fbpx
Wikipedia

Enzyme

January 31, 2023

"Biocatalyst" redirects here. For the use of natural catalysts in organic chemistry, see Biocatalysis.

Enzymes (/ˈɛnzmz/) are proteins that act as biological catalysts by accelerating chemical reactions. The molecules upon which enzymes may act are called substrates, and the enzyme converts the substrates into different molecules known as products. Almost all metabolic processes in the cell need enzyme catalysis in order to occur at rates fast enough to sustain life.[1]: 8.1  Metabolic pathways depend upon enzymes to catalyze individual steps. The study of enzymes is called enzymology and the field of pseudoenzyme analysis recognizes that during evolution, some enzymes have lost the ability to carry out biological catalysis, which is often reflected in their amino acid sequences and unusual 'pseudocatalytic' properties.[2][3]

The enzyme glucosidase converts the sugar maltose into two glucose sugars. Active site residues in red, maltose substrate in black, and NAD cofactor in yellow. (PDB: 1OBB​)

Enzymes are known to catalyze more than 5,000 biochemical reaction types.[4] Other biocatalysts are catalytic RNA molecules, called ribozymes. Enzymes' specificity comes from their unique three-dimensional structures.

Like all catalysts, enzymes increase the reaction rate by lowering its activation energy. Some enzymes can make their conversion of substrate to product occur many millions of times faster. An extreme example is orotidine 5'-phosphate decarboxylase, which allows a reaction that would otherwise take millions of years to occur in milliseconds.[5][6] Chemically, enzymes are like any catalyst and are not consumed in chemical reactions, nor do they alter the equilibrium of a reaction. Enzymes differ from most other catalysts by being much more specific. Enzyme activity can be affected by other molecules: inhibitors are molecules that decrease enzyme activity, and activators are molecules that increase activity. Many therapeutic drugs and poisons are enzyme inhibitors. An enzyme's activity decreases markedly outside its optimal temperature and pH, and many enzymes are (permanently) denatured when exposed to excessive heat, losing their structure and catalytic properties.

Some enzymes are used commercially, for example, in the synthesis of antibiotics. Some household products use enzymes to speed up chemical reactions: enzymes in biological washing powders break down protein, starch or fat stains on clothes, and enzymes in meat tenderizer break down proteins into smaller molecules, making the meat easier to chew.

Etymology and history

 
Eduard Buchner

By the late 17th and early 18th centuries, the digestion of meat by stomach secretions[7] and the conversion of starch to sugars by plant extracts and saliva were known but the mechanisms by which these occurred had not been identified.[8]

French chemist Anselme Payen was the first to discover an enzyme, diastase, in 1833.[9] A few decades later, when studying the fermentation of sugar to alcohol by yeast, Louis Pasteur concluded that this fermentation was caused by a vital force contained within the yeast cells called "ferments", which were thought to function only within living organisms. He wrote that "alcoholic fermentation is an act correlated with the life and organization of the yeast cells, not with the death or putrefaction of the cells."[10]

In 1877, German physiologist Wilhelm Kühne (1837–1900) first used the term enzyme, which comes from Greek ἔνζυμον, "leavened" or "in yeast", to describe this process.[11] The word enzyme was used later to refer to nonliving substances such as pepsin, and the word ferment was used to refer to chemical activity produced by living organisms.[12]

Eduard Buchner submitted his first paper on the study of yeast extracts in 1897. In a series of experiments at the University of Berlin, he found that sugar was fermented by yeast extracts even when there were no living yeast cells in the mixture.[13] He named the enzyme that brought about the fermentation of sucrose "zymase".[14] In 1907, he received the Nobel Prize in Chemistry for "his discovery of cell-free fermentation". Following Buchner's example, enzymes are usually named according to the reaction they carry out: the suffix -ase is combined with the name of the substrate (e.g., lactase is the enzyme that cleaves lactose) or to the type of reaction (e.g., DNA polymerase forms DNA polymers).[15]

The biochemical identity of enzymes was still unknown in the early 1900s. Many scientists observed that enzymatic activity was associated with proteins, but others (such as Nobel laureate Richard Willstätter) argued that proteins were merely carriers for the true enzymes and that proteins per se were incapable of catalysis.[16] In 1926, James B. Sumner showed that the enzyme urease was a pure protein and crystallized it; he did likewise for the enzyme catalase in 1937. The conclusion that pure proteins can be enzymes was definitively demonstrated by John Howard Northrop and Wendell Meredith Stanley, who worked on the digestive enzymes pepsin (1930), trypsin and chymotrypsin. These three scientists were awarded the 1946 Nobel Prize in Chemistry.[17]

The discovery that enzymes could be crystallized eventually allowed their structures to be solved by x-ray crystallography. This was first done for lysozyme, an enzyme found in tears, saliva and egg whites that digests the coating of some bacteria; the structure was solved by a group led by David Chilton Phillips and published in 1965.[18] This high-resolution structure of lysozyme marked the beginning of the field of structural biology and the effort to understand how enzymes work at an atomic level of detail.[19]

Classification and nomenclature

Enzymes can be classified by two main criteria: either amino acid sequence similarity (and thus evolutionary relationship) or enzymatic activity.

Enzyme activity. An enzyme's name is often derived from its substrate or the chemical reaction it catalyzes, with the word ending in -ase.[1]: 8.1.3  Examples are lactase, alcohol dehydrogenase and DNA polymerase. Different enzymes that catalyze the same chemical reaction are called isozymes.[1]: 10.3 

The International Union of Biochemistry and Molecular Biology have developed a nomenclature for enzymes, the EC numbers (for "Enzyme Commission"). Each enzyme is described by "EC" followed by a sequence of four numbers which represent the hierarchy of enzymatic activity (from very general to very specific). That is, the first number broadly classifies the enzyme based on its mechanism while the other digits add more and more specificity.[20]

The top-level classification is:

These sections are subdivided by other features such as the substrate, products, and chemical mechanism. An enzyme is fully specified by four numerical designations. For example, hexokinase (EC 2.7.1.1) is a transferase (EC 2) that adds a phosphate group (EC 2.7) to a hexose sugar, a molecule containing an alcohol group (EC 2.7.1).[21]

Sequence similarity. EC categories do not reflect sequence similarity. For instance, two ligases of the same EC number that catalyze exactly the same reaction can have completely different sequences. Independent of their function, enzymes, like any other proteins, have been classified by their sequence similarity into numerous families. These families have been documented in dozens of different protein and protein family databases such as Pfam.[22]

Structure

 
Enzyme activity initially increases with temperature (Q10 coefficient) until the enzyme's structure unfolds (denaturation), leading to an optimal rate of reaction at an intermediate temperature.
See also: Protein structure

Enzymes are generally globular proteins, acting alone or in larger complexes. The sequence of the amino acids specifies the structure which in turn determines the catalytic activity of the enzyme.[23] Although structure determines function, a novel enzymatic activity cannot yet be predicted from structure alone.[24] Enzyme structures unfold (denature) when heated or exposed to chemical denaturants and this disruption to the structure typically causes a loss of activity.[25] Enzyme denaturation is normally linked to temperatures above a species' normal level; as a result, enzymes from bacteria living in volcanic environments such as hot springs are prized by industrial users for their ability to function at high temperatures, allowing enzyme-catalysed reactions to be operated at a very high rate.

Enzymes are usually much larger than their substrates. Sizes range from just 62 amino acid residues, for the monomer of 4-oxalocrotonate tautomerase,[26] to over 2,500 residues in the animal fatty acid synthase.[27] Only a small portion of their structure (around 2–4 amino acids) is directly involved in catalysis: the catalytic site.[28] This catalytic site is located next to one or more binding sites where residues orient the substrates. The catalytic site and binding site together compose the enzyme's active site. The remaining majority of the enzyme structure serves to maintain the precise orientation and dynamics of the active site.[29]

In some enzymes, no amino acids are directly involved in catalysis; instead, the enzyme contains sites to bind and orient catalytic cofactors.[29] Enzyme structures may also contain allosteric sites where the binding of a small molecule causes a conformational change that increases or decreases activity.[30]

A small number of RNA-based biological catalysts called ribozymes exist, which again can act alone or in complex with proteins. The most common of these is the ribosome which is a complex of protein and catalytic RNA components.[1]: 2.2 

Mechanism

 
Organisation of enzyme structure and lysozyme example. Binding sites in blue, catalytic site in red and peptidoglycan substrate in black. (PDB: 9LYZ​)

Substrate binding

Enzymes must bind their substrates before they can catalyse any chemical reaction. Enzymes are usually very specific as to what substrates they bind and then the chemical reaction catalysed. Specificity is achieved by binding pockets with complementary shape, charge and hydrophilic/hydrophobic characteristics to the substrates. Enzymes can therefore distinguish between very similar substrate molecules to be chemoselective, regioselective and stereospecific.[31]

Some of the enzymes showing the highest specificity and accuracy are involved in the copying and expression of the genome. Some of these enzymes have "proof-reading" mechanisms. Here, an enzyme such as DNA polymerase catalyzes a reaction in a first step and then checks that the product is correct in a second step.[32] This two-step process results in average error rates of less than 1 error in 100 million reactions in high-fidelity mammalian polymerases.[1]: 5.3.1  Similar proofreading mechanisms are also found in RNA polymerase,[33] aminoacyl tRNA synthetases[34] and ribosomes.[35]

Conversely, some enzymes display enzyme promiscuity, having broad specificity and acting on a range of different physiologically relevant substrates. Many enzymes possess small side activities which arose fortuitously (i.e. neutrally), which may be the starting point for the evolutionary selection of a new function.[36][37]

 
Enzyme changes shape by induced fit upon substrate binding to form enzyme-substrate complex. Hexokinase has a large induced fit motion that closes over the substrates adenosine triphosphate and xylose. Binding sites in blue, substrates in black and Mg2+ cofactor in yellow. (PDB: 2E2N​, 2E2Q​)

"Lock and key" model

To explain the observed specificity of enzymes, in 1894 Emil Fischer proposed that both the enzyme and the substrate possess specific complementary geometric shapes that fit exactly into one another.[38] This is often referred to as "the lock and key" model.[1]: 8.3.2  This early model explains enzyme specificity, but fails to explain the stabilization of the transition state that enzymes achieve.[39]

Induced fit model

In 1958, Daniel Koshland suggested a modification to the lock and key model: since enzymes are rather flexible structures, the active site is continuously reshaped by interactions with the substrate as the substrate interacts with the enzyme.[40] As a result, the substrate does not simply bind to a rigid active site; the amino acid side-chains that make up the active site are molded into the precise positions that enable the enzyme to perform its catalytic function. In some cases, such as glycosidases, the substrate molecule also changes shape slightly as it enters the active site.[41] The active site continues to change until the substrate is completely bound, at which point the final shape and charge distribution is determined.[42] Induced fit may enhance the fidelity of molecular recognition in the presence of competition and noise via the conformational proofreading mechanism.[43]

Catalysis

See also: Enzyme catalysis and Transition state theory

Enzymes can accelerate reactions in several ways, all of which lower the activation energy (ΔG, Gibbs free energy)[44]

  1. By stabilizing the transition state:
    • Creating an environment with a charge distribution complementary to that of the transition state to lower its energy[45]
  2. By providing an alternative reaction pathway:
    • Temporarily reacting with the substrate, forming a covalent intermediate to provide a lower energy transition state[46]
  3. By destabilising the substrate ground state:
    • Distorting bound substrate(s) into their transition state form to reduce the energy required to reach the transition state[47]
    • By orienting the substrates into a productive arrangement to reduce the reaction entropy change[48] (the contribution of this mechanism to catalysis is relatively small)[49]

Enzymes may use several of these mechanisms simultaneously. For example, proteases such as trypsin perform covalent catalysis using a catalytic triad, stabilise charge build-up on the transition states using an oxyanion hole, complete hydrolysis using an oriented water substrate.[50]

Dynamics

See also: Protein dynamics

Enzymes are not rigid, static structures; instead they have complex internal dynamic motions – that is, movements of parts of the enzyme's structure such as individual amino acid residues, groups of residues forming a protein loop or unit of secondary structure, or even an entire protein domain. These motions give rise to a conformational ensemble of slightly different structures that interconvert with one another at equilibrium. Different states within this ensemble may be associated with different aspects of an enzyme's function. For example, different conformations of the enzyme dihydrofolate reductase are associated with the substrate binding, catalysis, cofactor release, and product release steps of the catalytic cycle,[51] consistent with catalytic resonance theory.

Substrate presentation

Substrate presentation is a process where the enzyme is sequestered away from its substrate. Enzymes can be sequestered to the plasma membrane away from a substrate in the nucleus or cytosol. Or within the membrane, an enzyme can be sequestered into lipid rafts away from its substrate in the disordered region. When the enzyme is released it mixes with its substrate. Alternatively, the enzyme can be sequestered near its substrate to activate the enzyme. For example, the enzyme can be soluble and upon activation bind to a lipid in the plasma membrane and then act upon molecules in the plasma membrane.

Allosteric modulation

Main article: Allosteric regulation

Allosteric sites are pockets on the enzyme, distinct from the active site, that bind to molecules in the cellular environment. These molecules then cause a change in the conformation or dynamics of the enzyme that is transduced to the active site and thus affects the reaction rate of the enzyme.[52] In this way, allosteric interactions can either inhibit or activate enzymes. Allosteric interactions with metabolites upstream or downstream in an enzyme's metabolic pathway cause feedback regulation, altering the activity of the enzyme according to the flux through the rest of the pathway.[53]

Cofactors

 
Chemical structure for thiamine pyrophosphate and protein structure of transketolase. Thiamine pyrophosphate cofactor in yellow and xylulose 5-phosphate substrate in black. (PDB: 4KXV​)
Main article: Cofactor (biochemistry)

Some enzymes do not need additional components to show full activity. Others require non-protein molecules called cofactors to be bound for activity.[54] Cofactors can be either inorganic (e.g., metal ions and iron–sulfur clusters) or organic compounds (e.g., flavin and heme). These cofactors serve many purposes; for instance, metal ions can help in stabilizing nucleophilic species within the active site.[55] Organic cofactors can be either coenzymes, which are released from the enzyme's active site during the reaction, or prosthetic groups, which are tightly bound to an enzyme. Organic prosthetic groups can be covalently bound (e.g., biotin in enzymes such as pyruvate carboxylase).[56]

An example of an enzyme that contains a cofactor is carbonic anhydrase, which uses a zinc cofactor bound as part of its active site.[57] These tightly bound ions or molecules are usually found in the active site and are involved in catalysis.[1]: 8.1.1  For example, flavin and heme cofactors are often involved in redox reactions.[1]: 17 

Enzymes that require a cofactor but do not have one bound are called apoenzymes or apoproteins. An enzyme together with the cofactor(s) required for activity is called a holoenzyme (or haloenzyme). The term holoenzyme can also be applied to enzymes that contain multiple protein subunits, such as the DNA polymerases; here the holoenzyme is the complete complex containing all the subunits needed for activity.[1]: 8.1.1 

Coenzymes

Coenzymes are small organic molecules that can be loosely or tightly bound to an enzyme. Coenzymes transport chemical groups from one enzyme to another.[58] Examples include NADH, NADPH and adenosine triphosphate (ATP). Some coenzymes, such as flavin mononucleotide (FMN), flavin adenine dinucleotide (FAD), thiamine pyrophosphate (TPP), and tetrahydrofolate (THF), are derived from vitamins. These coenzymes cannot be synthesized by the body de novo and closely related compounds (vitamins) must be acquired from the diet. The chemical groups carried include:

Since coenzymes are chemically changed as a consequence of enzyme action, it is useful to consider coenzymes to be a special class of substrates, or second substrates, which are common to many different enzymes. For example, about 1000 enzymes are known to use the coenzyme NADH.[59]

Coenzymes are usually continuously regenerated and their concentrations maintained at a steady level inside the cell. For example, NADPH is regenerated through the pentose phosphate pathway and S-adenosylmethionine by methionine adenosyltransferase. This continuous regeneration means that small amounts of coenzymes can be used very intensively. For example, the human body turns over its own weight in ATP each day.[60]

Thermodynamics

 
The energies of the stages of a chemical reaction. Uncatalysed (dashed line), substrates need a lot of activation energy to reach a transition state, which then decays into lower-energy products. When enzyme catalysed (solid line), the enzyme binds the substrates (ES), then stabilizes the transition state (ES) to reduce the activation energy required to produce products (EP) which are finally released.
Main articles: Activation energy, Thermodynamic equilibrium, and Chemical equilibrium

As with all catalysts, enzymes do not alter the position of the chemical equilibrium of the reaction. In the presence of an enzyme, the reaction runs in the same direction as it would without the enzyme, just more quickly.[1]: 8.2.3  For example, carbonic anhydrase catalyzes its reaction in either direction depending on the concentration of its reactants:[61]

  (in tissues; high CO2 concentration)

 

 

 

 

(1)

  (in lungs; low CO2 concentration)

 

 

 

 

(2)

The rate of a reaction is dependent on the activation energy needed to form the transition state which then decays into products. Enzymes increase reaction rates by lowering the energy of the transition state. First, binding forms a low energy enzyme-substrate complex (ES). Second, the enzyme stabilises the transition state such that it requires less energy to achieve compared to the uncatalyzed reaction (ES). Finally the enzyme-product complex (EP) dissociates to release the products.[1]: 8.3 

Enzymes can couple two or more reactions, so that a thermodynamically favorable reaction can be used to "drive" a thermodynamically unfavourable one so that the combined energy of the products is lower than the substrates. For example, the hydrolysis of ATP is often used to drive other chemical reactions.[62]

Kinetics

 
A chemical reaction mechanism with or without enzyme catalysis. The enzyme (E) binds substrate (S) to produce product (P).
 
