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结合重组工程和末端外同源重组系统地表征果蝇基因家族:以Rab GTPases为例进行研究

Combining recombineering and ends-out homologous recombination to systematically characterize Drosophila gene families: Rab GTPases as a case study.

作者信息

Chan Chih-Chiang, Scoggin Shane, Hiesinger P Robin, Buszczak Michael

出版信息

Commun Integr Biol. 2012 Mar 1;5(2):179-83. doi: 10.4161/cib.18788.

Abstract

Evaluating how an individual gene contributes to a particular biological process benefits greatly from a comprehensive understanding of all members of its gene family. Such knowledge is ideally obtained using multicellular model organisms, which provide rapid and decisive platforms for determining gene function. We recently established a novel transgenesis platform in Drosophila to systematically knock out all members of the Rab small GTPase family of membrane regulators. This platform combines BAC transgenesis/recombineering with ends-out homologous recombinations and Gateway(TM) technologies and provides a new rapid and scalable method that eases the manipulation of endogenous loci. This method not only allows for the generation of molecularly defined lesions, but also the precise replacement or tagging of genes in their endogenous loci. Using this method, we found that up to half of all Rab GTPases exhibit enriched expression at synapses in the nervous system. Here we provide critical details about the underlying recombineering and transgenesis method, new cassettes for tagging endogenous loci and information on important parameters that will allow Drosophila researchers to target members of other gene families.

摘要

从对某个基因家族所有成员的全面了解中,能极大地受益于评估单个基因如何促成特定的生物学过程。理想情况下,此类知识是通过多细胞模式生物获得的,这些生物为确定基因功能提供了快速且决定性的平台。我们最近在果蝇中建立了一个新型转基因平台,用于系统性敲除膜调节因子Rab小GTP酶家族的所有成员。该平台将BAC转基因/重组工程与末端外同源重组及Gateway(TM)技术相结合,提供了一种新的快速且可扩展的方法,简化了对内源基因座的操作。这种方法不仅能产生分子定义明确的损伤,还能在其内源基因座精确替换或标记基因。使用这种方法,我们发现所有Rab GTP酶中多达一半在神经系统的突触处表现出富集表达。在此,我们提供了关于基础重组工程和转基因方法的关键细节、用于标记内源基因座的新盒式结构以及重要参数的信息,这将使果蝇研究人员能够靶向其他基因家族的成员。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6ea5/3376058/424a72f63ff8/cib-5-179-g1.jpg

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