Enzyme immunoassay of calpain I and calpastatin and its application to the analysis of human erythrocyte hemolysate.

Journal of applied biochemistry Pub Date : 1984-06-01
E Takano, A Kitahara, R Kannagi, T Murachi
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Abstract

A highly sensitive sandwich enzyme immunoassay for a Ca2+-dependent cysteine proteinase (calpain I) and its specific endogenous inhibitor protein (calpastatin) was developed. The calpain I and calpastatin used as immunogens were purified from human erythrocytes. Anti-calpastatin antisera having sufficiently high titer were obtained only when the immunogen was purified by preparative sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The assay method was principally based on the report by M. Imagawa et al. (1982, J. Appl. Biochem. 4, 41-57), using a specific antibody-coated polystyrene ball and horseradish peroxidase-conjugated Fab' fragment of the antibody. The sensitivity was 0.1 ng of calpain I or calpastatin per assay tube. Starting with 50 microliter of the hemolysate from human erythrocytes, the method permitted direct and simultaneous determination of calpain I and calpastatin, without prior separation of these two enzymatically counteracting components by chromatography. The present method as applied to the erythrocytes from 14 healthy adults gave 120-170 micrograms for calpain I and 164-211 micrograms for calpastatin per gram of hemoglobin, respectively.

钙蛋白酶I和钙pastatin的酶免疫分析及其在人红细胞溶血分析中的应用。
开发了一种高灵敏度的夹心酶免疫分析法,用于检测Ca2+依赖性半胱氨酸蛋白酶(calpain I)及其特异性内源性抑制剂蛋白(calpastatin)。作为免疫原的钙蛋白酶I和钙pastatin是从人红细胞中纯化出来的。免疫原经制备性十二烷基硫酸钠-聚丙烯酰胺凝胶电泳纯化后,获得了足够高滴度的抗钙pastatin抗血清。测定方法主要基于M. Imagawa等人(1982年)的报告。使用特异性抗体包被的聚苯乙烯球和辣根过氧化物酶偶联的抗体Fab'片段。灵敏度为每管0.1 ng calpain I或calpastatin。从50微升人红细胞的溶血液开始,该方法允许直接和同时测定钙蛋白酶I和钙pastatin,而无需事先用色谱法分离这两种酶抵消成分。本方法应用于14名健康成人的红细胞,每克血红蛋白中钙蛋白酶I含量为120 ~ 170微克,钙pastatin含量为164 ~ 211微克。
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