Saturation curve for an enzyme reaction showing the relation between the substrate concentration and reaction rate.
Main article: Enzyme kinetics

Enzyme kinetics is the investigation of how enzymes bind substrates and turn them into products.[63] The rate data used in kinetic analyses are commonly obtained from enzyme assays. In 1913 Leonor Michaelis and Maud Leonora Menten proposed a quantitative theory of enzyme kinetics, which is referred to as Michaelis–Menten kinetics.[64] The major contribution of Michaelis and Menten was to think of enzyme reactions in two stages. In the first, the substrate binds reversibly to the enzyme, forming the enzyme-substrate complex. This is sometimes called the Michaelis–Menten complex in their honor. The enzyme then catalyzes the chemical step in the reaction and releases the product. This work was further developed by G. E. Briggs and J. B. S. Haldane, who derived kinetic equations that are still widely used today.[65]

Enzyme rates depend on solution conditions and substrate concentration. To find the maximum speed of an enzymatic reaction, the substrate concentration is increased until a constant rate of product formation is seen. This is shown in the saturation curve on the right. Saturation happens because, as substrate concentration increases, more and more of the free enzyme is converted into the substrate-bound ES complex. At the maximum reaction rate (Vmax) of the enzyme, all the enzyme active sites are bound to substrate, and the amount of ES complex is the same as the total amount of enzyme.[1]: 8.4 

Vmax is only one of several important kinetic parameters. The amount of substrate needed to achieve a given rate of reaction is also important. This is given by the Michaelis–Menten constant (Km), which is the substrate concentration required for an enzyme to reach one-half its maximum reaction rate; generally, each enzyme has a characteristic KM for a given substrate. Another useful constant is kcat, also called the turnover number, which is the number of substrate molecules handled by one active site per second.[1]: 8.4 

The efficiency of an enzyme can be expressed in terms of kcat/Km. This is also called the specificity constant and incorporates the rate constants for all steps in the reaction up to and including the first irreversible step. Because the specificity constant reflects both affinity and catalytic ability, it is useful for comparing different enzymes against each other, or the same enzyme with different substrates. The theoretical maximum for the specificity constant is called the diffusion limit and is about 108 to 109 (M−1 s−1). At this point every collision of the enzyme with its substrate will result in catalysis, and the rate of product formation is not limited by the reaction rate but by the diffusion rate. Enzymes with this property are called catalytically perfect or kinetically perfect. Example of such enzymes are triose-phosphate isomerase, carbonic anhydrase, acetylcholinesterase, catalase, fumarase, β-lactamase, and superoxide dismutase.[1]: 8.4.2  The turnover of such enzymes can reach several million reactions per second.[1]: 9.2  But most enzymes are far from perfect: the average values of   and   are about   and  , respectively.[66]

Michaelis–Menten kinetics relies on the law of mass action, which is derived from the assumptions of free diffusion and thermodynamically driven random collision. Many biochemical or cellular processes deviate significantly from these conditions, because of macromolecular crowding and constrained molecular movement.[67] More recent, complex extensions of the model attempt to correct for these effects.[68]

Inhibition

 
 
The coenzyme folic acid (left) and the anti-cancer drug methotrexate (right) are very similar in structure (differences show in green). As a result, methotrexate is a competitive inhibitor of many enzymes that use folates.
Main article: Enzyme inhibitor

Enzyme reaction rates can be decreased by various types of enzyme inhibitors.[69]: 73–74 

Types of inhibition

Competitive

A competitive inhibitor and substrate cannot bind to the enzyme at the same time.[70] Often competitive inhibitors strongly resemble the real substrate of the enzyme. For example, the drug methotrexate is a competitive inhibitor of the enzyme dihydrofolate reductase, which catalyzes the reduction of dihydrofolate to tetrahydrofolate.[71] The similarity between the structures of dihydrofolate and this drug are shown in the accompanying figure. This type of inhibition can be overcome with high substrate concentration. In some cases, the inhibitor can bind to a site other than the binding-site of the usual substrate and exert an allosteric effect to change the shape of the usual binding-site.[72]

Non-competitive

A non-competitive inhibitor binds to a site other than where the substrate binds. The substrate still binds with its usual affinity and hence Km remains the same. However the inhibitor reduces the catalytic efficiency of the enzyme so that Vmax is reduced. In contrast to competitive inhibition, non-competitive inhibition cannot be overcome with high substrate concentration.[69]: 76–78 

Uncompetitive

An uncompetitive inhibitor cannot bind to the free enzyme, only to the enzyme-substrate complex; hence, these types of inhibitors are most effective at high substrate concentration. In the presence of the inhibitor, the enzyme-substrate complex is inactive.[69]: 78  This type of inhibition is rare.[73]

Mixed

A mixed inhibitor binds to an allosteric site and the binding of the substrate and the inhibitor affect each other. The enzyme's function is reduced but not eliminated when bound to the inhibitor. This type of inhibitor does not follow the Michaelis–Menten equation.[69]: 76–78 

Irreversible

An irreversible inhibitor permanently inactivates the enzyme, usually by forming a covalent bond to the protein.[74] Penicillin[75] and aspirin[76] are common drugs that act in this manner.

Functions of inhibitors

In many organisms, inhibitors may act as part of a feedback mechanism. If an enzyme produces too much of one substance in the organism, that substance may act as an inhibitor for the enzyme at the beginning of the pathway that produces it, causing production of the substance to slow down or stop when there is sufficient amount. This is a form of negative feedback. Major metabolic pathways such as the citric acid cycle make use of this mechanism.[1]: 17.2.2 

Since inhibitors modulate the function of enzymes they are often used as drugs. Many such drugs are reversible competitive inhibitors that resemble the enzyme's native substrate, similar to methotrexate above; other well-known examples include statins used to treat high cholesterol,[77] and protease inhibitors used to treat retroviral infections such as HIV.[78] A common example of an irreversible inhibitor that is used as a drug is aspirin, which inhibits the COX-1 and COX-2 enzymes that produce the inflammation messenger prostaglandin.[76] Other enzyme inhibitors are poisons. For example, the poison cyanide is an irreversible enzyme inhibitor that combines with the copper and iron in the active site of the enzyme cytochrome c oxidase and blocks cellular respiration.[79]

Factors affecting enzyme activity

As enzymes are made up of proteins, their actions are sensitive to change in many physio chemical factors such as pH, temperature, substrate concentration, etc.

The following table shows pH optima for various enzymes.[80]

Enzyme Optimum pH pH description
Pepsin 1.5–1.6 Highly acidic
Invertase 4.5 Acidic
Lipase (stomach) 4.0–5.0 Acidic
Lipase (castor oil) 4.7 Acidic
Lipase (pancreas) 8.0 Alkaline
Amylase (malt) 4.6–5.2 Acidic
Amylase (pancreas) 6.7–7.0 Acidic-neutral
Cellobiase 5.0 Acidic
Maltase 6.1–6.8 Acidic
Sucrase 6.2 Acidic
Catalase 7.0 Neutral
Urease 7.0 Neutral
Cholinesterase 7.0 Neutral
Ribonuclease 7.0–7.5 Neutral
Fumarase 7.8 Alkaline
Trypsin 7.8–8.7 Alkaline
Adenosine triphosphate 9.0 Alkaline
Arginase 10.0 Highly alkaline

Biological function

Enzymes serve a wide variety of functions inside living organisms. They are indispensable for signal transduction and cell regulation, often via kinases and phosphatases.[81] They also generate movement, with myosin hydrolyzing adenosine triphosphate (ATP) to generate muscle contraction, and also transport cargo around the cell as part of the cytoskeleton.[82] Other ATPases in the cell membrane are ion pumps involved in active transport. Enzymes are also involved in more exotic functions, such as luciferase generating light in fireflies.[83] Viruses can also contain enzymes for infecting cells, such as the HIV integrase and reverse transcriptase, or for viral release from cells, like the influenza virus neuraminidase.[84]

An important function of enzymes is in the digestive systems of animals. Enzymes such as amylases and proteases break down large molecules (starch or proteins, respectively) into smaller ones, so they can be absorbed by the intestines. Starch molecules, for example, are too large to be absorbed from the intestine, but enzymes hydrolyze the starch chains into smaller molecules such as maltose and eventually glucose, which can then be absorbed. Different enzymes digest different food substances. In ruminants, which have herbivorous diets, microorganisms in the gut produce another enzyme, cellulase, to break down the cellulose cell walls of plant fiber.[85]

Metabolism

 
The metabolic pathway of glycolysis releases energy by converting glucose to pyruvate via a series of intermediate metabolites. Each chemical modification (red box) is performed by a different enzyme.

Several enzymes can work together in a specific order, creating metabolic pathways.[1]: 30.1  In a metabolic pathway, one enzyme takes the product of another enzyme as a substrate. After the catalytic reaction, the product is then passed on to another enzyme. Sometimes more than one enzyme can catalyze the same reaction in parallel; this can allow more complex regulation: with, for example, a low constant activity provided by one enzyme but an inducible high activity from a second enzyme.[86]

Enzymes determine what steps occur in these pathways. Without enzymes, metabolism would neither progress through the same steps and could not be regulated to serve the needs of the cell. Most central metabolic pathways are regulated at a few key steps, typically through enzymes whose activity involves the hydrolysis of ATP. Because this reaction releases so much energy, other reactions that are thermodynamically unfavorable can be coupled to ATP hydrolysis, driving the overall series of linked metabolic reactions.[1]: 30.1 

Control of activity

There are five main ways that enzyme activity is controlled in the cell.[1]: 30.1.1 

Regulation

Enzymes can be either activated or inhibited by other molecules. For example, the end product(s) of a metabolic pathway are often inhibitors for one of the first enzymes of the pathway (usually the first irreversible step, called committed step), thus regulating the amount of end product made by the pathways. Such a regulatory mechanism is called a negative feedback mechanism, because the amount of the end product produced is regulated by its own concentration.[87]: 141–48  Negative feedback mechanism can effectively adjust the rate of synthesis of intermediate metabolites according to the demands of the cells. This helps with effective allocations of materials and energy economy, and it prevents the excess manufacture of end products. Like other homeostatic devices, the control of enzymatic action helps to maintain a stable internal environment in living organisms.[87]: 141 

Post-translational modification

Examples of post-translational modification include phosphorylation, myristoylation and glycosylation.[87]: 149–69  For example, in the response to insulin, the phosphorylation of multiple enzymes, including glycogen synthase, helps control the synthesis or degradation of glycogen and allows the cell to respond to changes in blood sugar.[88] Another example of post-translational modification is the cleavage of the polypeptide chain. Chymotrypsin, a digestive protease, is produced in inactive form as chymotrypsinogen in the pancreas and transported in this form to the stomach where it is activated. This stops the enzyme from digesting the pancreas or other tissues before it enters the gut. This type of inactive precursor to an enzyme is known as a zymogen[87]: 149–53  or proenzyme.

Quantity

Enzyme production (transcription and translation of enzyme genes) can be enhanced or diminished by a cell in response to changes in the cell's environment. This form of gene regulation is called enzyme induction. For example, bacteria may become resistant to antibiotics such as penicillin because enzymes called beta-lactamases are induced that hydrolyse the crucial beta-lactam ring within the penicillin molecule.[89] Another example comes from enzymes in the liver called cytochrome P450 oxidases, which are important in drug metabolism. Induction or inhibition of these enzymes can cause drug interactions.[90] Enzyme levels can also be regulated by changing the rate of enzyme degradation.[1]: 30.1.1  The opposite of enzyme induction is enzyme repression.

Subcellular distribution

Enzymes can be compartmentalized, with different metabolic pathways occurring in different cellular compartments. For example, fatty acids are synthesized by one set of enzymes in the cytosol, endoplasmic reticulum and Golgi and used by a different set of enzymes as a source of energy in the mitochondrion, through β-oxidation.[91] In addition, trafficking of the enzyme to different compartments may change the degree of protonation (e.g., the neutral cytoplasm and the acidic lysosome) or oxidative state (e.g., oxidizing periplasm or reducing cytoplasm) which in turn affects enzyme activity.[92] In contrast to partitioning into membrane bound organelles, enzyme subcellular localisation may also be altered through polymerisation of enzymes into macromolecular cytoplasmic filaments.[93][94]

Organ specialization

In multicellular eukaryotes, cells in different organs and tissues have different patterns of gene expression and therefore have different sets of enzymes (known as isozymes) available for metabolic reactions. This provides a mechanism for regulating the overall metabolism of the organism. For example, hexokinase, the first enzyme in the glycolysis pathway, has a specialized form called glucokinase expressed in the liver and pancreas that has a lower affinity for glucose yet is more sensitive to glucose concentration.[95] This enzyme is involved in sensing blood sugar and regulating insulin production.[96]

Involvement in disease

 
In phenylalanine hydroxylase over 300 different mutations throughout the structure cause phenylketonuria. Phenylalanine substrate and tetrahydrobiopterin coenzyme in black, and Fe2+ cofactor in yellow. (PDB: 1KW0​)
 
Hereditary defects in enzymes are generally inherited in an autosomal fashion because there are more non-X chromosomes than X-chromosomes, and a recessive fashion because the enzymes from the unaffected genes are generally sufficient to prevent symptoms in carriers.
See also: Genetic disorder

Since the tight control of enzyme activity is essential for homeostasis, any malfunction (mutation, overproduction, underproduction or deletion) of a single critical enzyme can lead to a genetic disease. The malfunction of just one type of enzyme out of the thousands of types present in the human body can be fatal. An example of a fatal genetic disease due to enzyme insufficiency is Tay–Sachs disease, in which patients lack the enzyme hexosaminidase.[97][98]

One example of enzyme deficiency is the most common type of phenylketonuria. Many different single amino acid mutations in the enzyme phenylalanine hydroxylase, which catalyzes the first step in the degradation of phenylalanine, result in build-up of phenylalanine and related products. Some mutations are in the active site, directly disrupting binding and catalysis, but many are far from the active site and reduce activity by destabilising the protein structure, or affecting correct oligomerisation.[99][100] This can lead to intellectual disability if the disease is untreated.[101] Another example is pseudocholinesterase deficiency, in which the body's ability to break down choline ester drugs is impaired.[102] Oral administration of enzymes can be used to treat some functional enzyme deficiencies, such as pancreatic insufficiency[103] and lactose intolerance.[104]

Another way enzyme malfunctions can cause disease comes from germline mutations in genes coding for DNA repair enzymes. Defects in these enzymes cause cancer because cells are less able to repair mutations in their genomes. This causes a slow accumulation of mutations and results in the development of cancers. An example of such a hereditary cancer syndrome is xeroderma pigmentosum, which causes the development of skin cancers in response to even minimal exposure to ultraviolet light.[105][106]

Evolution

Similar to any other protein, enzymes change over time through mutations and sequence divergence. Given their central role in metabolism, enzyme evolution plays a critical role in adaptation. A key question is therefore whether and how enzymes can change their enzymatic activities alongside. It is generally accepted that many new enzyme activities have evolved through gene duplication and mutation of the duplicate copies although evolution can also happen without duplication. One example of an enzyme that has changed its activity is the ancestor of methionyl aminopeptidase (MAP) and creatine amidinohydrolase (creatinase) which are clearly homologous but catalyze very different reactions (MAP removes the amino-terminal methionine in new proteins while creatinase hydrolyses creatine to sarcosine and urea). In addition, MAP is metal-ion dependent while creatinase is not, hence this property was also lost over time.[107] Small changes of enzymatic activity are extremely common among enzymes. In particular, substrate binding specificity (see above) can easily and quickly change with single amino acid changes in their substrate binding pockets. This is frequently seen in the main enzyme classes such as kinases.[108]

Artificial (in vitro) evolution is now commonly used to modify enzyme activity or specificity for industrial applications (see below).

