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RuBisCO

February 15, 2024

Ribulose-1,5-bisphosphate carboxylase/oxygenase, commonly known by the abbreviations RuBisCo, rubisco,[1] RuBPCase,[2] or RuBPco,[3] is an enzyme (EC 4.1.1.39) involved in light-independent (or "dark") part of photosynthesis, including the carbon fixation by which atmospheric carbon dioxide is converted by plants and other photosynthetic organisms to energy-rich molecules such as glucose. It emerged approximately four billion years ago in primordial metabolism prior to the presence of oxygen on Earth.[4] It is probably the most abundant enzyme on Earth. In chemical terms, it catalyzes the carboxylation of ribulose-1,5-bisphosphate (also known as RuBP).[5][6][7]

Ribulose-1,5-bisphosphate carboxylase oxygenase
A 3d depiction of the activated RuBisCO from spinach in open form with active site accessible. The active site Lys175 residues are marked in pink, and a close-up of the residue is provided to the right for one of the monomers composing the enzyme.
Identifiers
EC no.4.1.1.39
CAS no.9027-23-0
Databases
IntEnzIntEnz view
BRENDABRENDA entry
ExPASyNiceZyme view
KEGGKEGG entry
MetaCycmetabolic pathway
PRIAMprofile
PDB structuresRCSB PDB PDBe PDBsum
Gene OntologyAmiGO / QuickGO
Search
PMCarticles
PubMedarticles
NCBIproteins

Alternative carbon fixation pathways edit

RuBisCO is important biologically because it catalyzes the primary chemical reaction by which inorganic carbon enters the biosphere. While many autotrophic bacteria and archaea fix carbon via the reductive acetyl CoA pathway, the 3-hydroxypropionate cycle, or the reverse Krebs cycle, these pathways are relatively small contributors to global carbon fixation compared to that catalyzed by RuBisCO. Phosphoenolpyruvate carboxylase, unlike RuBisCO, only temporarily fixes carbon. Reflecting its importance, RuBisCO is the most abundant protein in leaves, accounting for 50% of soluble leaf protein in C3 plants (20–30% of total leaf nitrogen) and 30% of soluble leaf protein in C4 plants (5–9% of total leaf nitrogen).[7] Given its important role in the biosphere, the genetic engineering of RuBisCO in crops is of continuing interest (see below).

Structure edit

 
Active site of RuBisCO of Galdieria sulphuraria with CO2: Residues involved in both the active site and stabilizing CO2 for enzyme catalysis are shown in color and labeled. Distances of the hydrogen bonding interactions are shown in angstroms. Mg2+ ion (green sphere) is shown coordinated to CO2, and is followed by three water molecules (red spheres). All other residues are placed in grayscale.
 
Location of the rbcL gene in the chloroplast genome of Arabidopsis thaliana (positions ca. 55-56.4 kb). rbcL is one of the 21 protein-coding genes involved in photosynthesis (green boxes).

In plants, algae, cyanobacteria, and phototrophic and chemoautotrophic Pseudomonadota (formerly proteobacteria), the enzyme usually consists of two types of protein subunit, called the large chain (L, about 55,000 Da) and the small chain (S, about 13,000 Da). The large-chain gene (rbcL) is encoded by the chloroplast DNA in plants.[8] There are typically several related small-chain genes in the nucleus of plant cells, and the small chains are imported to the stromal compartment of chloroplasts from the cytosol by crossing the outer chloroplast membrane.[6][9] The enzymatically active substrate (ribulose 1,5-bisphosphate) binding sites are located in the large chains that form dimers in which amino acids from each large chain contribute to the binding sites. A total of eight large chains (= four dimers) and eight small chains assemble into a larger complex of about 540,000 Da.[10] In some Pseudomonadota and dinoflagellates, enzymes consisting of only large subunits have been found.[a]

Magnesium ions (Mg2+) are needed for enzymatic activity. Correct positioning of Mg2+ in the active site of the enzyme involves addition of an "activating" carbon dioxide molecule (CO2) to a lysine in the active site (forming a carbamate).[12] Mg2+ operates by driving deprotonation of the Lys210 residue, causing the Lys residue to rotate by 120 degrees to the trans conformer, decreasing the distance between the nitrogen of Lys and the carbon of CO2. The close proximity allows for the formation of a covalent bond, resulting in the carbamate.[13] Mg2+ is first enabled to bind to the active site by the rotation of His335 to an alternate conformation. Mg2+ is then coordinated by the His residues of the active site (His300, His302, His335), and is partially neutralized by the coordination of three water molecules and their conversion to OH.[13] This coordination results in an unstable complex, but produces a favorable environment for the binding of Mg2+. Formation of the carbamate is favored by an alkaline pH. The pH and the concentration of magnesium ions in the fluid compartment (in plants, the stroma of the chloroplast) increases in the light. The role of changing pH and magnesium ion levels in the regulation of RuBisCO enzyme activity is discussed below. Once the carbamate is formed, His335 finalizes the activation by returning to its initial position through thermal fluctuation.[13]

RuBisCO large chain,
catalytic domain
Identifiers
SymbolRuBisCO_large
PfamPF00016
InterProIPR000685
PROSITEPDOC00142
SCOP23rub / SCOPe / SUPFAM
CDDcd08148
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary
PDB1aa1​, 1aus​, 1bwv​, 1bxn​, 1ej7​, 1geh​, 1gk8​, 1ir1​, 1ir2​, 1iwa​, 1rba​, 1rbl​, 1rbo​, 1rco​, 1rcx​, 1rld​, 1rsc​, 1rus​, 1rxo​, 1svd​, 1tel​, 1upm​, 1upp​, 1uw9​, 1uwa​, 1uzd​, 1uzh​, 1wdd​, 1ykw​, 2cwx​, 2cxe​, 2d69​, 2qyg​, 2rus​, 2v63​, 2v67​, 2v68​, 2v69​, 2v6a​, 3rub​, 4rub​, 5rub​, 8ruc​, 9rub
RuBisCO, N-terminal domain
Identifiers
SymbolRuBisCO_large_N
PfamPF02788
InterProIPR017444
SCOP23rub / SCOPe / SUPFAM
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary
PDB1aa1​, 1aus​, 1bwv​, 1bxn​, 1ej7​, 1geh​, 1gk8​, 1ir1​, 1ir2​, 1iwa​, 1rba​, 1rbl​, 1rbo​, 1rco​, 1rcx​, 1rld​, 1rsc​, 1rus​, 1rxo​, 1svd​, 1tel​, 1upm​, 1upp​, 1uw9​, 1uwa​, 1uzd​, 1uzh​, 1wdd​, 1ykw​, 2cwx​, 2cxe​, 2d69​, 2qyg​, 2rus​, 2v63​, 2v67​, 2v68​, 2v69​, 2v6a​, 3rub​, 4rub​, 5rub​, 8ruc​, 9rub
RuBisCO, small chain
Identifiers
SymbolRuBisCO_small
PfamPF00101
InterProIPR000894
SCOP23rub / SCOPe / SUPFAM
CDDcd03527
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary
PDB1aa1​, 1aus​, 1bwv​, 1bxn​, 1ej7​, 1gk8​, 1ir1​, 1ir2​, 1iwa​, 1rbl​, 1rbo​, 1rco​, 1rcx​, 1rlc​, 1rld​, 1rsc​, 1rxo​, 1svd​, 1upm​, 1upp​, 1uw9​, 1uwa​, 1uzd​, 1uzh​, 1wdd​, 2v63​, 2v67​, 2v68​, 2v69​, 2v6a​, 3rub​, 4rub​, 8ruc

Enzymatic activity edit

 
Two main reactions of RuBisCo: CO2 fixation and oxygenation.

RuBisCO is one of many enzymes in the Calvin cycle. When Rubisco facilitates the attack of CO2 at the C2 carbon of RuBP and subsequent bond cleavage between the C3 and C2 carbon, 2 molecules of glycerate-3-phosphate are formed. The conversion involves these steps: enolisation, carboxylation, hydration, C-C bond cleavage, and protonation.[14][15][16]

Substrates edit

Substrates for RuBisCO are ribulose-1,5-bisphosphate and carbon dioxide (distinct from the "activating" carbon dioxide). RuBisCO also catalyses a reaction of ribulose-1,5-bisphosphate and molecular oxygen (O2) instead of carbon dioxide (CO2).[17] Discriminating between the substrates CO2 and O2 is attributed to the differing interactions of the substrate's quadrupole moments and a high electrostatic field gradient.[13] This gradient is established by the dimer form of the minimally active RuBisCO, which with its two components provides a combination of oppositely charged domains required for the enzyme's interaction with O2 and CO2. These conditions help explain the low turnover rate found in RuBisCO: In order to increase the strength of the electric field necessary for sufficient interaction with the substrates’ quadrupole moments, the C- and N- terminal segments of the enzyme must be closed off, allowing the active site to be isolated from the solvent and lowering the dielectric constant.[18] This isolation has a significant entropic cost, and results in the poor turnover rate.

Binding RuBP edit

Carbamylation of the ε-amino group of Lys210 is stabilized by coordination with the Mg2+.[19] This reaction involves binding of the carboxylate termini of Asp203 and Glu204 to the Mg2+ ion. The substrate RuBP binds Mg2+ displacing two of the three aquo ligands.[14][20][21]

Enolisation edit

Enolisation of RuBP is the conversion of the keto tautomer of RuBP to an enediol(ate). Enolisation is initiated by deprotonation at C3. The enzyme base in this step has been debated,[20][22] but the steric constraints observed in crystal structures have made Lys210 the most likely candidate.[14] Specifically, the carbamate oxygen on Lys210 that is not coordinated with the Mg ion deprotonates the C3 carbon of RuBP to form a 2,3-enediolate.[20][21]

Carboxylation edit

 
A 3D image of the active site of spinach RuBisCO complexed with the inhibitor 2-carboxyarabinitol-1,5-bisphosphate, CO2, and Mg2+. (PDB: 1IR1; Ligand View [CAP]501:A)

Carboxylation of the 2,3-enediolate results in the intermediate 3-keto-2-carboxyarabinitol-1,5-bisphosphate and Lys334 is positioned to facilitate the addition of the CO2 substrate as it replaces the third Mg2+-coordinated water molecule and add directly to the enediol. No Michaelis complex is formed in this process.[14][22] Hydration of this ketone results in an additional hydroxy group on C3, forming a gem-diol intermediate.[20][23] Carboxylation and hydration have been proposed as either a single concerted step[20] or as two sequential steps.[23] Concerted mechanism is supported by the proximity of the water molecule to C3 of RuBP in multiple crystal structures. Within the spinach structure, other residues are well placed to aid in the hydration step as they are within hydrogen bonding distance of the water molecule.[14]

C-C bond cleavage edit

The gem-diol intermediate cleaves at the C2-C3 bond to form one molecule of glycerate-3-phosphate and a negatively charged carboxylate.[14] Stereo specific protonation of C2 of this carbanion results in another molecule of glycerate-3-phosphate. This step is thought to be facilitated by Lys175 or potentially the carbamylated Lys210.[14]

Products edit

When carbon dioxide is the substrate, the product of the carboxylase reaction is an unstable six-carbon phosphorylated intermediate known as 3-keto-2-carboxyarabinitol-1,5-bisphosphate, which decays rapidly into two molecules of glycerate-3-phosphate. This product, also known as 3-phosphoglycerate, can be used to produce larger molecules such as glucose.

When molecular oxygen is the substrate, the products of the oxygenase reaction are phosphoglycolate and 3-phosphoglycerate. Phosphoglycolate is recycled through a sequence of reactions called photorespiration, which involves enzymes and cytochromes located in the mitochondria and peroxisomes (this is a case of metabolite repair). In this process, two molecules of phosphoglycolate are converted to one molecule of carbon dioxide and one molecule of 3-phosphoglycerate, which can reenter the Calvin cycle. Some of the phosphoglycolate entering this pathway can be retained by plants to produce other molecules such as glycine. At ambient levels of carbon dioxide and oxygen, the ratio of the reactions is about 4 to 1, which results in a net carbon dioxide fixation of only 3.5. Thus, the inability of the enzyme to prevent the reaction with oxygen greatly reduces the photosynthetic capacity of many plants. Some plants, many algae, and photosynthetic bacteria have overcome this limitation by devising means to increase the concentration of carbon dioxide around the enzyme, including C4 carbon fixation, crassulacean acid metabolism, and the use of pyrenoid.

