Purification of the i-antigen 51A fromParamecium tetraurelia by immunoaffinity chromatography

Richard H. Davis Jr., Edward Steers Jr.
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引用次数: 8

Abstract

Purification of the surface antigen ofParamecium tetraurelia (termed i-antigen) by previously published procedures has been shown to result in preparations which frequently contain contaminating proteins including a thiol-activated protease. Alternate procedures for the purification of i-antigen were developed using ion-exchange chromatography. While certain of these procedures result in a homogeneous preparation of i-antigen, the poor yields obtained make these procedures impractical. An alternate method for the purification of i-antigen was developed using immunoaffinity chromatography. Purification by this technique proved to be superior to the various standard procedures described previously. The immunoaffinity column is rapid and results in a recovery, on the average, of over 95% of the applied material. The columns are readily regenerated and may be used numerous times without loss of capacity or purification ability. The i-antigen purified by this method appears homogeneous immunologically and electrophoretically on polyacrylamide gel electrophoresis and isoelectric focusing.

免疫亲和层析法纯化四甲草履虫i抗原51A
通过先前公布的程序纯化四片草履虫表面抗原(称为i-抗原)已被证明会导致制备中经常含有污染蛋白质,包括硫醇活化蛋白酶。采用离子交换色谱法纯化i抗原。虽然某些程序导致i抗原的均匀制备,但获得的低产量使这些程序不切实际。采用免疫亲和层析法纯化i抗原。经证明,该技术的纯化优于前面描述的各种标准程序。免疫亲和柱是快速的,结果回收率,平均而言,超过95%的应用材料。柱很容易再生,可以多次使用而不损失容量或净化能力。该方法纯化的i抗原在聚丙烯酰胺凝胶电泳和等电聚焦上具有均匀的免疫和电泳特性。
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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