Industrial applications

Main article: Industrial enzymes

Enzymes are used in the chemical industry and other industrial applications when extremely specific catalysts are required. Enzymes in general are limited in the number of reactions they have evolved to catalyze and also by their lack of stability in organic solvents and at high temperatures. As a consequence, protein engineering is an active area of research and involves attempts to create new enzymes with novel properties, either through rational design or in vitro evolution.[109][110] These efforts have begun to be successful, and a few enzymes have now been designed "from scratch" to catalyze reactions that do not occur in nature.[111]

Application Enzymes used Uses
Biofuel industry Cellulases Break down cellulose into sugars that can be fermented to produce cellulosic ethanol.[112]
Ligninases Pretreatment of biomass for biofuel production.[112]
Biological detergent Proteases, amylases, lipases Remove protein, starch, and fat or oil stains from laundry and dishware.[113]
Mannanases Remove food stains from the common food additive guar gum.[113]
Brewing industry Amylase, glucanases, proteases Split polysaccharides and proteins in the malt.[114]: 150–9 
Betaglucanases Improve the wort and beer filtration characteristics.[114]: 545 
Amyloglucosidase and pullulanases Make low-calorie beer and adjust fermentability.[114]: 575 
Acetolactate decarboxylase (ALDC) Increase fermentation efficiency by reducing diacetyl formation.[115]
Culinary uses Papain Tenderize meat for cooking.[116]
Dairy industry Rennin Hydrolyze protein in the manufacture of cheese.[117]
Lipases Produce Camembert cheese and blue cheeses such as Roquefort.[118]
Food processing Amylases Produce sugars from starch, such as in making high-fructose corn syrup.[119]
Proteases Lower the protein level of flour, as in biscuit-making.[120]
Trypsin Manufacture hypoallergenic baby foods.[120]
Cellulases, pectinases Clarify fruit juices.[121]
Molecular biology Nucleases, DNA ligase and polymerases Use restriction digestion and the polymerase chain reaction to create recombinant DNA.[1]: 6.2 
Paper industry Xylanases, hemicellulases and lignin peroxidases Remove lignin from kraft pulp.[122]
Personal care Proteases Remove proteins on contact lenses to prevent infections.[123]
Starch industry Amylases Convert starch into glucose and various syrups.[124]

