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钙离子结合至凝血因子X轻链的蛋白质结构要求。使用包含γ-羧基谷氨酸区域和/或表皮生长因子样结构域的分离完整片段进行的研究。

Protein structural requirements for Ca2+ binding to the light chain of factor X. Studies using isolated intact fragments containing the gamma-carboxyglutamic acid region and/or the epidermal growth factor-like domains.

作者信息

Persson E, Björk I, Stenflo J

机构信息

Department of Clinical Chemistry, University of Lund, Malmö General Hospital, Sweden.

出版信息

J Biol Chem. 1991 Feb 5;266(4):2444-52.

PMID:1989996
Abstract

Coagulation factor X is a multidomain proenzyme of a serine protease. Calcium ions bind to the vitamin K-dependent gamma-carboxyglutamic acid (Gla) residues and to a site in the NH2-terminal of two epidermal growth factor (EGF)-like domains. To study structure-function relationships in the NH2-terminal part of factor X and to determine the structure of isolated domains, we have developed methods that allow the subsequent isolation of the first or both EGF-like domains with or without an attached Gla domain from controlled proteolytic digests of the protein. The Ca2(+)-induced changes of the intrinsic protein fluorescence were measured to elucidate whether the isolated fragments retain their native conformation. Changes in the fluorescence caused by Ca2+ binding were found to result from perturbations of the environment of the Trp residue in position 41. Calcium ion binding to the Gla-containing region linked to the NH2-terminal EGF-like domain was identical with that to intact factor X, indicating a native orientation of the ligand binding groups in the fragment. In contrast, the isolated Gla peptide had a lower affinity for Ca2+, suggesting that the NH2-terminal EGF-like domain serves as a scaffold for the folding of the Gla region. Similarly, the presence of the Gla region was found to increase the affinity of the Gla-independent site in the first EGF-like domain for Ca2+. The metal ion-induced resistance against chymotryptic cleavage COOH-terminal of Tyr-44 in intact factor X is similar in the isolated fragment that contains the Gla region linked to one EGF-like domain, indicating a native conformation of the fragment in the presence of Ca2+. Furthermore, the Gla-independent metal ion binding site binds Ca2+ but does not appear to bind Mg2+.

摘要

凝血因子X是一种丝氨酸蛋白酶的多结构域酶原。钙离子与维生素K依赖的γ-羧基谷氨酸(Gla)残基以及两个表皮生长因子(EGF)样结构域的NH2末端的一个位点结合。为了研究因子X NH2末端部分的结构-功能关系并确定分离结构域的结构,我们开发了一些方法,这些方法能够从该蛋白的可控蛋白水解消化物中随后分离出带有或不带有连接的Gla结构域的第一个或两个EGF样结构域。测量了Ca2+诱导的内在蛋白荧光变化,以阐明分离的片段是否保留其天然构象。发现由Ca2+结合引起的荧光变化是由41位色氨酸残基环境的扰动导致的。钙离子与连接到NH2末端EGF样结构域的含Gla区域的结合与与完整因子X的结合相同,表明片段中配体结合基团的天然取向。相比之下,分离的Gla肽对Ca2+的亲和力较低,这表明NH2末端EGF样结构域作为Gla区域折叠的支架。同样,发现Gla区域的存在增加了第一个EGF样结构域中与Gla无关的位点对Ca2+的亲和力。在完整因子X中,金属离子诱导的对Tyr-44羧基末端胰凝乳蛋白酶切割的抗性在包含与一个EGF样结构域相连的Gla区域的分离片段中是相似的,这表明在Ca2+存在下片段的天然构象。此外,与Gla无关的金属离子结合位点结合Ca2+,但似乎不结合Mg2+。

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