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P-Element Homing Is Facilitated by engrailed Polycomb-Group Response Elements in Drosophila melanogaster

机译:果蝇的参与的多梳子群响应元素促进了P元素归巢

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摘要

P-element vectors are commonly used to make transgenic Drosophila and generally insert in the genome in a nonselective manner. However, when specific fragments of regulatory DNA from a few Drosophila genes are incorporated into P-transposons, they cause the vectors to be inserted near the gene from which the DNA fragment was derived. This is called P-element homing. We mapped the minimal DNA fragment that could mediate homing to the engrailed/invected region of the genome. A 1.6 kb fragment of engrailed regulatory DNA that contains two Polycomb-group response elements (PREs) was sufficient for homing. We made flies that contain a 1.5kb deletion of engrailed DNA (enΔ1.5) in situ, including the PREs and the majority of the fragment that mediates homing. Remarkably, homing still occurs onto the enΔ1. 5 chromosome. In addition to homing to en, P[en] inserts near Polycomb group target genes at an increased frequency compared to P[EPgy2], a vector used to generate 18,214 insertions for the Drosophila gene disruption project. We suggest that homing is mediated by interactions between multiple proteins bound to the homing fragment and proteins bound to multiple areas of the engrailed/invected chromatin domain. Chromatin structure may also play a role in homing.
机译:P-元件载体通常用于制备转基因果蝇,并通常以非选择性方式插入基因组中。但是,当将来自几个果蝇基因的特定调控DNA片段掺入P-转座子时,它们会使载体插入到DNA片段所源自的基因附近。这称为P元素归位。我们绘制了最小的DNA片段,该片段可以介导归巢到基因组的受侵袭/受感染区域。包含两个Polycomb-group响应元件(PRE)的进化调控DNA的1.6 kb片段足以进行归巢。我们制作的果蝇原位含有1.5kb缺失的衔接DNA(en Δ1.5),包括PRE和介导归巢的大部分片段。明显地,归巢仍然发生在enΔ1上。 5 染色体。除了归巢到en之外,P [en]还以比P [EPgy2]更高的频率插入到Polycomb组靶基因附近,P [EPgy2]是一种用于为果蝇基因破坏计划生成18,214个插入的载体。我们建议归巢是由绑定到归巢片段的多个蛋白质和绑定到被侵染的染色质域的多个区域之间的蛋白质之间的相互作用介导的。染色质结构也可能在归巢中起作用。

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