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有证据表明,无配体的人纤溶酶原的构象是通过kringle 5的赖氨酸结合位点与N端肽之间的分子内相互作用来维持的。

Evidence that the conformation of unliganded human plasminogen is maintained via an intramolecular interaction between the lysine-binding site of kringle 5 and the N-terminal peptide.

作者信息

Cockell C S, Marshall J M, Dawson K M, Cederholm-Williams S A, Ponting C P

机构信息

University of Oxford, Laboratory of Molecular Biophysics, Department of Biochemistry, Rex Richards Building, South Parks Road, Oxford OX1 3QU, U.K.

出版信息

Biochem J. 1998 Jul 1;333 ( Pt 1)(Pt 1):99-105. doi: 10.1042/bj3330099.

Abstract

Human Glu-plasminogen adopts at least three conformations that provide a means for regulating the specificity of its activation in vivo. It has been proposed previously that the closed (alpha) conformation of human Glu-plasminogen is maintained through physical interaction of the kringle 5 domain and a lysine residue within the N-terminal peptide (NTP). To examine this hypothesis, site-directed mutagenesis was used to generate variant proteins containing substitutions either for aspartic acid residues within the anionic centre of the kringle 5 domain or for conserved lysine residues within the NTP. Size-exclusion HPLC and rates of plasminogen activation by urokinase-type plasminogen activator were used to determine the conformational states of these variants. Variants with substitutions within the kringle 5 lysine-binding site demonstrated extended conformations, as did variants with alanine substitutions for Lys50 and Lys62. In contrast, molecules in which NTP residues Lys20 or Lys33 were replaced were shown to adopt closed conformations. We conclude that the lysine-binding site of kringle 5 is involved in maintaining the closed conformation of human Glu-plasminogen via an interaction with the NTP, probably through Lys50 and/or Lys62. These conclusions advance the current model for the initial stages of fibrinolysis during which fibrin is thought to compete with the NTP for the kringle 5 lysine-binding site.

摘要

人谷氨酸纤溶酶原至少采用三种构象,这为调节其在体内激活的特异性提供了一种方式。先前有人提出,人谷氨酸纤溶酶原的封闭(α)构象是通过kringle 5结构域与N端肽(NTP)内的一个赖氨酸残基的物理相互作用来维持的。为了验证这一假设,采用定点诱变技术生成了变体蛋白,这些变体蛋白要么是kringle 5结构域阴离子中心内的天冬氨酸残基被取代,要么是NTP内保守的赖氨酸残基被取代。使用尺寸排阻高效液相色谱法和尿激酶型纤溶酶原激活剂激活纤溶酶原的速率来确定这些变体的构象状态。在kringle 5赖氨酸结合位点有取代的变体表现出伸展构象,用丙氨酸取代Lys50和Lys62的变体也是如此。相比之下,NTP残基Lys20或Lys33被取代的分子被证明采用封闭构象。我们得出结论,kringle 5的赖氨酸结合位点通过与NTP相互作用,可能通过Lys50和/或Lys62,参与维持人谷氨酸纤溶酶原的封闭构象。这些结论推进了目前关于纤维蛋白溶解初始阶段的模型,在此阶段,纤维蛋白被认为与NTP竞争kringle 5赖氨酸结合位点。

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