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Antithrombin

February 16, 2024

Antithrombin (AT) is a small glycoprotein that inactivates several enzymes of the coagulation system. It is a 464-amino-acid protein produced by the liver. It contains three disulfide bonds and a total of four possible glycosylation sites. α-Antithrombin is the dominant form of antithrombin found in blood plasma and has an oligosaccharide occupying each of its four glycosylation sites. A single glycosylation site remains consistently un-occupied in the minor form of antithrombin, β-antithrombin.[5] Its activity is increased manyfold by the anticoagulant drug heparin, which enhances the binding of antithrombin to factor IIa (thrombin) and factor Xa.[6]

SERPINC1
Available structures
PDBOrtholog search: PDBe RCSB
Identifiers
AliasesSERPINC1, AT3, AT3D, ATIII, THPH7, serpin family C member 1, ATIII-R2, ATIII-T2, ATIII-T1
External IDsOMIM: 107300 MGI: 88095 HomoloGene: 20139 GeneCards: SERPINC1
Orthologs
SpeciesHumanMouse
Entrez

462

11905

Ensembl

ENSG00000117601

ENSMUSG00000026715

UniProt

P01008

P32261

RefSeq (mRNA)

NM_000488
NM_001365052

NM_080844
NM_001379302

RefSeq (protein)

NP_000479
NP_001351981

NP_543120
NP_001366231

Location (UCSC)Chr 1: 173.9 – 173.92 MbChr 1: 160.81 – 160.83 Mb
PubMed search[3][4]
Wikidata
View/Edit HumanView/Edit Mouse

Structure edit

Antithrombin is also termed antithrombin III (AT III). The designations antithrombin I through to antithrombin IV originate in early studies carried out in the 1950s by Seegers, Johnson and Fell.[7]

Antithrombin I (AT I) refers to the binding of thrombin to fibrin, after thrombin has activated fibrinogen, at a non-catalytic binding site of thrombin. Antithrombin II (AT II) refers to a cofactor in plasma, which together with heparin interferes with the interaction of thrombin and fibrinogen. Antithrombin III (AT III) refers to a substance in plasma that inactivates thrombin. Antithrombin IV (AT IV) refers to an antithrombin that becomes activated during and shortly after blood coagulation.[8] Only AT III and possibly AT I are medically significant. AT III is generally referred to solely as "antithrombin" and it is antithrombin III that is discussed in this article.

 
Figure 1. The location of the four potential glycosylation sites within the tertiary structure of an antithrombin monomer are shown, as taken from the protein data bank file 2ANT. In this structure only Asn 155 is glycosylated by the addition of a single N-acetylglucosamine residue.

Antithrombin has a half-life in blood plasma of around 3 days.[9] The normal antithrombin concentration in human blood plasma is high at approximately 0.12 mg/ml, which is equivalent to a molar concentration of 2.3 μM.[10] Antithrombin has been isolated from the plasma of a large number of species additional to humans.[11] As deduced from protein and cDNA sequencing, cow, sheep, rabbit and mouse antithrombins are all 433 amino acids in length, which is one amino acid longer than human antithrombin. The extra amino acid is thought to occur at amino acid position 6. Cow, sheep, rabbit, mouse, and human antithrombins share between 84 and 89% amino acid sequence identity.[12] Six of the amino acids form three intramolecular disulfide bonds, Cys8-Cys128, Cys21-Cys95, and Cys248-Cys430. They all have four potential N-glycosylation sites. These occur at asparagine (Asn) amino acid numbers 96, 135, 155, and 192 in humans and at similar amino acid numbers in other species. All these sites are occupied by covalently attached oligosaccharide side-chains in the predominant form of human antithrombin, α-antithrombin, resulting in a molecular weight for this form of antithrombin of 58,200.[5] The potential glycosylation site at asparagine 135 is not occupied in a minor form (around 10%) of antithrombin, β-antithrombin (see Figure 1).[13]

Recombinant antithrombins with properties similar to those of normal human antithrombin have been produced using baculovirus-infected insect cells and mammalian cell lines grown in cell culture.[14][15][16][17] These recombinant antithrombins generally have different glycosylation patterns to normal antithrombin and are typically used in antithrombin structural studies. For this reason many of the antithrombin structures stored in the protein data bank and presented in this article show variable glycosylation patterns.

Antithrombin begins in its native state, which has a higher free energy compared to the latent state, which it decays to on average after 3 days. The latent state has the same form as the activated state - that is, when it is inhibiting thrombin. As such it is a classic example of the utility of kinetic vs thermodynamic control of protein folding.

Function edit

 
Figure 2. The reactive arg 393 - ser 394 bond is located on an exposed loop at the surface of the molecule. This loop is termed the reactive site loop (RSL) or reactive centre loop (RCL).
 
Figure 3. The amino acid sequence of the reactive site loop of human antithrombin is shown.[18] The reactive site loop comprises amino acid sequence numbers 377 to 400 (numbers shown below the above sequence) or amino acids P1 to P17 and P1' to P7' using the Schechter and Berger convention (number shown above the above sequence).[19] The reactive bond is indicated by an arrow.

Antithrombin is a serpin (serine protease inhibitor) and is thus similar in structure to most other plasma protease inhibitors, such as alpha 1-antichymotrypsin, alpha 2-antiplasmin and Heparin cofactor II.

The physiological target proteases of antithrombin are those of the contact activation pathway (formerly known as the intrinsic pathway), namely the activated forms of Factor X (Xa), Factor IX (IXa), Factor XI (XIa), Factor XII (XIIa) and, to a greater extent, Factor II (thrombin) (IIa), and also the activated form of Factor VII (VIIa) from the tissue factor pathway (formerly known as the extrinsic pathway).[20] The inhibitor also inactivates kallikrein and plasmin[citation needed], also involved in blood coagulation. However it inactivates certain other serine proteases that are not involved in coagulation such as trypsin and the C1s subunit of the enzyme C1 involved in the classical complement pathway.[12][21]

Protease inactivation results as a consequence of trapping the protease in an equimolar complex with antithrombin in which the active site of the protease enzyme is inaccessible to its usual substrate.[12] The formation of an antithrombin-protease complex involves an interaction between the protease and a specific reactive peptide bond within antithrombin. In human antithrombin this bond is between arginine (arg) 393 and serine (ser) 394 (see Figure 2 and Figure 3).[12]