See also

Enzyme databases

References

  1. ^ a b c d e f g h i j k l m n o p q r s t u Stryer L, Berg JM, Tymoczko JL (2002). Biochemistry (5th ed.). San Francisco: W.H. Freeman. ISBN 0-7167-4955-6. 
  2. ^ Murphy JM, Farhan H, Eyers PA (2017). "Bio-Zombie: the rise of pseudoenzymes in biology". Biochem Soc Trans. 45 (2): 537–544. doi:10.1042/bst20160400. PMID 28408493.
  3. ^ Murphy JM, et al. (2014). "A robust methodology to subclassify pseudokinases based on their nucleotide-binding properties". Biochemical Journal. 457 (2): 323–334. doi:10.1042/BJ20131174. PMC 5679212. PMID 24107129.
  4. ^ Schomburg I, Chang A, Placzek S, Söhngen C, Rother M, Lang M, Munaretto C, Ulas S, Stelzer M, Grote A, Scheer M, Schomburg D (January 2013). "BRENDA in 2013: integrated reactions, kinetic data, enzyme function data, improved disease classification: new options and contents in BRENDA". Nucleic Acids Research. 41 (Database issue): D764–72. doi:10.1093/nar/gks1049. PMC 3531171. PMID 23203881.
  5. ^ Radzicka A, Wolfenden R (January 1995). "A proficient enzyme". Science. 267 (5194): 90–931. Bibcode:1995Sci...267...90R. doi:10.1126/science.7809611. PMID 7809611. S2CID 8145198.
  6. ^ Callahan BP, Miller BG (December 2007). "OMP decarboxylase—An enigma persists". Bioorganic Chemistry. 35 (6): 465–9. doi:10.1016/j.bioorg.2007.07.004. PMID 17889251.
  7. ^ de Réaumur RA (1752). "Observations sur la digestion des oiseaux". Histoire de l'Académie Royale des Sciences. 1752: 266, 461.
  8. ^ Williams HS (1904). A History of Science: in Five Volumes. Volume IV: Modern Development of the Chemical and Biological Sciences. Harper and Brothers.
  9. ^ Payen A, Persoz JF (1833). "Mémoire sur la diastase, les principaux produits de ses réactions et leurs applications aux arts industriels" [Memoir on diastase, the principal products of its reactions, and their applications to the industrial arts]. Annales de chimie et de physique. 2nd (in French). 53: 73–92.
  10. ^ Manchester KL (December 1995). "Louis Pasteur (1822–1895)–chance and the prepared mind". Trends in Biotechnology. 13 (12): 511–5. doi:10.1016/S0167-7799(00)89014-9. PMID 8595136.
  11. ^ Kühne coined the word "enzyme" in: Kühne W (1877). "Über das Verhalten verschiedener organisirter und sog. ungeformter Fermente" [On the behavior of various organized and so-called unformed ferments]. Verhandlungen des Naturhistorisch-medicinischen Vereins zu Heidelberg. new series (in German). 1 (3): 190–193. Relevant passage on page 190: "Um Missverständnissen vorzubeugen und lästige Umschreibungen zu vermeiden schlägt Vortragender vor, die ungeformten oder nicht organisirten Fermente, deren Wirkung ohne Anwesenheit von Organismen und ausserhalb derselben erfolgen kann, als Enzyme zu bezeichnen." (Translation: In order to obviate misunderstandings and avoid cumbersome periphrases, [the author, a university lecturer] suggests designating as "enzymes" the unformed or not organized ferments, whose action can occur without the presence of organisms and outside of the same.)
  12. ^ Holmes FL (2003). "Enzymes". In Heilbron JL (ed.). The Oxford Companion to the History of Modern Science. Oxford: Oxford University Press. p. 270. ISBN 9780199743766.
  13. ^ "Eduard Buchner". Nobel Laureate Biography. Nobelprize.org. Retrieved 23 February 2015.
  14. ^ "Eduard Buchner – Nobel Lecture: Cell-Free Fermentation". Nobelprize.org. 1907. Retrieved 23 February 2015.
  15. ^ The naming of enzymes by adding the suffix "-ase" to the substrate on which the enzyme acts, has been traced to French scientist Émile Duclaux (1840–1904), who intended to honor the discoverers of diastase – the first enzyme to be isolated – by introducing this practice in his book Duclaux E (1899). Traité de microbiologie: Diastases, toxines et venins [Microbiology Treatise: diastases, toxins and venoms] (in French). Paris, France: Masson and Co. See Chapter 1, especially page 9.
  16. ^ Willstätter R (1927). "Faraday lecture. Problems and methods in enzyme research". Journal of the Chemical Society (Resumed): 1359–1381. doi:10.1039/JR9270001359. quoted in Blow D (April 2000). "So do we understand how enzymes work?". Structure. 8 (4): R77–R81. doi:10.1016/S0969-2126(00)00125-8. PMID 10801479.
  17. ^ "Nobel Prizes and Laureates: The Nobel Prize in Chemistry 1946". Nobelprize.org. Retrieved 23 February 2015.
  18. ^ Blake CC, Koenig DF, Mair GA, North AC, Phillips DC, Sarma VR (May 1965). "Structure of hen egg-white lysozyme. A three-dimensional Fourier synthesis at 2 Ångström resolution". Nature. 206 (4986): 757–61. Bibcode:1965Natur.206..757B. doi:10.1038/206757a0. PMID 5891407. S2CID 4161467.
  19. ^ Johnson LN, Petsko GA (1999). "David Phillips and the origin of structural enzymology". Trends Biochem. Sci. 24 (7): 287–9. doi:10.1016/S0968-0004(99)01423-1. PMID 10390620.
  20. ^ Moss GP. "Recommendations of the Nomenclature Committee of the International Union of Biochemistry and Molecular Biology on the Nomenclature and Classification of Enzymes by the Reactions they Catalyse". International Union of Biochemistry and Molecular Biology. Retrieved 28 August 2021.
  21. ^ Nomenclature Committee. . International Union of Biochemistry and Molecular Biology (NC-IUBMB). School of Biological and Chemical Sciences, Queen Mary, University of London. Archived from the original on 1 December 2014. Retrieved 6 March 2015.
  22. ^ Mulder NJ (28 September 2007). "Protein Family Databases". eLS. Chichester, UK: John Wiley & Sons, Ltd. pp. a0003058.pub2. doi:10.1002/9780470015902.a0003058.pub2. ISBN 978-0-470-01617-6.
  23. ^ Anfinsen CB (July 1973). "Principles that govern the folding of protein chains". Science. 181 (4096): 223–30. Bibcode:1973Sci...181..223A. doi:10.1126/science.181.4096.223. PMID 4124164.
  24. ^ Dunaway-Mariano D (November 2008). "Enzyme function discovery". Structure. 16 (11): 1599–600. doi:10.1016/j.str.2008.10.001. PMID 19000810.
  25. ^ Petsko GA, Ringe D (2003). "Chapter 1: From sequence to structure". Protein structure and function. London: New Science. p. 27. ISBN 978-1405119221.
  26. ^ Chen LH, Kenyon GL, Curtin F, Harayama S, Bembenek ME, Hajipour G, Whitman CP (September 1992). "4-Oxalocrotonate tautomerase, an enzyme composed of 62 amino acid residues per monomer". The Journal of Biological Chemistry. 267 (25): 17716–21. doi:10.1016/S0021-9258(19)37101-7. PMID 1339435.
  27. ^ Smith S (December 1994). "The animal fatty acid synthase: one gene, one polypeptide, seven enzymes". FASEB Journal. 8 (15): 1248–59. doi:10.1096/fasebj.8.15.8001737. PMID 8001737. S2CID 22853095.
  28. ^ "The Catalytic Site Atlas". The European Bioinformatics Institute. Retrieved 4 April 2007.
  29. ^ a b Suzuki H (2015). "Chapter 7: Active Site Structure". How Enzymes Work: From Structure to Function. Boca Raton, FL: CRC Press. pp. 117–140. ISBN 978-981-4463-92-8.
  30. ^ Krauss G (2003). "The Regulations of Enzyme Activity". Biochemistry of Signal Transduction and Regulation (3rd ed.). Weinheim: Wiley-VCH. pp. 89–114. ISBN 9783527605767.
  31. ^ Jaeger KE, Eggert T (August 2004). "Enantioselective biocatalysis optimized by directed evolution". Current Opinion in Biotechnology. 15 (4): 305–13. doi:10.1016/j.copbio.2004.06.007. PMID 15358000.
  32. ^ Shevelev IV, Hübscher U (May 2002). "The 3' 5' exonucleases". Nature Reviews Molecular Cell Biology. 3 (5): 364–76. doi:10.1038/nrm804. PMID 11988770. S2CID 31605786.
  33. ^ Zenkin N, Yuzenkova Y, Severinov K (July 2006). "Transcript-assisted transcriptional proofreading". Science. 313 (5786): 518–20. Bibcode:2006Sci...313..518Z. doi:10.1126/science.1127422. PMID 16873663. S2CID 40772789.
  34. ^ Ibba M, Soll D (2000). "Aminoacyl-tRNA synthesis". Annual Review of Biochemistry. 69: 617–50. doi:10.1146/annurev.biochem.69.1.617. PMID 10966471.
  35. ^ Rodnina MV, Wintermeyer W (2001). "Fidelity of aminoacyl-tRNA selection on the ribosome: kinetic and structural mechanisms". Annual Review of Biochemistry. 70: 415–35. doi:10.1146/annurev.biochem.70.1.415. PMID 11395413.
  36. ^ Khersonsky O, Tawfik DS (2010). "Enzyme promiscuity: a mechanistic and evolutionary perspective". Annual Review of Biochemistry. 79: 471–505. doi:10.1146/annurev-biochem-030409-143718. PMID 20235827.
  37. ^ O'Brien PJ, Herschlag D (April 1999). "Catalytic promiscuity and the evolution of new enzymatic activities". Chemistry & Biology. 6 (4): R91–R105. doi:10.1016/S1074-5521(99)80033-7. PMID 10099128.
  38. ^ Fischer E (1894). "Einfluss der Configuration auf die Wirkung der Enzyme" [Influence of configuration on the action of enzymes]. Berichte der Deutschen Chemischen Gesellschaft zu Berlin (in German). 27 (3): 2985–93. doi:10.1002/cber.18940270364. From page 2992: "Um ein Bild zu gebrauchen, will ich sagen, dass Enzym und Glucosid wie Schloss und Schlüssel zu einander passen müssen, um eine chemische Wirkung auf einander ausüben zu können." (To use an image, I will say that an enzyme and a glucoside [i.e., glucose derivative] must fit like a lock and key, in order to be able to exert a chemical effect on each other.)
  39. ^ Cooper GM (2000). "Chapter 2.2: The Central Role of Enzymes as Biological Catalysts". The Cell: a Molecular Approach (2nd ed.). Washington (DC ): ASM Press. ISBN 0-87893-106-6.
  40. ^ Koshland DE (February 1958). "Application of a Theory of Enzyme Specificity to Protein Synthesis". Proceedings of the National Academy of Sciences of the United States of America. 44 (2): 98–104. Bibcode:1958PNAS...44...98K. doi:10.1073/pnas.44.2.98. PMC 335371. PMID 16590179.
  41. ^ Vasella A, Davies GJ, Böhm M (October 2002). "Glycosidase mechanisms". Current Opinion in Chemical Biology. 6 (5): 619–29. doi:10.1016/S1367-5931(02)00380-0. PMID 12413546.
  42. ^ Boyer R (2002). "Chapter 6: Enzymes I, Reactions, Kinetics, and Inhibition". Concepts in Biochemistry (2nd ed.). New York, Chichester, Weinheim, Brisbane, Singapore, Toronto.: John Wiley & Sons, Inc. pp. 137–8. ISBN 0-470-00379-0. OCLC 51720783.
  43. ^ Savir Y, Tlusty T (2007). Scalas E (ed.). "Conformational proofreading: the impact of conformational changes on the specificity of molecular recognition". PLOS ONE. 2 (5): e468. Bibcode:2007PLoSO...2..468S. doi:10.1371/journal.pone.0000468. PMC 1868595. PMID 17520027.
  44. ^ Fersht A (1985). Enzyme Structure and Mechanism. San Francisco: W.H. Freeman. pp. 50–2. ISBN 978-0-7167-1615-0.
  45. ^ Warshel A, Sharma PK, Kato M, Xiang Y, Liu H, Olsson MH (August 2006). "Electrostatic basis for enzyme catalysis". Chemical Reviews. 106 (8): 3210–35. doi:10.1021/cr0503106. PMID 16895325.
  46. ^ Cox MM, Nelson DL (2013). "Chapter 6.2: How enzymes work". Lehninger Principles of Biochemistry (6th ed.). New York, N.Y.: W.H. Freeman. p. 195. ISBN 978-1464109621.
  47. ^ Benkovic SJ, Hammes-Schiffer S (August 2003). "A perspective on enzyme catalysis". Science. 301 (5637): 1196–202. Bibcode:2003Sci...301.1196B. doi:10.1126/science.1085515. PMID 12947189. S2CID 7899320.
  48. ^ Jencks WP (1987). Catalysis in Chemistry and Enzymology. Mineola, N.Y: Dover. ISBN 978-0-486-65460-7.
  49. ^ Villa J, Strajbl M, Glennon TM, Sham YY, Chu ZT, Warshel A (October 2000). "How important are entropic contributions to enzyme catalysis?". Proceedings of the National Academy of Sciences of the United States of America. 97 (22): 11899–904. Bibcode:2000PNAS...9711899V. doi:10.1073/pnas.97.22.11899. PMC 17266. PMID 11050223.
  50. ^ Polgár L (October 2005). "The catalytic triad of serine peptidases". Cellular and Molecular Life Sciences. 62 (19–20): 2161–2172. doi:10.1007/s00018-005-5160-x. PMID 16003488. S2CID 3343824.
  51. ^ Ramanathan A, Savol A, Burger V, Chennubhotla CS, Agarwal PK (2014). "Protein conformational populations and functionally relevant substates". Acc. Chem. Res. 47 (1): 149–56. doi:10.1021/ar400084s. OSTI 1565147. PMID 23988159.
  52. ^ Tsai CJ, Del Sol A, Nussinov R (2009). "Protein allostery, signal transmission and dynamics: a classification scheme of allosteric mechanisms" (PDF). Mol Biosyst. 5 (3): 207–16. doi:10.1039/b819720b. PMC 2898650. PMID 19225609.
  53. ^ Changeux JP, Edelstein SJ (June 2005). "Allosteric mechanisms of signal transduction". Science. 308 (5727): 1424–8. Bibcode:2005Sci...308.1424C. doi:10.1126/science.1108595. PMID 15933191. S2CID 10621930.
  54. ^ de Bolster MW (1997). . International Union of Pure and Applied Chemistry. Archived from the original on 21 January 2017. Retrieved 30 October 2007.
  55. ^ Voet D, Voet J, Pratt C (2016). Fundamentals of Biochemistry. Hoboken, New Jersey: John Wiley & Sons, Inc. p. 336. ISBN 978-1-118-91840-1.
  56. ^ Chapman-Smith A, Cronan JE (September 1999). "The enzymatic biotinylation of proteins: a post-translational modification of exceptional specificity". Trends in Biochemical Sciences. 24 (9): 359–363. doi:10.1016/s0968-0004(99)01438-3. PMID 10470036.
  57. ^ Fisher Z, Hernandez Prada JA, Tu C, Duda D, Yoshioka C, An H, Govindasamy L, Silverman DN, McKenna R (February 2005). "Structural and kinetic characterization of active-site histidine as a proton shuttle in catalysis by human carbonic anhydrase II". Biochemistry. 44 (4): 1097–115. doi:10.1021/bi0480279. PMID 15667203.
  58. ^ a b Wagner AL (1975). Vitamins and Coenzymes. Krieger Pub Co. ISBN 0-88275-258-8.
  59. ^ "BRENDA The Comprehensive Enzyme Information System". Technische Universität Braunschweig. Retrieved 23 February 2015.