Rubisco side activities can lead to useless or inhibitory by-products. Important inhibitory by-products include xylulose 1,5-bisphosphate and glycero-2,3-pentodiulose 1,5-bisphosphate, both caused by "misfires" halfway in the enolisation-carboxylation reaction. In higher plants, this process causes RuBisCO self-inhibition, which can be triggered by saturating CO2 and RuBP concentrations and solved by Rubisco activase (see below).[24]

Rate of enzymatic activity edit

 
Overview of the Calvin cycle and carbon fixation.

Some enzymes can carry out thousands of chemical reactions each second. However, RuBisCO is slow, fixing only 3-10 carbon dioxide molecules each second per molecule of enzyme.[25] The reaction catalyzed by RuBisCO is, thus, the primary rate-limiting factor of the Calvin cycle during the day. Nevertheless, under most conditions, and when light is not otherwise limiting photosynthesis, the speed of RuBisCO responds positively to increasing carbon dioxide concentration.

RuBisCO is usually only active during the day, as ribulose 1,5-bisphosphate is not regenerated in the dark. This is due to the regulation of several other enzymes in the Calvin cycle. In addition, the activity of RuBisCO is coordinated with that of the other enzymes of the Calvin cycle in several other ways:

By ions edit

Upon illumination of the chloroplasts, the pH of the stroma rises from 7.0 to 8.0 because of the proton (hydrogen ion, H+) gradient created across the thylakoid membrane. The movement of protons into thylakoids is driven by light and is fundamental to ATP synthesis in chloroplasts (Further reading: Photosynthetic reaction centre; Light-dependent reactions). To balance ion potential across the membrane, magnesium ions (Mg2+) move out of the thylakoids in response, increasing the concentration of magnesium in the stroma of the chloroplasts. RuBisCO has a high optimal pH (can be >9.0, depending on the magnesium ion concentration) and, thus, becomes "activated" by the introduction of carbon dioxide and magnesium to the active sites as described above.

By RuBisCO activase edit

In plants and some algae, another enzyme, RuBisCO activase (Rca, GO:0046863, P10896), is required to allow the rapid formation of the critical carbamate in the active site of RuBisCO.[26][27] This is required because ribulose 1,5-bisphosphate (RuBP) binds more strongly to the active sites of RuBisCO when excess carbamate is present, preventing processes from moving forward. In the light, RuBisCO activase promotes the release of the inhibitory (or — in some views — storage) RuBP from the catalytic sites of RuBisCO. Activase is also required in some plants (e.g., tobacco and many beans) because, in darkness, RuBisCO is inhibited (or protected from hydrolysis) by a competitive inhibitor synthesized by these plants, a substrate analog 2-carboxy-D-arabitinol 1-phosphate (CA1P).[28] CA1P binds tightly to the active site of carbamylated RuBisCO and inhibits catalytic activity to an even greater extent. CA1P has also been shown to keep RuBisCO in a conformation that is protected from proteolysis.[29] In the light, RuBisCO activase also promotes the release of CA1P from the catalytic sites. After the CA1P is released from RuBisCO, it is rapidly converted to a non-inhibitory form by a light-activated CA1P-phosphatase. Even without these strong inhibitors, once every several hundred reactions, the normal reactions with carbon dioxide or oxygen are not completed; other inhibitory substrate analogs are still formed in the active site. Once again, RuBisCO activase can promote the release of these analogs from the catalytic sites and maintain the enzyme in a catalytically active form. However, at high temperatures, RuBisCO activase aggregates and can no longer activate RuBisCO. This contributes to the decreased carboxylating capacity observed during heat stress.[30][31]

By activase edit

The removal of the inhibitory RuBP, CA1P, and the other inhibitory substrate analogs by activase requires the consumption of ATP. This reaction is inhibited by the presence of ADP, and, thus, activase activity depends on the ratio of these compounds in the chloroplast stroma. Furthermore, in most plants, the sensitivity of activase to the ratio of ATP/ADP is modified by the stromal reduction/oxidation (redox) state through another small regulatory protein, thioredoxin. In this manner, the activity of activase and the activation state of RuBisCO can be modulated in response to light intensity and, thus, the rate of formation of the ribulose 1,5-bisphosphate substrate.[32]

By phosphate edit

In cyanobacteria, inorganic phosphate (Pi) also participates in the co-ordinated regulation of photosynthesis: Pi binds to the RuBisCO active site and to another site on the large chain where it can influence transitions between activated and less active conformations of the enzyme. In this way, activation of bacterial RuBisCO might be particularly sensitive to Pi levels, which might cause it to act in a similar way to how RuBisCO activase functions in higher plants.[33]

By carbon dioxide edit

Since carbon dioxide and oxygen compete at the active site of RuBisCO, carbon fixation by RuBisCO can be enhanced by increasing the carbon dioxide level in the compartment containing RuBisCO (chloroplast stroma). Several times during the evolution of plants, mechanisms have evolved for increasing the level of carbon dioxide in the stroma (see C4 carbon fixation). The use of oxygen as a substrate appears to be a puzzling process, since it seems to throw away captured energy. However, it may be a mechanism for preventing carbohydrate overload during periods of high light flux. This weakness in the enzyme is the cause of photorespiration, such that healthy leaves in bright light may have zero net carbon fixation when the ratio of O2 to CO2 available to RuBisCO shifts too far towards oxygen. This phenomenon is primarily temperature-dependent: high temperatures can decrease the concentration of CO2 dissolved in the moisture of leaf tissues. This phenomenon is also related to water stress: since plant leaves are evaporatively cooled, limited water causes high leaf temperatures. C4 plants use the enzyme PEP carboxylase initially, which has a higher affinity for CO2. The process first makes a 4-carbon intermediate compound, hence the name C4 plants, which is shuttled into a site of C3 photosynthesis then decarboxylated, releasing CO2 to boost the concentration of CO2.

Crassulacean acid metabolism (CAM) plants keep their stomata closed during the day, which conserves water but prevents the light-independent reactions (a.k.a. the Calvin Cycle) from taking place, since these reactions require CO2 to pass by gas exchange through these openings. Evaporation through the upper side of a leaf is prevented by a layer of wax.

Genetic engineering edit

Since RuBisCO is often rate-limiting for photosynthesis in plants, it may be possible to improve photosynthetic efficiency by modifying RuBisCO genes in plants to increase catalytic activity and/or decrease oxygenation rates.[34][35][36][37] This could improve sequestration of CO2 and be a strategy to increase crop yields.[38] Approaches under investigation include transferring RuBisCO genes from one organism into another organism, engineering Rubisco activase from thermophilic cyanobacteria into temperature sensitive plants, increasing the level of expression of RuBisCO subunits, expressing RuBisCO small chains from the chloroplast DNA, and altering RuBisCO genes to increase specificity for carbon dioxide or otherwise increase the rate of carbon fixation.[39][40]

Mutagenesis in plants edit

In general, site-directed mutagenesis of RuBisCO has been mostly unsuccessful,[38] though mutated forms of the protein have been achieved in tobacco plants with subunit C4 species,[41] and a RuBisCO with more C4-like kinetic characteristics have been attained in rice via nuclear transformation.[42] Robust and reliable engineering for yield of RuBisCO and other enzymes in the C3 cycle was shown to be possible,[43] and it was first achieved in 2019 through a synthetic biology approach.[37]

One avenue is to introduce RuBisCO variants with naturally high specificity values such as the ones from the red alga Galdieria partita into plants. This may improve the photosynthetic efficiency of crop plants, although possible negative impacts have yet to be studied.[44] Advances in this area include the replacement of the tobacco enzyme with that of the purple photosynthetic bacterium Rhodospirillum rubrum.[45] In 2014, two transplastomic tobacco lines with functional RuBisCO from the cyanobacterium Synechococcus elongatus PCC7942 (Se7942) were created by replacing the RuBisCO with the large and small subunit genes of the Se7942 enzyme, in combination with either the corresponding Se7942 assembly chaperone, RbcX, or an internal carboxysomal protein, CcmM35. Both mutants had increased CO2 fixation rates when measured as carbon molecules per RuBisCO. However, the mutant plants grew more slowly than wild-type.[46]

A recent theory explores the trade-off between the relative specificity (i.e., ability to favour CO2 fixation over O2 incorporation, which leads to the energy-wasteful process of photorespiration) and the rate at which product is formed. The authors conclude that RuBisCO may actually have evolved to reach a point of 'near-perfection' in many plants (with widely varying substrate availabilities and environmental conditions), reaching a compromise between specificity and reaction rate.[47] It has been also suggested that the oxygenase reaction of RuBisCO prevents CO2 depletion near its active sites and provides the maintenance of the chloroplast redox state.[48]

Since photosynthesis is the single most effective natural regulator of carbon dioxide in the Earth's atmosphere,[49] a biochemical model of RuBisCO reaction is used as the core module of climate change models. Thus, a correct model of this reaction is essential to the basic understanding of the relations and interactions of environmental models.

Expression in bacterial hosts edit

There currently are very few effective methods for expressing functional plant Rubisco in bacterial hosts for genetic manipulation studies. This is largely due to Rubisco's requirement of complex cellular machinery for its biogenesis and metabolic maintenance including the nuclear-encoded RbcS subunits, which are typically imported into chloroplasts as unfolded proteins.[50][51] Furthermore, sufficient expression and interaction with Rubisco activase are major challenges as well.[39] One successful method for expression of Rubisco in E. coli involves the co-expression of multiple chloroplast chaperones, though this has only been shown for Arabidopsis thaliana Rubisco.[52]

Depletion in proteomic studies edit

Due to its high abundance in plants (generally 40% of the total protein content), RuBisCO often impedes analysis of important signaling proteins such as transcription factors, kinases, and regulatory proteins found in lower abundance (10-100 molecules per cell) within plants.[53] For example, using mass spectrometry on plant protein mixtures would result in multiple intense RuBisCO subunit peaks that interfere and hide those of other proteins.

Recently, one efficient method for precipitating out RuBisCO involves the usage of protamine sulfate solution.[54] Other existing methods for depleting RuBisCO and studying lower abundance proteins include fractionation techniques with calcium and phytate,[55] gel electrophoresis with polyethylene glycol,[56][57] affinity chromatography,[58][59] and aggregation using DTT,[60] though these methods are more time-consuming and less efficient when compared to protamine sulfate precipitation.[53]

Evolution of RuBisCO edit

Phylogenetic studies edit

The chloroplast gene rbcL, which codes for the large subunit of RuBisCO has been widely used as an appropriate locus for analysis of phylogenetics in plant taxonomy.[61]

Origin edit

Non-carbon-fixing proteins similar to RuBisCO, termed RuBisCO-like proteins (RLPs), are also found in the wild in organisms as common as Bacillus subtilis. This bacterium has a rbcL-like protein with a 2,3-diketo-5-methylthiopentyl-1-phosphate enolase function, part of the methionine salvage pathway.[62] Later identifications found functionally divergent examples dispersed all over bacteria and archaea, as well as transitionary enzymes performing both RLP-type enolase and RuBisCO functions. It is now believed that the current RuBisCO evolved from a dimeric RLP ancestor, acquiring its carboxylase function first before further oligomerizing and then recruiting the small subunit to form the familiar modern enzyme.[15] The small subunit probably first evolved in anaerobic and thermophilic organisms, where it enabled RuBisCO to catalyze its reaction at higher temperatures.[63] In addition to its effect on stabilizing catalysis, it enabled the evolution of higher specificities for CO2 over O2 by modulating the effect that substitutions within RuBisCO have on enzymatic function. Substitutions that do not have an effect without the small subunit suddenly become beneficial when it is bound. Furthermore, the small subunit enabled the accumulation of substitutions that are only tolerated in its presence. Accumulation of such substitutions leads to a strict dependence on the small subunit, which is observed in extant Rubiscos that bind a small subunit.

