Purification and characterisation of the fourth component of bovine complement.

Complement (Basel, Switzerland) Pub Date : 1987-01-01 DOI:10.1159/000463002

D M Groth, J D Wetherall, B A Umotong, P Sparrow, I R Lee, M J Carrick

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引用次数: 6

Abstract

A relatively rapid method for the isolation of complement protein C4 from bovine plasma is described. The method consists of DEAE Sephacel anion exchange chromatography of plasminogen-depleted bovine plasma followed by cation exchange chromatography on CM Sepharose and finally gel filtration on a TSK G3000 SW column. A yield of approximately 20% was obtained. Conventional SDS-PAGE of purified bovine C4 showed the presence of alpha, beta and gamma polypeptide chains, the molecular weights of which were determined from Ferguson plots to be 95,000 +/- 2,500, 80,500 +/- 2,000 and 30,000 +/- 500 daltons, respectively. SDS-PAGE of C4 immunoprecipitated from the plasma of individual cattle in gels with a reduced proportion of crosslinker showed size polymorphism of the alpha chain. The presence of dual alpha chains was confirmed by radiolabelling their reactive thiol ester moiety with 14C methylamine. The difference in size of the two bovine alpha chains is approximately 1,800 daltons. On activation of bovine C4 both alpha chains were cleaved into alpha' chains (87,000 and 85,000 daltons) characteristic of C4b.

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牛补体第四组分的纯化与鉴定。

本文描述了一种从牛血浆中相对快速分离补体蛋白C4的方法。该方法采用DEAE sepphacel阴离子交换层析法，用CM Sepharose进行阳离子交换层析，最后用TSK G3000 SW柱进行凝胶过滤。产率约为20%。纯化牛C4的常规SDS-PAGE显示存在α、β和γ多肽链，其分子量分别为95,000 +/- 2,500、80,500 +/- 2,000和30,000 +/- 500道尔顿。在减少交联剂比例的凝胶中，从牛个体血浆中免疫沉淀C4的SDS-PAGE显示α链的大小多态性。双α链的存在通过用14C甲胺放射性标记其活性硫醇酯部分证实。两种牛α链的大小差异约为1800道尔顿。在牛C4活化后，两个α链被裂解为C4b特征的α '链(87,000道尔顿和85,000道尔顿)。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Complement (Basel, Switzerland)

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