  60. ^ Törnroth-Horsefield S, Neutze R (December 2008). "Opening and closing the metabolite gate". Proceedings of the National Academy of Sciences of the United States of America. 105 (50): 19565–6. Bibcode:2008PNAS..10519565T. doi:10.1073/pnas.0810654106. PMC 2604989. PMID 19073922.
  61. ^ McArdle WD, Katch F, Katch VL (2006). "Chapter 9: The Pulmonary System and Exercise". Essentials of Exercise Physiology (3rd ed.). Baltimore, Maryland: Lippincott Williams & Wilkins. pp. 312–3. ISBN 978-0781749916.
  62. ^ Ferguson SJ, Nicholls D, Ferguson S (2002). Bioenergetics 3 (3rd ed.). San Diego: Academic. ISBN 0-12-518121-3.
  63. ^ Bisswanger H (2017). Enzyme kinetics : principles and methods (Third, enlarged and improved ed.). Weinheim, Germany. ISBN 9783527806461. OCLC 992976641.
  64. ^ Michaelis L, Menten M (1913). "Die Kinetik der Invertinwirkung" [The Kinetics of Invertase Action]. Biochem. Z. (in German). 49: 333–369.; Michaelis L, Menten ML, Johnson KA, Goody RS (2011). "The original Michaelis constant: translation of the 1913 Michaelis–Menten paper". Biochemistry. 50 (39): 8264–9. doi:10.1021/bi201284u. PMC 3381512. PMID 21888353.
  65. ^ Briggs GE, Haldane JB (1925). "A Note on the Kinetics of Enzyme Action". The Biochemical Journal. 19 (2): 338–9. doi:10.1042/bj0190338. PMC 1259181. PMID 16743508.
  66. ^ Bar-Even A, Noor E, Savir Y, Liebermeister W, Davidi D, Tawfik DS, Milo R (2011). "The moderately efficient enzyme: evolutionary and physicochemical trends shaping enzyme parameters". Biochemistry. 50 (21): 4402–10. doi:10.1021/bi2002289. PMID 21506553.
  67. ^ Ellis RJ (October 2001). "Macromolecular crowding: obvious but underappreciated". Trends in Biochemical Sciences. 26 (10): 597–604. doi:10.1016/S0968-0004(01)01938-7. PMID 11590012.
  68. ^ Kopelman R (September 1988). "Fractal reaction kinetics". Science. 241 (4873): 1620–26. Bibcode:1988Sci...241.1620K. doi:10.1126/science.241.4873.1620. PMID 17820893. S2CID 23465446.
  69. ^ a b c d Cornish-Bowden A (2004). Fundamentals of Enzyme Kinetics (3 ed.). London: Portland Press. ISBN 1-85578-158-1.
  70. ^ Price NC (1979). "What is meant by 'competitive inhibition'?". Trends in Biochemical Sciences. 4 (11): N272–N273. doi:10.1016/0968-0004(79)90205-6.
  71. ^ Goodsell DS (1 August 1999). "The Molecular Perspective: Methotrexate". The Oncologist. 4 (4): 340–341. doi:10.1634/theoncologist.4-4-340. ISSN 1083-7159. PMID 10476546.
  72. ^ Wu P, Clausen MH, Nielsen TE (December 2015). "Allosteric small-molecule kinase inhibitors" (PDF). Pharmacology & Therapeutics. 156: 59–68. doi:10.1016/j.pharmthera.2015.10.002. PMID 26478442.
  73. ^ Cornish-Bowden A (July 1986). "Why is uncompetitive inhibition so rare? A possible explanation, with implications for the design of drugs and pesticides". FEBS Letters. 203 (1): 3–6. doi:10.1016/0014-5793(86)81424-7. PMID 3720956. S2CID 45356060.
  74. ^ Strelow JM (1 January 2017). "A Perspective on the Kinetics of Covalent and Irreversible Inhibition". SLAS Discovery. 22 (1): 3–20. doi:10.1177/1087057116671509. ISSN 2472-5552. PMID 27703080.
  75. ^ Fisher JF, Meroueh SO, Mobashery S (February 2005). "Bacterial resistance to beta-lactam antibiotics: compelling opportunism, compelling opportunity". Chemical Reviews. 105 (2): 395–424. doi:10.1021/cr030102i. PMID 15700950.
  76. ^ a b Johnson DS, Weerapana E, Cravatt BF (June 2010). "Strategies for discovering and derisking covalent, irreversible enzyme inhibitors". Future Medicinal Chemistry. 2 (6): 949–64. doi:10.4155/fmc.10.21. PMC 2904065. PMID 20640225.
  77. ^ Endo A (1 November 1992). "The discovery and development of HMG-CoA reductase inhibitors". J. Lipid Res. 33 (11): 1569–82. doi:10.1016/S0022-2275(20)41379-3. PMID 1464741.
  78. ^ Wlodawer A, Vondrasek J (1998). "Inhibitors of HIV-1 protease: a major success of structure-assisted drug design". Annual Review of Biophysics and Biomolecular Structure. 27: 249–84. doi:10.1146/annurev.biophys.27.1.249. PMID 9646869. S2CID 10205781.
  79. ^ Yoshikawa S, Caughey WS (May 1990). "Infrared evidence of cyanide binding to iron and copper sites in bovine heart cytochrome c oxidase. Implications regarding oxygen reduction". The Journal of Biological Chemistry. 265 (14): 7945–58. doi:10.1016/S0021-9258(19)39023-4. PMID 2159465.
  80. ^ Jain JL (May 1999). Fundamentals of biochemistry. New Delhi: S. Chand and Co. ISBN 8121903432. OCLC 818809626.
  81. ^ Hunter T (January 1995). "Protein kinases and phosphatases: the yin and yang of protein phosphorylation and signaling". Cell. 80 (2): 225–36. doi:10.1016/0092-8674(95)90405-0. PMID 7834742. S2CID 13999125.
  82. ^ Berg JS, Powell BC, Cheney RE (April 2001). "A millennial myosin census". Molecular Biology of the Cell. 12 (4): 780–94. doi:10.1091/mbc.12.4.780. PMC 32266. PMID 11294886.
  83. ^ Meighen EA (March 1991). "Molecular biology of bacterial bioluminescence". Microbiological Reviews. 55 (1): 123–42. doi:10.1128/MMBR.55.1.123-142.1991. PMC 372803. PMID 2030669.
  84. ^ De Clercq E (2002). "Highlights in the development of new antiviral agents". Mini Rev Med Chem. 2 (2): 163–75. doi:10.2174/1389557024605474. PMID 12370077.
  85. ^ Mackie RI, White BA (October 1990). "Recent advances in rumen microbial ecology and metabolism: potential impact on nutrient output". Journal of Dairy Science. 73 (10): 2971–95. doi:10.3168/jds.S0022-0302(90)78986-2. PMID 2178174.
  86. ^ Rouzer CA, Marnett LJ (2009). "Cyclooxygenases: structural and functional insights". J. Lipid Res. 50 (Suppl): S29–34. doi:10.1194/jlr.R800042-JLR200. PMC 2674713. PMID 18952571.
  87. ^ a b c d Suzuki H (2015). "Chapter 8: Control of Enzyme Activity". How Enzymes Work: From Structure to Function. Boca Raton, FL: CRC Press. pp. 141–69. ISBN 978-981-4463-92-8.
  88. ^ Doble BW, Woodgett JR (April 2003). "GSK-3: tricks of the trade for a multi-tasking kinase". Journal of Cell Science. 116 (Pt 7): 1175–86. doi:10.1242/jcs.00384. PMC 3006448. PMID 12615961.
  89. ^ Bennett PM, Chopra I (1993). "Molecular basis of beta-lactamase induction in bacteria". Antimicrob. Agents Chemother. 37 (2): 153–8. doi:10.1128/aac.37.2.153. PMC 187630. PMID 8452343.
  90. ^ Skett P, Gibson GG (2001). "Chapter 3: Induction and Inhibition of Drug Metabolism". Introduction to Drug Metabolism (3 ed.). Cheltenham, UK: Nelson Thornes Publishers. pp. 87–118. ISBN 978-0748760114.
  91. ^ Faergeman NJ, Knudsen J (April 1997). "Role of long-chain fatty acyl-CoA esters in the regulation of metabolism and in cell signalling". The Biochemical Journal. 323 (Pt 1): 1–12. doi:10.1042/bj3230001. PMC 1218279. PMID 9173866.
  92. ^ Suzuki H (2015). "Chapter 4: Effect of pH, Temperature, and High Pressure on Enzymatic Activity". How Enzymes Work: From Structure to Function. Boca Raton, FL: CRC Press. pp. 53–74. ISBN 978-981-4463-92-8.
  93. ^ Noree C, Sato BK, Broyer RM, Wilhelm JE (August 2010). "Identification of novel filament-forming proteins in Saccharomyces cerevisiae and Drosophila melanogaster". The Journal of Cell Biology. 190 (4): 541–51. doi:10.1083/jcb.201003001. PMC 2928026. PMID 20713603.
  94. ^ Aughey GN, Liu JL (2015). "Metabolic regulation via enzyme filamentation". Critical Reviews in Biochemistry and Molecular Biology. 51 (4): 282–93. doi:10.3109/10409238.2016.1172555. PMC 4915340. PMID 27098510.
  95. ^ Kamata K, Mitsuya M, Nishimura T, Eiki J, Nagata Y (March 2004). "Structural basis for allosteric regulation of the monomeric allosteric enzyme human glucokinase". Structure. 12 (3): 429–38. doi:10.1016/j.str.2004.02.005. PMID 15016359.
  96. ^ Froguel P, Zouali H, Vionnet N, Velho G, Vaxillaire M, Sun F, Lesage S, Stoffel M, Takeda J, Passa P (March 1993). "Familial hyperglycemia due to mutations in glucokinase. Definition of a subtype of diabetes mellitus". The New England Journal of Medicine. 328 (10): 697–702. doi:10.1056/NEJM199303113281005. PMID 8433729.
  97. ^ Okada S, O'Brien JS (August 1969). "Tay–Sachs disease: generalized absence of a beta-D-N-acetylhexosaminidase component". Science. 165 (3894): 698–700. Bibcode:1969Sci...165..698O. doi:10.1126/science.165.3894.698. PMID 5793973. S2CID 8473726.
  98. ^ "Learning About Tay–Sachs Disease". U.S. National Human Genome Research Institute. Retrieved 1 March 2015.
  99. ^ Erlandsen H, Stevens RC (October 1999). "The structural basis of phenylketonuria". Molecular Genetics and Metabolism. 68 (2): 103–25. doi:10.1006/mgme.1999.2922. PMID 10527663.
  100. ^ Flatmark T, Stevens RC (August 1999). "Structural Insight into the Aromatic Amino Acid Hydroxylases and Their Disease-Related Mutant Forms". Chemical Reviews. 99 (8): 2137–2160. doi:10.1021/cr980450y. PMID 11849022.
  101. ^ "Phenylketonuria". Genes and Disease [Internet]. Bethesda (MD): National Center for Biotechnology Information (US). 1998–2015.
  102. ^ "Pseudocholinesterase deficiency". U.S. National Library of Medicine. Retrieved 5 September 2013.
  103. ^ Fieker A, Philpott J, Armand M (2011). "Enzyme replacement therapy for pancreatic insufficiency: present and future". Clinical and Experimental Gastroenterology. 4: 55–73. doi:10.2147/CEG.S17634. PMC 3132852. PMID 21753892.
  104. ^ Misselwitz B, Pohl D, Frühauf H, Fried M, Vavricka SR, Fox M (June 2013). "Lactose malabsorption and intolerance: pathogenesis, diagnosis and treatment". United European Gastroenterology Journal. 1 (3): 151–9. doi:10.1177/2050640613484463. PMC 4040760. PMID 24917953.
  105. ^ Cleaver JE (May 1968). "Defective repair replication of DNA in xeroderma pigmentosum". Nature. 218 (5142): 652–6. Bibcode:1968Natur.218..652C. doi:10.1038/218652a0. PMID 5655953. S2CID 4171859.
  106. ^ James WD, Elston D, Berger TG (2011). Andrews' Diseases of the Skin: Clinical Dermatology (11th ed.). London: Saunders/ Elsevier. p. 567. ISBN 978-1437703146.
  107. ^ Murzin AG (November 1993). "Can homologous proteins evolve different enzymatic activities?". Trends in Biochemical Sciences. 18 (11): 403–405. doi:10.1016/0968-0004(93)90132-7. PMID 8291080.
  108. ^ Ochoa D, Bradley D, Beltrao P (February 2018). "Evolution, dynamics and dysregulation of kinase signalling". Current Opinion in Structural Biology. 48: 133–140. doi:10.1016/j.sbi.2017.12.008. PMID 29316484.
  109. ^ Renugopalakrishnan V, Garduño-Juárez R, Narasimhan G, Verma CS, Wei X, Li P (November 2005). "Rational design of thermally stable proteins: relevance to bionanotechnology". Journal of Nanoscience and Nanotechnology. 5 (11): 1759–1767. doi:10.1166/jnn.2005.441. PMID 16433409.
  110. ^ Hult K, Berglund P (August 2003). "Engineered enzymes for improved organic synthesis". Current Opinion in Biotechnology. 14 (4): 395–400. doi:10.1016/S0958-1669(03)00095-8. PMID 12943848.
  111. ^ Jiang L, Althoff EA, Clemente FR, Doyle L, Röthlisberger D, Zanghellini A, Gallaher JL, Betker JL, Tanaka F, Barbas CF, Hilvert D, Houk KN, Stoddard BL, Baker D (March 2008). "De novo computational design of retro-aldol enzymes". Science. 319 (5868): 1387–91. Bibcode:2008Sci...319.1387J. doi:10.1126/science.1152692. PMC 3431203. PMID 18323453.
  112. ^ a b Sun Y, Cheng J (May 2002). "Hydrolysis of lignocellulosic materials for ethanol production: a review". Bioresource Technology. 83 (1): 1–11. doi:10.1016/S0960-8524(01)00212-7. PMID 12058826.
  113. ^ a b Kirk O, Borchert TV, Fuglsang CC (August 2002). "Industrial enzyme applications". Current Opinion in Biotechnology. 13 (4): 345–351. doi:10.1016/S0958-1669(02)00328-2. PMID 12323357.
  114. ^ a b c Briggs DE (1998). Malts and Malting (1st ed.). London: Blackie Academic. ISBN 978-0412298004.
  115. ^ Dulieu C, Moll M, Boudrant J, Poncelet D (2000). "Improved performances and control of beer fermentation using encapsulated alpha-acetolactate decarboxylase and modeling". Biotechnology Progress. 16 (6): 958–65. doi:10.1021/bp000128k. PMID 11101321. S2CID 25674881.
  116. ^ Tarté R (2008). Ingredients in Meat Products Properties, Functionality and Applications. New York: Springer. p. 177. ISBN 978-0-387-71327-4.
  117. ^ . GMO Compass. European Union. 10 July 2010. Archived from the original on 26 March 2015. Retrieved 1 March 2015.
  118. ^ Molimard P, Spinnler HE (February 1996). "Review: Compounds Involved in the Flavor of Surface Mold-Ripened Cheeses: Origins and Properties". Journal of Dairy Science. 79 (2): 169–184. doi:10.3168/jds.S0022-0302(96)76348-8.
  119. ^ Guzmán-Maldonado H, Paredes-López O (September 1995). "Amylolytic enzymes and products derived from starch: a review". Critical Reviews in Food Science and Nutrition. 35 (5): 373–403. doi:10.1080/10408399509527706. PMID 8573280.
  120. ^ a b . GMO Compass. European Union. 10 July 2010. Archived from the original on 24 February 2015. Retrieved 28 February 2015.
  121. ^ Alkorta I, Garbisu C, Llama MJ, Serra JL (January 1998). "Industrial applications of pectic enzymes: a review". Process Biochemistry. 33 (1): 21–28. doi:10.1016/S0032-9592(97)00046-0.
  122. ^ Bajpai P (March 1999). "Application of enzymes in the pulp and paper industry". Biotechnology Progress. 15 (2): 147–157. doi:10.1021/bp990013k. PMID 10194388. S2CID 26080240.
  123. ^ Begley CG, Paragina S, Sporn A (March 1990). "An analysis of contact lens enzyme cleaners". Journal of the American Optometric Association. 61 (3): 190–4. PMID 2186082.
  124. ^ Farris PL (2009). "Economic Growth and Organization of the U.S. Starch Industry". In BeMiller JN, Whistler RL (eds.). Starch Chemistry and Technology (3rd ed.). London: Academic. ISBN 9780080926551.