C4 edit

With the mass convergent evolution of the C4-fixation pathway in a diversity of plant lineages, ancestral C3-type RuBisCO evolved to have faster turnover of CO2 in exchange for lower specificity as a result of the greater localization of CO2 from the mesophyll cells into the bundle sheath cells.[64] This was achieved through enhancement of conformational flexibility of the “open-closed” transition in the Calvin cycle. Laboratory-based phylogenetic studies have shown that this evolution was constrained by the trade-off between stability and activity brought about by the series of necessary mutations for C4 RuBisCO.[65] Moreover, in order to sustain the destabilizing mutations, the evolution to C4 RuBisCO was preceded by a period in which mutations granted the enzyme increased stability, establishing a buffer to sustain and maintain the mutations required for C4 RuBisCO. To assist with this buffering process, the newly-evolved enzyme was found to have further developed a series of stabilizing mutations. While RuBisCO has always been accumulating new mutations, most of these mutations that have survived have not had significant effects on protein stability. The destabilizing C4 mutations on RuBisCO has been sustained by environmental pressures such as low CO2 concentrations, requiring a sacrifice of stability for new adaptive functions.[65]

History of the term edit

The term "RuBisCO" was coined humorously in 1979, by David Eisenberg at a seminar honouring the retirement of the early, prominent RuBisCO researcher, Sam Wildman, and also alluded to the snack food trade name "Nabisco" in reference to Wildman's attempts to create an edible protein supplement from tobacco leaves.[66][67]

The capitalization of the name has been long debated. It can be capitalized for each letter of the full name (Ribulose-1,5 bisphosphate carboxylase/oxygenase), but it has also been argued that is should all be in lower case (rubisco), similar to other terms like scuba or laser.[1]

