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Mos as a tool for genome-wide insertional mutagenesis in Caenorhabditis elegans: results of a pilot study.

机译:Mos作为秀丽隐杆线虫全基因组插入诱变的工具:一项初步研究的结果。

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The sequence of the Caenorhabditis elegans genome contains approximately 19 000 genes. Available mutants currently exist for <20% of these genes. The existence of a Mos-based inducible transposon system in C. elegans could theoretically serve as a tool to saturate the genome with insertions. We report here the results of a pilot study aimed at assaying this strategy. We generated 914 independent random Mos insertions and determined their location by inverse PCR. The distribution of the insertions throughout the genome does not reveal any gross distortion, with the exception of a major hotspot on chromosome I (rDNA locus). Transposons are evenly distributed between the genic and intergenic regions. Within genes, transposons insert preferentially into the introns. We derived the consensus target site for Mos in C. elegans (ATATAT), which is common to Tc1, another mariner element. Finally, we assayed the mutagenic properties of insertions located in exons by comparing the phenotype of homozygous strains to that of known mutations or RNAi of the same gene. This pilot experiment shows that a Mos-based approach is a viable strategy that can contribute to the constitution of genome-wide collections of identified C. elegans mutants.
机译:秀丽隐杆线虫基因组的序列包含大约19000个基因。目前,这些基因的不足20%存在可用的突变体。秀丽隐杆线虫中基于Mos的诱导型转座子系统的存在在理论上可以用作通过插入使基因组饱和的工具。我们在这里报告旨在分析该策略的初步研究的结果。我们生成了914个独立的随机Mos插入片段,并通过反向PCR确定了它们的位置。除了整个染色体上的主要热点(rDNA基因座)外,整个基因组中插入的分布都没有发现任何明显的畸变。转座子在基因和基因间区域之间均匀分布。在基因内,转座子优先插入内含子。我们推导了秀丽隐杆线虫中的Mos的共有目标位点(ATATAT),这是另一种水手元素Tc1共有的。最后,我们通过将纯合菌株的表型与相同基因的已知突变或RNAi的表型进行比较,分析了位于外显子中的插入的诱变特性。该初步实验表明,基于Mos的方法是可行的策略,可有助于构建已鉴定秀丽隐杆线虫突变体的全基因组集合。

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