The complete N-terminal extension of heparin cofactor II is required for maximal effectiveness as a thrombin exosite 1 ligand

Boyle, Amanda J.; Roddick, Leigh Ann; Bhakta, Varsha; Lambourne, Melissa D.; Junop, M.S.; Liaw, Patricia C.; Weitz, Jeffrey I.; Sheffield, William P.

doi:10.1186/1471-2091-14-6

Cited by 6 publications

(13 citation statements)

References 47 publications

(62 reference statements)

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“…A small recombinant protein, 84 amino acids in size, comprising residues 1-75 of HCII with an N-terminal nonapeptide tag MSGH 6 (designated HCII 1-75), was expressed in a pBAD-based plasmid and purified from sonicated cell lysates by nickel-chelate affinity chromatography as described [ 36 ].…”

Section: Methodsmentioning

confidence: 99%

“…Human citrated plasma was combined in a 1:3:5 volume ratio of plasma: veronal buffer: Thrombin 10 calcified thrombin reagent, and the time to clot was determined. The veronal buffer (sodium acetate trihydrate 7.14 mM/ sodium diethyl barbiturate 7.4 mM/ NaCl 0.131 M pH7.4) was employed with or without supplementation with purified recombinant serpins or synthetic peptides, as described [ 36 ].…”

Section: Methodsmentioning

confidence: 99%

“…A previously described assay was employed in order to characterize the relative affinity of recombinant serpins and peptides for either α-thrombin or α-thrombin rendered inactive at its active site by incubation with FPR-chloromethylketone [ 36 ]. Briefly, purified HCII 1-75 was immobilized on microtiter plates and purified human α-thrombin was incubated with or without competitor peptides or proteins.…”

Section: Methodsmentioning

confidence: 99%

“…The acidic extension of HCII accelerates thrombin inhibition by binding to thrombin exosite 1, a cluster of charged residues involved in binding thrombin co-factors such as thrombomodulin and substrates such as fibrinogen and coagulation factor V [ 30 ]. This deduction is supported by: a partially resolved X-ray crystal structure of the HCII-S195A thrombin structure [ 31 ]; reduced rates of inhibition of HCII and HCII fusion proteins on exosite-1-disrupted forms of thrombin [ 32 - 35 ]; and direct binding studies of either HCII 1-75 or its smaller derivatives [ 36 , 37 ]. The leech anticoagulant protein hirudin is the most potent known polypeptide inhibitor of thrombin [ 38 ], and owes some of its high affinity for thrombin to the binding of its 11-13 C-terminal residues, depending on the isoform [ 39 ], to thrombin exosite 1.…”

Section: Introductionmentioning

confidence: 99%

“…The leech anticoagulant protein hirudin is the most potent known polypeptide inhibitor of thrombin [ 38 ], and owes some of its high affinity for thrombin to the binding of its 11-13 C-terminal residues, depending on the isoform [ 39 ], to thrombin exosite 1. We [ 36 ] and others [ 37 ] have demonstrated that hirudin C-terminal peptides bind more tightly to thrombin than HCII 1-75 or its derivatives. Accordingly, in the current study we tested the primary hypothesis that fusion of the C-terminal 13 amino acids of hirudin variant 3 (HV3), the most potent hirudin isoform [ 39 ], to API M358R, would increase the rate of thrombin inhibition of API M358R by conferring on this mutant serpin the ability to bind thrombin exosite 1.…”

Section: Introductionmentioning

confidence: 99%

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Fusion of the C-terminal triskaidecapeptide of hirudin variant 3 to alpha1-proteinase inhibitor M358R increases the serpin-mediated rate of thrombin inhibition

2013

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BackgroundAlpha-1 proteinase inhibitor (API) is a plasma serpin superfamily member that inhibits neutrophil elastase; variant API M358R inhibits thrombin and activated protein C (APC). Fusing residues 1-75 of another serpin, heparin cofactor II (HCII), to API M358R (in HAPI M358R) was previously shown to accelerate thrombin inhibition over API M358R by conferring thrombin exosite 1 binding properties. We hypothesized that replacing HCII 1-75 region with the 13 C-terminal residues (triskaidecapeptide) of hirudin variant 3 (HV354-66) would further enhance the inhibitory potency of API M358R fusion proteins. We therefore expressed HV3API M358R (HV354-66 fused to API M358R) and HV3API RCL5 (HV354-66 fused to API F352A/L353V/E354V/A355I/I356A/I460L/M358R) API M358R) as N-terminally hexahistidine-tagged polypeptides in E. coli.ResultsHV3API M358R inhibited thrombin 3.3-fold more rapidly than API M358R; for HV3API RCL5 the rate enhancement was 1.9-fold versus API RCL5; neither protein inhibited thrombin as rapidly as HAPI M358R. While the thrombin/Activated Protein C rate constant ratio was 77-fold higher for HV3API RCL5 than for HV3API M358R, most of the increased specificity derived from the API F352A/L353V/E354V/A355I/I356A/I460L API RCL 5 mutations, since API RCL5 remained 3-fold more specific than HV3API RCL5. An HV3 54-66 peptide doubled the Thrombin Clotting Time (TCT) and halved the binding of thrombin to immobilized HCII 1-75 at lower concentrations than free HCII 1-75. HV3API RCL5 bound active site-inhibited FPR-chloromethyl ketone-thrombin more effectively than HAPI RCL5. Transferring the position of the fused HV3 triskaidecapeptide to the C-terminus of API M358R decreased the rate of thrombin inhibition relative to that mediated by HV3API M358R by 11-to 14-fold.ConclusionsFusing the C-terminal triskaidecapeptide of HV3 to API M358R-containing serpins significantly increased their effectiveness as thrombin inhibitors, but the enhancement was less than that seen in HCII 1-75–API M358R fusion proteins. HCII 1-75 was a superior fusion partner, in spite of the greater affinity of the HV3 triskaidecapeptide, manifested both in isolated and API-fused form, for thrombin exosite 1. Our results suggest that HCII 1-75 binds thrombin exosite 1 and orients the attached serpin scaffold for more efficient interaction with the active site of thrombin than the HV3 triskaidecapeptide.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%