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野生型粗糙脉孢菌质膜的分离与鉴定

Isolation and characterization of plasma membranes from wild type Neurospora crassa.

作者信息

Bowman E J, Bowman B J, Slayman C W

出版信息

J Biol Chem. 1981 Dec 10;256(23):12336-42.

PMID:6457833
Abstract

A method has been developed to isolate plasma membranes with high ATPase activity from wild type Neurospora. Cells are treated with snail enzyme to weaken their cell walls, disrupted by gentle homogenization in a medium designed to keep mitochondria and other organelles intact, and fractionated by differential centrifugation. After removal of mitochondria, several higher speed particulate fractions (particularly one sedimenting at 40,000 X g) contain an ATPase that can be identified as the plasma membrane enzyme on the basis of sensitivity to vanadate and kinetic properties. Its [S]0.5 for Mg.ATP, specificity for nucleotides and divalent cations, and pH optimum are virtually identical with those reported previously for plasma membrane ATPase from the slime mutant of Neurospora (Bowman, B. J., and Slayman, C. W. (1977) J. Biol. Chem. 252, 3357-3363). By contrast, ATPase specific activities in the wild type plasma membranes are much higher than in slime, ranging up to 7.3 mumol/min/mg of protein (the highest value yet reported for Neurospora). The best preparations appear homogeneous upon sucrose density gradient centrifugation, and band at an equilibrium density of 1.15 g/cm3. Two other markers, chitin synthetase and [acetyl-3H] concanavalin A binding, show approximate co-purification with the plasma membrane ATPase through membrane fractionation and sucrose gradient centrifugation.

摘要

已开发出一种从野生型脉孢菌中分离具有高ATP酶活性的质膜的方法。用蜗牛酶处理细胞以削弱其细胞壁,在一种旨在保持线粒体和其他细胞器完整的培养基中通过温和匀浆使其破碎,然后通过差速离心进行分级分离。去除线粒体后,几个更高速度的颗粒级分(特别是在40,000×g下沉淀的一个级分)含有一种ATP酶,根据其对钒酸盐的敏感性和动力学特性可鉴定为质膜酶。其对Mg.ATP的[S]0.5、对核苷酸和二价阳离子的特异性以及最适pH与先前报道的脉孢菌黏液突变体质膜ATP酶的几乎相同(鲍曼,B.J.,和斯莱曼,C.W.(1977年)《生物化学杂志》252,3357 - 3363)。相比之下,野生型质膜中的ATP酶比活性远高于黏液突变体,高达7.3 μmol/分钟/毫克蛋白质(脉孢菌迄今报道的最高值)。最佳制剂在蔗糖密度梯度离心时看起来均匀,并且在平衡密度为1.15 g/cm³处形成条带。另外两个标志物,几丁质合成酶和[乙酰 - ³H]伴刀豆球蛋白A结合,在通过膜分级分离和蔗糖梯度离心时与质膜ATP酶显示出大致共纯化。

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