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重组杆状病毒表达的人DNA聚合酶δ催化亚基的特性分析

Characterization of the human DNA polymerase delta catalytic subunit expressed by a recombinant baculovirus.

作者信息

Suzuki S, Suzuki M, Yoshida S

机构信息

Medical Biological Institute, Nagoya, Japan.

出版信息

Nagoya J Med Sci. 2000 Nov;63(3-4):99-113.

PMID:11201990
Abstract

The catalytic subunit of human DNA polymerase (pol) delta, p125, was expressed in recombinant baculovirus-infected insect cells, separated from a baculovirus-encoded DNA polymerase, and was purified to homogeneity by affinity trapping with a histidine-octapeptide at the C-terminus of p125 as the ligand. Purified p125 showed DNA polymerase activity resembling conventionally purified calf thymus pol delta. However, the two differed in four ways: 1) the specific activity of recombinant p125 was one quarter of the calf thymus pol delta; 2) the recombinant p125 was relatively resistant to aphidicolin; 3) the apparent Km for dTTP of the recombinant p125 was estimated at 33 microM, 15-fold the value for calf thymus pol delta; and 4) the recombinant p125 was not stimulated by recombinant PCNA, while activity of calf thymus pol delta increased 150-fold in response. Furthermore, PCNA did not stimulate either the p125 incubated with p50, a small subunit of pol delta, or co-expressed with p50 in insect cells. The full length recombinant p125 migrated slightly faster than pol delta from human cell lines, Jurkat or HeLa, upon SDS-polyacrylamide gel electrophoresis, suggesting a post-translational modification. The results indicate that in vivo assembly of the fully active complex of pol delta requires factors in addition to p125 and p50 subunits, and/or a post-translational modification of p125.

摘要

人DNA聚合酶(pol)δ的催化亚基p125在重组杆状病毒感染的昆虫细胞中表达,与杆状病毒编码的DNA聚合酶分离,并通过以p125 C末端的组氨酸八肽为配体进行亲和捕获纯化至同质。纯化的p125显示出与常规纯化的小牛胸腺pol δ相似的DNA聚合酶活性。然而,两者在四个方面存在差异:1)重组p125的比活性是小牛胸腺pol δ的四分之一;2)重组p125对阿非科林相对耐药;3)重组p125对dTTP的表观Km估计为33μM,是小牛胸腺pol δ值的15倍;4)重组p125不受重组PCNA的刺激,而小牛胸腺pol δ的活性则增加150倍。此外,PCNA对与pol δ的小亚基p50一起孵育或在昆虫细胞中与p50共表达的p125均无刺激作用。在SDS-聚丙烯酰胺凝胶电泳中,全长重组p125的迁移速度略快于来自人细胞系Jurkat或HeLa的pol δ,提示存在翻译后修饰。结果表明,pol δ全活性复合物的体内组装除了需要p125和p50亚基外,还需要其他因子,和/或p125的翻译后修饰。

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引用本文的文献

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An in vivo analysis of the localisation and interactions of human p66 DNA polymerase delta subunit.人p66 DNA聚合酶δ亚基的定位及相互作用的体内分析
BMC Mol Biol. 2005 Jul 6;6:17. doi: 10.1186/1471-2199-6-17.