Structural Architecture of Prothrombin in Solution Revealed by Single Molecule Spectroscopy

Pozzi, Nicola; Bystranowska, Dominika; Zuo, Xiaobing; Di, Enrico

doi:10.1074/jbc.m116.738310

Cited by 36 publications

(60 citation statements)

References 49 publications

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“…Notably, the subtilisin cleavage sites in ProT perfectly match with the regions of highest segmental flexibility of the zymogen, as deduced from the B-factor plot of the crystallographic structure in the solid state (4) and single-molecule FRET studies in solution ( Fig. 3C) (31). In particular, CS-1 and CS-2 are embedded in the highly dynamic inter-domain linker regions, whereas CS-3 is in the highly flexible 148-loop of the Pre2 domain ( Fig.…”

Section: Limited Proteolysis Of Prot By Subtilisinmentioning

confidence: 99%

“…3) (4,32), corresponding to the autolysis loop in the mature ␣T (33). Of note, the structure of ProT we used here is that of the zymogen deletion mutant, ProT⌬(154 -167), solved at 2.2-Å resolution and lacking 14 amino acids in the linker-2 region, while retaining the conformational properties of the wild-type ProT in the extended conformation (29,31). A key aspect that emerges by comparing the time-course increase of hydrolytic activity at 37°C (Fig.…”

Section: Limited Proteolysis Of Prot By Subtilisinmentioning

confidence: 99%

“…difference can be accounted for by the following: (i) the lower number of subtilisin cleavages sites present on Pre2 structure compared with ProT; (ii) the lack of glycosylation at Asn-60g that in the natural glycosylated ProT is expected protect the zymogen from subtilisin cleavage (30); and (iii) the possible shielding of the 148-loop operated by the N-terminal F1 region, which in the solution structure of ProT has been proposed to fold back on the Pre2 domain (31).…”

Section: Limited Proteolysis Of Rpre2 By Subtilisinmentioning

confidence: 99%

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Non-canonical proteolytic activation of human prothrombin by subtilisin from Bacillus subtilis may shift the procoagulant–anticoagulant equilibrium toward thrombosis

Pontarollo

Acquasaliente

Peterle

et al. 2017

Journal of Biological Chemistry

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Blood coagulation is a finely regulated physiological process culminating with the factor Xa (FXa)-mediated conversion of the prothrombin (ProT) zymogen to active ␣-thrombin (␣T). In the prothrombinase complex on the platelet surface, FXa cleaves ProT at Arg-271, generating the inactive precursor prethrombin-2 (Pre2), which is further attacked at Arg-320 -Ile-321 to yield mature ␣T. Whereas the mechanism of physiological ProT activation has been elucidated in great detail, little is known about the role of bacterial proteases, possibly released in the bloodstream during infection, in inducing blood coagulation by direct proteolytic ProT activation. This knowledge gap is particularly concerning, as bacterial infections are frequently complicated by severe coagulopathies. Here, we show that addition of subtilisin (50 nM to 2 M), a serine protease secreted by the non-pathogenic bacterium Bacillus subtilis, induces plasma clotting by proteolytically converting ProT into active Pre2, a nicked Pre2 derivative with a single cleaved Ala-470 -Asn-471 bond. Notably, we found that this non-canonical cleavage at Ala-470 -Asn-471 is instrumental for the onset of catalysis in Pre2, which was, however, reduced about 100 -200-fold compared with ␣T. Of note, Pre2 could generate fibrin clots from fibrinogen, either in solution or in blood plasma, and could aggregate human platelets, either isolated or in whole blood. Our findings demonstrate that alternative cleavage of ProT by proteases, even by those secreted by non-virulent bacteria such as B. subtilis, can shift the delicate procoagulant-anticoagulant equilibrium toward thrombosis.Blood coagulation is a finely regulated physiological process that culminates with the factor Xa-mediated conversion of the prothrombin (ProT) 3 zymogen to the active ␣-thrombin (␣T) enzyme, which in turn is responsible for the generation of insoluble fibrin and activation of platelets via the GpIb␣-PAR1 pathway (1, 2). ProT (ϳ72 kDa) is a vitamin K-dependent glycoprotein produced in the liver and circulating at a relatively high plasma concentration (0.1 mg/ml) (3). The domain architecture of ProT includes a Gla domain (residues 1-46), a kringle-1 (residues 65-143) and a kringle-2 (residues 170 -248) domain, and a chymotrypsin-like protease domain (residues 285-579) connected by three intervening linker regions (Lnk-1, -2, and -3) (4). Isolated factor Xa (FXa) has low intrinsic ProTconverting activity, but when it is assembled in the presence of Ca 2ϩ with cofactor Va in the prothrombinase complex on the platelet surface, its ability to activate ProT is increased by about 5 orders of magnitude (5). FXa cleaves ProT in a concerted manner at two sites, i.e. Arg-271 and Arg-320, but the order of peptide bond cleavage is highly context-dependent. On the platelet surface, FXa first cleaves ProT at Arg-271 generating the inactive precursor prethrombin-2 (Pre2), which is attacked by FXa at Arg-320 to generate the active ␣T species, formed by the polypeptide chains Thr-272-Arg-320 and Ile-321-Glu-579 (6). ...

