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大鼠肝脏线粒体质子ATP酶:一种使用改良氯仿法纯化稳定的、具有重组活性的F1制剂的快速方法。

Proton ATPase of rat liver mitochondria: a rapid procedure for purification of a stable, reconstitutively active F1 preparation using a modified chloroform method.

作者信息

Williams N, Amzel L M, Pedersen P L

出版信息

Anal Biochem. 1984 Aug 1;140(2):581-8. doi: 10.1016/0003-2697(84)90210-0.

Abstract

A method is described for the purification of rat liver F1-ATPase by a modification of the chloroform extraction procedure originally described by Beechey et al. (Biochem. J. (1975) 148, 533). Purified liver membrane vesicles are extracted with chloroform in the presence of ATP and EDTA. The procedure yields pure F1 in only 2-3 h without the necessity of ion-exchange chromatography. The enzyme exhibits the alpha, beta, gamma, delta, and epsilon bands characteristic of F1-ATPase. It has a high ATPase specific activity, and is reconstitutively active, catalyzing high rates of ATP synthesis. Significantly, it can be readily crystallized. If desired, the enzyme can be passed over a gel filtration column to place it in a stabilizing phosphate-EDTA buffer, lyophilized and stored indefinitely at -20 degrees C.

摘要

本文描述了一种通过改进最初由Beechey等人(《生物化学杂志》(1975年)148卷,533页)描述的氯仿提取方法来纯化大鼠肝脏F1 - ATP酶的方法。在ATP和EDTA存在的情况下,用氯仿提取纯化的肝膜囊泡。该方法仅需2 - 3小时就能得到纯的F1,无需离子交换色谱法。该酶呈现出F1 - ATP酶特有的α、β、γ、δ和ε条带。它具有高ATP酶比活性,并且具有重组活性,能催化高速率的ATP合成。值得注意的是,它很容易结晶。如果需要,该酶可以通过凝胶过滤柱,置于稳定的磷酸盐 - EDTA缓冲液中,冻干并在 - 20℃下无限期储存。

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