It is thought that protease enzymes become trapped in inactive antithrombin-protease complexes as a consequence of their attack on the reactive bond. Although attacking a similar bond within the normal protease substrate results in rapid proteolytic cleavage of the substrate, initiating an attack on the antithrombin reactive bond causes antithrombin to become activated and trap the enzyme at an intermediate stage of the proteolytic process. Given time, thrombin is able to cleave the reactive bond within antithrombin and an inactive antithrombin-thrombin complex will dissociate, however the time it takes for this to occur may be greater than 3 days.[22] However, bonds P3-P4 and P1'-P2' can be rapidly cleaved by neutrophil elastase and the bacterial enzyme thermolysin, respectively, resulting in inactive antithrombins no longer able to inhibit thrombin activity.[23]

The rate of antithrombin's inhibition of protease activity is greatly enhanced by its additional binding to heparin, as is its inactivation by neutrophil elastase.[23]

Antithrombin and heparin edit

Antithrombin inactivates its physiological target enzymes, Thrombin, Factor Xa and Factor IXa with rate constants of 7–11 x 103, 2.5 x 103 M−1 s−1 and 1 x 10 M−1 s−1 respectively.[5][24] The rate of antithrombin-thrombin inactivation increases to 1.5 - 4 x 107 M−1 s−1 in the presence of heparin, i.e. the reaction is accelerated 2000-4000 fold.[25][26][27][28] Factor Xa inhibition is accelerated by only 500 to 1000 fold in the presence of heparin and the maximal rate constant is 10 fold lower than that of thrombin inhibition.[25][28] The rate enhancement of antithrombin-Factor IXa inhibition shows an approximate 1 million fold enhancement in the presence of heparin and physiological levels of calcium.[24]

AT-III binds to a specific pentasaccharide sulfation sequence contained within the heparin polymer

GlcNAc/NS(6S)-GlcA-GlcNS(3S,6S)-IdoA(2S)-GlcNS(6S)

Upon binding to this pentasaccharide sequence, inhibition of protease activity is increased by heparin as a result of two distinct mechanisms.[29] In one mechanism heparin stimulation of Factor IXa and Xa inhibition depends on a conformational change within antithrombin involving the reactive site loop and is thus allosteric.[30] In another mechanism stimulation of thrombin inhibition depends on the formation of a ternary complex between AT-III, thrombin, and heparin.[30]

Allosteric activation edit

 
Figure 4. Two crystal structures for antithrombin. Model A is taken from the pdb file 2ANT and model B from pdb file 1AZX. Model B is complexed with a pentasaccharide while model A is uncomplexed.

Increased Factor IXa and Xa inhibition requires the minimal heparin pentasaccharide sequence. The conformational changes that occur within antithrombin in response to pentasaccharide binding are well documented.[18][31][32]

In the absence of heparin, amino acids P14 and P15 (see Figure 3) from the reactive site loop are embedded within the main body of the protein (specifically the top of beta sheet A). This feature is in common with other serpins such as heparin cofactor II, alpha 1-antichymotrypsin and MENT.

The conformational change most relevant for Factor IXa and Xa inhibition involves the P14 and P15 amino acids within the N-terminal region of the reactive site loop (circled in Figure 4 model B). This region has been termed the hinge region. The conformational change within the hinge region in response to heparin binding results in the expulsion of P14 and P15 from the main body of the protein and it has been shown that by preventing this conformational change, increased Factor IXa and Xa inhibition does not occur.[30] It is thought that the increased flexibility given to the reactive site loop as a result of the hinge region conformational change is a key factor in influencing increased Factor IXa and Xa inhibition. It has been calculated that in the absence of the pentasaccharide only one in every 400 antithrombin molecules (0.25%) is in an active conformation with the P14 and P15 amino acids expelled.[30]

Non-allosteric activation edit

 
Figure 5. The structure of an antithrombin-thrombin-heparin ternary complex taken from pdb 1TB6.

Increased thrombin inhibition requires the minimal heparin pentasaccharide plus at least an additional 13 monomeric units.[33] This is thought to be due to a requirement that antithrombin and thrombin must bind to the same heparin chain adjacent to each other. This can be seen in the series of models shown in Figure 5.

In the structures shown in Figure 5 the C-terminal portion (P' side) of the reactive site loop is in an extended conformation when compared with other un-activated or heparin activated antithrombin structures.[34] The P' region of antithrombin is unusually long relative to the P' region of other serpins and in un-activated or heparin activated antithrombin structures forms a tightly hydrogen bonded β-turn. P' elongation occurs through the breaking of all hydrogen bonds involved in the β-turn.[34]

The hinge region of antithrombin in the Figure 5 complex could not be modelled due to its conformational flexibility, and amino acids P9-P14 are not seen in this structure. This conformational flexibility indicates an equilibrium may exist within the complex between a P14 P15 reactive site loop inserted antithrombin conformation and a P14 P15 reactive site loop expelled conformation. In support of this, analysis of the positioning of P15 Gly in the Figure 5 complex (labelled in model B) shows it to be inserted into beta sheet A (see model C).[34]

Effect of glycosylation on activity edit

α-Antithrombin and β-antithrombin differ in their affinity for heparin.[35] The difference in dissociation constant between the two is threefold for the pentasaccharide shown in Figure 3 and greater than tenfold for full length heparin, with β-antithrombin having a higher affinity.[36] The higher affinity of β-antithrombin is thought to be due to the increased rate at which subsequent conformational changes occur within the protein upon initial heparin binding. For α-antithrombin, the additional glycosylation at Asn-135 is not thought to interfere with initial heparin binding, but rather to inhibit any resulting conformational changes.[35]

Even though it is present at only 5–10% the levels of α-antithrombin, due to its increased heparin affinity, it is thought that β-antithrombin is more important than α-antithrombin in controlling thrombogenic events resulting from tissue injury. Indeed, thrombin inhibition after injury to the aorta has been attributed solely to β-antithrombin.[37]

Deficiencies edit

Further information: Antithrombin III deficiency

Evidence for the important role antithrombin plays in regulating normal blood coagulation is demonstrated by the correlation between inherited or acquired antithrombin deficiencies and an increased risk of any affected individual developing thrombotic disease.[38] Antithrombin deficiency generally comes to light when a patient suffers recurrent venous thrombosis and pulmonary embolism.