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Section: Limited Proteolysis Of Prot By Subtilisinmentioning

confidence: 99%

Section: Limited Proteolysis Of Prot By Subtilisinmentioning

confidence: 99%

Section: Limited Proteolysis Of Rpre2 By Subtilisinmentioning

confidence: 99%

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Non-canonical proteolytic activation of human prothrombin by subtilisin from Bacillus subtilis may shift the procoagulant–anticoagulant equilibrium toward thrombosis

Pontarollo

Acquasaliente

Peterle

et al. 2017

Journal of Biological Chemistry

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“…The high ionic strength used in the crystallization buffers may destabilize hydrogen bonds and favor hydrophobic interactions thus forcing the protein to assume a non-native conformation(2). To address this concern, we applied smFRET to β 2 GPI(37, 41, 42). By recording the energy that is transferred from an excited molecule (Donor) to a second molecule with spectral overlap (Acceptor) at the single molecule level, smFRET measures distances on a nanometer scale thus serving as a molecular ruler.…”

Section: Resultsmentioning

confidence: 99%

X-ray and solution structures of human beta-2 glycoprotein I reveal a new mechanism of autoantibody recognition

Ruben

Planer

Chinnaraj

et al. 2020

Preprint

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31Venous and arterial thromboses in patients suffering from the autoimmune disorder Antiphospholipid 32 Syndrome (APS) are caused by the presence of antiphospholipid antibodies (aPL). Emerging evidence 33 indicates that autoantibodies targeting the epitope R39-R43 in the N-terminal domain, Domain I (DI), of 34 b2-glycoprotein I (b2GPI) are among the most pathogenic aPL in patients with APS. How such 35 autoantibodies engage b2GPI at the molecular level remains incompletely understood. Here, we have 36 used X-ray crystallography, single-molecule FRET, and small-angle X-ray scattering to demonstrate that, 37 in the free form, under physiological pH and salt concentrations, human recombinant b2GPI adopts an 38 elongated, flexible conformation in which DI is exposed to the solvent, thus available for autoantibody 39 recognition. Consistent with this structural model, binding and mutagenesis studies revealed that the 40 elongated form interacts with a pathogenic anti-DI antibody in solution, without the need of phospholipids. 41Furthermore, complex formation was affected neither by the neighboring domains, nor by the presence 42 of the linkers, nor by the glycosylations. Since the pathogenic autoantibody requires residues R39 and 43 R43 for optimal binding, these findings challenge longstanding postulates in the field envisioning b2GPI 44 adopting immunologic inert conformations featuring inaccessibility of the epitope R39-R43 in DI and 45 support an alternative model whereby the preferential binding of anti-DI antibodies towards phospholipid-46 bound b2GPI arises from the ability of the pre-existing elongated form to bind to the membranes and then 47 oligomerize, processes that are likely to be supported by protein conformational changes. Interfering with 48 these steps may limit the pathogenic effects of anti-DI antibodies in APS patients. 