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将高分辨率小DNA片段从聚丙烯酰胺凝胶高效转移至重氮苄氧甲基纸。

Efficient transfer of highly resolved small DNA fragments from polyacrylamide gels to DBM paper.

作者信息

Levy A, Frei E, Noll M

出版信息

Gene. 1980 Nov;11(3-4):283-90. doi: 10.1016/0378-1119(80)90068-2.

Abstract

A procedure is described that combines high resolution of small DNA molecules (10 to 250 bases) with high transfer efficiency from polyacrylamide gels to diazobenzyloxymethyl (DBM) paper. The DNA fragments are separated electrophoretically in denaturing or nondenaturing step gels. These consist of a short gel of relatively high polyacrylamide concentration (8%) above a long gel of relatively low polyacrylamide concentration (4%). Step gels permit a high resolution of small DNA fragments in gels of sufficiently low polyacrylamide concentration from which efficient transfer to DBM paper is feasible. The combination of the step gel with a short treatment of the gel before transfer ensures a high transfer efficiency. As much as 30% and 50% of the DNA applied to nondenaturing and denaturing gels, respectively, are bound covalently to the DBM-paper. Optimal conditions for hybridization to DBM-linked DNA molecules of 30 to 250 base length are described.

摘要

本文描述了一种程序,该程序将小DNA分子(10至250个碱基)的高分辨率与从聚丙烯酰胺凝胶到重氮苄氧基甲基(DBM)纸的高转移效率相结合。DNA片段在变性或非变性梯度凝胶中进行电泳分离。这些梯度凝胶由一个相对高聚丙烯酰胺浓度(8%)的短凝胶置于一个相对低聚丙烯酰胺浓度(4%)的长凝胶之上组成。梯度凝胶能够在足够低聚丙烯酰胺浓度的凝胶中对小DNA片段进行高分辨率分离,从而实现向DBM纸的高效转移。梯度凝胶与转移前对凝胶的简短处理相结合可确保高转移效率。分别施加到非变性和变性凝胶上的DNA中,多达30%和50%共价结合到DBM纸上。文中还描述了与长度为30至250个碱基的DBM连接的DNA分子杂交的最佳条件。

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