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源自小鼠浆细胞瘤MOPC 315的脱氧核糖核酸依赖性核糖核酸聚合酶II的纯化及亚基结构

Purification and subunit structure of deoxyribonucleic acid-dependent ribonucleic acid polymerase II from the mouse plasmacytoma, MOPC 315.

作者信息

Schwartz L B, Roeder R G

出版信息

J Biol Chem. 1975 May 10;250(9):3221-8.

PMID:1168191
Abstract

DNA-dependent RNA polymerase II was purified from the mouse plasmacytoma, MOPC 315. Soluble enzyme was obtained from a nucleoplasmic fraction and subjected to chromatography on phosphocellulose, DEAE-cellulose, and DEAE-Sephadex ion exchange resins and was subjected to sedimentation in sucrose density gradients. A chromatographically homogeneous enzyme was obtained which was purified about 25,000-fold relative to whole cell extracts and which had a specific activity (on native DNA) similar to those reported for other purified eukaryotic class II RNA polymerase preparations. Analysis of purified RNA polymerase II by polyacrylamide gel electrophoresis under nondenaturing conditions revealed three protein bands, designated II-O, II-A, and II-B in order of electrophoretic mobility. The subunit compositions of these nondenatured bands were subsequently analyzed by electrophoresis under denaturing conditions. Each enzyme II form contained subunits with molecular weights of 140,000 (II-c), 41,000 (II-d), 30,000 (II-e), 25,000 (II-f), 22,000 (II-g), 20,000 (II-h), and 16,000 (II-i). Molar ratios were unity for all subunits except subunit II-h which had a molar ratio of 2. Each enzyme form was distinguished by its highest molecular weight subunit. II-O contained subunit II-o (molecular weight 240,000), II-A contained subunit II-a (molecular weight 205,000), and II-B contained subunit II-b (molecular weight 170,000). Total molecular weights for II-O, II-A, and II-B were calculated as 554,000, 519,000, and 484,000, respectively. In addition, the number of RNA polymerase II molecules per MOPC 315 tumor cell was calculated to be about 5 times 10-4.

摘要

从鼠浆细胞瘤MOPC 315中纯化出依赖DNA的RNA聚合酶II。从核质部分获得可溶性酶,并使其通过磷酸纤维素、DEAE - 纤维素和DEAE - 葡聚糖离子交换树脂进行色谱分析,然后在蔗糖密度梯度中进行沉降。获得了一种色谱均一的酶,相对于全细胞提取物,其纯化了约25000倍,并且其比活性(基于天然DNA)与其他纯化的真核II类RNA聚合酶制剂报道的相似。在非变性条件下通过聚丙烯酰胺凝胶电泳对纯化的RNA聚合酶II进行分析,显示出三条蛋白带,按照电泳迁移率顺序命名为II - O、II - A和II - B。随后在变性条件下通过电泳分析这些非变性条带的亚基组成。每种II型酶形式都包含分子量分别为140000(II - c)、41000(II - d)、30000(II - e)、25000(II - f)、22000(II - g)、20000(II - h)和16000(II - i)的亚基。除亚基II - h的摩尔比为2外,所有亚基的摩尔比均为1。每种酶形式以其分子量最高的亚基为特征。II - O包含亚基II - o(分子量240000),II - A包含亚基II - a(分子量205000),II - B包含亚基II - b(分子量170000)。II - O、II - A和II - B的总分子量分别计算为554000、519000和484000。此外,计算出每个MOPC 315肿瘤细胞中RNA聚合酶II分子的数量约为5×10⁻⁴。

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