Acquired antithrombin deficiency edit

Acquired antithrombin deficiency occurs as a result of three distinctly different mechanisms. The first mechanism is increased excretion which may occur with renal failure associated with proteinuria nephrotic syndrome. The second mechanism results from decreased production as seen in liver failure or cirrhosis or an immature liver secondary to premature birth. The third mechanism results from accelerated consumption which is most pronounced as consequence of severe injury trauma but also may be seen on a lesser scale as a result of interventions such as major surgery or cardiopulmonary bypass.[39]

Inherited antithrombin deficiency edit

The incidence of inherited antithrombin deficiency has been estimated at between 1:2000 and 1:5000 in the normal population, with the first family suffering from inherited antithrombin deficiency being described in 1965.[40][41] Subsequently, it was proposed that the classification of inherited antithrombin deficiency be designated as either type I or type II, based upon functional and immunochemical antithrombin analyses.[42] Maintenance of an adequate level of antithrombin activity, which is at least 70% that of a normal functional level, is essential to ensure effective inhibition of blood coagulation proteases.[43] Typically as a result of type I or type II antithrombin deficiency, functional antithrombin levels are reduced to below 50% of normal.[44]

Type I antithrombin deficiency edit

Type I antithrombin deficiency is characterized by a decrease in both antithrombin activity and antithrombin concentration in the blood of affected individuals. Type I deficiency was originally further divided into two subgroups, Ia and Ib, based upon heparin affinity. The antithrombin of subgroup Ia individuals showed a normal affinity for heparin while the antithrombin of subgroup Ib individuals showed a reduced affinity for heparin.[45] Subsequent functional analysis of a group of 1b cases found them not only to have reduced heparin affinity but multiple or 'pleiotrophic' abnormalities affecting the reactive site, the heparin binding site and antithrombin blood concentration. In a revised system of classification adopted by the Scientific and Standardization Committee of the International Society on Thrombosis and Haemostasis, type Ib cases are now designated as type II PE, Pleiotrophic effect.[46]

Most cases of type I deficiency are due to point mutations, deletions or minor insertions within the antithrombin gene. These genetic mutations result in type I deficiency through a variety of mechanisms:

  • Mutations may produce unstable antithrombins that either may be not exported into the blood correctly upon completion biosynthesis or exist in the blood for a shortened period of time, e.g., the deletion of 6 base pairs in codons 106–108.[47]
  • Mutations may affect mRNA processing of the antithrombin gene.
  • Minor insertions or deletions may lead to frame shift mutations and premature termination of the antithrombin gene.
  • Point mutations may also result in the premature generation of a termination or stop codon e.g. the mutation of codon 129, CGATGA (UGA after transcription), replaces a normal codon for arginine with a termination codon.[48]

Type II antithrombin deficiency edit

Type II antithrombin deficiency is characterized by normal antithrombin levels but reduced antithrombin activity in the blood of affected individuals. It was originally proposed that type II deficiency be further divided into three subgroups (IIa, IIb, and IIc) depending on which antithrombin functional activity is reduced or retained.[45]

  • Subgroup IIa - Decreased thrombin inactivation, decreased factor Xa inactivation and decreased heparin affinity.
  • Subgroup IIb - Decreased thrombin inactivation and normal heparin affinity.
  • Subgroup IIc - Normal thrombin inactivation, normal factor Xa inactivation and decreased heparin affinity.

In the revised system of classification again adopted by the Scientific and Standardization Committee of the International Society on Thrombosis and Haemostasis, type II antithrombin deficiency remains subdivided into three subgroups: the already mentioned type II PE, along with type II RS, where mutations effect the reactive site and type II HBS, where mutations effect the antithrombin heparin binding site.[46] For the purposes of an antithrombin mutational database compiled by members of the Plasma Coagulation Inhibitors Subcommittee of the Scientific and Standardization Committee of the International Society on Thrombosis and Haemostasis, type IIa cases are now classified as type II PE, type IIb cases as type II RS and type IIc cases as type II HBS.[49]

Toponyms edit

Presently it is relatively easy to characterise a specific antithrombin genetic mutation. However prior to the use of modern characterisation techniques investigators named mutations for the town or city where the individual suffering from the deficiency resided i.e. the antithrombin mutation was designated a toponym.[50] Modern mutational characterisation has since shown that many individual antithrombin toponyms are actually the result of the same genetic mutation, for example antithrombin-Toyama, is equivalent to antithrombin-Kumamoto, -Amien, -Tours, -Paris-1, -Paris-2, -Alger, -Padua-2 and -Barcelona.[49]

  •  
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Medical uses edit

Antithrombin is used as a protein therapeutic that can be purified from human plasma[51] or produced recombinantly (for example Atryn, which is produced in the milk of genetically modified goats[52][53]).

It is approved by the FDA as an anticoagulant for the prevention of clots before, during, or after surgery or birthing in patients with hereditary antithrombin deficiency.[51][53]

It has been studied in sepsis to reduce diffuse intravascular coagulation and other outcomes. It has not been found to confer any benefit in critically ill people with sepsis.[54]

Cleaved and latent antithrombin edit

 
Figure 6. Latent antithrombin

Cleavage at the reactive site results in entrapment of the thrombin protease, with movement of the cleaved reactive site loop together with the bound protease, such that the loop forms an extra sixth strand in the middle of beta sheet A. This movement of the reactive site loop can also be induced without cleavage, with the resulting crystallographic structure being identical to that of the physiologically latent conformation of plasminogen activator inhibitor-1 (PAI-1).[55] For this reason the conformation of antithrombin in which the reactive site loop is incorporated uncleaved into the main body of the protein is referred to as latent antithrombin. In contrast to PAI-1 the transition for antithrombin from a normal or native conformation to a latent conformation is irreversible.

Native antithrombin can be converted to latent antithrombin (L-antithrombin) by heating alone or heating in the presence of citrate.[56][57] However, without extreme heating and at 37 °C (body temperature) 10% of all antithrombin circulating in the blood is converted to the L-antithrombin over a 24-hour period.[58][59] The structure of L-antithrombin is shown in Figure 6.

