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一种改进的纯化2',5'-寡腺苷酸合成酶的方法。

An improved method for purifying 2',5'-oligoadenylate synthetases.

作者信息

Wells J A, Swyryd E A, Stark G R

出版信息

J Biol Chem. 1984 Jan 25;259(2):1363-70.

PMID:6693390
Abstract

We describe a new, rapid, and convenient procedure for purifying 2',5'-oligoadenylate synthetases, employing precipitation with ammonium sulfate, fractionation by gel filtration, rapid binding to poly(I) X poly(C) cellulose, and elution with 0.35 M KCl. Unlike previously published methods, the procedure does not require sedimentation of the enzyme at 200,000 X g. Therefore, it is more general and more likely to succeed with synthetases extracted from a variety of cells or tissues, or from different subcellular fractions. We have purified the enzymes from two sources to apparent homogeneity, about 2500-fold from the cytoplasm of HeLa cells in 40% yield and more than 400,000-fold from the cytoplasm of rabbit reticulocytes in 25% yield. The specific activity of the HeLa enzyme is about 4 times higher than reported previously. The physical and functional properties of the pure enzymes are very similar to those reported by others for preparations of 2',5'-oligoadenylate synthetase from rabbit reticulocytes, mouse L cells, and human HeLa cells. A new affinity matrix was prepared by linking periodate-oxidized poly(I) X poly(C) to a hydrazide derivative of finely divided cellulose. Poly(I) X poly(C) cellulose binds about twice as much synthetase as the corresponding amount of poly(I) X poly(C) paper and activates the bound enzyme about three times better.

摘要

我们描述了一种新的、快速且便捷的纯化2',5'-寡腺苷酸合成酶的方法,该方法采用硫酸铵沉淀、凝胶过滤分级分离、快速结合到聚(I)×聚(C)纤维素上,并用0.35 M KCl洗脱。与先前发表的方法不同,该方法不需要在200,000×g下对酶进行沉降。因此,它更具通用性,更有可能成功用于从多种细胞或组织,或不同亚细胞组分中提取的合成酶。我们已从两种来源纯化出酶,达到表观均一性,从HeLa细胞胞质中纯化的酶回收率为40%,纯化倍数约为2500倍;从兔网织红细胞胞质中纯化的酶回收率为25%,纯化倍数超过400,000倍。HeLa酶的比活性比先前报道的高约4倍。纯化酶的物理和功能特性与其他人报道的从兔网织红细胞、小鼠L细胞和人HeLa细胞制备的2',5'-寡腺苷酸合成酶的特性非常相似。通过将高碘酸盐氧化的聚(I)×聚(C)与细碎纤维素的酰肼衍生物连接,制备了一种新的亲和基质。聚(I)×聚(C)纤维素结合的合成酶量约为相应量聚(I)×聚(C)纸的两倍,并且对结合酶的激活效果约为其3倍。

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