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来自人类精子纯化细胞核和DNA合成复合物的DNA聚合酶的性质

Properties of a DNA polymerase from purified nuclei and DNA-synthesizing complexes of human spermatozoa.

作者信息

Witkin S S

出版信息

J Reprod Fertil. 1980 Jul;59(2):409-19. doi: 10.1530/jrf.0.0590409.

Abstract

A DNA polymerase was isolated from human spermatozoa. In one procedure, spermatozoa were decapitated with detergent, the heads purified and then lysed with dithiothreitol, trypsin and deoxyribonuclease. DNA polymerase was isolated from the lysate by sedimentation through an 18% Metrizamide solution, solubilization with 0.8 M-KCl-0.5% Triton X-100 and sequential chromatography on DEAE cellulose, phosphocellulose and hydroxylapatite. Alternatively, the heads of intact spermatozoa, untreated with detergent, were lysed as above; the subsequent Metrizamide pellet fraction was isolated and further fractionated by gel filtration and buoyant density centrifugation. The enzyme in this fraction was solubilized with KCl-Triton X-100. Characterization by velocity centrifugation and phosphocellulose chromatography revealed that it possessed properties indistinguishable from those of the enzyme purified from isolated sperm nuclei. The DNA polymerase had an apparent molecular weight of 79,000-89,000, Mn2+ (1 mM) was the preferred divalent cation and ativity was inhibited by concentrations of potassium phosphate greater than 10 mM. The synthetic template preferences of the enzyme were dT12-18 . poly rA > poly(dA-dT) > dT12-18 . poly dA; no activity was observed with dG12-18 . poly rC or dT10.

摘要

从人类精子中分离出一种DNA聚合酶。在一种方法中,用去污剂将精子断头,纯化头部,然后用二硫苏糖醇、胰蛋白酶和脱氧核糖核酸酶裂解。通过在18%的甲泛葡胺溶液中沉降从裂解物中分离出DNA聚合酶,用0.8M - KCl - 0.5% Triton X - 100溶解,并依次在DEAE纤维素、磷酸纤维素和羟基磷灰石上进行层析。或者,未用去污剂处理的完整精子头部按上述方法裂解;分离随后的甲泛葡胺沉淀部分,并通过凝胶过滤和浮力密度离心进一步分级分离。该部分中的酶用KCl - Triton X - 100溶解。通过速度离心和磷酸纤维素层析进行表征表明,它具有与从分离的精子核中纯化的酶无法区分的特性。该DNA聚合酶的表观分子量为79,000 - 89,000,Mn2 +(1 mM)是首选的二价阳离子,浓度大于10 mM的磷酸钾会抑制其活性。该酶的合成模板偏好为dT12 - 18·聚rA > 聚(dA - dT)> dT12 - 18·聚dA;用dG12 - 18·聚rC或dT10未观察到活性。

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