See also edit

References edit

  1. ^ The structure of RuBisCO from the photosynthetic bacterium Rhodospirillum rubrum has been determined by X-ray crystallography, see: PDB: 9RUB​. A comparison of the structures of eukaryotic and bacterial RuBisCO is shown in the Protein Data Bank "Molecule of the Month" #11.[11]
  1. ^ a b Sharkey TD (May 2019). "Discovery of the canonical Calvin-Benson cycle". Photosynthesis Research. 140 (2): 235–252. Bibcode:2019PhoRe.140..235S. doi:10.1007/s11120-018-0600-2. OSTI 1607740. PMID 30374727. S2CID 53092349.
  2. ^ Nivison, Helen; Stocking, C. (1983). "Ribulose Bisphosphate Carboxylase Synthesis in Barley Leaves". Plant Physiology. 73 (4): 906–911. doi:10.1104/pp.73.4.906. PMC 1066578. PMID 16663341.
  3. ^ Mächler, Felix; Nösberger, Josef (1988). "Bicarbonate Inhibits Ribulose-1,5-Bisphosphate Carboxylase". Plant Physiology. 88 (2): 462–465. doi:10.1104/pp.88.2.462. PMC 1055600. PMID 16666327.
  4. ^ Back to the future of photosynthesis: Resurrecting billon-year-old enzymes reveals how photosynthesis adapted to the rise of oxygen., News from the Max Planck Society, October 13, 2022
  5. ^ Cooper GM (2000). "10.The Chloroplast Genome". The Cell: A Molecular Approach (2nd ed.). Washington, D.C: ASM Press. ISBN 978-0-87893-106-4. , one of the subunits of ribulose bisphosphate carboxylase (rubisco) is encoded by chloroplast DNA. Rubisco is the critical enzyme that catalyzes the addition of CO2 to ribulose-1,5-bisphosphate during the Calvin cycle. It is also thought to be the single most abundant protein on Earth, so it is noteworthy that one of its subunits is encoded by the chloroplast genome.
  6. ^ a b Dhingra A, Portis AR, Daniell H (April 2004). "Enhanced translation of a chloroplast-expressed RbcS gene restores small subunit levels and photosynthesis in nuclear RbcS antisense plants". Proceedings of the National Academy of Sciences of the United States of America. 101 (16): 6315–6320. Bibcode:2004PNAS..101.6315D. doi:10.1073/pnas.0400981101. PMC 395966. PMID 15067115. (Rubisco) is the most prevalent enzyme on this planet, accounting for 30–50% of total soluble protein in the chloroplast;
  7. ^ a b Feller U, Anders I, Mae T (2008). "Rubiscolytics: fate of Rubisco after its enzymatic function in a cell is terminated". Journal of Experimental Botany. 59 (7): 1615–1624. doi:10.1093/jxb/erm242. PMID 17975207.
  8. ^ Vitlin Gruber A, Feiz L (2018). "Rubisco Assembly in the Chloroplast". Frontiers in Molecular Biosciences. 5: 24. doi:10.3389/fmolb.2018.00024. PMC 5859369. PMID 29594130.
  9. ^ Arabidopsis thaliana has four RuBisCO small chain genes.
    Yoon M, Putterill JJ, Ross GS, Laing WA (April 2001). "Determination of the relative expression levels of rubisco small subunit genes in Arabidopsis by rapid amplification of cDNA ends". Analytical Biochemistry. 291 (2): 237–244. doi:10.1006/abio.2001.5042. PMID 11401297.
  10. ^ Stryer L, Berg JM, Tymoczko JL (2002). "Chapter 20: The Calvin Cycle and the Pentose Phosphate Pathway". Biochemistry (5th ed.). San Francisco: W.H. Freeman. ISBN 978-0-7167-3051-4. Figure 20.3. Structure of Rubisco.] (Color-coded ribbon diagram)
  11. ^ Goodsell D (November 2000). "Rubisco". Molecule of the Month. RCSB PDB (Research Collaboratory for Structural Bioinformatics PDB). doi:10.2210/rcsb_pdb/mom_2000_11.
  12. ^ Lodish H, Berk A, Zipursky SL, Matsudaira P, Baltimore D, Darnell JE (2000). "Molecular Cell Biology" (4th ed.). New York: W. H. Freeman & Co. Figure 16-48 shows a structural model of the active site, including the involvement of magnesium.
  13. ^ a b c d Stec B (November 2012). "Structural mechanism of RuBisCO activation by carbamylation of the active site lysine". Proceedings of the National Academy of Sciences of the United States of America. 109 (46): 18785–18790. Bibcode:2012PNAS..10918785S. doi:10.1073/pnas.1210754109. PMC 3503183. PMID 23112176.
  14. ^ a b c d e f g Andersson I (May 2008). "Catalysis and regulation in Rubisco". Journal of Experimental Botany. 59 (7): 1555–1568. doi:10.1093/jxb/ern091. PMID 18417482.
  15. ^ a b Erb TJ, Zarzycki J (February 2018). "A short history of RubisCO: the rise and fall (?) of Nature's predominant CO2 fixing enzyme". Current Opinion in Biotechnology. 49: 100–107. doi:10.1016/j.copbio.2017.07.017. PMC 7610757. PMID 28843191.
  16. ^ Lundqvist T, Schneider G (July 1991). "Crystal structure of activated ribulose-1,5-bisphosphate carboxylase complexed with its substrate, ribulose-1,5-bisphosphate". The Journal of Biological Chemistry. 266 (19): 12604–12611. doi:10.1016/S0021-9258(18)98942-8. PMID 1905726.
  17. ^ Goodsell D (November 2000). "Rubisco". Molecule of the Month. RCSB PDB (Research Collaboratory for Structural Bioinformatics PDB). doi:10.2210/rcsb_pdb/mom_2000_11.
  18. ^ Satagopan S, Spreitzer RJ (July 2008). "Plant-like substitutions in the large-subunit carboxy terminus of Chlamydomonas Rubisco increase CO2/O2 specificity". BMC Plant Biology. 8: 85. doi:10.1186/1471-2229-8-85. PMC 2527014. PMID 18664299.
  19. ^ Lorimer GH, Miziorko HM (November 1980). "Carbamate formation on the epsilon-amino group of a lysyl residue as the basis for the activation of ribulosebisphosphate carboxylase by CO2 and Mg2+". Biochemistry. 19 (23): 5321–5328. doi:10.1021/bi00564a027. PMID 6778504.
  20. ^ a b c d e Cleland WW, Andrews TJ, Gutteridge S, Hartman FC, Lorimer GH (April 1998). "Mechanism of Rubisco: The Carbamate as General Base". Chemical Reviews. 98 (2): 549–562. doi:10.1021/cr970010r. PMID 11848907.
  21. ^ a b Andersson I, Knight S, Schneider G, Lindqvist Y, Lundqvist T, Brändén CI, Lorimer GH (1989). "Crystal structure of the active site of ribulose-bisphosphate carboxylase". Nature. 337 (6204): 229–234. Bibcode:1989Natur.337..229A. doi:10.1038/337229a0. S2CID 4370073.
  22. ^ a b Hartman FC, Harpel MR (1994). "Structure, function, regulation, and assembly of D-ribulose-1,5-bisphosphate carboxylase/oxygenase". Annual Review of Biochemistry. 63: 197–234. doi:10.1146/annurev.bi.63.070194.001213. PMID 7979237.
  23. ^ a b Taylor TC, Andersson I (January 1997). "The structure of the complex between rubisco and its natural substrate ribulose 1,5-bisphosphate". Journal of Molecular Biology. 265 (4): 432–444. doi:10.1006/jmbi.1996.0738. PMID 9034362.
  24. ^ Pearce FG (November 2006). "Catalytic by-product formation and ligand binding by ribulose bisphosphate carboxylases from different phylogenies". The Biochemical Journal. 399 (3): 525–534. doi:10.1042/BJ20060430. PMC 1615894. PMID 16822231.
  25. ^ Ellis RJ (January 2010). "Biochemistry: Tackling unintelligent design". Nature. 463 (7278): 164–165. Bibcode:2010Natur.463..164E. doi:10.1038/463164a. PMID 20075906. S2CID 205052478.
  26. ^ Portis AR (2003). "Rubisco activase - Rubisco's catalytic chaperone". Photosynthesis Research. 75 (1): 11–27. doi:10.1023/A:1022458108678. PMID 16245090. S2CID 2632.
  27. ^ Jin SH, Jiang DA, Li XQ, Sun JW (August 2004). "Characteristics of photosynthesis in rice plants transformed with an antisense Rubisco activase gene". Journal of Zhejiang University Science. 5 (8): 897–899. doi:10.1631/jzus.2004.0897. PMID 15236471. S2CID 1496584.
  28. ^ Andralojc PJ, Dawson GW, Parry MA, Keys AJ (December 1994). "Incorporation of carbon from photosynthetic products into 2-carboxyarabinitol-1-phosphate and 2-carboxyarabinitol". The Biochemical Journal. 304 (3): 781–786. doi:10.1042/bj3040781. PMC 1137402. PMID 7818481.
  29. ^ Khan S, Andralojc PJ, Lea PJ, Parry MA (December 1999). "2'-carboxy-D-arabitinol 1-phosphate protects ribulose 1, 5-bisphosphate carboxylase/oxygenase against proteolytic breakdown". European Journal of Biochemistry. 266 (3): 840–847. doi:10.1046/j.1432-1327.1999.00913.x. PMID 10583377.
  30. ^ Salvucci ME, Osteryoung KW, Crafts-Brandner SJ, Vierling E (November 2001). "Exceptional sensitivity of Rubisco activase to thermal denaturation in vitro and in vivo". Plant Physiology. 127 (3): 1053–1064. doi:10.1104/pp.010357. PMC 129275. PMID 11706186.
  31. ^ Crafts-Brandner SJ, Salvucci ME (November 2000). "Rubisco activase constrains the photosynthetic potential of leaves at high temperature and CO2". Proceedings of the National Academy of Sciences of the United States of America. 97 (24): 13430–13435. Bibcode:2000PNAS...9713430C. doi:10.1073/pnas.230451497. PMC 27241. PMID 11069297.
  32. ^ Zhang N, Kallis RP, Ewy RG, Portis AR (March 2002). "Light modulation of Rubisco in Arabidopsis requires a capacity for redox regulation of the larger Rubisco activase isoform". Proceedings of the National Academy of Sciences of the United States of America. 99 (5): 3330–3334. Bibcode:2002PNAS...99.3330Z. doi:10.1073/pnas.042529999. PMC 122518. PMID 11854454.
  33. ^ Marcus Y, Gurevitz M (October 2000). "Activation of cyanobacterial RuBP-carboxylase/oxygenase is facilitated by inorganic phosphate via two independent mechanisms". European Journal of Biochemistry. 267 (19): 5995–6003. doi:10.1046/j.1432-1327.2000.01674.x. PMID 10998060.
  34. ^ Spreitzer RJ, Salvucci ME (2002). "Rubisco: structure, regulatory interactions, and possibilities for a better enzyme". Annual Review of Plant Biology. 53: 449–475. doi:10.1146/annurev.arplant.53.100301.135233. PMID 12221984. S2CID 9387705.
  35. ^ Timmer J (7 December 2017). "We may now be able to engineer the most important lousy enzyme on the planet". Ars Technica. Retrieved 5 January 2019.
  36. ^ Timmer J (3 January 2019). "Fixing photosynthesis by engineering it to recycle a toxic mistake". Ars Technica. Retrieved 5 January 2019.
  37. ^ a b South PF, Cavanagh AP, Liu HW, Ort DR (January 2019). "Synthetic glycolate metabolism pathways stimulate crop growth and productivity in the field". Science. 363 (6422): eaat9077. doi:10.1126/science.aat9077. PMC 7745124. PMID 30606819.
  38. ^ a b Furbank RT, Quick WP, Sirault XR (2015). "Improving photosynthesis and yield potential in cereal crops by targeted genetic manipulation: Prospects, progress and challenges". Field Crops Research. 182: 19–29. doi:10.1016/j.fcr.2015.04.009.
  39. ^ a b Parry MA, Andralojc PJ, Mitchell RA, Madgwick PJ, Keys AJ (May 2003). "Manipulation of Rubisco: the amount, activity, function and regulation". Journal of Experimental Botany. 54 (386): 1321–1333. doi:10.1093/jxb/erg141. PMID 12709478.
  40. ^ Ogbaga CC, Stepien P, Athar HU, Ashraf M (June 2018). "Engineering Rubisco activase from thermophilic cyanobacteria into high-temperature sensitive plants". Critical Reviews in Biotechnology. 38 (4): 559–572. doi:10.1080/07388551.2017.1378998. PMID 28937283. S2CID 4191791.
  41. ^ Whitney SM, Sharwood RE, Orr D, White SJ, Alonso H, Galmés J (August 2011). "Isoleucine 309 acts as a C4 catalytic switch that increases ribulose-1,5-bisphosphate carboxylase/oxygenase (rubisco) carboxylation rate in Flaveria". Proceedings of the National Academy of Sciences of the United States of America. 108 (35): 14688–14693. Bibcode:2011PNAS..10814688W. doi:10.1073/pnas.1109503108. PMC 3167554. PMID 21849620.
  42. ^ Ishikawa C, Hatanaka T, Misoo S, Miyake C, Fukayama H (July 2011). "Functional incorporation of sorghum small subunit increases the catalytic turnover rate of Rubisco in transgenic rice". Plant Physiology. 156 (3): 1603–1611. doi:10.1104/pp.111.177030. PMC 3135941. PMID 21562335.
  43. ^ Stracquadanio G, Umeton R, Papini A, Lio P, Nicosia G (2010). "Analysis and Optimization of C3 Photosynthetic Carbon Metabolism". 2010 IEEE International Conference on BioInformatics and BioEngineering. Philadelphia, PA, USA: IEEE. pp. 44–51. doi:10.1109/BIBE.2010.17. hdl:1721.1/101094. ISBN 978-1-4244-7494-3. S2CID 5568464.
  44. ^ Whitney SM, Andrews TJ (December 2001). "Plastome-encoded bacterial ribulose-1,5-bisphosphate carboxylase/oxygenase (RubisCO) supports photosynthesis and growth in tobacco". Proceedings of the National Academy of Sciences of the United States of America. 98 (25): 14738–14743. Bibcode:2001PNAS...9814738W. doi:10.1073/pnas.261417298. PMC 64751. PMID 11724961.
  45. ^ John Andrews T, Whitney SM (June 2003). "Manipulating ribulose bisphosphate carboxylase/oxygenase in the chloroplasts of higher plants". Archives of Biochemistry and Biophysics. 414 (2): 159–169. doi:10.1016/S0003-9861(03)00100-0. PMID 12781767.
  46. ^ Lin MT, Occhialini A, Andralojc PJ, Parry MA, Hanson MR (September 2014). "A faster Rubisco with potential to increase photosynthesis in crops". Nature. 513 (7519): 547–550. Bibcode:2014Natur.513..547L. doi:10.1038/nature13776. PMC 4176977. PMID 25231869.
  47. ^ Tcherkez GG, Farquhar GD, Andrews TJ (May 2006). "Despite slow catalysis and confused substrate specificity, all ribulose bisphosphate carboxylases may be nearly perfectly optimized". Proceedings of the National Academy of Sciences of the United States of America. 103 (19): 7246–7251. Bibcode:2006PNAS..103.7246T. doi:10.1073/pnas.0600605103. PMC 1464328. PMID 16641091.
  48. ^ Igamberdiev AU (2015). "Control of Rubisco function via homeostatic equilibration of CO2 supply". Frontiers in Plant Science. 6: 106. doi:10.3389/fpls.2015.00106. PMC 4341507. PMID 25767475.
  49. ^ Igamberdiev AU, Lea PJ (February 2006). "Land plants equilibrate O2 and CO2 concentrations in the atmosphere". Photosynthesis Research. 87 (2): 177–194. Bibcode:2006PhoRe..87..177I. doi:10.1007/s11120-005-8388-2. PMID 16432665. S2CID 10709679.
  50. ^ Bracher A, Whitney SM, Hartl FU, Hayer-Hartl M (April 2017). "Biogenesis and Metabolic Maintenance of Rubisco". Annual Review of Plant Biology. 68: 29–60. doi:10.1146/annurev-arplant-043015-111633. PMID 28125284.
  51. ^ Sjuts I, Soll J, Bölter B (2017). "Import of Soluble Proteins into Chloroplasts and Potential Regulatory Mechanisms". Frontiers in Plant Science. 8: 168. doi:10.3389/fpls.2017.00168. PMC 5296341. PMID 28228773.
  52. ^ Aigner H, Wilson RH, Bracher A, Calisse L, Bhat JY, Hartl FU, Hayer-Hartl M (December 2017). "Plant RuBisCo assembly in E. coli with five chloroplast chaperones including BSD2". Science. 358 (6368): 1272–1278. Bibcode:2017Sci...358.1272A. doi:10.1126/science.aap9221. hdl:11858/00-001M-0000-002E-8B4D-B. PMID 29217567.
  53. ^ a b Heazlewood J (2012). Proteomic applications in biology. New York: InTech Manhattan. ISBN 978-953-307-613-3.
  54. ^ Gupta R, Kim ST (2015). "Depletion of RuBisCO Protein Using the Protamine Sulfate Precipitation Method". Proteomic Profiling. Methods in Molecular Biology. Vol. 1295. New York, NY: Humana Press. pp. 225–33. doi:10.1007/978-1-4939-2550-6_17. ISBN 978-1-4939-2549-0. PMID 25820725.
  55. ^ Krishnan HB, Natarajan SS (December 2009). "A rapid method for depletion of Rubisco from soybean (Glycine max) leaf for proteomic analysis of lower abundance proteins". Phytochemistry. 70 (17–18): 1958–1964. Bibcode:2009PChem..70.1958K. doi:10.1016/j.phytochem.2009.08.020. PMID 19766275.
  56. ^ Kim ST, Cho KS, Jang YS, Kang KY (June 2001). "Two-dimensional electrophoretic analysis of rice proteins by polyethylene glycol fractionation for protein arrays". Electrophoresis. 22 (10): 2103–2109. doi:10.1002/1522-2683(200106)22:10<2103::aid-elps2103>3.0.co;2-w. PMID 11465512. S2CID 38878805.
  57. ^ Xi J, Wang X, Li S, Zhou X, Yue L, Fan J, Hao D (November 2006). "Polyethylene glycol fractionation improved detection of low-abundant proteins by two-dimensional electrophoresis analysis of plant proteome". Phytochemistry. 67 (21): 2341–2348. Bibcode:2006PChem..67.2341X. doi:10.1016/j.phytochem.2006.08.005. PMID 16973185.
  58. ^ Cellar NA, Kuppannan K, Langhorst ML, Ni W, Xu P, Young SA (January 2008). "Cross species applicability of abundant protein depletion columns for ribulose-1,5-bisphosphate carboxylase/oxygenase". Journal of Chromatography. B, Analytical Technologies in the Biomedical and Life Sciences. 861 (1): 29–39. doi:10.1016/j.jchromb.2007.11.024. PMID 18063427.
  59. ^ Agrawal GK, Jwa NS, Rakwal R (February 2009). "Rice proteomics: ending phase I and the beginning of phase II". Proteomics. 9 (4): 935–963. doi:10.1002/pmic.200800594. PMID 19212951. S2CID 2455432.
  60. ^ Cho JH, Hwang H, Cho MH, Kwon YK, Jeon JS, Bhoo SH, Hahn TR (July 2008). "The effect of DTT in protein preparations for proteomic analysis: Removal of a highly abundant plant enzyme, ribulose bisphosphate carboxylase/oxygenase". Journal of Plant Biology. 51 (4): 297–301. Bibcode:2008JPBio..51..297C. doi:10.1007/BF03036130. ISSN 1226-9239. S2CID 23636617.
  61. ^ Chase MW, Soltis DE, Olmstead RG, Morgan D, Les DH, Mishler BD, et al. (1993). "Phylogenetics of Seed Plants: An Analysis of Nucleotide Sequences from the Plastid Gene rbcL" (PDF). Annals of the Missouri Botanical Garden. 80 (3): 528–580. doi:10.2307/2399846. hdl:1969.1/179875. JSTOR 2399846.
  62. ^ Ashida H, Saito Y, Nakano T, Tandeau de Marsac N, Sekowska A, Danchin A, Yokota A (19 June 2007). "RuBisCO-like proteins as the enolase enzyme in the methionine salvage pathway: functional and evolutionary relationships between RuBisCO-like proteins and photosynthetic RuBisCO". Journal of Experimental Botany. 59 (7): 1543–1554. doi:10.1093/jxb/ern104. PMID 18403380.
  63. ^ Schulz, L; Guo, Z; Zarzycki, J; Steinchen, W; Schuller, JM; Heimerl, T; Prinz, S; Mueller-Cajar, O; Erb, TJ; Hochberg, GKA (2022-10-14). "Evolution of increased complexity and specificity at the dawn of form I Rubiscos". Science. 378 (6616): 155–160. Bibcode:2022Sci...378..155S. doi:10.1126/science.abq1416. PMID 36227987. S2CID 252897276.
  64. ^ Sage RF, Sage TL, Kocacinar F (2012). "Photorespiration and the evolution of C4 photosynthesis". Annual Review of Plant Biology. 63: 19–47. doi:10.1146/annurev-arplant-042811-105511. PMID 22404472. S2CID 24199852.
  65. ^ a b Studer RA, Christin PA, Williams MA, Orengo CA (February 2014). "Stability-activity tradeoffs constrain the adaptive evolution of RubisCO". Proceedings of the National Academy of Sciences of the United States of America. 111 (6): 2223–2228. Bibcode:2014PNAS..111.2223S. doi:10.1073/pnas.1310811111. PMC 3926066. PMID 24469821.
  66. ^ Wildman SG (2002). "Along the trail from Fraction I protein to Rubisco (ribulose bisphosphate carboxylase-oxygenase)". Photosynthesis Research. 73 (1–3): 243–250. doi:10.1023/A:1020467601966. PMID 16245127. S2CID 7622999.
  67. ^ Portis AR, Parry MA (October 2007). "Discoveries in Rubisco (Ribulose 1,5-bisphosphate carboxylase/oxygenase): a historical perspective". Photosynthesis Research. 94 (1): 121–143. Bibcode:2007PhoRe..94..121P. doi:10.1007/s11120-007-9225-6. PMID 17665149. S2CID 39767233.
 