Further reading

External links

  •   Media related to Enzymes at Wikimedia Commons

January 31, 2023
enzyme, biocatalyst, redirects, here, natural, catalysts, organic, chemistry, biocatalysis, proteins, that, biological, catalysts, accelerating, chemical, reactions, molecules, upon, which, enzymes, called, substrates, enzyme, converts, substrates, into, diffe. Biocatalyst redirects here For the use of natural catalysts in organic chemistry see Biocatalysis Enzymes ˈ ɛ n z aɪ m z are proteins that act as biological catalysts by accelerating chemical reactions The molecules upon which enzymes may act are called substrates and the enzyme converts the substrates into different molecules known as products Almost all metabolic processes in the cell need enzyme catalysis in order to occur at rates fast enough to sustain life 1 8 1 Metabolic pathways depend upon enzymes to catalyze individual steps The study of enzymes is called enzymology and the field of pseudoenzyme analysis recognizes that during evolution some enzymes have lost the ability to carry out biological catalysis which is often reflected in their amino acid sequences and unusual pseudocatalytic properties 2 3 The enzyme glucosidase converts the sugar maltose into two glucose sugars Active site residues in red maltose substrate in black and NAD cofactor in yellow PDB 1OBB Enzymes are known to catalyze more than 5 000 biochemical reaction types 4 Other biocatalysts are catalytic RNA molecules called ribozymes Enzymes specificity comes from their unique three dimensional structures Like all catalysts enzymes increase the reaction rate by lowering its activation energy Some enzymes can make their conversion of substrate to product occur many millions of times faster An extreme example is orotidine 5 phosphate decarboxylase which allows a reaction that would otherwise take millions of years to occur in milliseconds 5 6 Chemically enzymes are like any catalyst and are not consumed in chemical reactions nor do they alter the equilibrium of a reaction Enzymes differ from most other catalysts by being much more specific Enzyme activity can be affected by other molecules inhibitors are molecules that decrease enzyme activity and activators are molecules that increase activity Many therapeutic drugs and poisons are enzyme inhibitors An enzyme s activity decreases markedly outside its optimal temperature and pH and many enzymes are permanently denatured when exposed to excessive heat losing their structure and catalytic properties Some enzymes are used commercially for example in the synthesis of antibiotics Some household products use enzymes to speed up chemical reactions enzymes in biological washing powders break down protein starch or fat stains on clothes and enzymes in meat tenderizer break down proteins into smaller molecules making the meat easier to chew Contents 1 Etymology and history 2 Classification and nomenclature 3 Structure 4 Mechanism 4 1 Substrate binding 4 1 1 Lock and key model 4 1 2 Induced fit model 4 2 Catalysis 4 3 Dynamics 4 4 Substrate presentation 4 5 Allosteric modulation 5 Cofactors 5 1 Coenzymes 6 Thermodynamics 7 Kinetics 8 Inhibition 8 1 Types of inhibition 8 1 1 Competitive 8 1 2 Non competitive 8 1 3 Uncompetitive 8 1 4 Mixed 8 1 5 Irreversible 8 2 Functions of inhibitors 9 Factors affecting enzyme activity 10 Biological function 10 1 Metabolism 10 2 Control of activity 10 2 1 Regulation 10 2 2 Post translational modification 10 2 3 Quantity 10 2 4 Subcellular distribution 10 2 5 Organ specialization 10 3 Involvement in disease 11 Evolution 12 Industrial applications 13 See also 13 1 Enzyme databases 14 References 15 Further reading 16 External linksEtymology and history Eduard Buchner By the late 17th and early 18th centuries the digestion of meat by stomach secretions 7 and the conversion of starch to sugars by plant extracts and saliva were known but the mechanisms by which these occurred had not been identified 8 French chemist Anselme Payen was the first to discover an enzyme diastase in 1833 9 A few decades later when studying the fermentation of sugar to alcohol by yeast Louis Pasteur concluded that this fermentation was caused by a vital force contained within the yeast cells called ferments which were thought to function only within living organisms He wrote that alcoholic fermentation is an act correlated with the life and organization of the yeast cells not with the death or putrefaction of the cells 10 In 1877 German physiologist Wilhelm Kuhne 1837 1900 first used the term enzyme which comes from Greek ἔnzymon leavened or in yeast to describe this process 11 The word enzyme was used later to refer to nonliving substances such as pepsin and the word ferment was used to refer to chemical activity produced by living organisms 12 Eduard Buchner submitted his first paper on the study of yeast extracts in 1897 In a series of experiments at the University of Berlin he found that sugar was fermented by yeast extracts even when there were no living yeast cells in the mixture 13 He named the enzyme that brought about the fermentation of sucrose zymase 14 In 1907 he received the Nobel Prize in Chemistry for his discovery of cell free fermentation Following Buchner s example enzymes are usually named according to the reaction they carry out the suffix ase is combined with the name of the substrate e g lactase is the enzyme that cleaves lactose or to the type of reaction e g DNA polymerase forms DNA polymers 15 The biochemical identity of enzymes was still unknown in the early 1900s Many scientists observed that enzymatic activity was associated with proteins but others such as Nobel laureate Richard Willstatter argued that proteins were merely carriers for the true enzymes and that proteins per se were incapable of catalysis 16 In 1926 James B Sumner showed that the enzyme urease was a pure protein and crystallized it he did likewise for the enzyme catalase in 1937 The conclusion that pure proteins can be enzymes was definitively demonstrated by John Howard Northrop and Wendell Meredith Stanley who worked on the digestive enzymes pepsin 1930 trypsin and chymotrypsin These three scientists were awarded the 1946 Nobel Prize in Chemistry 17 The discovery that enzymes could be crystallized eventually allowed their structures to be solved by x ray crystallography This was first done for lysozyme an enzyme found in tears saliva and egg whites that digests the coating of some bacteria the structure was solved by a group led by David Chilton Phillips and published in 1965 18 This high resolution structure of lysozyme marked the beginning of the field of structural biology and the effort to understand how enzymes work at an atomic level of detail 19 Classification and nomenclatureEnzymes can be classified by two main criteria either amino acid sequence similarity and thus evolutionary relationship or enzymatic activity Enzyme activity An enzyme s name is often derived from its substrate or the chemical reaction it catalyzes with the word ending in ase 1 8 1 3 Examples are lactase alcohol dehydrogenase and DNA polymerase Different enzymes that catalyze the same chemical reaction are called isozymes 1 10 3 The International Union of Biochemistry and Molecular Biology have developed a nomenclature for enzymes the EC numbers for Enzyme Commission Each enzyme is described by EC followed by a sequence of four numbers which represent the hierarchy of enzymatic activity from very general to very specific That is the first number broadly classifies the enzyme based on its mechanism while the other digits add more and more specificity 20 The top level classification is EC 1 Oxidoreductases catalyze oxidation reduction reactions EC 2 Transferases transfer a functional group e g a methyl or phosphate group EC 3 Hydrolases catalyze the hydrolysis of various bonds EC 4 Lyases cleave various bonds by means other than hydrolysis and oxidation EC 5 Isomerases catalyze isomerization changes within a single molecule EC 6 Ligases join two molecules with covalent bonds EC 7 Translocases catalyze the movement of ions or molecules across membranes or their separation within membranes These sections are subdivided by other features such as the substrate products and chemical mechanism An enzyme is fully specified by four numerical designations For example hexokinase EC 2 7 1 1 is a transferase EC 2 that adds a phosphate group EC 2 7 to a hexose sugar a molecule containing an alcohol group EC 2 7 1 21 Sequence similarity EC categories do not reflect sequence similarity For instance two ligases of the same EC number that catalyze exactly the same reaction can have completely different sequences Independent of their function enzymes like any other proteins have been classified by their sequence similarity into numerous families These families have been documented in dozens of different protein and protein family databases such as Pfam 22 Structure Enzyme activity initially increases with temperature Q10 coefficient until the enzyme s structure unfolds denaturation leading to an optimal rate of reaction at an intermediate temperature See also Protein structure Enzymes are generally globular proteins acting alone or in larger complexes The sequence of the amino acids specifies the structure which in turn determines the catalytic activity of the enzyme 23 Although structure determines function a novel enzymatic activity cannot yet be predicted from structure alone 24 Enzyme structures unfold denature when heated or exposed to chemical denaturants and this disruption to the structure typically causes a loss of activity 25 Enzyme denaturation is normally linked to temperatures above a species normal level as a result enzymes from bacteria living in volcanic environments such as hot springs are prized by industrial users for their ability to function at high temperatures allowing enzyme catalysed reactions to be operated at a very high rate Enzymes are usually much larger than their substrates Sizes range from just 62 amino acid residues for the monomer of 4 oxalocrotonate tautomerase 26 to over 2 500 residues in the animal fatty acid synthase 27 Only a small portion of their structure around 2 4 amino acids is directly involved in catalysis the catalytic site 28 This catalytic site is located next to one or more binding sites where residues orient the substrates The catalytic site and binding site together compose the enzyme s active site The remaining majority of the enzyme structure serves to maintain the precise orientation and dynamics of the active site 29 In some enzymes no amino acids are directly involved in catalysis instead the enzyme contains sites to bind and orient catalytic cofactors 29 Enzyme structures may also contain allosteric sites where the binding of a small molecule causes a conformational change that increases or decreases activity 30 A small number of RNA based biological catalysts called ribozymes exist which again can act alone or in complex with proteins The most common of these is the ribosome which is a complex of protein and catalytic RNA components 1 2 2 Mechanism Organisation of enzyme structure and lysozyme example Binding sites in blue catalytic site in red and peptidoglycan substrate in black PDB 9LYZ Substrate binding Enzymes must bind their substrates before they can catalyse any chemical reaction Enzymes are usually very specific as to what substrates they bind and then the chemical reaction catalysed Specificity is achieved by binding pockets with complementary shape charge and hydrophilic hydrophobic characteristics to the substrates Enzymes can therefore distinguish between very similar substrate molecules to be chemoselective regioselective and stereospecific 31 Some of the enzymes showing the highest specificity and accuracy are involved in the copying and expression of the genome Some of these enzymes have proof reading mechanisms Here an enzyme such as DNA polymerase catalyzes a reaction in a first step and then checks that the product is correct in a second step 32 This two step process results in average error rates of less than 1 error in 100 million reactions in high fidelity mammalian polymerases 1 5 3 1 Similar proofreading mechanisms are also found in RNA polymerase 33 aminoacyl tRNA synthetases 34 and ribosomes 35 Conversely some enzymes display enzyme promiscuity having broad specificity and acting on a range of different physiologically relevant substrates Many enzymes possess small side activities which arose fortuitously i e neutrally which may be the starting point for the evolutionary selection of a new function 36 37 Enzyme changes shape by induced fit upon substrate binding to form enzyme substrate complex Hexokinase has a large induced fit motion that closes over the substrates adenosine triphosphate and xylose Binding sites in blue substrates in black and Mg2 cofactor in yellow PDB 2E2N 2E2Q Lock and key model To explain the observed specificity of enzymes in 1894 Emil Fischer proposed that both the enzyme and the substrate possess specific complementary geometric shapes that fit exactly into one another 38 This is often referred to as the lock and key model 1 8 3 2 This early model explains enzyme specificity but fails to explain the stabilization of the transition state that enzymes achieve 39 Induced fit model In 1958 Daniel Koshland suggested a modification to the lock and key model since enzymes are rather flexible structures the active site is continuously reshaped by interactions with the substrate as the substrate interacts with the enzyme 40 As a result the substrate does not simply bind to a rigid active site the amino acid side chains that make up the active site are molded into the precise positions that enable the enzyme to perform its catalytic function In some cases such as glycosidases the substrate molecule also changes shape slightly as it enters the active site 41 The active site continues to change until the substrate is completely bound at which point the final shape and charge distribution is determined 42 Induced fit may enhance the fidelity of molecular recognition in the presence of competition and noise via the conformational proofreading mechanism 43 Catalysis See also Enzyme catalysis and Transition state theory Enzymes can accelerate reactions in several ways all of which lower the activation energy DG Gibbs free energy 44 By stabilizing the transition state Creating an environment with a charge distribution complementary to that of the transition state to lower its energy 45 By providing an alternative reaction pathway Temporarily reacting with the substrate forming a covalent intermediate to provide a lower energy transition state 46 By destabilising the substrate ground state Distorting bound substrate s into their transition state form to reduce the energy required to reach the transition state 47 By orienting the substrates into a productive arrangement to reduce the reaction entropy change 48 the contribution of this mechanism to catalysis is relatively small 49 Enzymes may use several of these mechanisms simultaneously For example proteases such as trypsin perform covalent catalysis using a catalytic triad stabilise charge build up on the transition states using an oxyanion hole complete hydrolysis using an oriented water substrate 50 Dynamics See also Protein dynamics Enzymes are not rigid static structures instead they have complex internal dynamic motions that is movements of parts of the enzyme s structure such as individual amino acid residues groups of residues forming a protein loop or unit of secondary structure or even an entire protein domain These motions give rise to a conformational ensemble of slightly different structures that interconvert with one another at equilibrium Different states within this ensemble may be associated with different aspects of an enzyme s function For example different conformations of the enzyme dihydrofolate reductase are associated with the substrate binding catalysis cofactor release and product release steps of the catalytic cycle 51 consistent with catalytic resonance theory Substrate presentation Substrate presentation is a process where the enzyme is sequestered away from its substrate Enzymes can be sequestered to the plasma membrane away from a substrate in the nucleus or cytosol Or within the membrane an enzyme can be sequestered into lipid rafts away from its substrate in the disordered region When the enzyme is released it mixes with its substrate Alternatively the enzyme can be sequestered near its substrate to activate the enzyme For example the enzyme can be soluble and upon activation bind to a lipid in the plasma membrane and then act upon molecules in the plasma membrane Allosteric modulation Main article Allosteric regulation Allosteric sites are pockets on the enzyme distinct from the active site that bind to molecules in the cellular environment These molecules then cause a change in the conformation or dynamics of the enzyme that is transduced to the active site and thus affects the reaction rate of the enzyme 52 In this way allosteric interactions can either inhibit or activate enzymes Allosteric interactions with metabolites upstream or downstream in an enzyme s metabolic pathway cause feedback regulation altering the activity of the enzyme according to the flux through the rest of the pathway 53 Cofactors Chemical structure for thiamine pyrophosphate and protein structure of transketolase Thiamine pyrophosphate cofactor in yellow and xylulose 5 phosphate substrate in black PDB 4KXV Main article Cofactor biochemistry Some enzymes do not need additional components to show full activity Others require non protein molecules called cofactors to be bound for activity 54 Cofactors can be either inorganic e g metal ions and iron sulfur clusters or organic compounds e g flavin and heme These cofactors serve many purposes for instance metal ions can help in stabilizing nucleophilic species within the active site 55 Organic cofactors can be either coenzymes which are released from the enzyme s active site during the reaction or prosthetic groups which are tightly bound to an enzyme Organic prosthetic groups can be covalently bound e g biotin in enzymes such as pyruvate carboxylase 56 An example of an enzyme that contains a cofactor is carbonic anhydrase which uses a zinc cofactor bound as part of its active site 57 These tightly bound ions or molecules are usually found in the active site and are involved in catalysis 1 8 1 1 For example flavin and heme cofactors are often involved in redox reactions 1 17 Enzymes that require a cofactor but do not have one bound are called apoenzymes or apoproteins An enzyme together with the cofactor s required for activity is called a holoenzyme or haloenzyme The term holoenzyme can also be applied to enzymes that contain multiple protein subunits such as the DNA polymerases here the holoenzyme is the complete complex containing all the subunits needed for activity 1 8 1 1 Coenzymes Coenzymes are small organic molecules that can be loosely or tightly bound to an enzyme Coenzymes transport chemical groups from one enzyme to another 58 Examples include NADH NADPH and adenosine triphosphate ATP Some coenzymes such as flavin mononucleotide FMN flavin adenine dinucleotide FAD thiamine pyrophosphate TPP and tetrahydrofolate THF are derived from vitamins These coenzymes cannot be synthesized by the body de novo and closely related compounds vitamins must be acquired from the diet The chemical groups carried include the hydride ion H carried by NAD or NADP the phosphate group carried by adenosine triphosphate the acetyl group carried by coenzyme A formyl methenyl or methyl groups carried by folic acid and the methyl group carried by S adenosylmethionine 58 Since coenzymes are chemically changed as a consequence of enzyme action it is useful to consider coenzymes to be a special class of substrates or second substrates which are common to many different enzymes For example about 1000 enzymes are known to use the coenzyme NADH 59 Coenzymes are usually continuously regenerated and their concentrations maintained at a steady level inside the cell For example NADPH is regenerated through the pentose phosphate pathway and S adenosylmethionine by methionine adenosyltransferase This continuous regeneration means that small amounts of coenzymes can be used very intensively For example the human body turns over its own weight in ATP each day 60 Thermodynamics The energies of the stages of a chemical reaction Uncatalysed dashed line substrates need a lot of activation energy to reach a transition state which then decays into lower energy products When enzyme catalysed solid line the enzyme binds the substrates ES then stabilizes the transition state ES to reduce the activation energy required to produce products EP which are finally released Main articles Activation energy Thermodynamic equilibrium and Chemical equilibrium As with all catalysts enzymes do not alter the position of the chemical equilibrium of the reaction In the presence of an enzyme the reaction runs in the same direction as it would without the enzyme just more quickly 1 8 2 3 For example carbonic anhydrase catalyzes its reaction in either direction depending on the concentration of its reactants 61 CO 2 H 2 O Carbonic anhydrase H 2 CO 3 displaystyle ce CO2 H2O gt text Carbonic anhydrase H2CO3 in tissues high CO2 concentration 1 CO 2 H 2 O Carbonic anhydrase H 2 CO 3 displaystyle ce CO2 H2O lt text Carbonic anhydrase H2CO3 in lungs low CO2 concentration 2 The rate of a reaction is dependent on the activation energy needed to form the transition state which then decays into products Enzymes increase reaction rates by lowering the energy of the transition state First binding forms a low energy enzyme substrate complex ES Second the enzyme stabilises the transition state such that it requires less energy to achieve compared to the uncatalyzed reaction ES Finally the enzyme product complex EP dissociates to release the products 1 8 3 Enzymes can couple two or more reactions so that a thermodynamically favorable reaction can be used to drive a thermodynamically unfavourable one so that the combined energy of the products is lower than the substrates For example the hydrolysis of ATP is often used to drive other chemical reactions 62 Kinetics A chemical reaction mechanism with or without enzyme catalysis The enzyme E binds substrate S to produce product P Saturation curve for an enzyme reaction showing the relation between the substrate concentration and reaction rate Main article Enzyme kinetics Enzyme kinetics is the investigation