The 3-dimensional structure of native antithrombin was first determined in 1994.[31][32] Unexpectedly the protein crystallized as a heterodimer composed of one molecule of native antithrombin and one molecule of latent antithrombin. Latent antithrombin on formation immediately links to a molecule of native antithrombin to form the heterodimer, and it is not until the concentration of latent antithrombin exceeds 50% of the total antithrombin that it can be detected analytically.[59] Not only is the latent form of antithrombin inactive against its target coagulation proteases, but its dimerisation with an otherwise active native antithrombin molecule also results in the native molecules inactivation. The physiological impact of the loss of antithrombin activity either through latent antithrombin formation or through subsequent dimer formation is exacerbated by the preference for dimerisation to occur between heparin activated β-antithrombin and latent antithrombin as opposed to α-antithrombin.[59]

A form of antithrombin that is an intermediate in the conversion between native and latent forms of antithrombin has also been isolated and this has been termed prelatent antithrombin.[60]

Antiangiogenic antithrombin edit

Angiogenesis is a physiological process involving the growth of new blood vessels from pre-existing vessels. Under normal physiological conditions angiogenesis is tightly regulated and is controlled by a balance of angiogenic stimulators and angiogenic inhibitors. Tumor growth is dependent upon angiogenesis and during tumor development a sustained production of angiogenic stimulatory factors is required along with a reduction in the quantity of angiogenic inhibitory factors tumor cells produce.[61] The cleaved and latent form of antithrombin potently inhibit angiogenesis and tumor growth in animal models.[62] The prelatent form of antithrombin has been shown to inhibit angiogenesis in-vitro but to date has not been tested in experimental animal models.

References edit

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Further reading edit

  • Panzer-Heinig, Sabine (2009). Antithrombin (III) - Establishing Pediatric Reference Values, Relevance for DIC 1992 versus 2007 (Thesis). Medizinische Fakultät Charité - Universitätsmedizin Berlin.

External links edit

  • The MEROPS online database for peptidases and their inhibitors: I04.018
  • Antithrombin+III at the U.S. National Library of Medicine Medical Subject Headings (MeSH)
  • Human SERPINC1 genome location and SERPINC1 gene details page in the UCSC Genome Browser.