Figure 3. In this figure, each protein chain in the (LS)2 complex is given its own color for easy identification.

Further reading edit

  • Marcus Y, Altman-Gueta H, Finkler A, Gurevitz M (June 2005). "Mutagenesis at two distinct phosphate-binding sites unravels their differential roles in regulation of Rubisco activation and catalysis". Journal of Bacteriology. 187 (12): 4222–4228. doi:10.1128/JB.187.12.4222-4228.2005. PMC 1151729. PMID 15937184.
  • Sugawara H, Yamamoto H, Shibata N, Inoue T, Okada S, Miyake C, et al. (May 1999). "Crystal structure of carboxylase reaction-oriented ribulose 1, 5-bisphosphate carboxylase/oxygenase from a thermophilic red alga, Galdieria partita". The Journal of Biological Chemistry. 274 (22): 15655–15661. doi:10.1074/jbc.274.22.15655. PMID 10336462.

External links edit

  • Gerritsen VB (September 2003). "The Plant Kingdom's sloth". Protein Spotlight. Swiss Institute of Bioinformatics (SIB). Rubisco plods along at a mere three molecules per second... To bypass such slothfulness, plants synthesize a gross amount of Rubisco, sometimes up to 50% of their total protein content!

February 15, 2024
rubisco, ribulose, bisphosphate, carboxylase, oxygenase, commonly, known, abbreviations, rubisco, rubisco, rubpcase, rubpco, enzyme, involved, light, independent, dark, part, photosynthesis, including, carbon, fixation, which, atmospheric, carbon, dioxide, con. Ribulose 1 5 bisphosphate carboxylase oxygenase commonly known by the abbreviations RuBisCo rubisco 1 RuBPCase 2 or RuBPco 3 is an enzyme EC 4 1 1 39 involved in light independent or dark part of photosynthesis including the carbon fixation by which atmospheric carbon dioxide is converted by plants and other photosynthetic organisms to energy rich molecules such as glucose It emerged approximately four billion years ago in primordial metabolism prior to the presence of oxygen on Earth 4 It is probably the most abundant enzyme on Earth In chemical terms it catalyzes the carboxylation of ribulose 1 5 bisphosphate also known as RuBP 5 6 7 Ribulose 1 5 bisphosphate carboxylase oxygenaseA 3d depiction of the activated RuBisCO from spinach in open form with active site accessible The active site Lys175 residues are marked in pink and a close up of the residue is provided to the right for one of the monomers composing the enzyme IdentifiersEC no 4 1 1 39CAS no 9027 23 0DatabasesIntEnzIntEnz viewBRENDABRENDA entryExPASyNiceZyme viewKEGGKEGG entryMetaCycmetabolic pathwayPRIAMprofilePDB structuresRCSB PDB PDBe PDBsumGene OntologyAmiGO QuickGOSearchPMCarticlesPubMedarticlesNCBIproteins Contents 1 Alternative carbon fixation pathways 2 Structure 3 Enzymatic activity 3 1 Substrates 3 1 1 Binding RuBP 3 1 2 Enolisation 3 1 3 Carboxylation 3 1 4 C C bond cleavage 3 2 Products 3 3 Rate of enzymatic activity 3 3 1 By ions 3 3 2 By RuBisCO activase 3 3 3 By activase 3 3 4 By phosphate 3 3 5 By carbon dioxide 4 Genetic engineering 4 1 Mutagenesis in plants 4 2 Expression in bacterial hosts 5 Depletion in proteomic studies 6 Evolution of RuBisCO 6 1 Phylogenetic studies 6 2 Origin 6 3 C4 7 History of the term 8 See also 9 References 10 Further reading 11 External linksAlternative carbon fixation pathways editRuBisCO is important biologically because it catalyzes the primary chemical reaction by which inorganic carbon enters the biosphere While many autotrophic bacteria and archaea fix carbon via the reductive acetyl CoA pathway the 3 hydroxypropionate cycle or the reverse Krebs cycle these pathways are relatively small contributors to global carbon fixation compared to that catalyzed by RuBisCO Phosphoenolpyruvate carboxylase unlike RuBisCO only temporarily fixes carbon Reflecting its importance RuBisCO is the most abundant protein in leaves accounting for 50 of soluble leaf protein in C3 plants 20 30 of total leaf nitrogen and 30 of soluble leaf protein in C4 plants 5 9 of total leaf nitrogen 7 Given its important role in the biosphere the genetic engineering of RuBisCO in crops is of continuing interest see below Structure edit nbsp Active site of RuBisCO of Galdieria sulphuraria with CO2 Residues involved in both the active site and stabilizing CO2 for enzyme catalysis are shown in color and labeled Distances of the hydrogen bonding interactions are shown in angstroms Mg2 ion green sphere is shown coordinated to CO2 and is followed by three water molecules red spheres All other residues are placed in grayscale nbsp Location of the rbcL gene in the chloroplast genome of Arabidopsis thaliana positions ca 55 56 4 kb rbcL is one of the 21 protein coding genes involved in photosynthesis green boxes In plants algae cyanobacteria and phototrophic and chemoautotrophic Pseudomonadota formerly proteobacteria the enzyme usually consists of two types of protein subunit called the large chain L about 55 000 Da and the small chain S about 13 000 Da The large chain gene rbcL is encoded by the chloroplast DNA in plants 8 There are typically several related small chain genes in the nucleus of plant cells and the small chains are imported to the stromal compartment of chloroplasts from the cytosol by crossing the outer chloroplast membrane 6 9 The enzymatically active substrate ribulose 1 5 bisphosphate binding sites are located in the large chains that form dimers in which amino acids from each large chain contribute to the binding sites A total of eight large chains four dimers and eight small chains assemble into a larger complex of about 540 000 Da 10 In some Pseudomonadota and dinoflagellates enzymes consisting of only large subunits have been found a Magnesium ions Mg2 are needed for enzymatic activity Correct positioning of Mg2 in the active site of the enzyme involves addition of an activating carbon dioxide molecule CO2 to a lysine in the active site forming a carbamate 12 Mg2 operates by driving deprotonation of the Lys210 residue causing the Lys residue to rotate by 120 degrees to the trans conformer decreasing the distance between the nitrogen of Lys and the carbon of CO2 The close proximity allows for the formation of a covalent bond resulting in the carbamate 13 Mg2 is first enabled to bind to the active site by the rotation of His335 to an alternate conformation Mg2 is then coordinated by the His residues of the active site His300 His302 His335 and is partially neutralized by the coordination of three water molecules and their conversion to OH 13 This coordination results in an unstable complex but produces a favorable environment for the binding of Mg2 Formation of the carbamate is favored by an alkaline pH The pH and the concentration of magnesium ions in the fluid compartment in plants the stroma of the chloroplast increases in the light The role of changing pH and magnesium ion levels in the regulation of RuBisCO enzyme activity is discussed below Once the carbamate is formed His335 finalizes the activation by returning to its initial position through thermal fluctuation 13 RuBisCO large chain catalytic domainIdentifiersSymbolRuBisCO largePfamPF00016InterProIPR000685PROSITEPDOC00142SCOP23rub SCOPe SUPFAMCDDcd08148Available protein structures Pfam structures ECOD PDBRCSB PDB PDBe PDBjPDBsumstructure summaryPDB1aa1 1aus 1bwv 1bxn 1ej7 1geh 1gk8 1ir1 1ir2 1iwa 1rba 1rbl 1rbo 1rco 1rcx 1rld 1rsc 1rus 1rxo 1svd 1tel 1upm 1upp 1uw9 1uwa 1uzd 1uzh 1wdd 1ykw 2cwx 2cxe 2d69 2qyg 2rus 2v63 2v67 2v68 2v69 2v6a 3rub 4rub 5rub 8ruc 9rub RuBisCO N terminal domainIdentifiersSymbolRuBisCO large NPfamPF02788InterProIPR017444SCOP23rub SCOPe SUPFAMAvailable protein structures Pfam structures ECOD PDBRCSB PDB PDBe PDBjPDBsumstructure summaryPDB1aa1 1aus 1bwv 1bxn 1ej7 1geh 1gk8 1ir1 1ir2 1iwa 1rba 1rbl 1rbo 1rco 1rcx 1rld 1rsc 1rus 1rxo 1svd 1tel 1upm 1upp 1uw9 1uwa 1uzd 1uzh 1wdd 1ykw 2cwx 2cxe 2d69 2qyg 2rus 2v63 2v67 2v68 2v69 2v6a 3rub 4rub 5rub 8ruc 9rub RuBisCO small chainIdentifiersSymbolRuBisCO smallPfamPF00101InterProIPR000894SCOP23rub SCOPe SUPFAMCDDcd03527Available protein structures Pfam structures ECOD PDBRCSB PDB PDBe PDBjPDBsumstructure summaryPDB1aa1 1aus 1bwv 1bxn 1ej7 1gk8 1ir1 1ir2 1iwa 1rbl 1rbo 1rco 1rcx 1rlc 1rld 1rsc 1rxo 1svd 1upm 1upp 1uw9 1uwa 1uzd 1uzh 1wdd 2v63 2v67 2v68 2v69 2v6a 3rub 4rub 8ruc Enzymatic activity edit nbsp Two main reactions of RuBisCo CO2 fixation and oxygenation RuBisCO is one of many enzymes in the Calvin cycle When Rubisco facilitates the attack of CO2 at the C2 carbon of RuBP and subsequent bond cleavage between the C3 and C2 carbon 2 molecules of glycerate 3 phosphate are formed The conversion involves these steps enolisation carboxylation hydration C C bond cleavage and protonation 14 15 16 Substrates edit Substrates for RuBisCO are ribulose 1 5 bisphosphate and carbon dioxide distinct from the activating carbon dioxide RuBisCO also catalyses a reaction of ribulose 1 5 bisphosphate and molecular oxygen O2 instead of carbon dioxide CO2 17 Discriminating between the substrates CO2 and O2 is attributed to the differing interactions of the substrate s quadrupole moments and a high electrostatic field gradient 13 This gradient is established by the dimer form of the minimally active RuBisCO which with its two components provides a combination of oppositely charged domains required for the enzyme s interaction with O2 and CO2 These conditions help explain the low turnover rate found in RuBisCO In order to increase the strength of the electric field necessary for sufficient interaction with the substrates quadrupole moments the C and N terminal segments of the enzyme must be closed off allowing the active site to be isolated from the solvent and lowering the dielectric constant 18 This isolation has a significant entropic cost and results in the poor turnover rate Binding RuBP edit Carbamylation of the e amino group of Lys210 is stabilized by coordination with the Mg2 19 This reaction involves binding of the carboxylate termini of Asp203 and Glu204 to the Mg2 ion The substrate RuBP binds Mg2 displacing two of the three aquo ligands 14 20 21 Enolisation edit Enolisation of RuBP is the conversion of the keto tautomer of RuBP to an enediol ate Enolisation is initiated by deprotonation at C3 The enzyme base in this step has been debated 20 22 but the steric constraints observed in crystal structures have made Lys210 the most likely candidate 14 Specifically the carbamate oxygen on Lys210 that is not coordinated with the Mg ion deprotonates the C3 carbon of RuBP to form a 2 3 enediolate 20 21 Carboxylation edit nbsp A 3D image of the active site of spinach RuBisCO complexed with the inhibitor 2 carboxyarabinitol 1 5 bisphosphate CO2 and Mg2 PDB 1IR1 Ligand View CAP 501 A Carboxylation of the 2 3 enediolate results in the intermediate 3 keto 2 carboxyarabinitol 1 5 bisphosphate and Lys334 is positioned to facilitate the addition of the CO2 substrate as it replaces the third Mg2 coordinated water molecule and add directly to the enediol No Michaelis complex is formed in this process 14 22 Hydration of this ketone results in an additional hydroxy group on C3 forming a gem diol intermediate 20 23 Carboxylation and hydration have been proposed as either a single concerted step 20 or as two sequential steps 23 Concerted mechanism is supported by the proximity of the water molecule to C3 of RuBP in multiple crystal structures Within the spinach structure other residues are well placed to aid in the hydration step as they are within hydrogen bonding distance of the water molecule 14 C C bond cleavage edit The gem diol intermediate cleaves at the C2 C3 bond to form one molecule of glycerate 3 phosphate and a negatively charged carboxylate 14 Stereo specific protonation of C2 of this carbanion results in another molecule of glycerate 3 phosphate This step is thought to be