of how enzymes bind substrates and turn them into products 63 The rate data used in kinetic analyses are commonly obtained from enzyme assays In 1913 Leonor Michaelis and Maud Leonora Menten proposed a quantitative theory of enzyme kinetics which is referred to as Michaelis Menten kinetics 64 The major contribution of Michaelis and Menten was to think of enzyme reactions in two stages In the first the substrate binds reversibly to the enzyme forming the enzyme substrate complex This is sometimes called the Michaelis Menten complex in their honor The enzyme then catalyzes the chemical step in the reaction and releases the product This work was further developed by G E Briggs and J B S Haldane who derived kinetic equations that are still widely used today 65 Enzyme rates depend on solution conditions and substrate concentration To find the maximum speed of an enzymatic reaction the substrate concentration is increased until a constant rate of product formation is seen This is shown in the saturation curve on the right Saturation happens because as substrate concentration increases more and more of the free enzyme is converted into the substrate bound ES complex At the maximum reaction rate Vmax of the enzyme all the enzyme active sites are bound to substrate and the amount of ES complex is the same as the total amount of enzyme 1 8 4 Vmax is only one of several important kinetic parameters The amount of substrate needed to achieve a given rate of reaction is also important This is given by the Michaelis Menten constant Km which is the substrate concentration required for an enzyme to reach one half its maximum reaction rate generally each enzyme has a characteristic KM for a given substrate Another useful constant is kcat also called the turnover number which is the number of substrate molecules handled by one active site per second 1 8 4 The efficiency of an enzyme can be expressed in terms of kcat Km This is also called the specificity constant and incorporates the rate constants for all steps in the reaction up to and including the first irreversible step Because the specificity constant reflects both affinity and catalytic ability it is useful for comparing different enzymes against each other or the same enzyme with different substrates The theoretical maximum for the specificity constant is called the diffusion limit and is about 108 to 109 M 1 s 1 At this point every collision of the enzyme with its substrate will result in catalysis and the rate of product formation is not limited by the reaction rate but by the diffusion rate Enzymes with this property are called catalytically perfect or kinetically perfect Example of such enzymes are triose phosphate isomerase carbonic anhydrase acetylcholinesterase catalase fumarase b lactamase and superoxide dismutase 1 8 4 2 The turnover of such enzymes can reach several million reactions per second 1 9 2 But most enzymes are far from perfect the average values of k c a t K m displaystyle k rm cat K rm m and k c a t displaystyle k rm cat are about 10 5 s 1 M 1 displaystyle 10 5 rm s 1 rm M 1 and 10 s 1 displaystyle 10 rm s 1 respectively 66 Michaelis Menten kinetics relies on the law of mass action which is derived from the assumptions of free diffusion and thermodynamically driven random collision Many biochemical or cellular processes deviate significantly from these conditions because of macromolecular crowding and constrained molecular movement 67 More recent complex extensions of the model attempt to correct for these effects 68 Inhibition The coenzyme folic acid left and the anti cancer drug methotrexate right are very similar in structure differences show in green As a result methotrexate is a competitive inhibitor of many enzymes that use folates Main article Enzyme inhibitor Enzyme reaction rates can be decreased by various types of enzyme inhibitors 69 73 74 Types of inhibition Competitive A competitive inhibitor and substrate cannot bind to the enzyme at the same time 70 Often competitive inhibitors strongly resemble the real substrate of the enzyme For example the drug methotrexate is a competitive inhibitor of the enzyme dihydrofolate reductase which catalyzes the reduction of dihydrofolate to tetrahydrofolate 71 The similarity between the structures of dihydrofolate and this drug are shown in the accompanying figure This type of inhibition can be overcome with high substrate concentration In some cases the inhibitor can bind to a site other than the binding site of the usual substrate and exert an allosteric effect to change the shape of the usual binding site 72 Non competitive A non competitive inhibitor binds to a site other than where the substrate binds The substrate still binds with its usual affinity and hence Km remains the same However the inhibitor reduces the catalytic efficiency of the enzyme so that Vmax is reduced In contrast to competitive inhibition non competitive inhibition cannot be overcome with high substrate concentration 69 76 78 Uncompetitive An uncompetitive inhibitor cannot bind to the free enzyme only to the enzyme substrate complex hence these types of inhibitors are most effective at high substrate concentration In the presence of the inhibitor the enzyme substrate complex is inactive 69 78 This type of inhibition is rare 73 Mixed A mixed inhibitor binds to an allosteric site and the binding of the substrate and the inhibitor affect each other The enzyme s function is reduced but not eliminated when bound to the inhibitor This type of inhibitor does not follow the Michaelis Menten equation 69 76 78 Irreversible An irreversible inhibitor permanently inactivates the enzyme usually by forming a covalent bond to the protein 74 Penicillin 75 and aspirin 76 are common drugs that act in this manner Functions of inhibitors In many organisms inhibitors may act as part of a feedback mechanism If an enzyme produces too much of one substance in the organism that substance may act as an inhibitor for the enzyme at the beginning of the pathway that produces it causing production of the substance to slow down or stop when there is sufficient amount This is a form of negative feedback Major metabolic pathways such as the citric acid cycle make use of this mechanism 1 17 2 2 Since inhibitors modulate the function of enzymes they are often used as drugs Many such drugs are reversible competitive inhibitors that resemble the enzyme s native substrate similar to methotrexate above other well known examples include statins used to treat high cholesterol 77 and protease inhibitors used to treat retroviral infections such as HIV 78 A common example of an irreversible inhibitor that is used as a drug is aspirin which inhibits the COX 1 and COX 2 enzymes that produce the inflammation messenger prostaglandin 76 Other enzyme inhibitors are poisons For example the poison cyanide is an irreversible enzyme inhibitor that combines with the copper and iron in the active site of the enzyme cytochrome c oxidase and blocks cellular respiration 79 Factors affecting enzyme activityAs enzymes are made up of proteins their actions are sensitive to change in many physio chemical factors such as pH temperature substrate concentration etc The following table shows pH optima for various enzymes 80 Enzyme Optimum pH pH descriptionPepsin 1 5 1 6 Highly acidicInvertase 4 5 AcidicLipase stomach 4 0 5 0 AcidicLipase castor oil 4 7 AcidicLipase pancreas 8 0 AlkalineAmylase malt 4 6 5 2 AcidicAmylase pancreas 6 7 7 0 Acidic neutralCellobiase 5 0 AcidicMaltase 6 1 6 8 AcidicSucrase 6 2 AcidicCatalase 7 0 NeutralUrease 7 0 NeutralCholinesterase 7 0 NeutralRibonuclease 7 0 7 5 NeutralFumarase 7 8 AlkalineTrypsin 7 8 8 7 AlkalineAdenosine triphosphate 9 0 AlkalineArginase 10 0 Highly alkalineBiological functionEnzymes serve a wide variety of functions inside living organisms They are indispensable for signal transduction and cell regulation often via kinases and phosphatases 81 They also generate movement with myosin hydrolyzing adenosine triphosphate ATP to generate muscle contraction and also transport cargo around the cell as part of the cytoskeleton 82 Other ATPases in the cell membrane are ion pumps involved in active transport Enzymes are also involved in more exotic functions such as luciferase generating light in fireflies 83 Viruses can also contain enzymes for infecting cells such as the HIV integrase and reverse transcriptase or for viral release from cells like the influenza virus neuraminidase 84 An important function of enzymes is in the digestive systems of animals Enzymes such as amylases and proteases break down large molecules starch or proteins respectively into smaller ones so they can be absorbed by the intestines Starch molecules for example are too large to be absorbed from the intestine but enzymes hydrolyze the starch chains into smaller molecules such as maltose and eventually glucose which can then be absorbed Different enzymes digest different food substances In ruminants which have herbivorous diets microorganisms in the gut produce another enzyme cellulase to break down the cellulose cell walls of plant fiber 85 Metabolism The metabolic pathway of glycolysis releases energy by converting glucose to pyruvate via a series of intermediate metabolites Each chemical modification red box is performed by a different enzyme Several enzymes can work together in a specific order creating metabolic pathways 1 30 1 In a metabolic pathway one enzyme takes the product of another enzyme as a substrate After the catalytic reaction the product is then passed on to another enzyme Sometimes more than one enzyme can catalyze the same reaction in parallel this can allow more complex regulation with for example a low constant activity provided by one enzyme but an inducible high activity from a second enzyme 86 Enzymes determine what steps occur in these pathways Without enzymes metabolism would neither progress through the same steps and could not be regulated to serve the needs of the cell Most central metabolic pathways are regulated at a few key steps typically through enzymes whose activity involves the hydrolysis of ATP Because this reaction releases so much energy other reactions that are thermodynamically unfavorable can be coupled to ATP hydrolysis driving the overall series of linked metabolic reactions 1 30 1 Control of activity There are five main ways that enzyme activity is controlled in the cell 1 30 1 1 Regulation Enzymes can be either activated or inhibited by other molecules For example the end product s of a metabolic pathway are often inhibitors for one of the first enzymes of the pathway usually the first irreversible step called committed step thus regulating the amount of end product made by the pathways Such a regulatory mechanism is called a negative feedback mechanism because the amount of the end product produced is regulated by its own concentration 87 141 48 Negative feedback mechanism can effectively adjust the rate of synthesis of intermediate metabolites according to the demands of the cells This helps with effective allocations of materials and energy economy and it prevents the excess manufacture of end products Like other homeostatic devices the control of enzymatic action helps to maintain a stable internal environment in living organisms 87 141 Post translational modification Examples of post translational modification include phosphorylation myristoylation and glycosylation 87 149 69 For example in the response to insulin the phosphorylation of multiple enzymes including glycogen synthase helps control the synthesis or degradation of glycogen and allows the cell to respond to changes in blood sugar 88 Another example of post translational modification is the cleavage of the polypeptide chain Chymotrypsin a digestive protease is produced in inactive form as chymotrypsinogen in the pancreas and transported in this form to the stomach where it is activated This stops the enzyme from digesting the pancreas or other tissues before it enters the gut This type of inactive precursor to an enzyme is known as a zymogen 87 149 53 or proenzyme Quantity Enzyme production transcription and translation of enzyme genes can be enhanced or diminished by a cell in response to changes in the cell s environment This form of gene regulation is called enzyme induction For example bacteria may become resistant to antibiotics such as penicillin because enzymes called beta lactamases are induced that hydrolyse the crucial beta lactam ring within the penicillin molecule 89 Another example comes from enzymes in the liver called cytochrome P450 oxidases which are important in drug metabolism Induction or inhibition of these enzymes can cause drug interactions 90 Enzyme levels can also be regulated by changing the rate of enzyme degradation 1 30 1 1 The opposite of enzyme induction is enzyme repression Subcellular distribution Enzymes can be compartmentalized with different metabolic pathways occurring in different cellular compartments For example fatty acids are synthesized by one set of enzymes in the cytosol endoplasmic reticulum and Golgi and used by a different set of enzymes as a source of energy in the mitochondrion through b oxidation 91 In addition trafficking of the enzyme to different compartments may change the degree of protonation e g the neutral cytoplasm and the acidic lysosome or oxidative state e g oxidizing periplasm or reducing cytoplasm which in turn affects enzyme activity 92 In contrast to partitioning into membrane bound organelles enzyme subcellular localisation may also be altered through polymerisation of enzymes into macromolecular cytoplasmic filaments 93 94 Organ specialization In multicellular eukaryotes cells in different organs and tissues have different patterns of gene expression and therefore have different sets of enzymes known as isozymes available for metabolic reactions This provides a mechanism for regulating the overall metabolism of the organism For example hexokinase the first enzyme in the glycolysis pathway has a specialized form called glucokinase expressed in the liver and pancreas that has a lower affinity for glucose yet is more sensitive to glucose concentration 95 This enzyme is involved in sensing blood sugar and regulating insulin production 96 Involvement in disease In phenylalanine hydroxylase over 300 different mutations throughout the structure cause phenylketonuria Phenylalanine substrate and tetrahydrobiopterin coenzyme in black and Fe2 cofactor in yellow PDB 1KW0 Hereditary defects in enzymes are generally inherited in an autosomal fashion because there are more non X chromosomes than X chromosomes and a recessive fashion because the enzymes from the unaffected genes are generally sufficient to prevent symptoms in carriers See also Genetic disorder Since the tight control of enzyme activity is essential for homeostasis any malfunction mutation overproduction underproduction or deletion of a single critical enzyme can lead to a genetic disease The malfunction of just one type of enzyme out of the thousands of types present in the human body can be fatal An example of a fatal genetic disease due to enzyme insufficiency is Tay Sachs disease in which patients lack the enzyme hexosaminidase 97 98 One example of enzyme deficiency is the most common type of phenylketonuria Many different single amino acid mutations in the enzyme phenylalanine hydroxylase which catalyzes the first step in the degradation of phenylalanine result in build up of phenylalanine and related products Some mutations are in the active site directly disrupting binding and catalysis but many are far from the active site and reduce activity by destabilising the protein structure or affecting correct oligomerisation 99 100 This can lead to intellectual disability if the disease is untreated 101 Another example is pseudocholinesterase deficiency in which the body s ability to break down choline ester drugs is impaired 102 Oral administration of enzymes can be used to treat some functional enzyme deficiencies such as pancreatic insufficiency 103 and lactose intolerance 104 Another way enzyme malfunctions can cause disease comes from germline mutations in genes coding for DNA repair enzymes Defects in these enzymes cause cancer because cells are less able to repair mutations in their genomes This causes a slow accumulation of mutations and results in the development of cancers An example of such a hereditary cancer syndrome is xeroderma pigmentosum which causes the development of skin cancers in response to even minimal exposure to ultraviolet light 105 106 EvolutionSimilar to any other protein enzymes change over time through mutations and sequence divergence Given their central role in metabolism enzyme evolution plays a critical role in adaptation A key question is therefore whether and how enzymes can change their enzymatic activities alongside It is generally accepted that many new enzyme activities have evolved through gene duplication and mutation of the duplicate copies although evolution can also happen without duplication One example of an enzyme that has changed its activity is the ancestor of methionyl aminopeptidase MAP and creatine amidinohydrolase creatinase which are clearly homologous but catalyze very different reactions MAP removes the amino terminal methionine in new proteins while creatinase hydrolyses creatine to sarcosine and urea In addition MAP is metal ion dependent while creatinase is not hence this property was also lost over time 107 Small changes of enzymatic activity are extremely common among enzymes In particular substrate binding specificity see above can easily and quickly change with single amino acid changes in their substrate binding pockets This is frequently seen in the main enzyme classes such as kinases 108 Artificial in vitro evolution is now commonly used to modify enzyme activity or specificity for industrial applications see below Industrial applicationsMain article Industrial enzymes Enzymes are used in the chemical industry and other industrial applications when extremely specific catalysts are required Enzymes in general are limited in the number of reactions they have evolved to catalyze and also by their lack of stability in organic solvents and at high temperatures As a consequence protein engineering is an active area of research and involves attempts to create new enzymes with novel properties either through rational design or in vitro evolution 109 110 These efforts have begun to be successful and a few enzymes have now been designed from scratch to catalyze reactions that do not occur in nature 111 Application Enzymes used UsesBiofuel industry Cellulases Break down cellulose into sugars that can be fermented to produce cellulosic ethanol 112 Ligninases Pretreatment of biomass for biofuel production 112 Biological detergent Proteases amylases lipases Remove protein starch and fat or oil stains from laundry and dishware 113 Mannanases Remove food stains from the common food additive guar gum 113 Brewing industry Amylase glucanases proteases Split polysaccharides and proteins in the malt 114 150 9 Betaglucanases Improve the wort and beer filtration characteristics 114 545 Amyloglucosidase and pullulanases Make low calorie beer and adjust fermentability 114 575 Acetolactate decarboxylase ALDC Increase fermentation efficiency by reducing diacetyl formation 115 Culinary uses Papain Tenderize meat for cooking 116 Dairy industry Rennin Hydrolyze protein in the manufacture of cheese 117 Lipases Produce Camembert cheese and blue cheeses such as Roquefort 118 Food processing Amylases Produce sugars from starch such as in making high fructose corn syrup 119 Proteases Lower the protein level of flour as in biscuit making 120 Trypsin Manufacture hypoallergenic baby foods 120 Cellulases pectinases Clarify fruit juices 121 Molecular biology Nucleases DNA ligase and polymerases Use restriction digestion and the polymerase chain reaction to create recombinant DNA 1 6 2 Paper industry Xylanases hemicellulases and lignin peroxidases Remove lignin from kraft pulp 122 Personal care Proteases Remove proteins on contact lenses to prevent infections 123 Starch industry Amylases Convert starch into glucose and various syrups 124 See also Biology portal Food portalIndustrial enzymes List of enzymes Molecular machineEnzyme databases BRENDA ExPASy IntEnz KEGG MetaCycReferences a b c d e f g h i j k l m n o p q r s t u Stryer L Berg JM Tymoczko JL 2002 Biochemistry 5th ed San Francisco W H Freeman ISBN 0 7167 4955 6 Murphy JM Farhan H Eyers PA 2017 Bio Zombie the rise of pseudoenzymes in biology Biochem Soc Trans 45 2 537 544 doi 10 1042 bst20160400 PMID 28408493 Murphy JM et al 2014 A robust methodology to subclassify pseudokinases based on their nucleotide binding properties Biochemical Journal 457 2 323 334 doi 10 1042 BJ20131174 PMC 5679212 PMID 24107129 Schomburg I Chang A Placzek S Sohngen C Rother M Lang M Munaretto C Ulas S Stelzer M Grote A Scheer M Schomburg D January 2013 BRENDA in 2013 integrated reactions kinetic data enzyme function data improved disease classification new options and contents in BRENDA Nucleic Acids Research 41 Database issue D764 72 doi 10 1093 nar gks1049 PMC 3531171 PMID 23203881 Radzicka A Wolfenden R January 1995 A proficient enzyme Science 267 5194 90 931 Bibcode 1995Sci 267 90R doi 10 1126 science 7809611 PMID 7809611 S2CID 8145198 Callahan BP Miller BG December 2007 OMP decarboxylase An enigma persists Bioorganic Chemistry 35 6 465 9 doi 10 1016 j bioorg 2007 07 004 PMID 17889251 de Reaumur RA 1752 Observations sur la digestion des oiseaux Histoire de l Academie Royale des Sciences 1752 266 461 Williams HS 1904 A History of Science in Five Volumes Volume IV Modern Development of the Chemical and Biological Sciences Harper and Brothers Payen A Persoz JF 1833 Memoire sur la diastase les principaux produits de ses reactions et leurs applications aux arts industriels Memoir on diastase the principal products of its reactions and their applications to the industrial arts Annales de chimie et de physique 2nd in French 53 73 92 Manchester KL December 1995 Louis Pasteur 1822 1895 chance and the prepared mind Trends in Biotechnology 13 12 511 5 doi 10 1016 S0167 7799 00 89014 9 PMID 8595136 Kuhne coined the word enzyme in Kuhne W 1877 Uber das Verhalten verschiedener organisirter und sog ungeformter Fermente On the behavior of various organized and so called unformed ferments Verhandlungen des Naturhistorisch medicinischen Vereins zu Heidelberg new series in German 1 3 190 193 Relevant passage on page 190 Um Missverstandnissen vorzubeugen und lastige Umschreibungen zu vermeiden