February 16, 2024
antithrombin, small, glycoprotein, that, inactivates, several, enzymes, coagulation, system, amino, acid, protein, produced, liver, contains, three, disulfide, bonds, total, four, possible, glycosylation, sites, dominant, form, antithrombin, found, blood, plas. Antithrombin AT is a small glycoprotein that inactivates several enzymes of the coagulation system It is a 464 amino acid protein produced by the liver It contains three disulfide bonds and a total of four possible glycosylation sites a Antithrombin is the dominant form of antithrombin found in blood plasma and has an oligosaccharide occupying each of its four glycosylation sites A single glycosylation site remains consistently un occupied in the minor form of antithrombin b antithrombin 5 Its activity is increased manyfold by the anticoagulant drug heparin which enhances the binding of antithrombin to factor IIa thrombin and factor Xa 6 SERPINC1Available structuresPDBOrtholog search PDBe RCSBList of PDB id codes4EB1 1ANT 1ATH 1AZX 1BR8 1DZG 1DZH 1E03 1E04 1E05 1JVQ 1LK6 1NQ9 1OYH 1R1L 1SR5 1T1F 1TB6 2ANT 2B4X 2B5T 2BEH 2GD4 2HIJ 2ZNH 3EVJ 3KCGIdentifiersAliasesSERPINC1 AT3 AT3D ATIII THPH7 serpin family C member 1 ATIII R2 ATIII T2 ATIII T1External IDsOMIM 107300 MGI 88095 HomoloGene 20139 GeneCards SERPINC1Gene location Human Chr Chromosome 1 human 1 Band1q25 1Start173 903 804 bp 1 End173 917 378 bp 1 Gene location Mouse Chr Chromosome 1 mouse 2 Band1 H2 1 1 69 75 cMStart160 806 155 bp 2 End160 833 433 bp 2 RNA expression patternBgeeHumanMouse ortholog Top expressed inright lobe of liverstromal cell of endometriumkidneyislet of Langerhansgastrocnemius musclegastric mucosametanephrosbloodrenal cortexright coronary arteryTop expressed inleft lobe of livergallbladderyolk sacsecondary oocytesexually immature organismabdominal wallmorulaatrioventricular valvedermisstomachMore reference expression dataBioGPSMore reference expression dataGene ontologyMolecular functionpeptidase inhibitor activity protease binding heparin binding protein binding serine type endopeptidase inhibitor activity identical protein bindingCellular componentextracellular region plasma membrane blood microparticle extracellular exosome extracellular space endoplasmic reticulum lumen collagen containing extracellular matrixBiological processhemostasis negative regulation of peptidase activity blood coagulation regulation of blood coagulation intrinsic pathway response to nutrient negative regulation of endopeptidase activity lactation acute inflammatory response to antigenic stimulus regulation of blood coagulation post translational protein modificationSources Amigo QuickGOOrthologsSpeciesHumanMouseEntrez46211905EnsemblENSG00000117601ENSMUSG00000026715UniProtP01008P32261RefSeq mRNA NM 000488NM 001365052NM 080844NM 001379302RefSeq protein NP 000479NP 001351981NP 543120NP 001366231Location UCSC Chr 1 173 9 173 92 MbChr 1 160 81 160 83 MbPubMed search 3 4 WikidataView Edit HumanView Edit Mouse Contents 1 Structure 2 Function 3 Antithrombin and heparin 3 1 Allosteric activation 3 2 Non allosteric activation 4 Effect of glycosylation on activity 5 Deficiencies 5 1 Acquired antithrombin deficiency 5 2 Inherited antithrombin deficiency 5 2 1 Type I antithrombin deficiency 5 2 2 Type II antithrombin deficiency 5 3 Toponyms 6 Medical uses 7 Cleaved and latent antithrombin 8 Antiangiogenic antithrombin 9 References 10 Further reading 11 External linksStructure editAntithrombin is also termed antithrombin III AT III The designations antithrombin I through to antithrombin IV originate in early studies carried out in the 1950s by Seegers Johnson and Fell 7 Antithrombin I AT I refers to the binding of thrombin to fibrin after thrombin has activated fibrinogen at a non catalytic binding site of thrombin Antithrombin II AT II refers to a cofactor in plasma which together with heparin interferes with the interaction of thrombin and fibrinogen Antithrombin III AT III refers to a substance in plasma that inactivates thrombin Antithrombin IV AT IV refers to an antithrombin that becomes activated during and shortly after blood coagulation 8 Only AT III and possibly AT I are medically significant AT III is generally referred to solely as antithrombin and it is antithrombin III that is discussed in this article nbsp Figure 1 The location of the four potential glycosylation sites within the tertiary structure of an antithrombin monomer are shown as taken from the protein data bank file 2ANT In this structure only Asn 155 is glycosylated by the addition of a single N acetylglucosamine residue Antithrombin has a half life in blood plasma of around 3 days 9 The normal antithrombin concentration in human blood plasma is high at approximately 0 12 mg ml which is equivalent to a molar concentration of 2 3 mM 10 Antithrombin has been isolated from the plasma of a large number of species additional to humans 11 As deduced from protein and cDNA sequencing cow sheep rabbit and mouse antithrombins are all 433 amino acids in length which is one amino acid longer than human antithrombin The extra amino acid is thought to occur at amino acid position 6 Cow sheep rabbit mouse and human antithrombins share between 84 and 89 amino acid sequence identity 12 Six of the amino acids form three intramolecular disulfide bonds Cys8 Cys128 Cys21 Cys95 and Cys248 Cys430 They all have four potential N glycosylation sites These occur at asparagine Asn amino acid numbers 96 135 155 and 192 in humans and at similar amino acid numbers in other species All these sites are occupied by covalently attached oligosaccharide side chains in the predominant form of human antithrombin a antithrombin resulting in a molecular weight for this form of antithrombin of 58 200 5 The potential glycosylation site at asparagine 135 is not occupied in a minor form around 10 of antithrombin b antithrombin see Figure 1 13 Recombinant antithrombins with properties similar to those of normal human antithrombin have been produced using baculovirus infected insect cells and mammalian cell lines grown in cell culture 14 15 16 17 These recombinant antithrombins generally have different glycosylation patterns to normal antithrombin and are typically used in antithrombin structural studies For this reason many of the antithrombin structures stored in the protein data bank and presented in this article show variable glycosylation patterns Antithrombin begins in its native state which has a higher free energy compared to the latent state which it decays to on average after 3 days The latent state has the same form as the activated state that is when it is inhibiting thrombin As such it is a classic example of the utility of kinetic vs thermodynamic control of protein folding Function edit nbsp Figure 2 The reactive arg 393 ser 394 bond is located on an exposed loop at the surface of the molecule This loop is termed the reactive site loop RSL or reactive centre loop RCL nbsp Figure 3 The amino acid sequence of the reactive site loop of human antithrombin is shown 18 The reactive site loop comprises amino acid sequence numbers 377 to 400 numbers shown below the above sequence or amino acids P1 to P17 and P1 to P7 using the Schechter and Berger convention number shown above the above sequence 19 The reactive bond is indicated by an arrow Antithrombin is a serpin serine protease inhibitor and is thus similar in structure to most other plasma protease inhibitors such as alpha 1 antichymotrypsin alpha 2 antiplasmin and Heparin cofactor II The physiological target proteases of antithrombin are those of the contact activation pathway formerly known as the intrinsic pathway namely the activated forms of Factor X Xa Factor IX IXa Factor XI XIa Factor XII XIIa