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纤维蛋白原伯尔尼I:γ337位天冬酰胺替换为赖氨酸导致纤维蛋白单体聚合缺陷。

Fibrinogen Bern I: substitution gamma 337 Asn-->Lys is responsible for defective fibrin monomer polymerization.

作者信息

Steinmann C, Reber P, Jungo M, Lämmle B, Heinemann G, Wermuth B, Furlan M

机构信息

Central Hematology Laboratory, Inselspital, University of Bern, Switzerland.

出版信息

Blood. 1993 Oct 1;82(7):2104-8.

PMID:8400260
Abstract

An inherited fibrinogen variant, fibrinogen Bern I, was isolated from plasma of an asymptomatic woman. Routine coagulation studies showed prolonged thrombin and reptilase clotting times. Fibrinogen concentration was diminished when determined by a functional assay, but was normal by the heat precipitation method. The release of fibrinopeptides A and B was not delayed. Two-dimensional gel electrophoresis of mercaptolyzed fragments D of fibrinogen, obtained by digestion with plasmin, showed an abnormal electrophoretic mobility in the gamma-chain remnants of fragments D1 and D2 from fibrinogen Bern I, whereas conversion of D2 to D3 by plasmin resulted in the loss of the abnormal charge, suggesting that the structural abnormality in this variant is located in the region gamma 303 through 356. The molecular defect in fibrinogen Bern I was identified by sequence analysis of genomic DNA amplified by polymerase chain reaction and cloned in M13mp19. The triplet AAC coding for asparagine at position gamma 337 was found to be substituted by AAA coding for lysine. We conclude that the substitution gamma 337 Asn-->Lys in fibrinogen Bern I is responsible for defective polymerization of fibrin monomers and for impaired protection by calcium against plasmic degradation.

摘要

从一名无症状女性的血浆中分离出一种遗传性纤维蛋白原变体——纤维蛋白原伯尔尼I。常规凝血研究显示凝血酶和蛇毒凝血时间延长。通过功能测定法测定时,纤维蛋白原浓度降低,但通过热沉淀法测定则正常。纤维蛋白肽A和B的释放没有延迟。用纤溶酶消化纤维蛋白原得到的巯基化片段D进行二维凝胶电泳,结果显示纤维蛋白原伯尔尼I的片段D1和D2的γ链残余物电泳迁移异常,而纤溶酶将D2转化为D3导致异常电荷消失,这表明该变体的结构异常位于γ303至356区域。通过聚合酶链反应扩增并克隆到M13mp19中的基因组DNA序列分析,确定了纤维蛋白原伯尔尼I的分子缺陷。发现编码γ位337位天冬酰胺的三联体AAC被编码赖氨酸的AAA替代。我们得出结论,纤维蛋白原伯尔尼I中γ337位天冬酰胺被赖氨酸替代,导致纤维蛋白单体聚合缺陷以及钙对血浆降解的保护作用受损。

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