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密封的内翻和外翻质膜囊泡:形成和分离的最佳条件。

Sealed inside-out and right-side-out plasma membrane vesicles : optimal conditions for formation and separation.

作者信息

Palmgren M G, Askerlund P, Fredrikson K, Widell S, Sommarin M, Larsson C

机构信息

Department of Plant Biochemistry, University of Lund, P. O. Box 7007, S-220 07 Lund, Sweden.

出版信息

Plant Physiol. 1990 Apr;92(4):871-80. doi: 10.1104/pp.92.4.871.

Abstract

Plasma membrane preparations of high purity (about 95%) are easily obtained by partitioning in aqueous polymer two-phase systems. These preparations, however, mainly contain sealed right-side-out (apoplastic side out) vesicles. Part of these vesicles have been turned inside-out by freezing and thawing, and sealed inside-out and right-side-out vesicles subsequently separated by repeating the phase partition step. Increasing the KCI concentration in the freeze/thaw medium as well as increasing the number of freeze/thaw cycles significantly increased the yield of inside-out vesicles. At optimal conditions, 15 to 25% of total plasma membrane protein was recovered as inside-out vesicles, corresponding to 5 to 10 milligrams of protein from 500 grams of sugar beet (Beta vulgaris L.) leaves. Based on enzyme latency, trypsin inhibition of NADH-cytochrome c reductase, and H(+) pumping capacity, a cross-contamination of about 20% between the two fractions of oppositely oriented vesicles was estimated. Thus, preparations containing about 80% inside-out and 80% right-side-out vesicles, respectively, were obtained. ATPase activity and H(+) pumping were both completely inhibited by vanadate (K(i) approximately 10 micromolar), indicating that the fractions were completely free from nonplasma membrane ATPases. Furthermore, the polypeptide patterns of the two fractions were close to identical, which shows that the vesicles differed in sidedness only. Thus, preparations of both inside-out and right-side-out plasma membrane vesicles are now available. This permits studies on transport, signal transduction mechanisms, enzyme topology, etc., using plasma membrane vesicles of either orientation.

摘要

通过在水性聚合物双相系统中进行分配,可以轻松获得高纯度(约95%)的质膜制剂。然而,这些制剂主要包含密封的外翻(质外体侧向外)囊泡。其中一部分囊泡通过冻融变成了内翻,随后通过重复相分配步骤将密封的内翻和外翻囊泡分离。增加冻融介质中的KCI浓度以及增加冻融循环次数显著提高了内翻囊泡的产量。在最佳条件下,15%至25%的总质膜蛋白以内翻囊泡的形式回收,相当于从500克甜菜(Beta vulgaris L.)叶片中获得5至10毫克蛋白质。根据酶潜伏性、胰蛋白酶对NADH-细胞色素c还原酶的抑制作用以及H(+)泵送能力,估计两种相反取向囊泡组分之间的交叉污染约为20%。因此,分别获得了含有约80%内翻和80%外翻囊泡的制剂。钒酸盐(K(i)约为10微摩尔)完全抑制了ATPase活性和H(+)泵送,表明这些组分完全不含非质膜ATPase。此外,两种组分的多肽模式几乎相同,这表明囊泡仅在膜面性上有所不同。因此,现在可以获得内翻和外翻质膜囊泡的制剂。这使得能够使用任何一种取向的质膜囊泡研究转运、信号转导机制、酶拓扑结构等。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b061/1062389/cfb60b8b209d/plntphys00677-0018-a.jpg

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