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酵母DNA依赖性RNA聚合酶I。一种大规模纯化均一酶的快速方法。

Yeast DNA-dependent RNA polymerase I. A rapid procedure for the large scale purification of homogeneous enzyme.

作者信息

Valenzuela P, Weinberg F, Bell G, Rutter W J

出版信息

J Biol Chem. 1976 Mar 10;251(5):1464-70.

PMID:767334
Abstract

A procedure has been developed for the rapid purification of large amounts of yeast RNA polymerase I (A). The method involves batchwise treatment with phosphocellulose and DEAE-cellulose, ion filtration chromatography on DEAE-Sephadex, sucrose gradient centrifugation, and DNA-cellulose chromatography. The enzyme obtained is apparently homogeneous by sedimentation velocity analysis and has a specific activity of 300 nmol of UMP incorporated into RNA in 10 min per mg of protein. Between 30 and 45 mg of enzyme can be obtained in 5 days from 3.0 kg of yeast cells. The subunit composition of the enzyme was determined by polyacrylamide gel electrophoresis in the presence of 0.1% sodium dodecyl sulfate. The purified polymerase is composed of 11 putative subunits with molecular weights 185,000 (Ia), 137,000 (Ib), 48,000 (Ic), 44,000 (Id), 41,000 (Ie), 36,000 (If), 28,000 (Ig), 24,000 (Ih), 20,000 (Ii), 14,500 (Ij), and 12,000 (Ik). Yeast polymerase I separates into two forms when subjected to gel electrophoresis under nondenaturing conditions. The main component which migrates faster contains all the subunits except the polypeptides Ic and If. The slow migrating component which is present in lower amounts contains all the subunits.

摘要

已开发出一种用于快速纯化大量酵母RNA聚合酶I(A)的方法。该方法包括用磷酸纤维素和DEAE-纤维素进行分批处理、在DEAE-葡聚糖上进行离子过滤色谱、蔗糖梯度离心以及DNA-纤维素色谱。通过沉降速度分析,所获得的酶显然是均一的,其比活性为每毫克蛋白质在10分钟内将300 nmol的UMP掺入RNA中。从3.0千克酵母细胞中,5天内可获得30至45毫克的酶。在0.1%十二烷基硫酸钠存在下,通过聚丙烯酰胺凝胶电泳确定了该酶的亚基组成。纯化的聚合酶由11个推定的亚基组成,其分子量分别为185,000(Ia)、137,000(Ib)、48,000(Ic)、44,000(Id)、41,000(Ie)、36,000(If)、28,000(Ig)、24,000(Ih)、20,000(Ii)、14,500(Ij)和12,000(Ik)。在非变性条件下进行凝胶电泳时,酵母聚合酶I可分为两种形式。迁移较快的主要成分包含除多肽Ic和If之外的所有亚基。迁移较慢、含量较低的成分包含所有亚基。

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