503 Significance 51In the autoimmune disorder called Antiphospholipid Syndrome (APS), the presence of autoantibodies 52 targeting the plasma glycoprotein beta-2 glycoprotein I (b2GPI) is associated with arterial and venous 53 thrombosis as well as pregnancy complications. Understanding how b2GPI becomes immunogenic and 54 how autoantibodies in complex with b2GPI cause the blood to clot remains a top priority in the field. By 55 elucidating the structural architecture of b2GPI free in solution, our studies challenge longstanding 56 postulates in the field and shed new light on the pathogenic mechanisms of APS that may help the 57 development of new diagnostics and therapeutic approaches.58 59 4 Introduction 60β2GPI is a 50-kDa multi-domain glycoprotein that circulates in the plasma at a concentration of 0.2 61 mg/ml(1, 2)( Fig 1A). It acquired centerstage in hematology in 1990 when it was recognized by two 62 independent studies as the dominant antigen of antiphospholipid antibodies (aPL) in the Antiphospholipid 63 Syndrome (APS)(3-5), a life-threatening blood clotting disorder characterized by vascular thrombosis and 64 pregnancy morbidity(6). Autoantibodies against β2GPI (anti-β2...

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“…For this reason, molecules able to inhibit αT activity are the focus of intensive pharmacological research. αT displays a unique surface electrostatic potential (Figure ), generated by the asymmetry of charge distribution, where a negatively charged active‐site region is flanked by two positive patches opposite to the active site, that is, exosites 1 and 2, and responsible for physiological substrates binding . In hemostasis, αT exerts either procoagulant or anticoagulant functions .…”

Section: Incorporation Of Non‐coded Amino Acids For Sar Studies Of Himentioning

confidence: 99%

Protein engineering by chemical methods: Incorporation of nonnatural amino acids as a tool for studying protein folding, stability, and function

et al. 2018

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Proteins are large complex biomolecules that act as the effectors of essentially all cell functions. Due to the intrinsic complexity of protein architecture at the microscopic level and the inadequacy of theoretical methods to predict protein reactivity (ie, folding, stability, and function), protein engineering has emerged as a valuable tool to investigate structure–stability–activity relationships in proteins and nowadays recombinant DNA technologies are the “gold standard” for site‐specifically manipulating a given protein chain. The usefulness of current mutagenesis techniques, however, is limited by the relatively poor chemical diversity of the 20 DNA‐coded amino acids, such that it is difficult to precisely assign the observed change of protein stability or function to the variation of a single physicochemical property at a protein site (ie, hydrophobicity, conformational propensity, polarizability, hydrogen bonding, etc). In this article, we report relevant examples from our laboratory showing that chemical methods, that is, enzyme‐catalyzed semisynthesis and stepwise solid‐phase synthesis, allow to conveniently incorporate non‐natural amino acids with “tailored” side chains into small proteins and thus effectively transfer the structure–activity relationship methodology, typical of the medicinal chemistry approach on small molecules, to the study of folding, stability, and molecular recognition in macromolecular protein systems.

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Structural Architecture of Prothrombin in Solution Revealed by Single Molecule Spectroscopy

Cited by 36 publications

References 49 publications

Non-canonical proteolytic activation of human prothrombin by subtilisin from Bacillus subtilis may shift the procoagulant–anticoagulant equilibrium toward thrombosis

Non-canonical proteolytic activation of human prothrombin by subtilisin from Bacillus subtilis may shift the procoagulant–anticoagulant equilibrium toward thrombosis

X-ray and solution structures of human beta-2 glycoprotein I reveal a new mechanism of autoantibody recognition

Protein engineering by chemical methods: Incorporation of nonnatural amino acids as a tool for studying protein folding, stability, and function

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