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黑腹果蝇卵母细胞的诱变。I. 核和线粒体 DNA 的定时合成与非定时 DNA 合成。

Mutagenesis in Oocytes of DROSOPHILA MELANOGASTER. I. Scheduled Synthesis of Nuclear and Mitochondrial DNA and Unscheduled DNA Synthesis.

机构信息

Department of Zoology, Louisiana State University, Baton Rouge, Louisiana 70803.

出版信息

Genetics. 1983 Jun;104(2):279-99. doi: 10.1093/genetics/104.2.279.

Abstract

As a model system for studying mutagenesis, the oocyte of Drosophila melanogaster has exhibited considerable complexity. Very few experiments have been conducted on the effect of exposing oocytes to chemical mutagens, presumably due to their lower mutational response relative to sperm and spermatids. This lower response may be due either to a change in probability of mutation induction per adduct due to a change in the type of DNA repair or to a lower dose of the mutagen to the female germ line. To study molecular dosimetry and DNA repair in the oocyte, the large number of intracellular constituents (mtDNA, RNA, nucleic acid precursors and large quantities of proteins and lipids) must be separated from nuclear DNA. In this paper we present results showing reliable separation of such molecules enabling us to detect scheduled nuclear and mitochondrial DNA synthesis. We also, by understanding the precise timing of such events, can detect unscheduled DNA synthesis (UDS) as a measure of DNA repair. Furthermore, by comparing the UDS results in a repair competent (Ore-R) vs. a repair deficient (mei-9(L1 )) strain, we have shown the oocyte capable of DNA repair after treatment with ethyl methanesulfonate (EMS). We conclude that the important determinant of mutation induction in oocytes after treatment with EMS is the time interval between DNA alkylation and DNA synthesis after fertilization, i.e., the interruption of continuous DNA repair.

摘要

作为研究诱变的模型系统,黑腹果蝇的卵母细胞表现出相当的复杂性。由于与精子和精细胞相比,卵母细胞对化学诱变剂的暴露的突变反应较低,因此很少有实验在卵母细胞上进行。这种低反应可能是由于 DNA 修复类型的改变导致每个加合物的突变诱导概率发生变化,或者是由于雌性生殖系中诱变剂的剂量较低。为了研究卵母细胞中的分子剂量学和 DNA 修复,必须将大量的细胞内成分(mtDNA、RNA、核酸前体以及大量的蛋白质和脂质)与核 DNA 分离。在本文中,我们展示了可靠的分离这些分子的结果,使我们能够检测预定的核和线粒体 DNA 合成。我们还通过了解这些事件的精确时间,可以检测到未计划的 DNA 合成(UDS)作为 DNA 修复的衡量标准。此外,通过比较修复能力(Ore-R)与修复缺陷(mei-9(L1))菌株中的 UDS 结果,我们表明卵母细胞在乙磺酸(EMS)处理后能够进行 DNA 修复。我们得出结论,卵母细胞在 EMS 处理后诱导突变的重要决定因素是 DNA 烷化和受精后 DNA 合成之间的时间间隔,即连续 DNA 修复的中断。

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