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从高血压大鼠心脏中纯化和鉴定两种不同的钙激活蛋白酶。

Purification and characterization of two distinct Ca2+-activated proteinases from hearts of hypertensive rats.

作者信息

Spalla M, Tsang W, Kuo T H, Giacomelli F, Wiener J

出版信息

Biochim Biophys Acta. 1985 Aug 23;830(3):258-66. doi: 10.1016/0167-4838(85)90281-x.

Abstract

Two distinct Ca2+-activated proteinases were purified and characterized from hearts of hypertensive rats. Ca2+-activated proteinases I and II, having low and high Ca2+ requirements, respectively, were first separated by DEAE-cellulose chromatography. The enzymes were then purified individually by different column procedures: chromatography on phenyl-Sepharose, then Sephadex G-200 for proteinase I and reactive-red agarose for proteinase II. The apparent molecular weight of purified proteinase I was 125 000 and that for purified proteinase II was 110 000. Both enzymes are heterodimers made up of a larger catalytic subunit and a smaller subunit devoid of proteinase activity. Ca2+ concentrations for half-maximal activation were 5 microM for proteinase I and 200 microM for proteinase II. Both enzymes were inhibited by sulfhydryl-modifying agents, but exhibited different characteristics in the auto-digestion reaction in the presence of Ca2+. Proteinases I and II were also purified from hearts of normotensive rats and shown to be identical to their respective counterparts from hearts of hypertensive rats. However, proteinase II activity in hypertensive rat hearts was significantly elevated as compared to controls.

摘要

从高血压大鼠心脏中纯化并鉴定出两种不同的钙激活蛋白酶。钙激活蛋白酶I和II,分别具有低和高的钙需求,首先通过DEAE-纤维素色谱法分离。然后通过不同的柱程序分别纯化这些酶:蛋白酶I用苯基-琼脂糖色谱,然后用Sephadex G-200;蛋白酶II用活性红琼脂糖。纯化的蛋白酶I的表观分子量为125000,纯化的蛋白酶II的表观分子量为110000。两种酶都是异二聚体,由一个较大的催化亚基和一个没有蛋白酶活性的较小亚基组成。蛋白酶I的半最大激活钙浓度为5微摩尔,蛋白酶II为200微摩尔。两种酶都被巯基修饰剂抑制,但在钙存在下的自消化反应中表现出不同的特性。蛋白酶I和II也从正常血压大鼠心脏中纯化出来,并被证明与高血压大鼠心脏中的相应酶相同。然而,与对照组相比,高血压大鼠心脏中的蛋白酶II活性显著升高。

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