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来自硅藻梭形角毛藻的脱氧核糖核酸聚合酶。酶的亚细胞分布、核酸外切酶活性及异质性。

The deoxyribonucleic acid polymerases from the diatom Cylindrotheca fusiformis. Subcellular distribution, exonuclease activity and heterogeneity of the enzymes.

作者信息

Okita T W, Volcani B E

出版信息

Biochem J. 1977 Dec 1;167(3):611-9. doi: 10.1042/bj1670611.

Abstract

Four DNA polymerases from the marine diatom Cylindrotheca fusiformis, polymerases A, B, C and D, were further differentiated by their subcellular localization, presence of deoxyribonuclease activity, apparent heterogeneity and molecular weights. Polymerases A, B and D occur in significant amounts in the soluble fraction, suggesting that they were originally localized in the nuclei, whereas polymerase C predominates in the chloroplasts. A mitochondrial DNA polymerase was also isolated and characterized by ion-exchange chromatography. Polymerase D has an associated nuclease activity which prefers denatured DNA and Mg2+, and has a pH optimum higher than that for polymerase activity. Co-elution from a DEAE-Sephadex column and co-sedimentation in glycerol density gradients of deoxyribonuclease and polymerase D activity suggest a molecular association. Polymerases A, B and C are devoid of nuclease activity. Glycerol-gradient-sedimentation analysis showed that all DNA polymerase fractions are heterogeneous at low ionic strengths, with the appearance of a single homogeneous activity of 0.5M-KCl. Estimated molecular weights of 100000, 82000 and 120000 for polymerases A, B and C respectively were obtained from sedimentation analysis and gel filtration. Polymerase D was estimated to have a molecular weight of about 100000 as determined by sedimentation analysis alone.

摘要

从海洋硅藻纺锤硅藻(Cylindrotheca fusiformis)中提取的四种DNA聚合酶,即聚合酶A、B、C和D,通过它们的亚细胞定位、脱氧核糖核酸酶活性的存在、明显的异质性和分子量进一步区分。聚合酶A、B和D在可溶部分中大量存在,这表明它们最初定位于细胞核,而聚合酶C在叶绿体中占主导地位。还通过离子交换色谱法分离并鉴定了一种线粒体DNA聚合酶。聚合酶D具有一种相关的核酸酶活性,该活性更倾向于变性DNA和Mg2+,并且其最适pH高于聚合酶活性的最适pH。从DEAE-葡聚糖凝胶柱上的共洗脱以及脱氧核糖核酸酶和聚合酶D活性在甘油密度梯度中的共沉降表明存在分子关联。聚合酶A、B和C没有核酸酶活性。甘油梯度沉降分析表明,在低离子强度下,所有DNA聚合酶组分都是异质的,在0.5M-KCl时出现单一均匀活性。通过沉降分析和凝胶过滤分别获得聚合酶A、B和C的估计分子量为100000、82000和120000。仅通过沉降分析确定,聚合酶D的估计分子量约为100000。

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