[人红细胞RHoD抗原分子质量的分离和测定]。

Bilten za hematologiju i transfuziju Pub Date : 1984-01-01
V D Miletić, M Saracević
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引用次数: 0

摘要

采用2-巯基乙醇和非离子洗涤剂brij35膜增溶法从人红细胞中分离出RhoD抗原。初始用pH为12的水处理膜,不能溶解D抗原,证明D抗原是红细胞膜的一种完整蛋白。采用超滤法和凝胶过滤法研究D抗原分子质量。用超滤法测定了10-20 000道尔顿的分子质量,用凝胶过滤法测定了32 700道尔顿的分子质量。在Sephadex G-25上凝胶过滤,测定D抗原分子质量小于25 000,约为14 000道尔顿。凝胶过滤和超滤两种测定方法之间的差异可能是由于D抗原球形实际上不表达。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
[Isolation and determination of the molecular mass of the RHoD antigen in human erythrocytes].

RhoD antigen was isolated from human erythrocytes using membrane solubilization by 2-mercaptoethanol and nonionic detergents BRIJ 35. Initial treatment of membrane using water at pH 12, failed to solubilize D antigen, which proved that D antigen is an integral protein of erythrocyte membrane. D antigen molecule mass was investigated by ultrafiltration and gelfiltration. Molecular mass was determined by ultrafiltration in the range of 10-20 000 daltons, and by gelfiltration on Sephacryl S--200 as 32 700. Using gelfiltration on Sephadex G-25, D antigen molecular mass was determined to be less than 25 000 and was approximately 14 000 daltons. Discrepancy between those two ways of determination by gelfiltration and ultrafiltration could be explained by the possibility that D antigen globularity is practically unexpressed.

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