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A Genetic Screen Based on in Vivo RNA Imaging Reveals Centrosome-Independent Mechanisms for Localizing gurken Transcripts in Drosophila

机译:基于体内RNA成像的遗传筛选揭示了中心体独立的机制用于定位果蝇中的古根转录本。

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摘要

We have screened chromosome arm 3L for ethyl methanesulfonate−induced mutations that disrupt localization of fluorescently labeled gurken (grk) messenger (m)RNA, whose transport along microtubules establishes both major body axes of the developing Drosophila oocyte. Rapid identification of causative mutations by single-nucleotide polymorphism recombinational mapping and whole-genomic sequencing allowed us to define nine complementation groups affecting grk mRNA localization and other aspects of oogenesis, including alleles of elg1, scaf6, , nudE, Tsc2/gigas, rasp, and Chd5/Wrb, and several null alleles of the armitage Piwi-pathway gene. Analysis of a newly induced kinesin light chain allele shows that kinesin motor activity is required for both efficient grk mRNA localization and oocyte centrosome integrity. We also show that initiation of the dorsoanterior localization of grk mRNA precedes centrosome localization, suggesting that microtubule self-organization contributes to breaking axial symmetry to generate a unique dorsoventral axis.
机译:我们筛选了3L染色体臂上的甲磺酸乙酯诱导的突变,这些突变破坏了荧光标记的古肯(grk)信使(m)RNA的定位,该基因沿微管的运输建立了果蝇卵母细胞发育的两个主要身体轴。通过单核苷酸多态性重组作图和全基因组测序快速鉴定出致病突变,这使我们能够定义影响grk mRNA定位和卵子发生其他方面的9个互补基团,包括elg1,scaf6,nudE,Tsc2 / gigas,rasp等位基因,和Chd5 / Wrb,以及保护性Piwi途径基因的几个无效等位基因。对新诱导的驱动蛋白轻链等位基因的分析表明,有效的grk mRNA定位和卵母细胞中心体完整性均需要驱动蛋白运动。我们还显示,grk mRNA的背前部定位的启动先于中心体定位,这表明微管的自组织有助于打破轴向对称性以产生唯一的背腹轴。

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