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在由两性缓冲剂二元混合物构成的人工pH梯度中对蛋白质进行密度梯度等电聚焦。

Density gradient isoelectric focusing of proteins in artificial pH gradients made up of binary mixtures of amphoteric buffers.

作者信息

Tulp A, Verwoerd D, Hart A A

机构信息

The Netherlands Cancer Institute, Antoni van Leeuwenhoekhuis, Department of Cellular Biochemistry, Amsterdam.

出版信息

Electrophoresis. 1997 May;18(5):767-73. doi: 10.1002/elps.1150180518.

DOI:10.1002/elps.1150180518
PMID:9194604
Abstract

A density gradient electrophoresis apparatus made of Perspex (7 cm, O 2.2 cm) with a circular platinum anode and a palladium cathode was used for the separation of proteins in free liquid. Following a concept developed by M. Bier et al. (Electrophoresis 1993, 14, 1011-1018), mixtures of two suitable amphoteric buffers I and II provide for media with a fixed and electrophoretically stable pH or were used for the generation of preformed (electrophoretically stable) pH gradients covering about 1 pH unit. Amphoters I and II are considered suitable if there is overlap between (pK(1,1)-1-2) and the pK(2,II)+1+2) region. 3-(N-Morpholino)propanesulfonic acid (MOPS) and gamma-amino-n-butyric acid (GABA) were used as an example. Two approaches were followed: (i) rate-zonal separation of test proteins in a pH window, formed by a fixed ratio of MOPS/GABA. (ii) Isoelectric focusing in a shallow preformed pH gradient, made up of inverse reciprocal linear gradients of MOPS and GABA. At isopH, test proteins (bovine serum albumin, cytochrome c, ferritin, hemoglobin, lactoglobulin, myoglobin, and transferrin) were rate-zonally separated within a short time. Even the separation of the A and B forms of lactoglobulin was feasible at isopH. The glycoforms of transferrin were separated and enriched on a pH 5.2-6.1 pH gradient, indicating that pH differences of about 0.01 still permit resolution. Contrary to the ill-defined Ampholines, the cost of these well-defined amphoters is low.

摘要

一个由有机玻璃制成(7厘米,外径2.2厘米)、带有圆形铂阳极和钯阴极的密度梯度电泳仪用于在自由液体中分离蛋白质。遵循M. Bier等人提出的概念(《电泳》,1993年,第14卷,1011 - 1018页),两种合适的两性缓冲液I和II的混合物可提供具有固定且电泳稳定pH值的介质,或用于生成覆盖约1个pH单位的预制(电泳稳定)pH梯度。如果(pK(1,I) - 1 - 2)和(pK(2,II) + 1 + 2)区域存在重叠,则两性电解质I和II被认为是合适的。以3 -(N - 吗啉代)丙磺酸(MOPS)和γ - 氨基 - n - 丁酸(GABA)为例。采用了两种方法:(i)在由MOPS/GABA固定比例形成的pH窗口中对测试蛋白质进行速率区带分离。(ii)在由MOPS和GABA的反向倒数线性梯度组成的浅预制pH梯度中进行等电聚焦。在等pH值下,测试蛋白质(牛血清白蛋白、细胞色素c、铁蛋白、血红蛋白、乳球蛋白、肌红蛋白和转铁蛋白)在短时间内被速率区带分离。甚至在等pH值下分离乳球蛋白的A和B形式也是可行的。转铁蛋白的糖型在pH 5.2 - 6.1的pH梯度上被分离和富集,这表明约0.01的pH差异仍能实现分离。与定义不明确的两性电解质不同,这些定义明确的两性电解质成本较低。

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