Equivalence of UDS responses for established cell lines and primary cells derived from the mei-9a and mus201D1 excision repair-deficient strains of Drosophila melanogaster

Mutation Research/DNA Repair Reports Pub Date : 1988-11-01 DOI:10.1016/0167-8817(88)90027-2

Ruth L. Dusenbery, Shwu-Fei Lee-Chen

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引用次数: 6

Abstract

Autoradiographic analysis of unscheduled DNA synthesis in response to DNA damage produced by relatively high doses of the direct-acting, monofunctional alkylating agent, MMS, (4.5 mM) and UV (40 J/m²) demonstrates that established cell lines, derived from the mei-9^a and mus201^D1 excision repair-deficient strains of Drosophila melanogaster, perform no measurable incorporation of [³H]thymidine into repair patches, in accordance with the observations made for the corresponding primary embryonic cells derived from the two mutagen-sensitive strains of flies. These established cell lines can therefore be used as appropriate models for both examination of the biochemical basis of the genetic defects in the mei-9 and mus201 mutations and the role of excision-repair processes in spontaneous and induced mutation induction in eukaryotic cells.

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果蝇mei-9a和mus201D1切除修复缺陷株的已建立细胞系和原代细胞的UDS应答的等效性

高剂量直接作用单功能烷基化剂MMS (4.5 mM)和UV (40 J/m2)对DNA损伤反应的非计划性DNA合成的放射自显影分析表明，来自果蝇mei-9a和mus201D1切除修复缺陷菌株的已建立细胞系，在修复补丁中没有可测量的[3H]胸腺嘧啶的结合。根据对两种对诱变剂敏感的果蝇的相应原代胚胎细胞的观察。因此，这些已建立的细胞系可以作为检验mei-9和mus201突变中遗传缺陷的生化基础以及真核细胞中自发和诱导突变诱导中切除-修复过程的作用的适当模型。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Mutation Research/DNA Repair Reports

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