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生成针对果蝇异染色质 Tim17b 基因(编码线粒体转位酶亚基)的敲低转基因。

Generating a knockdown transgene against Drosophila heterochromatic Tim17b gene encoding mitochondrial translocase subunit.

机构信息

Fox Chase Cancer Center, Philadelphia, Pennsylvania, United States of America.

出版信息

PLoS One. 2011;6(10):e25945. doi: 10.1371/journal.pone.0025945. Epub 2011 Oct 6.

Abstract

Heterochromatic regions of eukaryotic genomes contain multiple functional elements involved in chromosomal dynamics, as well as multiple housekeeping genes. Cytological and molecular peculiarities of heterochromatic loci complicate genetic studies based on standard approaches developed using euchromatic genes. Here, we report the development of an RNAi-based knockdown transgenic construct and red fluorescent reporter transgene for a small gene, Tim17b, which localizes in constitutive heterochromatin of Drosophila melanogaster third chromosome and encodes a mitochondrial translocase subunit. We demonstrate that Tim17b protein is required strictly for protein delivery to mitochondrial matrix. Knockdown of Tim17b completely disrupts functions of the mitochondrial translocase complex. Using fluorescent recovery after photobleaching assay, we show that Tim17b protein has a very stable localization in the membranes of the mitochondrial network and that its exchange rate is close to zero when compared with soluble proteins of mitochondrial matrix. These results confirm that we have developed comprehensive tools to study functions of heterochromatic Tim17b gene.

摘要

真核基因组的异染色质区含有多个参与染色体动力学的功能元件,以及多个管家基因。异染色质位点的细胞学和分子特性使基于使用常染色质基因开发的标准方法进行的遗传研究变得复杂。在这里,我们报告了一种基于 RNAi 的敲低转基因构建体和红色荧光报告基因的开发,用于一个小基因 Tim17b,该基因定位于果蝇第三染色体的组成型异染色质中,编码线粒体转位酶亚基。我们证明 Tim17b 蛋白严格需要将蛋白质递送到线粒体基质中。Tim17b 的敲低完全破坏了线粒体转位酶复合物的功能。通过荧光恢复后光漂白测定,我们表明 Tim17b 蛋白在线粒体网络的膜上具有非常稳定的定位,并且与线粒体基质中的可溶性蛋白相比,其交换率接近零。这些结果证实,我们已经开发了全面的工具来研究异染色质 Tim17b 基因的功能。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9584/3188573/483d0ea0a63b/pone.0025945.g001.jpg

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