and to a greater extent Factor II thrombin IIa and also the activated form of Factor VII VIIa from the tissue factor pathway formerly known as the extrinsic pathway 20 The inhibitor also inactivates kallikrein and plasmin citation needed also involved in blood coagulation However it inactivates certain other serine proteases that are not involved in coagulation such as trypsin and the C1s subunit of the enzyme C1 involved in the classical complement pathway 12 21 Protease inactivation results as a consequence of trapping the protease in an equimolar complex with antithrombin in which the active site of the protease enzyme is inaccessible to its usual substrate 12 The formation of an antithrombin protease complex involves an interaction between the protease and a specific reactive peptide bond within antithrombin In human antithrombin this bond is between arginine arg 393 and serine ser 394 see Figure 2 and Figure 3 12 It is thought that protease enzymes become trapped in inactive antithrombin protease complexes as a consequence of their attack on the reactive bond Although attacking a similar bond within the normal protease substrate results in rapid proteolytic cleavage of the substrate initiating an attack on the antithrombin reactive bond causes antithrombin to become activated and trap the enzyme at an intermediate stage of the proteolytic process Given time thrombin is able to cleave the reactive bond within antithrombin and an inactive antithrombin thrombin complex will dissociate however the time it takes for this to occur may be greater than 3 days 22 However bonds P3 P4 and P1 P2 can be rapidly cleaved by neutrophil elastase and the bacterial enzyme thermolysin respectively resulting in inactive antithrombins no longer able to inhibit thrombin activity 23 The rate of antithrombin s inhibition of protease activity is greatly enhanced by its additional binding to heparin as is its inactivation by neutrophil elastase 23 Antithrombin and heparin editAntithrombin inactivates its physiological target enzymes Thrombin Factor Xa and Factor IXa with rate constants of 7 11 x 103 2 5 x 103 M 1 s 1 and 1 x 10 M 1 s 1 respectively 5 24 The rate of antithrombin thrombin inactivation increases to 1 5 4 x 107 M 1 s 1 in the presence of heparin i e the reaction is accelerated 2000 4000 fold 25 26 27 28 Factor Xa inhibition is accelerated by only 500 to 1000 fold in the presence of heparin and the maximal rate constant is 10 fold lower than that of thrombin inhibition 25 28 The rate enhancement of antithrombin Factor IXa inhibition shows an approximate 1 million fold enhancement in the presence of heparin and physiological levels of calcium 24 AT III binds to a specific pentasaccharide sulfation sequence contained within the heparin polymerGlcNAc NS 6S GlcA GlcNS 3S 6S IdoA 2S GlcNS 6S Upon binding to this pentasaccharide sequence inhibition of protease activity is increased by heparin as a result of two distinct mechanisms 29 In one mechanism heparin stimulation of Factor IXa and Xa inhibition depends on a conformational change within antithrombin involving the reactive site loop and is thus allosteric 30 In another mechanism stimulation of thrombin inhibition depends on the formation of a ternary complex between AT III thrombin and heparin 30 Allosteric activation edit nbsp Figure 4 Two crystal structures for antithrombin Model A is taken from the pdb file 2ANT and model B from pdb file 1AZX Model B is complexed with a pentasaccharide while model A is uncomplexed Increased Factor IXa and Xa inhibition requires the minimal heparin pentasaccharide sequence The conformational changes that occur within antithrombin in response to pentasaccharide binding are well documented 18 31 32 In the absence of heparin amino acids P14 and P15 see Figure 3 from the reactive site loop are embedded within the main body of the protein specifically the top of beta sheet A This feature is in common with other serpins such as heparin cofactor II alpha 1 antichymotrypsin and MENT The conformational change most relevant for Factor IXa and Xa inhibition involves the P14 and P15 amino acids within the N terminal region of the reactive site loop circled in Figure 4 model B This region has been termed the hinge region The conformational change within the hinge region in response to heparin binding results in the expulsion of P14 and P15 from the main body of the protein and it has been shown that by preventing this conformational change increased Factor IXa and Xa inhibition does not occur 30 It is thought that the increased flexibility given to the reactive site loop as a result of the hinge region conformational change is a key factor in influencing increased Factor IXa and Xa inhibition It has been calculated that in the absence of the pentasaccharide only one in every 400 antithrombin molecules 0 25 is in an active conformation with the P14 and P15 amino acids expelled 30 Non allosteric activation edit nbsp Figure 5 The structure of an antithrombin thrombin heparin ternary complex taken from pdb 1TB6 Increased thrombin inhibition requires the minimal heparin pentasaccharide plus at least an additional 13 monomeric units 33 This is thought to be due to a requirement that antithrombin and thrombin must bind to the same heparin chain adjacent to each other This can be seen in the series of models shown in Figure 5 In the structures shown in Figure 5 the C terminal portion P side of the reactive site loop is in an extended conformation when compared with other un activated or heparin activated antithrombin structures 34 The P region of antithrombin is unusually long relative to the P region of other serpins and in un activated or heparin activated antithrombin structures forms a tightly hydrogen bonded b turn P elongation occurs through the breaking of all hydrogen bonds involved in the b turn 34 The hinge region of antithrombin in the Figure 5 complex could not be modelled due to its conformational flexibility and amino acids P9 P14 are not seen in this structure This conformational flexibility indicates an equilibrium may exist within the complex between a P14 P15 reactive site loop inserted antithrombin conformation and a P14 P15 reactive site loop expelled conformation In support of this analysis of the positioning of P15 Gly in the Figure 5 complex labelled in model B shows it to be inserted into beta sheet A see model C 34 Effect of glycosylation on activity edita Antithrombin and b antithrombin differ in their affinity for heparin 35 The difference in dissociation constant between the two is threefold for the pentasaccharide shown in Figure 3 and greater than tenfold for full length heparin with b antithrombin having a higher affinity 36 The higher affinity of b antithrombin is thought to be due to the increased rate at which subsequent conformational changes occur within the protein upon initial heparin binding For a antithrombin the additional glycosylation at Asn 135 is not thought to interfere with initial heparin binding but rather to inhibit any resulting conformational changes 35 Even though it is present at only 5 10 the levels of a antithrombin due to its increased heparin affinity it is thought that b antithrombin is more important than a antithrombin in controlling thrombogenic events resulting from tissue injury Indeed thrombin inhibition after injury to the aorta has been attributed solely to b antithrombin 37 Deficiencies editFurther information Antithrombin III deficiency Evidence for the important role antithrombin plays in regulating normal blood coagulation is demonstrated by the correlation between inherited or acquired antithrombin deficiencies and an increased risk of any affected individual developing thrombotic