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人血小板血浆和细胞内膜钙离子泵对胰蛋白酶的不同敏感性。

Different sensitivity to trypsin of the human platelet plasma and intracellular membrane Ca2+ pumps.

作者信息

Enouf J, Lompré A M, Bredoux R, Bourdeau N, de La Bastie D, Levy-Toledano S

机构信息

U-150 Institut National de la Santé et de la Recherche Médicale, Hôpital Lariboisière, Paris, France.

出版信息

J Biol Chem. 1988 Sep 25;263(27):13922-9.

PMID:2458355
Abstract

The Ca2+ pumps associated with human platelet plasma and intracellular membranes have been further characterized by their sensitivity to trypsin. (a) Tryptic degradation of the Ca2+-ATPases has been followed by immunoblotting. It resulted in fragmentation into peptides of 80, 55, 35, and 24 kDa for both enzymes. Subcomplete hydrolysis obtained with a ratio of trypsin/membrane protein of 0.05-0.1 for the two Ca2+ pumps resulted in the total disappearance of the 100-, 80-, and 35-kDa fragments. However, maximum degradation was reached within 1 min for the intracellular enzyme but needed 5 min of incubation for the plasma membrane enzyme. (b) This effect of trypsin has been correlated with its effect on both the Ca2+-ATPase activities. The plasma membrane enzyme showed a maximum inhibition of 50-60% which was obtained using a trypsin/protein ratio of 0.1 and 5 min of incubation. A much higher trypsin sensitivity was observed for the intracellular enzyme because the maximum inhibition reached 80% after only 1 min of incubation. (c) Finally, the two Ca2+ transport systems studied showed different trypsin reactivities; the Ca2+ uptake by the plasma membrane vesicles was inhibited by 20-25%, and this maximum inhibition was observed after 5 min of incubation with trypsin. In contrast, the Ca2+ transport associated with the intracellular membrane vesicles was difficult to detect after trypsin treatment. Taken together, the results show that the two Ca2+ pumps can be distinguished by their trypsin sensitivity.

摘要

与人类血小板质膜和内膜相关的钙离子泵,已通过其对胰蛋白酶的敏感性得到进一步表征。(a) 通过免疫印迹追踪了钙离子ATP酶的胰蛋白酶降解情况。两种酶均导致裂解为80、55、35和24 kDa的肽段。对于两种钙离子泵,当胰蛋白酶与膜蛋白的比例为0.05 - 0.1时获得的不完全水解,导致100 kDa、80 kDa和35 kDa片段完全消失。然而,细胞内酶在1分钟内达到最大降解,而质膜酶则需要孵育5分钟。(b) 胰蛋白酶的这种作用与其对两种钙离子ATP酶活性的影响相关。质膜酶在胰蛋白酶与蛋白质比例为0.1且孵育5分钟的情况下,显示出最大50 - 60%的抑制率。细胞内酶对胰蛋白酶的敏感性更高,因为仅孵育1分钟后最大抑制率就达到了80%。(c) 最后,所研究的两种钙离子转运系统显示出不同的胰蛋白酶反应性;质膜囊泡对钙离子的摄取受到20 - 25%的抑制,在用胰蛋白酶孵育5分钟后观察到这种最大抑制。相比之下,胰蛋白酶处理后与内膜囊泡相关的钙离子转运很难检测到。综上所述,结果表明两种钙离子泵可通过其对胰蛋白酶的敏感性来区分。

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