facilitated by Lys175 or potentially the carbamylated Lys210 14 Products edit When carbon dioxide is the substrate the product of the carboxylase reaction is an unstable six carbon phosphorylated intermediate known as 3 keto 2 carboxyarabinitol 1 5 bisphosphate which decays rapidly into two molecules of glycerate 3 phosphate This product also known as 3 phosphoglycerate can be used to produce larger molecules such as glucose When molecular oxygen is the substrate the products of the oxygenase reaction are phosphoglycolate and 3 phosphoglycerate Phosphoglycolate is recycled through a sequence of reactions called photorespiration which involves enzymes and cytochromes located in the mitochondria and peroxisomes this is a case of metabolite repair In this process two molecules of phosphoglycolate are converted to one molecule of carbon dioxide and one molecule of 3 phosphoglycerate which can reenter the Calvin cycle Some of the phosphoglycolate entering this pathway can be retained by plants to produce other molecules such as glycine At ambient levels of carbon dioxide and oxygen the ratio of the reactions is about 4 to 1 which results in a net carbon dioxide fixation of only 3 5 Thus the inability of the enzyme to prevent the reaction with oxygen greatly reduces the photosynthetic capacity of many plants Some plants many algae and photosynthetic bacteria have overcome this limitation by devising means to increase the concentration of carbon dioxide around the enzyme including C4 carbon fixation crassulacean acid metabolism and the use of pyrenoid Rubisco side activities can lead to useless or inhibitory by products Important inhibitory by products include xylulose 1 5 bisphosphate and glycero 2 3 pentodiulose 1 5 bisphosphate both caused by misfires halfway in the enolisation carboxylation reaction In higher plants this process causes RuBisCO self inhibition which can be triggered by saturating CO2 and RuBP concentrations and solved by Rubisco activase see below 24 Rate of enzymatic activity edit nbsp Overview of the Calvin cycle and carbon fixation Some enzymes can carry out thousands of chemical reactions each second However RuBisCO is slow fixing only 3 10 carbon dioxide molecules each second per molecule of enzyme 25 The reaction catalyzed by RuBisCO is thus the primary rate limiting factor of the Calvin cycle during the day Nevertheless under most conditions and when light is not otherwise limiting photosynthesis the speed of RuBisCO responds positively to increasing carbon dioxide concentration RuBisCO is usually only active during the day as ribulose 1 5 bisphosphate is not regenerated in the dark This is due to the regulation of several other enzymes in the Calvin cycle In addition the activity of RuBisCO is coordinated with that of the other enzymes of the Calvin cycle in several other ways By ions edit Upon illumination of the chloroplasts the pH of the stroma rises from 7 0 to 8 0 because of the proton hydrogen ion H gradient created across the thylakoid membrane The movement of protons into thylakoids is driven by light and is fundamental to ATP synthesis in chloroplasts Further reading Photosynthetic reaction centre Light dependent reactions To balance ion potential across the membrane magnesium ions Mg2 move out of the thylakoids in response increasing the concentration of magnesium in the stroma of the chloroplasts RuBisCO has a high optimal pH can be gt 9 0 depending on the magnesium ion concentration and thus becomes activated by the introduction of carbon dioxide and magnesium to the active sites as described above By RuBisCO activase edit In plants and some algae another enzyme RuBisCO activase Rca GO 0046863 P10896 is required to allow the rapid formation of the critical carbamate in the active site of RuBisCO 26 27 This is required because ribulose 1 5 bisphosphate RuBP binds more strongly to the active sites of RuBisCO when excess carbamate is present preventing processes from moving forward In the light RuBisCO activase promotes the release of the inhibitory or in some views storage RuBP from the catalytic sites of RuBisCO Activase is also required in some plants e g tobacco and many beans because in darkness RuBisCO is inhibited or protected from hydrolysis by a competitive inhibitor synthesized by these plants a substrate analog 2 carboxy D arabitinol 1 phosphate CA1P 28 CA1P binds tightly to the active site of carbamylated RuBisCO and inhibits catalytic activity to an even greater extent CA1P has also been shown to keep RuBisCO in a conformation that is protected from proteolysis 29 In the light RuBisCO activase also promotes the release of CA1P from the catalytic sites After the CA1P is released from RuBisCO it is rapidly converted to a non inhibitory form by a light activated CA1P phosphatase Even without these strong inhibitors once every several hundred reactions the normal reactions with carbon dioxide or oxygen are not completed other inhibitory substrate analogs are still formed in the active site Once again RuBisCO activase can promote the release of these analogs from the catalytic sites and maintain the enzyme in a catalytically active form However at high temperatures RuBisCO activase aggregates and can no longer activate RuBisCO This contributes to the decreased carboxylating capacity observed during heat stress 30 31 By activase edit The removal of the inhibitory RuBP CA1P and the other inhibitory substrate analogs by activase requires the consumption of ATP This reaction is inhibited by the presence of ADP and thus activase activity depends on the ratio of these compounds in the chloroplast stroma Furthermore in most plants the sensitivity of activase to the ratio of ATP ADP is modified by the stromal reduction oxidation redox state through another small regulatory protein thioredoxin In this manner the activity of activase and the activation state of RuBisCO can be modulated in response to light intensity and thus the rate of formation of the ribulose 1 5 bisphosphate substrate 32 By phosphate edit In cyanobacteria inorganic phosphate Pi also participates in the co ordinated regulation of photosynthesis Pi binds to the RuBisCO active site and to another site on the large chain where it can influence transitions between activated and less active conformations of the enzyme In this way activation of bacterial RuBisCO might be particularly sensitive to Pi levels which might cause it to act in a similar way to how RuBisCO activase functions in higher plants 33 By carbon dioxide edit Since carbon dioxide and oxygen compete at the active site of RuBisCO carbon fixation by RuBisCO can be enhanced by increasing the carbon dioxide level in the compartment containing RuBisCO chloroplast stroma Several times during the evolution of plants mechanisms have evolved for increasing the level of carbon dioxide in the stroma see C4 carbon fixation The use of oxygen as a substrate appears to be a puzzling process since it seems to throw away captured energy However it may be a mechanism for preventing carbohydrate overload during periods of high light flux This weakness in the enzyme is the cause of photorespiration such that healthy leaves in bright light may have zero net carbon fixation when the ratio of O2 to CO2 available to RuBisCO shifts too far towards oxygen This phenomenon is primarily temperature dependent high temperatures can decrease the concentration of CO2 dissolved in the moisture of leaf tissues This phenomenon is also related to water stress since plant leaves are evaporatively cooled limited water causes high leaf temperatures C4 plants use the enzyme PEP carboxylase initially which has a higher affinity for CO2 The process first makes a 4 carbon intermediate compound hence the name C4 plants which is shuttled into a site of C3 photosynthesis then decarboxylated releasing CO2 to boost the concentration of CO2 Crassulacean acid metabolism CAM plants keep their stomata closed during the day which conserves water but prevents the light independent reactions a k a the Calvin Cycle from taking place since these reactions require CO2 to pass by gas exchange through these openings Evaporation through the upper side of a leaf is prevented by a layer of wax Genetic engineering editSince RuBisCO is often rate limiting for photosynthesis in plants it may be possible to improve photosynthetic efficiency by modifying RuBisCO genes in plants to increase catalytic activity and or decrease oxygenation rates 34 35 36 37 This could improve sequestration of CO2 and be a strategy to increase crop yields 38 Approaches under investigation include transferring RuBisCO genes from one organism into another organism engineering Rubisco activase from thermophilic cyanobacteria into temperature sensitive plants increasing the level of expression of RuBisCO subunits expressing RuBisCO small chains from the chloroplast DNA and altering RuBisCO genes to increase specificity for carbon dioxide or otherwise increase the rate of carbon fixation 39 40 Mutagenesis in plants edit In general site directed mutagenesis of RuBisCO has been mostly unsuccessful 38 though mutated forms of the protein have been achieved in tobacco plants with subunit C4 species 41 and a RuBisCO with more C4 like kinetic characteristics have been attained in rice via nuclear transformation 42 Robust and reliable engineering for yield of RuBisCO and other enzymes in the C3 cycle was shown to be possible 43 and it was first achieved in 2019 through a synthetic biology approach 37 One avenue is to introduce RuBisCO variants with naturally high specificity values such as the ones from the red alga Galdieria partita into plants This may improve the photosynthetic efficiency of crop plants although possible negative impacts have yet to be studied 44 Advances in this area include the replacement of the tobacco enzyme with that of the purple photosynthetic bacterium Rhodospirillum rubrum 45 In 2014 two transplastomic tobacco lines with functional RuBisCO from the cyanobacterium Synechococcus elongatus PCC7942 Se7942 were created by replacing the RuBisCO with the large and small subunit genes of the Se7942 enzyme in combination with either the corresponding Se7942 assembly chaperone RbcX or an internal carboxysomal protein CcmM35 Both mutants had increased CO2 fixation rates when measured as carbon molecules per RuBisCO However the mutant plants grew more slowly than wild type 46 A recent theory explores the trade off between the relative specificity i e ability to favour CO2 fixation over O2 incorporation which leads to the energy wasteful process of photorespiration and the rate at which product is formed The authors conclude that RuBisCO may actually have evolved to reach a point of near perfection in many plants with widely varying substrate availabilities and environmental conditions reaching a compromise between specificity and reaction rate 47 It has been also suggested that the oxygenase reaction of RuBisCO prevents CO2 depletion near its active sites and provides the maintenance of the chloroplast redox state 48 Since photosynthesis is the single most effective natural regulator of carbon dioxide in the Earth s atmosphere 49 a biochemical model of RuBisCO reaction is used as the core module of climate change models Thus a correct model of this reaction is essential to the basic understanding of the relations and interactions of environmental models Expression in bacterial hosts edit There currently are very few effective methods for expressing functional plant Rubisco in bacterial hosts for genetic manipulation studies This is largely due to Rubisco s requirement of complex cellular machinery for its biogenesis and metabolic maintenance including the nuclear encoded RbcS subunits