disease 38 Antithrombin deficiency generally comes to light when a patient suffers recurrent venous thrombosis and pulmonary embolism Acquired antithrombin deficiency edit Acquired antithrombin deficiency occurs as a result of three distinctly different mechanisms The first mechanism is increased excretion which may occur with renal failure associated with proteinuria nephrotic syndrome The second mechanism results from decreased production as seen in liver failure or cirrhosis or an immature liver secondary to premature birth The third mechanism results from accelerated consumption which is most pronounced as consequence of severe injury trauma but also may be seen on a lesser scale as a result of interventions such as major surgery or cardiopulmonary bypass 39 Inherited antithrombin deficiency edit The incidence of inherited antithrombin deficiency has been estimated at between 1 2000 and 1 5000 in the normal population with the first family suffering from inherited antithrombin deficiency being described in 1965 40 41 Subsequently it was proposed that the classification of inherited antithrombin deficiency be designated as either type I or type II based upon functional and immunochemical antithrombin analyses 42 Maintenance of an adequate level of antithrombin activity which is at least 70 that of a normal functional level is essential to ensure effective inhibition of blood coagulation proteases 43 Typically as a result of type I or type II antithrombin deficiency functional antithrombin levels are reduced to below 50 of normal 44 Type I antithrombin deficiency edit Type I antithrombin deficiency is characterized by a decrease in both antithrombin activity and antithrombin concentration in the blood of affected individuals Type I deficiency was originally further divided into two subgroups Ia and Ib based upon heparin affinity The antithrombin of subgroup Ia individuals showed a normal affinity for heparin while the antithrombin of subgroup Ib individuals showed a reduced affinity for heparin 45 Subsequent functional analysis of a group of 1b cases found them not only to have reduced heparin affinity but multiple or pleiotrophic abnormalities affecting the reactive site the heparin binding site and antithrombin blood concentration In a revised system of classification adopted by the Scientific and Standardization Committee of the International Society on Thrombosis and Haemostasis type Ib cases are now designated as type II PE Pleiotrophic effect 46 Most cases of type I deficiency are due to point mutations deletions or minor insertions within the antithrombin gene These genetic mutations result in type I deficiency through a variety of mechanisms Mutations may produce unstable antithrombins that either may be not exported into the blood correctly upon completion biosynthesis or exist in the blood for a shortened period of time e g the deletion of 6 base pairs in codons 106 108 47 Mutations may affect mRNA processing of the antithrombin gene Minor insertions or deletions may lead to frame shift mutations and premature termination of the antithrombin gene Point mutations may also result in the premature generation of a termination or stop codon e g the mutation of codon 129 CGA TGA UGA after transcription replaces a normal codon for arginine with a termination codon 48 Type II antithrombin deficiency edit Type II antithrombin deficiency is characterized by normal antithrombin levels but reduced antithrombin activity in the blood of affected individuals It was originally proposed that type II deficiency be further divided into three subgroups IIa IIb and IIc depending on which antithrombin functional activity is reduced or retained 45 Subgroup IIa Decreased thrombin inactivation decreased factor Xa inactivation and decreased heparin affinity Subgroup IIb Decreased thrombin inactivation and normal heparin affinity Subgroup IIc Normal thrombin inactivation normal factor Xa inactivation and decreased heparin affinity In the revised system of classification again adopted by the Scientific and Standardization Committee of the International Society on Thrombosis and Haemostasis type II antithrombin deficiency remains subdivided into three subgroups the already mentioned type II PE along with type II RS where mutations effect the reactive site and type II HBS where mutations effect the antithrombin heparin binding site 46 For the purposes of an antithrombin mutational database compiled by members of the Plasma Coagulation Inhibitors Subcommittee of the Scientific and Standardization Committee of the International Society on Thrombosis and Haemostasis type IIa cases are now classified as type II PE type IIb cases as type II RS and type IIc cases as type II HBS 49 Toponyms edit Presently it is relatively easy to characterise a specific antithrombin genetic mutation However prior to the use of modern characterisation techniques investigators named mutations for the town or city where the individual suffering from the deficiency resided i e the antithrombin mutation was designated a toponym 50 Modern mutational characterisation has since shown that many individual antithrombin toponyms are actually the result of the same genetic mutation for example antithrombin Toyama is equivalent to antithrombin Kumamoto Amien Tours Paris 1 Paris 2 Alger Padua 2 and Barcelona 49 nbsp nbsp nbsp Medical uses editAntithrombin is used as a protein therapeutic that can be purified from human plasma 51 or produced recombinantly for example Atryn which is produced in the milk of genetically modified goats 52 53 It is approved by the FDA as an anticoagulant for the prevention of clots before during or after surgery or birthing in patients with hereditary antithrombin deficiency 51 53 It has been studied in sepsis to reduce diffuse intravascular coagulation and other outcomes It has not been found to confer any benefit in critically ill people with sepsis 54 Cleaved and latent antithrombin edit nbsp Figure 6 Latent antithrombinCleavage at the reactive site results in entrapment of the thrombin protease with movement of the cleaved reactive site loop together with the bound protease such that the loop forms an extra sixth strand in the middle of beta sheet A This movement of the reactive site loop can also be induced without cleavage with the resulting crystallographic structure being identical to that of the physiologically latent conformation of plasminogen activator inhibitor 1 PAI 1 55 For this reason the conformation of antithrombin in which the reactive site loop is incorporated uncleaved into the main body of the protein is referred to as latent antithrombin In contrast to PAI 1 the transition for antithrombin from a normal or native conformation to a latent conformation is irreversible Native antithrombin can be converted to latent antithrombin L antithrombin by heating alone or heating in the presence of citrate 56 57 However without extreme heating and at 37 C body temperature 10 of all antithrombin circulating in the blood is converted to the L antithrombin over a 24 hour period 58 59 The structure of L antithrombin is shown in Figure 6 The 3 dimensional structure of native antithrombin was first determined in 1994 31 32 Unexpectedly the protein crystallized as a heterodimer composed of one molecule of native antithrombin and one molecule of latent antithrombin Latent antithrombin on formation immediately links to a molecule of native antithrombin to form the heterodimer and it is not until the concentration of latent antithrombin exceeds 50 of the total antithrombin that it can be detected analytically 59 Not only is the latent form of antithrombin inactive against its target coagulation proteases but its dimerisation