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线粒体质子腺苷三磷酸酶的抑制肽。钙调蛋白对其抑制作用的中和。

Inhibitor peptide of mitochondrial proton adenosine triphosphatase. Neutralization of its inhibitory action by calmodulin.

作者信息

Pedersen P L, Hullihen J

出版信息

J Biol Chem. 1984 Dec 25;259(24):15148-53.

PMID:6239865
Abstract

In the presence of ATP and Mg2+, the homogeneous ATPase peptide inhibitor of rat liver mitochondria markedly inhibits the proton ATPase from this source (Cintrón N. M., and Pedersen, P. L. (1979) J. Biol. Chem. 254, 3439-3443). Under these conditions, calmodulin prevents the inhibitor peptide from inhibiting the liver H+-ATPase. About 1.5 mol of calmodulin/mol of inhibitor is necessary to effect a half-maximal response (apparent Km = 0.5 microM calmodulin). The capacity of calmodulin to neutralize the action of the ATPase inhibitor peptide appears highly specific. This effect is not produced by insulin, trypsin inhibitor, lysozyme, ribonuclease, myoglobin, cytochrome c, ovalbumin, or bovine albumin. Only polyglutamate was found to mimic the action of calmodulin. However, when added together with calmodulin, polyglutamate failed to elicit an additive effect indicating that its site of interaction on the ATPase inhibitor peptide differs from that of calmodulin. Calcium is not essential in the assay medium for calmodulin to neutralize the action of the ATPase inhibitor peptide. The neutralization effect produced by calmodulin is also source-independent, with preparations of calmodulin from bovine brain and rat testes being equally competent. Calmodulin has no direct effect on the ATPase activity of the proton ATPase, nor does it affect the capacity of the enzyme to participate in either ATP synthesis or the ATP-dependent transhydrogenase reaction. Moreover, calmodulin fails to reverse inhibition of the H+-ATPase to which ATPase inhibitor peptide is already bound. Overall, these results indicate that calmodulin interacts in a direct and highly specific manner with the "free" ATPase peptide inhibitor of rat liver mitochondria.

摘要

在ATP和Mg2+存在的情况下,大鼠肝脏线粒体的均一ATP酶肽抑制剂能显著抑制该来源的质子ATP酶(辛特龙N.M.和佩德森P.L.(1979年)《生物化学杂志》254卷,3439 - 3443页)。在这些条件下,钙调蛋白可防止该抑制肽抑制肝脏H+-ATP酶。约1.5摩尔钙调蛋白/摩尔抑制剂对于产生半数最大反应是必需的(表观Km = 0.5微摩尔钙调蛋白)。钙调蛋白中和ATP酶抑制肽作用的能力似乎具有高度特异性。胰岛素、胰蛋白酶抑制剂、溶菌酶、核糖核酸酶、肌红蛋白、细胞色素c、卵清蛋白或牛血清白蛋白均不会产生这种效应。仅发现聚谷氨酸能模拟钙调蛋白的作用。然而,当与钙调蛋白一起添加时,聚谷氨酸未能引发相加效应,表明其在ATP酶抑制肽上的相互作用位点与钙调蛋白不同。在测定介质中,钙调蛋白中和ATP酶抑制肽的作用并不必需钙。钙调蛋白产生的中和效应也不依赖于来源,来自牛脑和大鼠睾丸的钙调蛋白制剂同样有效。钙调蛋白对质子ATP酶的ATP酶活性没有直接影响,也不影响该酶参与ATP合成或ATP依赖性转氢酶反应的能力。此外,钙调蛋白无法逆转已与ATP酶抑制肽结合的H+-ATP酶的抑制作用。总体而言,这些结果表明钙调蛋白以直接且高度特异性的方式与大鼠肝脏线粒体的“游离”ATP酶肽抑制剂相互作用。

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