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从小牛胸腺胞质提取物中分离并鉴定一种DNA解旋酶。

Isolation and characterization of a DNA helicase from cytosolic extracts of calf thymus.

作者信息

Zhang S, Grosse F

机构信息

German Primate Center, Department of Virology and Immunology, Göttingen.

出版信息

Chromosoma. 1992;102(1 Suppl):S100-6. doi: 10.1007/BF02451792.

Abstract

A DNA helicase has been isolated from calf thymus tissue. The enzyme was enriched from crude cytosolic extracts by batchwise chromatography on phosphocellulose, followed by 35% ammonium sulfate precipitation, and subsequent chromatography on phenyl-Sepharose, single-stranded DNA cellulose, and AcA 44 gel filtration. The DNA helicase had a Stokes' radius of about 45 A and a sedimentation coefficient of 4.3 S. The most purified fractions contained three polypeptides with apparent molecular weights of 110, 65, and 34 kDa. UV crosslinking with radioactive dATP stained all three major polypeptides. The helicase catalyzed the unwinding of a DNA primer from a single-stranded DNA template in an ATP- or dATP-dependent manner. DNA unwinding was also observed with CTP or dCTP, but with reduced efficiency. The helicase translocated from 3' to 5' on the single-stranded template it was bound to. Relationships between this DNA helicase and other calf thymus helicases will be discussed.

摘要

已从小牛胸腺组织中分离出一种DNA解旋酶。该酶通过在磷酸纤维素上进行分批色谱法从粗制胞质提取物中富集,随后进行35%硫酸铵沉淀,以及后续在苯基琼脂糖、单链DNA纤维素和AcA 44凝胶过滤柱上的色谱法。该DNA解旋酶的斯托克斯半径约为45 Å,沉降系数为4.3 S。最纯的组分含有三种表观分子量分别为110、65和34 kDa的多肽。用放射性dATP进行紫外交联可使所有三种主要多肽染色。该解旋酶以ATP或dATP依赖的方式催化从单链DNA模板上解开DNA引物。用CTP或dCTP时也观察到了DNA解链,但效率较低。该解旋酶在其结合的单链模板上从3'向5'方向移位。将讨论这种DNA解旋酶与其他小牛胸腺解旋酶之间的关系。

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