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心肌钙蛋白酶2被针对小的非催化亚基的单克隆抗体所抑制。

Myocardial calpain 2 is inhibited by monoclonal antibodies specific for the small, noncatalytic subunit.

作者信息

Mellgren R L, Lane R D

机构信息

Department of Pharmacology, Medical College of Ohio, Toledo 43699.

出版信息

Biochim Biophys Acta. 1988 May 18;954(2):154-60. doi: 10.1016/0167-4838(88)90066-0.

Abstract

Calpains (EC 3.4.22.17) are nonlysosomal intracellular proteinases which require calcium ion for activity. The calpains are heterodimers composed of a large catalytic subunit and a small subunit which may have a regulatory function during the catalytic cycle. However, whether calpains remain in the dimeric form or dissociate upon exposure to calcium is controversial. To resolve this issue, two monoclonal antibodies which specifically recognize the small calpain subunit were prepared using bovine calpain 2 heterodimer as the antigen. Both antibodies, designated P-1 and P-2, were capable of inhibiting bovine or canine calpain 2, and partially purified human erythrocyte calpain 1. However, neither could produce full inhibition. Further studies with P-1 and bovine calpain 2 indicated that the antibody decreased the calcium requirement for the proteinase. The Km for casein was increased and the Vmax was decreased. The addition of P-1 to the assay mixture several minutes after initiation of proteolytic activity resulted in a rapid inhibition. The P-1 antibody was also capable of decreasing the ability of the protein inhibitor of calpains (calpastatin) to inhibit bovine calpain 2. These studies indicate that the small subunit remains bound to the large subunit during catalysis and may influence its activity.

摘要

钙蛋白酶(EC 3.4.22.17)是一种非溶酶体胞内蛋白酶,其活性需要钙离子。钙蛋白酶是由一个大的催化亚基和一个小亚基组成的异二聚体,小亚基在催化循环中可能具有调节功能。然而,钙蛋白酶在暴露于钙离子时是保持二聚体形式还是解离,这存在争议。为了解决这个问题,以牛钙蛋白酶2异二聚体为抗原制备了两种特异性识别钙蛋白酶小亚基的单克隆抗体。这两种抗体分别命名为P-1和P-2,它们能够抑制牛或犬的钙蛋白酶2以及部分纯化的人红细胞钙蛋白酶1。然而,两者都不能产生完全抑制作用。对P-1和牛钙蛋白酶2的进一步研究表明,该抗体降低了蛋白酶对钙离子的需求。酪蛋白的米氏常数(Km)增加,最大反应速度(Vmax)降低。在蛋白水解活性开始几分钟后向测定混合物中加入P-1会导致快速抑制。P-1抗体还能够降低钙蛋白酶的蛋白抑制剂(钙蛋白酶抑制蛋白)抑制牛钙蛋白酶2的能力。这些研究表明,小亚基在催化过程中仍与大亚基结合,并且可能影响其活性。

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