Separation of functionally or highly pure C2 from human plasma with Sepharose and a lectin of Euonymus europeus.

D R Schultz, P I Arnold
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Abstract

A method is described for isolating both functionally and highly pure C2 from normal human serum or plasma. Functionally pure C2 was obtained by a two-step method of ammonium sulfate (AS) fractionation of plasma or serum and chromatography on AH-Sepharose containing a bound lectin of Euonymus europeus. The functionally pure C2 can be isolated in 2 days, and is used routinely as a reagent for functional hemolytic titrations of C3 and C4 in the Clinical Immunology Laboratory. Highly pure C2 was isolated by the two-step fractionation with AS followed by chromatography on CM-cellulose, aged CNBr-activated Sepharose 4B, and AH-Sepharose-lectin. The major difficulty for isolating highly pure C2 was its separation from Factor B of the alternative complement pathway. The yield of C2 varied from 30 to 40 per cent. Following electrophoresis and staining on polyacrylamide gels, the single band was hemolytically active C2.

用Sepharose和Euonymus凝集素从人血浆中分离功能或高纯度的C2。
描述了一种从正常人血清或血浆中分离功能性和高纯度C2的方法。采用硫酸铵两步法分离血浆或血清,并对含有欧洲卫矛凝集素的AH-Sepharose进行层析,得到功能纯净的C2。功能纯的C2可在2天内分离出来,在临床免疫学实验室常规用作C3和C4的功能溶血滴定试剂。采用AS两步分离,然后在cm -纤维素、老化的cnbr活化的Sepharose 4B和ah -Sepharose-凝集素上进行层析,分离出高纯度的C2。分离高纯度C2的主要困难是它与替代补体途径的因子B的分离。C2的产率从30%到40%不等。在聚丙烯酰胺凝胶上电泳和染色后,单带是溶血活性的C2。
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