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体外和体内高度交联的人纤维蛋白形成的α-聚合物结构

Structure of alpha-polymer from in vitro and in vivo highly cross-linked human fibrin.

作者信息

Fretto L J, McKee P A

出版信息

J Biol Chem. 1978 Sep 25;253(18):6614-22.

PMID:150419
Abstract

Peptides derived from plasmic and cyanogen bromide (CNBr) cleavage of highly cross-linked fibrin were isolated and characterized by sodium dodecyl sulfate-gel electrophoresis, amino acid analyses, cyanoethylation, and NH2-terminal analyses. Extended plasmic digestions of human fibrin containing four epsilon-(gamma-glutamyl)lysine cross-links per molecule produced a peptide of alpha-chain origin (Mr congruent to 21,000) which was comprised of a small donor peptide cross-linked to the acceptor site peptide from the middle of the alpha-chain. CNBr cleavage of highly cross-linked in vitro fibrin or of fibrin from a spontaneously formed in vivo arterial embolus produced about three cross-linked species of molecular weights 30,000 to 40,000, each of which contained the largest CNBr fragment (Mr = 29,000) from the alpha-chain. The predominant cross-link-containing CNBr fragments derived their donor group from the near COOH-terminal region of the alpha-chain as judged by difference amino acid compositions and NH2-terminal analyses. Additionally, cross-linked fragments of molecular weights 68,000 to 70,000 which appeared to contain two acceptor site peptides (Mr = 29,000) were detected in minor amounts in the CNBr digests of fibrin formed from whole plasma or from purified, plasminogen-free fibrinogen. No larger polymeric cross-linked CNBr fragment was generated from any of the highly cross-linked fibrin preparations examined. A model for the predominant mode of alpha-chain polymerization is proposed.

摘要

从高度交联的纤维蛋白经血浆酶解和溴化氰(CNBr)裂解得到的肽段,通过十二烷基硫酸钠 - 凝胶电泳、氨基酸分析、氰乙基化和氨基末端分析进行分离和表征。对每分子含有四个ε - (γ - 谷氨酰基)赖氨酸交联的人纤维蛋白进行延长的血浆酶解,产生了一个α链来源的肽段(Mr约为21,000),它由一个小的供体肽与来自α链中部的受体位点肽交联组成。对高度交联的体外纤维蛋白或来自体内自发形成的动脉栓子中的纤维蛋白进行CNBr裂解,产生了约三种分子量为30,000至40,000的交联物种,每种都包含来自α链的最大CNBr片段(Mr = 29,000)。通过氨基酸组成差异和氨基末端分析判断,主要的含交联的CNBr片段的供体基团来自α链的近羧基末端区域。此外,在由全血浆或纯化的、无纤溶酶原的纤维蛋白原形成的纤维蛋白的CNBr消化物中,少量检测到分子量为68,000至70,000的似乎含有两个受体位点肽(Mr = 29,000)的交联片段。在所检查的任何高度交联的纤维蛋白制剂中均未产生更大的聚合交联CNBr片段。提出了α链聚合主要模式的模型。

相似文献

1
Structure of alpha-polymer from in vitro and in vivo highly cross-linked human fibrin.体外和体内高度交联的人纤维蛋白形成的α-聚合物结构
J Biol Chem. 1978 Sep 25;253(18):6614-22.
2
Localization of the alpha-chain cross-link acceptor sites of human fibrin.人纤维蛋白α链交联受体位点的定位
J Biol Chem. 1978 Apr 10;253(7):2184-95.
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Identification of a site in fibrin(ogen) which is involved in the acceleration of plasminogen activation by tissue-type plasminogen activator.鉴定纤维蛋白(原)中一个与组织型纤溶酶原激活物加速纤溶酶原激活有关的位点。
Biochim Biophys Acta. 1983 Oct 17;748(1):86-92. doi: 10.1016/0167-4838(83)90030-4.
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Primary structure of human fibrinogen and fibrin. Structural studies on NH2-terminal part of B beta chain.人纤维蛋白原和纤维蛋白的一级结构。Bβ链氨基末端部分的结构研究。
Eur J Biochem. 1979 Aug 1;98(2):521-34. doi: 10.1111/j.1432-1033.1979.tb13213.x.
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Amino acid sequence studies on the alpha chain of human fibrinogen. Isolation and characterization of two linked alpha-chained cyanogen bromide fragments from fully cross-linked fibrin.人纤维蛋白原α链的氨基酸序列研究。从完全交联的纤维蛋白中分离并鉴定两个相连的α链溴化氰片段。
Biochemistry. 1977 Apr 19;16(8):1715-9. doi: 10.1021/bi00627a030.

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Platelet binding to polymerizing fibrin is avidity driven and requires activated αIIbβ3 but not fibrin cross-linking.血小板与聚合纤维蛋白的结合是由亲合力驱动的,需要激活的 αIIbβ3,但不需要纤维蛋白交联。
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Dominant role of αIIbβ3 in platelet interactions with cross-linked fibrin fragment D-dimer.
αIIbβ3 在血小板与交联纤维蛋白片段 D-二聚体相互作用中的主要作用。
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Rapid formation of large molecular weight alpha-polymers in cross-linked fibrin induced by high factor XIII concentrations. Role of platelet factor XIII.高浓度因子XIII诱导交联纤维蛋白中大分子α聚合物的快速形成。血小板因子XIII的作用。
J Clin Invest. 1987 Nov;80(5):1459-65. doi: 10.1172/JCI113226.