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一种来自野油菜黄单胞菌水稻致病变种的RNA聚合酶新蛋白亚基k

A new protein subunit k for RNA polymerase from Xanthomonas campestris pv. oryzae.

作者信息

Chen C K, Tu J, Kuo T T

机构信息

Department of Botany, National Taiwan University, Taipei, Republic of China.

出版信息

J Biol Chem. 1989 Mar 15;264(8):4362-6.

PMID:2647734
Abstract

During the purification of RNA polymerase from Xanthomonas campestris pv. oryzae, a new subunit named k was found to be associated with this enzyme. The removal of subunit k from holoenzyme by DEAE-cellulose column chromatography results in a decrease in specific activity of the enzyme. The readdition of subunit k to subunit k-depleted holoenzyme results in restoration of enzymatic activity. Subunit k increase the activity of RNA polymerase; the activation was in proportion to the concentration of subunit k added. Antiserum against holoenzyme devoid of subunit k was prepared. This antiserum did not react with purified subunit k; therefore, subunit k may not be the proteolytic fragment of the beta, beta', sigma, or alpha subunit. When this antiserum was used to precipitate RNA polymerase obtained from a crude extract of bacterial cells, subunit k was coprecipitated as determined by sodium dodecyl sulfate gel electrophoretic analysis. The molecular mass of subunit k is approximately 29 kDa, and the molar ratio of beta:beta':sigma:alpha:k was estimated to be 1:1:1:2:4. When native Xp10 DNA was used as template, subunit k stimulated subunit k-depleted holoenzyme, but not core enzyme. When the synthetic polynucleotide poly[d(A-T)] was used, subunit k activated both subunit k-depleted holoenzyme and core enzyme. Subunit k also activated the binding of RNA polymerase to template DNA.

摘要

在从水稻白叶枯病菌中纯化RNA聚合酶的过程中,发现一种名为k的新亚基与该酶相关联。通过DEAE-纤维素柱层析从全酶中去除亚基k会导致该酶的比活性降低。将亚基k重新添加到去除亚基k的全酶中会使酶活性恢复。亚基k增加了RNA聚合酶的活性;这种激活与添加的亚基k的浓度成正比。制备了针对不含亚基k的全酶的抗血清。这种抗血清不与纯化的亚基k反应;因此,亚基k可能不是β、β'、σ或α亚基的蛋白水解片段。当使用这种抗血清沉淀从细菌细胞粗提物中获得的RNA聚合酶时,通过十二烷基硫酸钠凝胶电泳分析确定亚基k会共沉淀。亚基k的分子量约为29 kDa,β:β':σ:α:k的摩尔比估计为1:1:1:2:4。当天然Xp10 DNA用作模板时,亚基k刺激去除亚基k的全酶,但不刺激核心酶。当使用合成多核苷酸聚[d(A-T)]时,亚基k激活去除亚基k的全酶和核心酶。亚基k还激活RNA聚合酶与模板DNA的结合。

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