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通过免疫亲和色谱联用技术分离维生素B-12结合蛋白。对分离和未分离蛋白的比较研究。

Isolation of vitamin B-12-binding proteins by combined immuno and affinity chromatography. Comparative studies on the isolated and unisolated proteins.

作者信息

Marcoullis G, Salonen E M, Gräsbeck R

出版信息

Biochim Biophys Acta. 1977 Dec 20;495(2):336-48. doi: 10.1016/0005-2795(77)90389-0.

Abstract

Intrinsic factor or cobalophilin were removed by incubating human gastric juice and pig pyloric extract with purified anti-intrinsic factor and anti-cobalophilin immunoglobulin-G, respectively, covalently coupled to Sepharose. Cobalophilin (transcobalamin I) was also removed from pig serum either by using anti-cobalophilin immunoglobulin-G Sepharose or by Sephadex G-200 chromatography. The one remaining semipurified vitamin B-12-binding protein (intrinsic factor, cobalophilin or transcobalamin II) was then isolated by vitamin B-12-Sepharose affinity chromatography. Intrinsic factors, cobalophilins and transcobalamin II isolated by this two-step procedure were compared by double isotope techniques with the corresponding protein not subjected to affinity chromatography and found to be identical in reaction to antiserum, gel filtration and electrofocusing. The avidity of the isolated and unisolated intrinsic factors for the ileal intrinsic factor receptor was also the same.

摘要

通过分别将人胃液和猪幽门提取物与共价偶联到琼脂糖凝胶上的纯化抗内因子和抗钴胺素免疫球蛋白G一起孵育,去除内因子或钴胺素结合蛋白。也可通过使用抗钴胺素免疫球蛋白G琼脂糖凝胶或通过葡聚糖凝胶G-200色谱法从猪血清中去除钴胺素结合蛋白(转钴胺素I)。然后通过维生素B-12琼脂糖凝胶亲和色谱法分离剩余的一种半纯化的维生素B-12结合蛋白(内因子、钴胺素结合蛋白或转钴胺素II)。通过双同位素技术将通过此两步法分离的内因子、钴胺素结合蛋白和转钴胺素II与未进行亲和色谱的相应蛋白质进行比较,发现它们在与抗血清反应、凝胶过滤和等电聚焦方面是相同的。分离的和未分离的内因子对回肠内因子受体的亲和力也是相同的。

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