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将蛋白质从变性或天然凝胶中同时电洗脱到孔状基质中。

Simultaneous electroelution of proteins from denaturing or native gels into a well matrix.

作者信息

Persidis A, Harcombe A A

机构信息

University of Cambridge Clinical School, Department of Medicine, Addenbrooke's Hospital, England.

出版信息

Anal Biochem. 1992 Feb 14;201(1):185-9. doi: 10.1016/0003-2697(92)90193-b.

Abstract

An electroelution device that is based on a semidry blotter and that allows the simultaneous elution of proteins or other charged macromolecules from one-dimensional gels is described. It consists of a central plate that has a matrix of oblong wells arranged in eight columns of 32 wells each, such that when a gel is placed on the plate each lane of bands is underlaid by a column of wells. The plate is placed between the electrodes of a semidry blotter and the wells are sealed by a dialysis membrane resting on polyacrylamide gel block, prior to being filled with transfer buffer. Using radiolabeled molecular weight standards resolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, elution is shown to require 30-60 min for 90% or better of proteins between 10 and 120 kDa to be removed from the gel. The recovery volume is 200 microliters per well and losses due to adsorption onto the dialysis membrane are minimal. beta-Galactosidase eluted from a nonreducing, nondenaturing gel was shown to be quantitatively active. The advantages of the device include its ease of assembly and operation, its speed, its reproducibility, and the fact that no gel slicing is required since all proteins are eluted simultaneously, allowing large-scale screening of multiple protein fractions.

摘要

本文描述了一种基于半干印迹仪的电洗脱装置,该装置可同时从一维凝胶中洗脱蛋白质或其他带电大分子。它由一个中心板组成,中心板上有一个长方形孔矩阵,排列成8列,每列32个孔,这样当凝胶放在板上时,每条带的泳道下面都有一列孔。将该板置于半干印迹仪的电极之间,在向孔中加入转移缓冲液之前,用置于聚丙烯酰胺凝胶块上的透析膜密封这些孔。使用经十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分离的放射性标记分子量标准品,结果表明,对于10至120 kDa之间的蛋白质,90%或更多的蛋白质从凝胶中洗脱出来需要30至60分钟。每个孔的回收体积为200微升,因吸附到透析膜上造成的损失极小。从非还原、非变性凝胶中洗脱的β-半乳糖苷酶显示具有定量活性。该装置的优点包括易于组装和操作、速度快、可重复性好,以及由于所有蛋白质同时洗脱,无需切割凝胶,从而可对多个蛋白质组分进行大规模筛选。

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