with an otherwise active native antithrombin molecule also results in the native molecules inactivation The physiological impact of the loss of antithrombin activity either through latent antithrombin formation or through subsequent dimer formation is exacerbated by the preference for dimerisation to occur between heparin activated b antithrombin and latent antithrombin as opposed to a antithrombin 59 A form of antithrombin that is an intermediate in the conversion between native and latent forms of antithrombin has also been isolated and this has been termed prelatent antithrombin 60 Antiangiogenic antithrombin editAngiogenesis is a physiological process involving the growth of new blood vessels from pre existing vessels Under normal physiological conditions angiogenesis is tightly regulated and is controlled by a balance of angiogenic stimulators and angiogenic inhibitors Tumor growth is dependent upon angiogenesis and during tumor development a sustained production of angiogenic stimulatory factors is required along with a reduction in the quantity of angiogenic inhibitory factors tumor cells produce 61 The cleaved and latent form of antithrombin potently inhibit angiogenesis and tumor growth in animal models 62 The prelatent form of antithrombin has been shown to inhibit angiogenesis in vitro but to date has not been tested in experimental animal models References edit a b c GRCh38 Ensembl release 89 ENSG00000117601 Ensembl May 2017 a b c GRCm38 Ensembl release 89 ENSMUSG00000026715 Ensembl May 2017 Human PubMed Reference National Center for Biotechnology Information U S National Library of Medicine Mouse PubMed Reference National Center for Biotechnology Information U S National Library of Medicine a b c Bjork I Olson JE 1997 Antithrombin A bloody important serpin in Chemistry and Biology of Serpins Plenum Press pp 17 33 ISBN 978 0 306 45698 5 Finley A Greenberg C 2013 06 01 Review article heparin sensitivity and resistance management during cardiopulmonary bypass Anesthesia and Analgesia 116 6 1210 1222 doi 10 1213 ANE 0b013e31827e4e62 ISSN 1526 7598 PMID 23408671 S2CID 22500786 Seegers WH Johnson JF Fell C 1954 An antithrombin reaction to prothrombin activation Am J Physiol 176 1 97 103 doi 10 1152 ajplegacy 1953 176 1 97 PMID 13124503 Yin ET Wessler S Stoll PJ 1971 Identity of plasma activated factor X inhibitor with antithrombin 3 and heparin cofactor J Biol Chem 246 11 3712 3719 doi 10 1016 S0021 9258 18 62185 4 PMID 4102937 Collen D Schetz J de Cock F Holmer E Verstraete M 1977 Metabolism of antithrombin III heparin cofactor in man Effects of venous thrombosis of heparin administration Eur J Clin Invest 7 1 27 35 doi 10 1111 j 1365 2362 1977 tb01566 x PMID 65284 S2CID 22494710 Conard J Brosstad F Lie Larsen M Samama M Abildgaard U 1983 Molar antithrombin concentration in normal human plasma Haemostasis 13 6 363 368 doi 10 1159 000214823 PMID 6667903 Jordan RE 1983 Antithrombin in vertebrate species Conservation of 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change contribution to heparin rate enhancement J Biol Chem 267 18 12528 12538 doi 10 1016 S0021 9258 18 42309 5 PMID 1618758 Johnson DJ Langdown J Li W Luis SA Baglin TP Huntington JA 2006 Crystal structure of monomeric native antithrombin reveals a novel reactive center loop conformation J Biol Chem 281 46 35478 35486 doi 10 1074 jbc M607204200 PMC 2679979 PMID 16973611 a b c d Langdown J Johnson DJ Baglin TP Huntington JA 2004 Allosteric activation of antithrombin critically depends upon hinge region extension J Biol Chem 279 45 47288 47297 doi 10 1074 jbc M408961200 PMID 15326167 a b Schreuder HA de Boer B Dijkema R Mulders J Theunissen HJ Grootenhuis PD Hol WG 1994 The intact and cleaved human antithrombin III complex as a model for serpin proteinase interactions Nature Structural amp Molecular Biology 1 1 48 54 doi 10 1038 nsb0194 48 PMID 7656006 S2CID 39110624 a b Carrell RW Stein PE Fermi G Wardell MR 1994 Biological implications of a 3 A structure of dimeric antithrombin Structure 2 4 257 270 doi 10 1016 S0969 2126 00 00028 9 PMID 8087553 Petitou M Herault JP Bernat A Driguez PA Duchaussoy P Lormeau JC Herbert JM 1999 Synthesis of Thrombin inhibiting Heparin mimetics without side effects Nature 398 6726 417 422 Bibcode 1999Natur 398 417P doi 10 1038 18877 PMID 10201371 S2CID 4339441 a b c Li W Johnson DJ Esmon CT Huntington JA 2004 Structure of the antithrombin thrombin heparin ternary complex reveals the antithrombotic mechanism of heparin Nature Structural amp Molecular Biology 11 9 857 862 doi 10 1038 nsmb811 PMID 15311269 S2CID 28790576 a b McCoy AJ Pei XY Skinner R Abrahams JP Carrell RW 2003 Structure of beta antithrombin and the effect of glycosylation on antithrombin s heparin affinity and activity J Mol Biol 326 3 823 833 doi 10 1016 S0022 2836 02 01382 7 hdl 1887 3620879 PMID 12581643 Turk B Brieditis I Bock SC Olson ST Bjork I 1997 The oligosaccharide side chain on Asn 135 of alpha antithrombin absent in beta antithrombin decreases the heparin affinity of the inhibitor by affecting the heparin induced conformational change Biochemistry 36 22 6682 6691 doi 10 1021 bi9702492 PMID 9184148 Frebelius S Isaksson S Swedenborg J 1996 Thrombin inhibition by antithrombin III on the subendothelium is explained by the isoform AT beta Arterioscler Thromb Vasc Biol 16 10 1292 1297 doi 10 1161 01 ATV 16 10 1292 PMID 8857927 van Boven HH Lane DA 1997 Antithrombin and its inherited deficiency states Semin Hematol 34 3 188 204 PMID 9241705 Maclean PS Tait RC 2007 Hereditary and acquired antithrombin deficiency epidemiology pathogenesis and treatment options Drugs 67 10 1429 1440 doi 10 2165 00003495 200767100 00005 PMID 17600391 S2CID 46971091 Lane DA Kunz G Olds RJ Thein SL 1996 Molecular genetics of antithrombin deficiency Blood Rev 10 2 59 74 doi 10 1016 S0268 960X 96 90034 X PMID 8813337 Egeberg O 1965 Inherited antithrombin deficiency causing thrombophilia Thromb Diath Haemorrh 13 2 516 530 doi 10 1055 s 0038 1656297 PMID 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Biochemistry 36 42 13133 13142 doi 10 1021 bi970664u PMID 9335576 Carrell RW Huntington JA Mushunje A Zhou A 2001 The conformational basis of thrombosis Thromb Haemost 86 1 14 22 doi 10 1055 s 0037 1616196 PMID 11487000 S2CID 21452323 a b c Zhou A Huntington JA Carrell RW 1999 Formation of the antithrombin heterodimer in vivo and the onset of thrombosis Blood 94 10 3388 3396 doi 10 1182 blood V94 10 3388 422k20 3388 3396 PMID 10552948 Larsson H Akerud P Nordling K Raub Segall E Claesson Welsh L Bjork I 2001 A novel anti angiogenic form of antithrombin with retained proteinase binding ability and heparin affinity J Biol Chem 276 15 11996 12002 doi 10 1074 jbc M010170200 PMID 11278631 O Reilly MS 2007 Antiangiogenic antithrombin Semin Thromb Hemost 33 7 660 666 doi 10 1055 s 2007 991533 PMID 18000792 S2CID 260321466 O Reilly MS Pirie Shepherd S Lane WS Folkman J 1999 Antiangiogenic activity of the cleaved conformation of the serpin antithrombin Science 285 5435 1926 1928 doi 10 1126 science 285 5435 1926 PMID 10489375 Further reading editPanzer Heinig Sabine 2009 Antithrombin III Establishing Pediatric Reference Values Relevance for DIC 1992 versus 2007 Thesis Medizinische Fakultat Charite Universitatsmedizin Berlin External links editThe MEROPS online database for peptidases and their inhibitors I04 018 Antithrombin III at the U S National Library of Medicine Medical Subject Headings MeSH Human SERPINC1 genome location and SERPINC1 gene details page in the UCSC Genome Browser Retrieved from https en wikipedia org w index php title Antithrombin amp oldid 1190755270, wikipedia, wiki, book, books, library,

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