which are typically imported into chloroplasts as unfolded proteins 50 51 Furthermore sufficient expression and interaction with Rubisco activase are major challenges as well 39 One successful method for expression of Rubisco in E coli involves the co expression of multiple chloroplast chaperones though this has only been shown for Arabidopsis thaliana Rubisco 52 Depletion in proteomic studies editDue to its high abundance in plants generally 40 of the total protein content RuBisCO often impedes analysis of important signaling proteins such as transcription factors kinases and regulatory proteins found in lower abundance 10 100 molecules per cell within plants 53 For example using mass spectrometry on plant protein mixtures would result in multiple intense RuBisCO subunit peaks that interfere and hide those of other proteins Recently one efficient method for precipitating out RuBisCO involves the usage of protamine sulfate solution 54 Other existing methods for depleting RuBisCO and studying lower abundance proteins include fractionation techniques with calcium and phytate 55 gel electrophoresis with polyethylene glycol 56 57 affinity chromatography 58 59 and aggregation using DTT 60 though these methods are more time consuming and less efficient when compared to protamine sulfate precipitation 53 Evolution of RuBisCO editPhylogenetic studies edit The chloroplast gene rbcL which codes for the large subunit of RuBisCO has been widely used as an appropriate locus for analysis of phylogenetics in plant taxonomy 61 Origin edit This section is missing information about explanation of the large only oligomeric forms up to L2 5 explanation of what the small subunit probably does improve CO2 O2 discrimination maybe a a href Template External image html class mw redirect title Template External image external image a pointing to the MotM and Erb 2018 pics Please expand the section to include this information Further details may exist on the talk page March 2022 Non carbon fixing proteins similar to RuBisCO termed RuBisCO like proteins RLPs are also found in the wild in organisms as common as Bacillus subtilis This bacterium has a rbcL like protein with a 2 3 diketo 5 methylthiopentyl 1 phosphate enolase function part of the methionine salvage pathway 62 Later identifications found functionally divergent examples dispersed all over bacteria and archaea as well as transitionary enzymes performing both RLP type enolase and RuBisCO functions It is now believed that the current RuBisCO evolved from a dimeric RLP ancestor acquiring its carboxylase function first before further oligomerizing and then recruiting the small subunit to form the familiar modern enzyme 15 The small subunit probably first evolved in anaerobic and thermophilic organisms where it enabled RuBisCO to catalyze its reaction at higher temperatures 63 In addition to its effect on stabilizing catalysis it enabled the evolution of higher specificities for CO2 over O2 by modulating the effect that substitutions within RuBisCO have on enzymatic function Substitutions that do not have an effect without the small subunit suddenly become beneficial when it is bound Furthermore the small subunit enabled the accumulation of substitutions that are only tolerated in its presence Accumulation of such substitutions leads to a strict dependence on the small subunit which is observed in extant Rubiscos that bind a small subunit C4 edit With the mass convergent evolution of the C4 fixation pathway in a diversity of plant lineages ancestral C3 type RuBisCO evolved to have faster turnover of CO2 in exchange for lower specificity as a result of the greater localization of CO2 from the mesophyll cells into the bundle sheath cells 64 This was achieved through enhancement of conformational flexibility of the open closed transition in the Calvin cycle Laboratory based phylogenetic studies have shown that this evolution was constrained by the trade off between stability and activity brought about by the series of necessary mutations for C4 RuBisCO 65 Moreover in order to sustain the destabilizing mutations the evolution to C4 RuBisCO was preceded by a period in which mutations granted the enzyme increased stability establishing a buffer to sustain and maintain the mutations required for C4 RuBisCO To assist with this buffering process the newly evolved enzyme was found to have further developed a series of stabilizing mutations While RuBisCO has always been accumulating new mutations most of these mutations that have survived have not had significant effects on protein stability The destabilizing C4 mutations on RuBisCO has been sustained by environmental pressures such as low CO2 concentrations requiring a sacrifice of stability for new adaptive functions 65 History of the term editThe term RuBisCO was coined humorously in 1979 by David Eisenberg at a seminar honouring the retirement of the early prominent RuBisCO researcher Sam Wildman and also alluded to the snack food trade name Nabisco in reference to Wildman s attempts to create an edible protein supplement from tobacco leaves 66 67 The capitalization of the name has been long debated It can be capitalized for each letter of the full name Ribulose 1 5 bisphosphate carboxylase oxygenase but it has also been argued that is should all be in lower case rubisco similar to other terms like scuba or laser 1 See also editCarbon cycle Photorespiration Pyrenoid C3 carbon fixation C4 carbon fixation Crassulacean acid metabolism CAM photosynthesis CarboxysomeReferences edit The structure of RuBisCO from the photosynthetic bacterium Rhodospirillum rubrum has been determined by X ray crystallography see PDB 9RUB A comparison of the structures of eukaryotic and bacterial RuBisCO is shown in the Protein Data Bank Molecule of the Month 11 11 a b Sharkey TD May 2019 Discovery of the canonical Calvin Benson cycle Photosynthesis Research 140 2 235 252 Bibcode 2019PhoRe 140 235S doi 10 1007 s11120 018 0600 2 OSTI 1607740 PMID 30374727 S2CID 53092349 Nivison Helen Stocking C 1983 Ribulose Bisphosphate Carboxylase Synthesis in Barley Leaves Plant Physiology 73 4 906 911 doi 10 1104 pp 73 4 906 PMC 1066578 PMID 16663341 Machler Felix Nosberger Josef 1988 Bicarbonate Inhibits Ribulose 1 5 Bisphosphate Carboxylase Plant Physiology 88 2 462 465 doi 10 1104 pp 88 2 462 PMC 1055600 PMID 16666327 Back to the future of photosynthesis Resurrecting billon year old enzymes reveals how photosynthesis adapted to the rise of oxygen News from the Max Planck Society October 13 2022 Cooper GM 2000 10 The Chloroplast Genome The Cell A Molecular Approach 2nd ed Washington D C ASM Press ISBN 978 0 87893 106 4 one of the subunits of ribulose bisphosphate carboxylase rubisco is encoded by chloroplast DNA Rubisco is the critical enzyme that catalyzes the addition of CO2 to ribulose 1 5 bisphosphate during the Calvin cycle It is also thought to be the single most abundant protein on Earth so it is noteworthy that one of its subunits is encoded by the chloroplast genome a b Dhingra A Portis AR Daniell H April 2004 Enhanced translation of a chloroplast expressed RbcS gene restores small subunit levels and photosynthesis in nuclear RbcS antisense plants Proceedings of the National Academy of Sciences of the United States of America 101 16 6315 6320 Bibcode 2004PNAS 101 6315D doi 10 1073 pnas 0400981101 PMC 395966 PMID 15067115 Rubisco is the most prevalent enzyme on this planet accounting for 30 50 of total soluble protein in the chloroplast a b Feller U Anders I Mae T 2008 Rubiscolytics fate of Rubisco after its enzymatic function in a cell is terminated Journal of Experimental Botany 59 7 1615 1624 doi 10 1093 jxb erm242 PMID 17975207 Vitlin Gruber A Feiz L 2018 Rubisco Assembly in the Chloroplast Frontiers in Molecular Biosciences 5 24 doi 10 3389 fmolb 2018 00024 PMC 5859369 PMID 29594130 Arabidopsis thaliana has four RuBisCO small chain genes Yoon M Putterill JJ Ross GS Laing WA April 2001 Determination of the relative expression levels of rubisco small subunit genes in Arabidopsis by rapid amplification of cDNA ends Analytical Biochemistry 291 2 237 244 doi 10 1006 abio 2001 5042 PMID 11401297 Stryer L Berg JM Tymoczko JL 2002 Chapter 20 The Calvin Cycle and the Pentose Phosphate Pathway Biochemistry 5th ed San Francisco W H Freeman ISBN 978 0 7167 3051 4 Figure 20 3 Structure of Rubisco Color coded ribbon diagram Goodsell D November 2000 Rubisco Molecule of the Month RCSB PDB Research Collaboratory for Structural Bioinformatics PDB doi 10 2210 rcsb pdb mom 2000 11 Lodish H Berk A Zipursky SL Matsudaira P Baltimore D Darnell JE 2000 Molecular Cell Biology 4th ed New York W H Freeman amp Co Figure 16 48 shows a structural model of the active site including the involvement of magnesium a b c d Stec B November 2012 Structural mechanism of RuBisCO activation by carbamylation of the active site lysine Proceedings of the National Academy of Sciences of the United States of America 109 46 18785 18790 Bibcode 2012PNAS 10918785S doi 10 1073 pnas 1210754109 PMC 3503183 PMID 23112176 a b c d e f g Andersson I May 2008 Catalysis and regulation in Rubisco Journal of Experimental Botany 59 7 1555 1568 doi 10 1093 jxb ern091 PMID 18417482 a b Erb TJ Zarzycki J February 2018 A short history of RubisCO the rise and fall of Nature s predominant CO2 fixing enzyme Current Opinion in Biotechnology 49 100 107 doi 10 1016 j copbio 2017 07 017 PMC 7610757 PMID 28843191 Lundqvist T Schneider G July 1991 Crystal structure of activated ribulose 1 5 bisphosphate carboxylase complexed with its substrate ribulose 1 5 bisphosphate The Journal of Biological Chemistry 266 19 12604 12611 doi 10 1016 S0021 9258 18 98942 8 PMID 1905726 Goodsell D November 2000 Rubisco Molecule of the Month RCSB PDB Research Collaboratory for Structural Bioinformatics PDB doi 10 2210 rcsb pdb mom 2000 11 Satagopan S Spreitzer RJ July 2008 Plant like substitutions in the large subunit carboxy terminus of Chlamydomonas Rubisco increase CO2 O2 specificity BMC Plant Biology 8 85 doi 10 1186 1471 2229 8 85 PMC 2527014 PMID 18664299 Lorimer GH Miziorko HM November 1980 Carbamate formation on the epsilon amino group of a lysyl residue as the basis for the activation of ribulosebisphosphate carboxylase by CO2 and Mg2 Biochemistry 19 23 5321 5328 doi 10 1021 bi00564a027 PMID 6778504 a b c d e Cleland WW Andrews TJ Gutteridge S Hartman FC Lorimer GH April 1998 Mechanism of Rubisco The Carbamate as General Base Chemical Reviews 98 2 549 562 doi 10 1021 cr970010r PMID 11848907 a b Andersson I Knight S Schneider G Lindqvist Y Lundqvist T Branden CI Lorimer GH 1989 Crystal structure of the active site of ribulose bisphosphate carboxylase Nature 337 6204 229 234 Bibcode 1989Natur 337 229A doi 10 1038 337229a0 S2CID 4370073 a b Hartman FC Harpel MR 1994 Structure function regulation and assembly of D ribulose 1 5 bisphosphate carboxylase oxygenase Annual Review of Biochemistry 63 197 234 doi 10 1146 annurev bi 63 070194 001213 PMID 7979237 a b Taylor TC Andersson I January 1997 The structure of the complex between rubisco and its natural substrate ribulose 1 5 bisphosphate Journal of Molecular Biology 265 4 432 444 doi 10 1006 jmbi 1996 0738 PMID 9034362 Pearce FG November 2006 Catalytic by product formation and ligand binding by ribulose bisphosphate carboxylases from different phylogenies The Biochemical Journal 399 3 525 534 doi 10 1042 BJ20060430 PMC 1615894 PMID 16822231 Ellis RJ January 2010 Biochemistry Tackling unintelligent design Nature 463 7278 164 165 Bibcode 2010Natur 463 164E doi 10 1038 463164a PMID 20075906 S2CID 205052478 Portis AR 2003 Rubisco activase Rubisco s catalytic chaperone Photosynthesis Research 75 1 11 27 doi 10 1023 A 1022458108678 PMID 16245090 