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蛋白质等速电泳

Isotachophoresis of proteins.

作者信息

Acevedo F

出版信息

J Chromatogr. 1989 May 26;470(2):407-14. doi: 10.1016/s0021-9673(01)83569-x.

Abstract

The analytical separation of proteins by isotachophoresis (ITP) was achieved in a short electrophoretic path and with a resolution comparable to that of isoelectric focusing by the appropriate selection of (1) a mixture of ampholytes as spacers to generate linear gradients of electrophoretic mobility and (2) the counter ions chosen to buffer the complete pH gradient generated. This ITP technique is exemplified by the analysis of plasma proteins in agarose gels. Upto 46 samples in the same gel plate were analysed. The resolution was such that at least 30 clear and discrete bands per sample could be observed after staining with Coomassie Brilliant Blue. The resolving power of ITP could be further increased for the study of a particular protein or zone by the selection of suitable spacers and counter ions.

摘要

通过等速电泳(ITP)对蛋白质进行分析分离,是在较短的电泳路径中实现的,并且通过适当选择(1)两性电解质混合物作为间隔物以产生电泳迁移率的线性梯度,以及(2)选择用于缓冲所产生的完整pH梯度的抗衡离子,其分辨率可与等电聚焦相媲美。这种ITP技术以琼脂糖凝胶中血浆蛋白的分析为例。在同一凝胶板上分析了多达46个样品。分辨率使得用考马斯亮蓝染色后,每个样品至少可以观察到30条清晰且离散的条带。通过选择合适的间隔物和抗衡离子,ITP的分辨能力可进一步提高,以用于研究特定的蛋白质或区域。

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