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大鼠甲胎蛋白的微观异质性

Microheterogeneity of rat alpha-fetoprotein.

作者信息

Watanabe A, Taketa K, Kosaka K

出版信息

Ann N Y Acad Sci. 1975 Aug 22;259:95-108. doi: 10.1111/j.1749-6632.1975.tb25406.x.

Abstract

A purified and homogeneous preparation of rat AFP, as judged by both electrophoresis on Cellogel and immunoelectrophoresis, was separated into two components, AFPa and AFPb, by disc electrophoresis on 7% polyacrylamide gel. These two components had a definite difference in electrostatic net charge and gave only a single band on SDS-electrophoresis. Immunological reactivity or electrophoretic separation or mobility of the two components could be altered by treatment with either sulfhydryl inhibitors or reducing agents but not by treatment with protein denaturants. Electrophoresis of neuraminidase-treated AFP on 5% polyacrylamide gel yielded clearly separable, slower moving four to six and finally two components depending on the time of incubation with neuraminidase. The time-dependent conversion of faster into slower migrating components of both AFPa and AFPb upon neuraminidase treatment was confirmed by reelectrophoresis of separated and similarly treated AFPa and AFPb. Two bands of sialized or desialized AFP were also observed on isoelectric focusing. Both AFPa and AFPb treated with and without neuraminidase gave single fused precipitin lines against the antiserum in Ouchterlony double-diffusion analysis. On the basis of the changes in electrophoretic mobilities of the intermediates following neuraminidase treatment, AFPa and AFPb were estimated to have at least 2.5 and 4.5 molecules of sialic acid per molecule, respectively.

摘要

通过在Cellogel上的电泳和免疫电泳判断,一种纯化且均一的大鼠甲胎蛋白制剂,在7%聚丙烯酰胺凝胶上进行圆盘电泳时被分离成两个组分,即甲胎蛋白a(AFPa)和甲胎蛋白b(AFPb)。这两个组分在静电荷方面有明确差异,在SDS电泳中仅呈现一条带。用巯基抑制剂或还原剂处理可改变这两个组分的免疫反应性、电泳分离或迁移率,但用蛋白质变性剂处理则无此效果。用神经氨酸酶处理后的甲胎蛋白在5%聚丙烯酰胺凝胶上进行电泳,根据与神经氨酸酶孵育的时间不同,可清晰分离出迁移较慢的四到六个组分,最终为两个组分。通过对分离并经类似处理的AFPa和AFPb进行再电泳,证实了神经氨酸酶处理后AFPa和AFPb中较快迁移组分向较慢迁移组分的时间依赖性转化。在等电聚焦中也观察到了两条唾液酸化或去唾液酸化甲胎蛋白的条带。在Ouchterlony双向扩散分析中,无论是否用神经氨酸酶处理,AFPa和AFPb与抗血清反应均产生单一融合沉淀线。根据神经氨酸酶处理后中间体电泳迁移率的变化,估计AFPa和AFPb每分子分别至少含有2.5个和4.5个唾液酸分子。

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