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钙可增强因子Xa的活性,且此作用不依赖于γ-羧基谷氨酸残基。

Calcium enhances factor Xa activity independent of gamma-carboxyglutamic acid residues.

作者信息

Sherrill G B, Meade J B, Kalayanamit T, Monroe D M, Church F C

机构信息

Division of Hematology, University of North Carolina School of Medicine, Chapel Hill 27599.

出版信息

Thromb Res. 1988 Oct 1;52(1):53-60. doi: 10.1016/0049-3848(88)90040-0.

Abstract

We investigated the gamma-carboxyglutamic acid (Gla) independent effect of calcium on the activity of human factor Xa. The effect of calcium on the reaction rate of factor Xa was compared using native and Gla-modified forms of human factor Xa [chemically decarboxylated (Gla-modified, 10 Gla residues modified/mol) and Gla-domainless (chymotrypsin-treated)]. Factor Xa activity was assessed by hydrolysis of a synthetic tripeptide nitroanilide substrate, by p-aminobenzamidine binding to the active site and by inhibition with antithrombin III. Calcium (1 mM) increased, by 25-35%, the amidolytic hydrolysis rates of all three factor Xa derivatives. Calcium had an apparent Kd of approximately 200 uM with both native and modified forms of factor Xa. However, there was no change in binding of p-aminobenzamidine, a small fluorescent probe, to factor Xa in the presence of calcium. Calcium (1 mM) increased the inhibition reaction rates of native and modified forms of factor Xa with antithrombin III by 20-30%. Magnesium (1 mM) showed greatly reduced effects on factor Xa activity relative to activities with calcium. We conclude that Gla-independent calcium interactions with factor Xa are important for some catalytic activities of this blood coagulation protease.

摘要

我们研究了钙对人凝血因子Xa活性的γ-羧基谷氨酸(Gla)非依赖性作用。使用天然形式和Gla修饰形式的人凝血因子Xa[化学脱羧(Gla修饰,每摩尔10个Gla残基被修饰)和无Gla结构域(经胰凝乳蛋白酶处理)]比较了钙对凝血因子Xa反应速率的影响。通过合成三肽硝基苯胺底物的水解、对氨基苯甲脒与活性位点的结合以及抗凝血酶III的抑制作用来评估凝血因子Xa的活性。钙(1 mM)使所有三种凝血因子Xa衍生物的酰胺水解速率提高了25% - 35%。钙与天然和修饰形式的凝血因子Xa的表观解离常数(Kd)约为200 μM。然而,在有钙存在的情况下,小荧光探针对氨基苯甲脒与凝血因子Xa的结合没有变化。钙(1 mM)使天然和修饰形式的凝血因子Xa与抗凝血酶III的抑制反应速率提高了20% - 30%。相对于钙的作用,镁(1 mM)对凝血因子Xa活性的影响大大降低。我们得出结论,钙与凝血因子Xa的Gla非依赖性相互作用对于这种血液凝固蛋白酶的某些催化活性很重要。

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