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抗栓酶抗凝机制。对纤维蛋白的直接蛋白水解作用。

Mechanism of ancrod anticoagulation. A direct proteolytic effect on fibrin.

作者信息

Pizzo S V, Schwartz M L, Hill R L, McKee P A

出版信息

J Clin Invest. 1972 Nov;51(11):2841-50. doi: 10.1172/JCI107107.

Abstract

Fibrin formed in response to ancrod, reptilase, or thrombin was reduced by beta-mercaptoethanol and examined by sodium dodecyl sulfate polyacrylamide gel electrophoresis. It was found that ancrod progressively and totally digested the alpha-chains of fibrin monomers at sites different than plasmin; however, further digestion of fibrin monomers by either reptilase or thrombin was not observed. Highly purified ancrod did not activate fibrin-stabilizing factor (FSF); however, the reptilase preparation used in these experiments, like thrombin, activated FSF and thereby promoted cross-link formation. Fibrin, formed by clotting purified human fibrinogen with ancrod, reptilase, or thrombin for increasing periods of time in the presence of plasminogen, was incubated with urokinase and observed for complete lysis. Fibrin formed by ancrod was strikingly more vulnerable to plasmin digestion than was fibrin formed by reptilase or thrombin. The lysis times for fibrin formed for 2 hr by ancrod, reptilase, or thrombin were 18, 89, and 120 min, respectively. Evidence was also obtained that neither ancrod nor reptilase activated human plasminogen. These results indicate that fibrin formed by ancrod is not cross-linked and has significantly degraded alpha-chains: as expected, ancrod-formed fibrin is markedly susceptible to digestion by plasmin.

摘要

由抗栓酶、蛇毒凝血酶或凝血酶诱导形成的纤维蛋白可被β-巯基乙醇降解,并通过十二烷基硫酸钠聚丙烯酰胺凝胶电泳进行检测。结果发现,抗栓酶能在与纤溶酶不同的位点逐步且完全地消化纤维蛋白单体的α链;然而,未观察到蛇毒凝血酶或凝血酶对纤维蛋白单体的进一步消化作用。高度纯化的抗栓酶不会激活纤维蛋白稳定因子(FSF);然而,本实验中所用的蛇毒凝血酶制剂,与凝血酶一样,能激活FSF,从而促进交联形成。在纤溶酶原存在的情况下,用抗栓酶、蛇毒凝血酶或凝血酶使纯化的人纤维蛋白原凝血不同时间形成纤维蛋白,再与尿激酶一起孵育,并观察其完全溶解情况。抗栓酶形成的纤维蛋白比蛇毒凝血酶或凝血酶形成的纤维蛋白对纤溶酶消化作用的敏感性明显更高。抗栓酶、蛇毒凝血酶或凝血酶作用2小时形成的纤维蛋白的溶解时间分别为18、89和120分钟。还获得证据表明,抗栓酶和蛇毒凝血酶均不能激活人纤溶酶原。这些结果表明,抗栓酶形成的纤维蛋白未发生交联且α链已显著降解:正如预期的那样,抗栓酶形成的纤维蛋白对纤溶酶消化作用明显敏感。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3705/292433/fc0a0485fa45/jcinvest00206-0073-a.jpg

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