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构建更好的纤维蛋白 knob 模拟物:在溶液中研究合成纤维蛋白 knob 肽结构及其与纤维蛋白原/纤维蛋白孔的动态结合。

Building better fibrin knob mimics: an investigation of synthetic fibrin knob peptide structures in solution and their dynamic binding with fibrinogen/fibrin holes.

机构信息

W. H. Coulter Department of Biomedical Engineering, Georgia Institute of Technology/Emory University, Atlanta, GA 30332, USA.

出版信息

Blood. 2010 Aug 26;116(8):1352-9. doi: 10.1182/blood-2009-11-251801. Epub 2010 May 18.

DOI:10.1182/blood-2009-11-251801
PMID:20484082
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2938242/
Abstract

Fibrin polymerizes via noncovalent and dynamic association of thrombin-exposed "knobs" with complementary "holes." Synthetic knob peptides have received significant interest as a means for understanding fibrin assembly mechanisms and inhibiting fibrin polymerization. Nevertheless, the inability to crystallize short peptides significantly limits our understanding of knob peptide structural features that regulate dynamic knob:hole interactions. In this study, we used molecular simulations to generate the first predicted structure(s) of synthetic knobs in solution before fibrin hole engagement. Combining surface plasmon resonance (SPR), we explored the role of structural and electrostatic properties of knob "A" mimics in regulating knob:hole binding kinetics. SPR results showed that association rates were most profoundly affected by the presence of both additional prolines as well as charged residues in the sixth to seventh positions. Importantly, analyzing the structural dynamics of the peptides through simulation indicated that the 3Arg side chain orientation and peptide backbone stability each contribute significantly to functional binding. These findings provide insights into early fibrin protofibril assembly dynamics as well as establishing essential design parameters for high-affinity knob mimics that more efficiently compete for hole occupancy, parameters realized here through a novel knob mimic displaying a 10-fold higher association rate than current mimics.

摘要

纤维蛋白通过凝血酶暴露的“栓钉”与互补的“孔”之间的非共价和动态结合进行聚合。合成栓钉肽作为一种理解纤维蛋白组装机制和抑制纤维蛋白聚合的手段引起了广泛关注。然而,由于短肽无法结晶,这极大地限制了我们对调节栓钉:孔相互作用的栓钉肽结构特征的理解。在这项研究中,我们使用分子模拟在纤维蛋白孔结合之前生成了第一个预测的合成栓钉在溶液中的结构。我们结合表面等离子体共振(SPR),探索了栓钉“A”模拟物的结构和静电特性在调节栓钉:孔结合动力学中的作用。SPR 结果表明,关联速率受第六至第七位额外脯氨酸和带电荷残基的存在的影响最大。重要的是,通过模拟分析肽的结构动力学表明,3Arg 侧链取向和肽骨架稳定性都对功能结合有重要贡献。这些发现为早期纤维蛋白原纤维组装动力学提供了深入了解,并为高亲和力栓钉模拟物建立了必要的设计参数,这些模拟物更有效地竞争孔占据,通过显示出比现有模拟物高 10 倍的结合速率的新型栓钉模拟物实现了这些参数。

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Integrin specificity and enhanced cellular activities associated with surfaces presenting a recombinant fibronectin fragment compared to RGD supports.与RGD载体相比,整合素特异性及与呈现重组纤连蛋白片段的表面相关的增强细胞活性。
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The structure of fibrinogen fragment D with the 'A' knob peptide GPRVVE.带有“A”旋钮肽GPRVVE的纤维蛋白原片段D的结构
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Folding very short peptides using molecular dynamics.使用分子动力学折叠极短肽段。
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