schlagt Vortragender vor die ungeformten oder nicht organisirten Fermente deren Wirkung ohne Anwesenheit von Organismen und ausserhalb derselben erfolgen kann alsEnzymezu bezeichnen Translation In order to obviate misunderstandings and avoid cumbersome periphrases the author a university lecturer suggests designating as enzymes the unformed or not organized ferments whose action can occur without the presence of organisms and outside of the same Holmes FL 2003 Enzymes In Heilbron JL ed The Oxford Companion to the History of Modern Science Oxford Oxford University Press p 270 ISBN 9780199743766 Eduard Buchner Nobel Laureate Biography Nobelprize org Retrieved 23 February 2015 Eduard Buchner Nobel Lecture Cell Free Fermentation Nobelprize org 1907 Retrieved 23 February 2015 The naming of enzymes by adding the suffix ase to the substrate on which the enzyme acts has been traced to French scientist Emile Duclaux 1840 1904 who intended to honor the discoverers of diastase the first enzyme to be isolated by introducing this practice in his book Duclaux E 1899 Traite de microbiologie Diastases toxines et venins Microbiology Treatise diastases toxins and venoms in French Paris France Masson and Co See Chapter 1 especially page 9 Willstatter R 1927 Faraday lecture Problems and methods in enzyme research Journal of the Chemical Society Resumed 1359 1381 doi 10 1039 JR9270001359 quoted in Blow D April 2000 So do we understand how enzymes work Structure 8 4 R77 R81 doi 10 1016 S0969 2126 00 00125 8 PMID 10801479 Nobel Prizes and Laureates The Nobel Prize in Chemistry 1946 Nobelprize org Retrieved 23 February 2015 Blake CC Koenig DF Mair GA North AC Phillips DC Sarma VR May 1965 Structure of hen egg white lysozyme A three dimensional Fourier synthesis at 2 Angstrom resolution Nature 206 4986 757 61 Bibcode 1965Natur 206 757B doi 10 1038 206757a0 PMID 5891407 S2CID 4161467 Johnson LN Petsko GA 1999 David Phillips and the origin of structural enzymology Trends Biochem Sci 24 7 287 9 doi 10 1016 S0968 0004 99 01423 1 PMID 10390620 Moss GP Recommendations of the Nomenclature Committee of the International Union of Biochemistry and Molecular Biology on the Nomenclature and Classification of Enzymes by the Reactions they Catalyse International Union of Biochemistry and Molecular Biology Retrieved 28 August 2021 Nomenclature Committee EC 2 7 1 1 International Union of Biochemistry and Molecular Biology NC IUBMB School of Biological and Chemical Sciences Queen Mary University of London Archived from the original on 1 December 2014 Retrieved 6 March 2015 Mulder NJ 28 September 2007 Protein Family Databases eLS Chichester UK John Wiley amp Sons Ltd pp a0003058 pub2 doi 10 1002 9780470015902 a0003058 pub2 ISBN 978 0 470 01617 6 Anfinsen CB July 1973 Principles that govern the folding of protein chains Science 181 4096 223 30 Bibcode 1973Sci 181 223A doi 10 1126 science 181 4096 223 PMID 4124164 Dunaway Mariano D November 2008 Enzyme function discovery Structure 16 11 1599 600 doi 10 1016 j str 2008 10 001 PMID 19000810 Petsko GA Ringe D 2003 Chapter 1 From sequence to structure Protein structure and function London New Science p 27 ISBN 978 1405119221 Chen LH Kenyon GL Curtin F Harayama S Bembenek ME Hajipour G Whitman CP September 1992 4 Oxalocrotonate tautomerase an enzyme composed of 62 amino acid residues per monomer The Journal of Biological Chemistry 267 25 17716 21 doi 10 1016 S0021 9258 19 37101 7 PMID 1339435 Smith S December 1994 The animal fatty acid synthase one gene one polypeptide seven enzymes FASEB Journal 8 15 1248 59 doi 10 1096 fasebj 8 15 8001737 PMID 8001737 S2CID 22853095 The Catalytic Site Atlas The European Bioinformatics Institute Retrieved 4 April 2007 a b Suzuki H 2015 Chapter 7 Active Site Structure How Enzymes Work From Structure to Function Boca Raton FL CRC Press pp 117 140 ISBN 978 981 4463 92 8 Krauss G 2003 The Regulations of Enzyme Activity Biochemistry of Signal Transduction and Regulation 3rd ed Weinheim Wiley VCH pp 89 114 ISBN 9783527605767 Jaeger KE Eggert T August 2004 Enantioselective biocatalysis optimized by directed evolution Current Opinion in Biotechnology 15 4 305 13 doi 10 1016 j copbio 2004 06 007 PMID 15358000 Shevelev IV Hubscher U May 2002 The 3 5 exonucleases Nature Reviews Molecular Cell Biology 3 5 364 76 doi 10 1038 nrm804 PMID 11988770 S2CID 31605786 Zenkin N Yuzenkova Y Severinov K July 2006 Transcript assisted transcriptional proofreading Science 313 5786 518 20 Bibcode 2006Sci 313 518Z doi 10 1126 science 1127422 PMID 16873663 S2CID 40772789 Ibba M Soll D 2000 Aminoacyl tRNA synthesis Annual Review of Biochemistry 69 617 50 doi 10 1146 annurev biochem 69 1 617 PMID 10966471 Rodnina MV Wintermeyer W 2001 Fidelity of aminoacyl tRNA selection on the ribosome kinetic and structural mechanisms Annual Review of Biochemistry 70 415 35 doi 10 1146 annurev biochem 70 1 415 PMID 11395413 Khersonsky O Tawfik DS 2010 Enzyme promiscuity a mechanistic and evolutionary perspective Annual Review of Biochemistry 79 471 505 doi 10 1146 annurev biochem 030409 143718 PMID 20235827 O Brien PJ Herschlag D April 1999 Catalytic promiscuity and the evolution of new enzymatic activities Chemistry amp Biology 6 4 R91 R105 doi 10 1016 S1074 5521 99 80033 7 PMID 10099128 Fischer E 1894 Einfluss der Configuration auf die Wirkung der Enzyme Influence of configuration on the action of enzymes Berichte der Deutschen Chemischen Gesellschaft zu Berlin in German 27 3 2985 93 doi 10 1002 cber 18940270364 From page 2992 Um ein Bild zu gebrauchen will ich sagen dass Enzym und Glucosid wie Schloss und Schlussel zu einander passen mussen um eine chemische Wirkung auf einander ausuben zu konnen To use an image I will say that an enzyme and a glucoside i e glucose derivative must fit like a lock and key in order to be able to exert a chemical effect on each other Cooper GM 2000 Chapter 2 2 The Central Role of Enzymes as Biological Catalysts The Cell a Molecular Approach 2nd ed Washington DC ASM Press ISBN 0 87893 106 6 Koshland DE February 1958 Application of a Theory of Enzyme Specificity to Protein Synthesis Proceedings of the National Academy of Sciences of the United States of America 44 2 98 104 Bibcode 1958PNAS 44 98K doi 10 1073 pnas 44 2 98 PMC 335371 PMID 16590179 Vasella A Davies GJ Bohm M October 2002 Glycosidase mechanisms Current Opinion in Chemical Biology 6 5 619 29 doi 10 1016 S1367 5931 02 00380 0 PMID 12413546 Boyer R 2002 Chapter 6 Enzymes I Reactions Kinetics and Inhibition Concepts in Biochemistry 2nd ed New York Chichester Weinheim Brisbane Singapore Toronto John Wiley amp Sons Inc pp 137 8 ISBN 0 470 00379 0 OCLC 51720783 Savir Y Tlusty T 2007 Scalas E ed Conformational proofreading the impact of conformational changes on the specificity of molecular recognition PLOS ONE 2 5 e468 Bibcode 2007PLoSO 2 468S doi 10 1371 journal pone 0000468 PMC 1868595 PMID 17520027 Fersht A 1985 Enzyme Structure and Mechanism San Francisco W H Freeman pp 50 2 ISBN 978 0 7167 1615 0 Warshel A Sharma PK Kato M Xiang Y Liu H Olsson MH August 2006 Electrostatic basis for enzyme catalysis Chemical Reviews 106 8 3210 35 doi 10 1021 cr0503106 PMID 16895325 Cox MM Nelson DL 2013 Chapter 6 2 How enzymes work Lehninger Principles of Biochemistry 6th ed New York N Y W H Freeman p 195 ISBN 978 1464109621 Benkovic SJ Hammes Schiffer S August 2003 A perspective on enzyme catalysis Science 301 5637 1196 202 Bibcode 2003Sci 301 1196B doi 10 1126 science 1085515 PMID 12947189 S2CID 7899320 Jencks WP 1987 Catalysis in Chemistry and Enzymology Mineola N Y Dover ISBN 978 0 486 65460 7 Villa J Strajbl M Glennon TM Sham YY Chu ZT Warshel A October 2000 How important are entropic contributions to enzyme catalysis Proceedings of the National Academy of Sciences of the United States of America 97 22 11899 904 Bibcode 2000PNAS 9711899V doi 10 1073 pnas 97 22 11899 PMC 17266 PMID 11050223 Polgar L October 2005 The catalytic triad of serine peptidases Cellular and Molecular Life Sciences 62 19 20 2161 2172 doi 10 1007 s00018 005 5160 x PMID 16003488 S2CID 3343824 Ramanathan A Savol A Burger V Chennubhotla CS Agarwal PK 2014 Protein conformational populations and functionally relevant substates Acc Chem Res 47 1 149 56 doi 10 1021 ar400084s OSTI 1565147 PMID 23988159 Tsai CJ Del Sol A Nussinov R 2009 Protein allostery signal transmission and dynamics a classification scheme of allosteric mechanisms PDF Mol Biosyst 5 3 207 16 doi 10 1039 b819720b PMC 2898650 PMID 19225609 Changeux JP Edelstein SJ June 2005 Allosteric mechanisms of signal transduction Science 308 5727 1424 8 Bibcode 2005Sci 308 1424C doi 10 1126 science 1108595 PMID 15933191 S2CID 10621930 de Bolster MW 1997 Glossary of Terms Used in Bioinorganic Chemistry Cofactor International Union of Pure and Applied Chemistry Archived from the original on 21 January 2017 Retrieved 30 October 2007 Voet D Voet J Pratt C 2016 Fundamentals of Biochemistry Hoboken New Jersey John Wiley amp Sons Inc p 336 ISBN 978 1 118 91840 1 Chapman Smith A Cronan JE September 1999 The enzymatic biotinylation of proteins a post translational modification of exceptional specificity Trends in Biochemical Sciences 24 9 359 363 doi 10 1016 s0968 0004 99 01438 3 PMID 10470036 Fisher Z Hernandez Prada JA Tu C Duda D Yoshioka C An H Govindasamy L Silverman DN McKenna R February 2005 Structural and kinetic characterization of active site histidine as a proton shuttle in catalysis by human carbonic anhydrase II Biochemistry 44 4 1097 115 doi 10 1021 bi0480279 PMID 15667203 a b Wagner AL 1975 Vitamins and Coenzymes Krieger Pub Co ISBN 0 88275 258 8 BRENDA The Comprehensive Enzyme Information System Technische Universitat Braunschweig Retrieved 23 February 2015 Tornroth Horsefield S Neutze R December 2008 Opening and closing the metabolite gate Proceedings of the National Academy of Sciences of the United States of America 105 50 19565 6 Bibcode 2008PNAS 10519565T doi 10 1073 pnas 0810654106 PMC 2604989 PMID 19073922 McArdle WD Katch F Katch VL 2006 Chapter 9 The Pulmonary System and Exercise Essentials of Exercise Physiology 3rd ed Baltimore Maryland Lippincott Williams amp Wilkins pp 312 3 ISBN 978 0781749916 Ferguson SJ Nicholls D Ferguson S 2002 Bioenergetics 3 3rd ed San Diego Academic ISBN 0 12 518121 3 Bisswanger H 2017 Enzyme kinetics principles and methods Third enlarged and improved ed Weinheim Germany ISBN 9783527806461 OCLC 992976641 Michaelis L Menten M 1913 Die Kinetik der Invertinwirkung The Kinetics of Invertase Action Biochem Z in German 49 333 369 Michaelis L Menten ML Johnson KA Goody RS 2011 The original Michaelis constant translation of the 1913 Michaelis Menten paper Biochemistry 50 39 8264 9 doi 10 1021 bi201284u PMC 3381512 PMID 21888353 Briggs GE Haldane JB 1925 A Note on the Kinetics of Enzyme Action The Biochemical Journal 19 2 338 9 doi 10 1042 bj0190338 PMC 1259181 PMID 16743508 Bar Even A Noor E Savir Y Liebermeister W Davidi D Tawfik DS Milo R 2011 The moderately efficient enzyme evolutionary and physicochemical trends shaping enzyme parameters Biochemistry 50 21 4402 10 doi 10 1021 bi2002289 PMID 21506553 Ellis RJ October 2001 Macromolecular crowding obvious but underappreciated Trends in Biochemical Sciences 26 10 597 604 doi 10 1016 S0968 0004 01 01938 7 PMID 11590012 Kopelman R September 1988 Fractal reaction kinetics Science 241 4873 1620 26 Bibcode 1988Sci 241 1620K doi 10 1126 science 241 4873 1620 PMID 17820893 S2CID 23465446 a b c d Cornish Bowden A 2004 Fundamentals of Enzyme Kinetics 3 ed London Portland Press ISBN 1 85578 158 1 Price NC 1979 What is meant by competitive inhibition Trends in Biochemical Sciences 4 11 N272 N273 doi 10 1016 0968 0004 79 90205 6 Goodsell DS 1 August 1999 The Molecular Perspective Methotrexate The Oncologist 4 4 340 341 doi 10 1634 theoncologist 4 4 340 ISSN 1083 7159 PMID 10476546 Wu P Clausen MH Nielsen TE December 2015 Allosteric small molecule kinase inhibitors PDF Pharmacology amp Therapeutics 156 59 68 doi 10 1016 j pharmthera 2015 10 002 PMID 26478442 Cornish Bowden A July 1986 Why is uncompetitive inhibition so rare A possible explanation with implications for the design of drugs and pesticides FEBS Letters 203 1 3 6 doi 10 1016 0014 5793 86 81424 7 PMID 3720956 S2CID 45356060 Strelow JM 1 January 2017 A Perspective on the Kinetics of Covalent and Irreversible Inhibition SLAS Discovery 22 1 3 20 doi 10 1177 1087057116671509 ISSN 2472 5552 PMID 27703080 Fisher JF Meroueh SO Mobashery S February 2005 Bacterial resistance to beta lactam antibiotics compelling opportunism compelling opportunity Chemical Reviews 105 2 395 424 doi 10 1021 cr030102i PMID 15700950 a b Johnson DS Weerapana E Cravatt BF June 2010 Strategies for discovering and derisking covalent irreversible enzyme inhibitors Future Medicinal Chemistry 2 6 949 64 doi 10 4155 fmc 10 21 PMC 2904065 PMID 20640225 Endo A 1 November 1992 The discovery and development of HMG CoA reductase inhibitors J Lipid Res 33 11 1569 82 doi 10 1016 S0022 2275 20 41379 3 PMID 1464741 Wlodawer A Vondrasek J 1998 Inhibitors of HIV 1 protease a major success of structure assisted drug design Annual Review of Biophysics and Biomolecular Structure 27 249 84 doi 10 1146 annurev biophys 27 1 249 PMID 9646869 S2CID 10205781 Yoshikawa S Caughey WS May 1990 Infrared evidence of cyanide binding to iron and copper sites in bovine heart cytochrome c oxidase Implications regarding oxygen reduction The Journal of Biological Chemistry 265 14 7945 58 doi 10 1016 S0021 9258 19 39023 4 PMID 2159465 Jain JL May 1999 Fundamentals of biochemistry New Delhi S Chand and Co ISBN 8121903432 OCLC 818809626 Hunter T January 1995 Protein kinases and phosphatases the yin and yang of protein phosphorylation and signaling Cell 80 2 225 36 doi 10 1016 0092 8674 95 90405 0 PMID 7834742 S2CID 13999125 Berg JS Powell BC Cheney RE April 2001 A millennial myosin census Molecular Biology of the Cell 12 4 780 94 doi 10 1091 mbc 12 4 780 PMC 32266 PMID 11294886 Meighen EA March 1991 Molecular biology of bacterial bioluminescence Microbiological Reviews 55 1 123 42 doi 10 1128 MMBR 55 1 123 142 1991 PMC 372803 PMID 2030669 De Clercq E 2002 Highlights in the development of new antiviral agents Mini Rev Med Chem 2 2 163 75 doi 10 2174 1389557024605474 PMID 12370077 Mackie RI White BA October 1990 Recent advances in rumen microbial ecology and metabolism potential impact on nutrient output Journal of Dairy Science 73 10 2971 95 doi 10 3168 jds S0022 0302 90 78986 2 PMID 2178174 Rouzer CA Marnett LJ 2009 Cyclooxygenases structural and functional insights J Lipid Res 50 Suppl S29 34 doi 10 1194 jlr R800042 JLR200 PMC 2674713 PMID 18952571 a b c d Suzuki H 2015 Chapter 8 Control of Enzyme Activity How Enzymes Work From Structure to Function Boca Raton FL CRC Press pp 141 69 ISBN 978 981 4463 92 8 Doble BW Woodgett JR April 2003 GSK 3 tricks of the trade for a multi tasking kinase Journal of Cell Science 116 Pt 7 1175 86 doi 10 1242 jcs 00384 PMC 3006448 PMID 12615961 Bennett PM Chopra I 1993 Molecular basis of beta lactamase induction in bacteria Antimicrob Agents Chemother 37 2 153 8 doi 10 1128 aac 37 2 153 PMC 187630 PMID 8452343 Skett P Gibson GG 2001 Chapter 3 Induction and Inhibition of Drug Metabolism Introduction to Drug Metabolism 3 ed Cheltenham UK Nelson Thornes Publishers pp 87 118 ISBN 978 0748760114 Faergeman NJ Knudsen J April 1997 Role of long chain fatty acyl CoA esters in the regulation of metabolism and in cell signalling The Biochemical Journal 323 Pt 1 1 12 doi 10 1042 bj3230001 PMC 1218279 PMID 9173866 Suzuki H 2015 Chapter 4 Effect of pH Temperature and High Pressure on Enzymatic Activity How Enzymes Work From Structure to Function Boca Raton FL CRC Press pp 53 74 ISBN 978 981 4463 92 8 Noree C Sato BK Broyer RM Wilhelm JE August 2010 Identification of novel filament forming proteins in Saccharomyces cerevisiae and Drosophila melanogaster The Journal of Cell Biology 190 4 541 51 doi 10 1083 jcb 201003001 PMC 2928026 PMID 20713603 Aughey GN Liu JL 2015 Metabolic regulation via enzyme filamentation Critical Reviews in Biochemistry and Molecular Biology 51 4 282 93 doi 10 3109 10409238 2016 1172555 PMC 4915340 PMID 27098510 Kamata K Mitsuya M Nishimura T Eiki J Nagata Y March 2004 Structural basis for allosteric regulation of the monomeric allosteric enzyme human glucokinase Structure 12 3 429 38 doi 10 1016 j str 2004 02 005 PMID 15016359 Froguel P Zouali H Vionnet N Velho G Vaxillaire M Sun F Lesage S Stoffel M Takeda J Passa P March 1993 Familial hyperglycemia due to mutations in glucokinase Definition of a subtype of diabetes mellitus The New England Journal of Medicine 328 10 697 702 doi 10 1056 NEJM199303113281005 PMID 8433729 Okada S O Brien JS August 1969 Tay Sachs disease generalized absence of a beta D N acetylhexosaminidase component Science 165 3894 698 700 Bibcode 1969Sci 165 698O doi 10 1126 science 165 3894 698 PMID 5793973 S2CID 8473726 Learning About Tay Sachs Disease U S National Human Genome Research Institute Retrieved 1 March 2015 Erlandsen H Stevens RC October 1999 The structural basis of phenylketonuria Molecular Genetics and Metabolism 68 2 103 25 doi 10 1006 mgme 1999 2922 PMID 10527663 Flatmark T Stevens RC August 1999 Structural Insight into the Aromatic Amino Acid Hydroxylases and Their Disease Related Mutant Forms Chemical Reviews 99 8 2137 2160 doi 10 1021 cr980450y PMID 11849022 Phenylketonuria Genes and Disease Internet Bethesda MD National Center for Biotechnology Information US 1998 2015 Pseudocholinesterase deficiency U S National Library of Medicine Retrieved 5 September 2013 Fieker A Philpott J Armand M 2011 Enzyme replacement therapy for pancreatic insufficiency present and future Clinical and Experimental Gastroenterology 4 55 73 doi 10 2147 CEG S17634 PMC 3132852 PMID 21753892 Misselwitz B Pohl D Fruhauf H Fried M Vavricka SR Fox M June 2013 Lactose malabsorption and intolerance pathogenesis diagnosis and treatment United European Gastroenterology Journal 1 3 151 9 doi 10 1177 2050640613484463 PMC 4040760 PMID 24917953 Cleaver JE May 1968 Defective repair replication of DNA in xeroderma pigmentosum Nature 218 5142 652 6 Bibcode 1968Natur 218 652C doi 10 1038 218652a0 PMID 5655953 S2CID 4171859 James WD Elston D Berger TG 2011 Andrews Diseases of the Skin Clinical Dermatology 11th ed London Saunders Elsevier p 567 ISBN 978 1437703146 Murzin AG November 1993 Can homologous proteins evolve different enzymatic activities Trends in Biochemical Sciences 18 11 403 405 doi 10 1016 0968 0004 93 90132 7 PMID 8291080 Ochoa D Bradley D Beltrao P February 2018 Evolution dynamics and dysregulation of kinase signalling Current Opinion in Structural Biology 48 133 140 doi 10 1016 j sbi 2017 12 008 PMID 29316484 Renugopalakrishnan V Garduno Juarez R Narasimhan G Verma CS Wei X Li P November 2005 Rational design of thermally stable proteins relevance to bionanotechnology Journal of Nanoscience and Nanotechnology 5 11 1759 1767 doi 10 1166 jnn 2005 441 PMID 16433409 Hult K Berglund P August 2003 Engineered enzymes for improved organic synthesis Current Opinion in Biotechnology 14 4 395 400 doi 10 1016 S0958 1669 03 00095 8 PMID 12943848 Jiang L Althoff EA Clemente FR Doyle L Rothlisberger D Zanghellini A Gallaher JL Betker JL Tanaka F Barbas CF Hilvert D Houk KN Stoddard BL Baker D March 2008 De novo computational design of retro aldol enzymes Science 319 5868 1387 91 Bibcode 2008Sci 319 1387J doi 10 1126 science 1152692 PMC 3431203 PMID 18323453 a b Sun Y Cheng J May 2002 Hydrolysis of lignocellulosic materials for ethanol production a review Bioresource Technology 83 1 1 11 doi 10 1016 S0960 8524 01 00212 7 PMID 12058826 a b Kirk O Borchert TV Fuglsang CC August 2002 Industrial enzyme applications Current Opinion in Biotechnology 13 4 345 351 doi 10 1016 S0958 1669 02 00328 2 PMID 12323357 a b c Briggs DE 1998 Malts and Malting 1st ed London Blackie Academic ISBN 978 0412298004 Dulieu C Moll M Boudrant J Poncelet D 2000 Improved performances and control of beer fermentation using encapsulated alpha acetolactate decarboxylase and modeling Biotechnology Progress 16 6 958 65 doi 10 1021 bp000128k PMID 11101321 S2CID 25674881 Tarte R 2008 Ingredients in Meat Products Properties Functionality and Applications New York Springer p 177 ISBN 978 0 387 71327 4 Chymosin GMO Database GMO Compass European Union 10 July 2010 Archived from the original on 26 March 2015 Retrieved 1 March 2015 Molimard P Spinnler HE February 1996 Review Compounds Involved in the Flavor of Surface Mold Ripened Cheeses Origins and Properties Journal of Dairy Science 79 2 169 184 doi 10 3168 jds S0022 0302 96 76348 8 Guzman Maldonado H Paredes Lopez O September 1995 Amylolytic enzymes and products derived from starch a review Critical Reviews in Food Science and Nutrition 35 5 373 403 doi 10 1080 10408399509527706 PMID 8573280 a b Protease GMO Database GMO Compass European Union 10 July 2010 Archived from the original on 24 February 2015 Retrieved 28 February 2015 Alkorta I Garbisu C Llama MJ Serra JL January 1998 Industrial applications of pectic enzymes a review Process Biochemistry 33 1 21 28 doi 10 1016 S0032 9592 97 00046 0 Bajpai P March 1999 Application of enzymes in the pulp and paper industry Biotechnology Progress 15 2 147 157 doi 10 1021 bp990013k PMID 10194388 S2CID 26080240 Begley CG Paragina S Sporn A March 1990 An analysis of contact lens enzyme cleaners Journal of the American Optometric Association 61 3 190 4 PMID 2186082 Farris PL 2009 Economic Growth and Organization of the U S Starch Industry In BeMiller JN Whistler RL eds Starch Chemistry and Technology 3rd ed London Academic ISBN 9780080926551 Further readingGeneralBerg JM Tymoczko JL Stryer L 2002 Biochemistry 5th ed New York NY W H Freeman ISBN 0 7167 3051 0 A biochemistry textbook available free online through NCBI Bookshelf Etymology and historyCornish Bowden A ed 1997 New Beer in an Old Bottle Eduard Buchner and the Growth of Biochemical Knowledge Universitat de Valencia ISBN 84 370 3328 4 Archived from the original on 13 December 2010 Retrieved 27 June 2006 A history of early enzymology Enzyme structure and mechanismSuzuki H 2015 How Enzymes Work From Structure to Function Boca Raton FL CRC Press ISBN 978 981 4463 92 8 Kinetics and inhibitionCornish Bowden A 2012 Fundamentals of Enzyme Kinetics 4th ed Weinheim Wiley VCH ISBN 978 3527330744 External links Media related to Enzymes at Wikimedia Commons Retrieved from https en wikipedia org w index php title Enzyme amp oldid 1132111677, wikipedia, wiki, book, books, library,

article

, read, download, free, free download, mp3, video, mp4, 3gp, jpg, jpeg, gif, png, picture, music, song, movie, book, game, games.