S2CID 2632 Jin SH Jiang DA Li XQ Sun JW August 2004 Characteristics of photosynthesis in rice plants transformed with an antisense Rubisco activase gene Journal of Zhejiang University Science 5 8 897 899 doi 10 1631 jzus 2004 0897 PMID 15236471 S2CID 1496584 Andralojc PJ Dawson GW Parry MA Keys AJ December 1994 Incorporation of carbon from photosynthetic products into 2 carboxyarabinitol 1 phosphate and 2 carboxyarabinitol The Biochemical Journal 304 3 781 786 doi 10 1042 bj3040781 PMC 1137402 PMID 7818481 Khan S Andralojc PJ Lea PJ Parry MA December 1999 2 carboxy D arabitinol 1 phosphate protects ribulose 1 5 bisphosphate carboxylase oxygenase against proteolytic breakdown European Journal of Biochemistry 266 3 840 847 doi 10 1046 j 1432 1327 1999 00913 x PMID 10583377 Salvucci ME Osteryoung KW Crafts Brandner SJ Vierling E November 2001 Exceptional sensitivity of Rubisco activase to thermal denaturation in vitro and in vivo Plant Physiology 127 3 1053 1064 doi 10 1104 pp 010357 PMC 129275 PMID 11706186 Crafts Brandner SJ Salvucci ME November 2000 Rubisco activase constrains the photosynthetic potential of leaves at high temperature and CO2 Proceedings of the National Academy of Sciences of the United States of America 97 24 13430 13435 Bibcode 2000PNAS 9713430C doi 10 1073 pnas 230451497 PMC 27241 PMID 11069297 Zhang N Kallis RP Ewy RG Portis AR March 2002 Light modulation of Rubisco in Arabidopsis requires a capacity for redox regulation of the larger Rubisco activase isoform Proceedings of the National Academy of Sciences of the United States of America 99 5 3330 3334 Bibcode 2002PNAS 99 3330Z doi 10 1073 pnas 042529999 PMC 122518 PMID 11854454 Marcus Y Gurevitz M October 2000 Activation of cyanobacterial RuBP carboxylase oxygenase is facilitated by inorganic phosphate via two independent mechanisms European Journal of Biochemistry 267 19 5995 6003 doi 10 1046 j 1432 1327 2000 01674 x PMID 10998060 Spreitzer RJ Salvucci ME 2002 Rubisco structure regulatory interactions and possibilities for a better enzyme Annual Review of Plant Biology 53 449 475 doi 10 1146 annurev arplant 53 100301 135233 PMID 12221984 S2CID 9387705 Timmer J 7 December 2017 We may now be able to engineer the most important lousy enzyme on the planet Ars Technica Retrieved 5 January 2019 Timmer J 3 January 2019 Fixing photosynthesis by engineering it to recycle a toxic mistake Ars Technica Retrieved 5 January 2019 a b South PF Cavanagh AP Liu HW Ort DR January 2019 Synthetic glycolate metabolism pathways stimulate crop growth and productivity in the field Science 363 6422 eaat9077 doi 10 1126 science aat9077 PMC 7745124 PMID 30606819 a b Furbank RT Quick WP Sirault XR 2015 Improving photosynthesis and yield potential in cereal crops by targeted genetic manipulation Prospects progress and challenges Field Crops Research 182 19 29 doi 10 1016 j fcr 2015 04 009 a b Parry MA Andralojc PJ Mitchell RA Madgwick PJ Keys AJ May 2003 Manipulation of Rubisco the amount activity function and regulation Journal of Experimental Botany 54 386 1321 1333 doi 10 1093 jxb erg141 PMID 12709478 Ogbaga CC Stepien P Athar HU Ashraf M June 2018 Engineering Rubisco activase from thermophilic cyanobacteria into high temperature sensitive plants Critical Reviews in Biotechnology 38 4 559 572 doi 10 1080 07388551 2017 1378998 PMID 28937283 S2CID 4191791 Whitney SM Sharwood RE Orr D White SJ Alonso H Galmes J August 2011 Isoleucine 309 acts as a C4 catalytic switch that increases ribulose 1 5 bisphosphate carboxylase oxygenase rubisco carboxylation rate in Flaveria Proceedings of the National Academy of Sciences of the United States of America 108 35 14688 14693 Bibcode 2011PNAS 10814688W doi 10 1073 pnas 1109503108 PMC 3167554 PMID 21849620 Ishikawa C Hatanaka T Misoo S Miyake C Fukayama H July 2011 Functional incorporation of sorghum small subunit increases the catalytic turnover rate of Rubisco in transgenic rice Plant Physiology 156 3 1603 1611 doi 10 1104 pp 111 177030 PMC 3135941 PMID 21562335 Stracquadanio G Umeton R Papini A Lio P Nicosia G 2010 Analysis and Optimization of C3 Photosynthetic Carbon Metabolism 2010 IEEE International Conference on BioInformatics and BioEngineering Philadelphia PA USA IEEE pp 44 51 doi 10 1109 BIBE 2010 17 hdl 1721 1 101094 ISBN 978 1 4244 7494 3 S2CID 5568464 Whitney SM Andrews TJ December 2001 Plastome encoded bacterial ribulose 1 5 bisphosphate carboxylase oxygenase RubisCO supports photosynthesis and growth in tobacco Proceedings of the National Academy of Sciences of the United States of America 98 25 14738 14743 Bibcode 2001PNAS 9814738W doi 10 1073 pnas 261417298 PMC 64751 PMID 11724961 John Andrews T Whitney SM June 2003 Manipulating ribulose bisphosphate carboxylase oxygenase in the chloroplasts of higher plants Archives of Biochemistry and Biophysics 414 2 159 169 doi 10 1016 S0003 9861 03 00100 0 PMID 12781767 Lin MT Occhialini A Andralojc PJ Parry MA Hanson MR September 2014 A faster Rubisco with potential to increase photosynthesis in crops Nature 513 7519 547 550 Bibcode 2014Natur 513 547L doi 10 1038 nature13776 PMC 4176977 PMID 25231869 Tcherkez GG Farquhar GD Andrews TJ May 2006 Despite slow catalysis and confused substrate specificity all ribulose bisphosphate carboxylases may be nearly perfectly optimized Proceedings of the National Academy of Sciences of the United States of America 103 19 7246 7251 Bibcode 2006PNAS 103 7246T doi 10 1073 pnas 0600605103 PMC 1464328 PMID 16641091 Igamberdiev AU 2015 Control of Rubisco function via homeostatic equilibration of CO2 supply Frontiers in Plant Science 6 106 doi 10 3389 fpls 2015 00106 PMC 4341507 PMID 25767475 Igamberdiev AU Lea PJ February 2006 Land plants equilibrate O2 and CO2 concentrations in the atmosphere Photosynthesis Research 87 2 177 194 Bibcode 2006PhoRe 87 177I doi 10 1007 s11120 005 8388 2 PMID 16432665 S2CID 10709679 Bracher A Whitney SM Hartl FU Hayer Hartl M April 2017 Biogenesis and Metabolic Maintenance of Rubisco Annual Review of Plant Biology 68 29 60 doi 10 1146 annurev arplant 043015 111633 PMID 28125284 Sjuts I Soll J Bolter B 2017 Import of Soluble Proteins into Chloroplasts and Potential Regulatory Mechanisms Frontiers in Plant Science 8 168 doi 10 3389 fpls 2017 00168 PMC 5296341 PMID 28228773 Aigner H Wilson RH Bracher A Calisse L Bhat JY Hartl FU Hayer Hartl M December 2017 Plant RuBisCo assembly in E coli with five chloroplast chaperones including BSD2 Science 358 6368 1272 1278 Bibcode 2017Sci 358 1272A doi 10 1126 science aap9221 hdl 11858 00 001M 0000 002E 8B4D B PMID 29217567 a b Heazlewood J 2012 Proteomic applications in biology New York InTech Manhattan ISBN 978 953 307 613 3 Gupta R Kim ST 2015 Depletion of RuBisCO Protein Using the Protamine Sulfate Precipitation Method Proteomic Profiling Methods in Molecular Biology Vol 1295 New York NY Humana Press pp 225 33 doi 10 1007 978 1 4939 2550 6 17 ISBN 978 1 4939 2549 0 PMID 25820725 Krishnan HB Natarajan SS December 2009 A rapid method for depletion of Rubisco from soybean Glycine max leaf for proteomic analysis of lower abundance proteins Phytochemistry 70 17 18 1958 1964 Bibcode 2009PChem 70 1958K doi 10 1016 j phytochem 2009 08 020 PMID 19766275 Kim ST Cho KS Jang YS Kang KY June 2001 Two dimensional electrophoretic analysis of rice proteins by polyethylene glycol fractionation for protein arrays Electrophoresis 22 10 2103 2109 doi 10 1002 1522 2683 200106 22 10 lt 2103 aid elps2103 gt 3 0 co 2 w PMID 11465512 S2CID 38878805 Xi J Wang X Li S Zhou X Yue L Fan J Hao D November 2006 Polyethylene glycol fractionation improved detection of low abundant proteins by two dimensional electrophoresis analysis of plant proteome Phytochemistry 67 21 2341 2348 Bibcode 2006PChem 67 2341X doi 10 1016 j phytochem 2006 08 005 PMID 16973185 Cellar NA Kuppannan K Langhorst ML Ni W Xu P Young SA January 2008 Cross species applicability of abundant protein depletion columns for ribulose 1 5 bisphosphate carboxylase oxygenase Journal of Chromatography B Analytical Technologies in the Biomedical and Life Sciences 861 1 29 39 doi 10 1016 j jchromb 2007 11 024 PMID 18063427 Agrawal GK Jwa NS Rakwal R February 2009 Rice proteomics ending phase I and the beginning of phase II Proteomics 9 4 935 963 doi 10 1002 pmic 200800594 PMID 19212951 S2CID 2455432 Cho JH Hwang H Cho MH Kwon YK Jeon JS Bhoo SH Hahn TR July 2008 The effect of DTT in protein preparations for proteomic analysis Removal of a highly abundant plant enzyme ribulose bisphosphate carboxylase oxygenase Journal of Plant Biology 51 4 297 301 Bibcode 2008JPBio 51 297C doi 10 1007 BF03036130 ISSN 1226 9239 S2CID 23636617 Chase MW Soltis DE Olmstead RG Morgan D Les DH Mishler BD et al 1993 Phylogenetics of Seed Plants An Analysis of Nucleotide Sequences from the Plastid Gene rbcL PDF Annals of the Missouri Botanical Garden 80 3 528 580 doi 10 2307 2399846 hdl 1969 1 179875 JSTOR 2399846 Ashida H Saito Y Nakano T Tandeau de Marsac N Sekowska A Danchin A Yokota A 19 June 2007 RuBisCO like proteins as the enolase enzyme in the methionine salvage pathway functional and evolutionary relationships between RuBisCO like proteins and photosynthetic RuBisCO Journal of Experimental Botany 59 7 1543 1554 doi 10 1093 jxb ern104 PMID 18403380 Schulz L Guo Z Zarzycki J Steinchen W Schuller JM Heimerl T Prinz S Mueller Cajar O Erb TJ Hochberg GKA 2022 10 14 Evolution of increased complexity and specificity at the dawn of form I Rubiscos Science 378 6616 155 160 Bibcode 2022Sci 378 155S doi 10 1126 science abq1416 PMID 36227987 S2CID 252897276 Sage RF Sage TL Kocacinar F 2012 Photorespiration and the evolution of C4 photosynthesis Annual Review of Plant Biology 63 19 47 doi 10 1146 annurev arplant 042811 105511 PMID 22404472 S2CID 24199852 a b Studer RA Christin PA Williams MA Orengo CA February 2014 Stability activity tradeoffs constrain the adaptive evolution of RubisCO Proceedings of the National Academy of Sciences of the United States of America 111 6 2223 2228 Bibcode 2014PNAS 111 2223S doi 10 1073 pnas 1310811111 PMC 3926066 PMID 24469821 Wildman SG 2002 Along the trail from Fraction I protein to Rubisco ribulose bisphosphate carboxylase oxygenase Photosynthesis Research 73 1 3 243 250 doi 10 1023 A 1020467601966 PMID 16245127 S2CID 7622999 Portis AR Parry MA October 2007 Discoveries in Rubisco Ribulose 1 5 bisphosphate carboxylase oxygenase a historical perspective Photosynthesis Research 94 1 121 143 Bibcode 2007PhoRe 94 121P doi 10 1007 s11120 007 9225 6 PMID 17665149 S2CID 39767233 nbsp Figure 3 In this figure each protein chain in the LS 2 complex is given its own color for easy identification Further reading editMarcus Y Altman Gueta H Finkler A Gurevitz M June 2005 Mutagenesis at two distinct phosphate binding sites unravels their differential roles in regulation of Rubisco activation and catalysis Journal of Bacteriology 187 12 4222 4228 doi 10 1128 JB 187 12 4222 4228 2005 PMC 1151729 PMID 15937184 Sugawara H Yamamoto H Shibata N Inoue T Okada S Miyake C et al May 1999 Crystal structure of carboxylase reaction oriented ribulose 1 5 bisphosphate carboxylase oxygenase from a thermophilic red alga Galdieria partita The Journal of Biological Chemistry 274 22 15655 15661 doi 10 1074 jbc 274 22 15655 PMID 10336462 External links editGerritsen VB September 2003 The Plant Kingdom s sloth Protein Spotlight Swiss Institute of Bioinformatics SIB Rubisco plods along at a mere three molecules per second To bypass such slothfulness plants synthesize a gross amount of Rubisco sometimes up to 50 of their total protein content Retrieved from https en wikipedia org w index php title RuBisCO amp oldid 1200891664, wikipedia, wiki, book, books, library,

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