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使用一种新型转座子介导的方法确定大肠杆菌中DNA元件的最佳染色体位置

Determination of the Optimal Chromosomal Location(s) for a DNA Element in Escherichia coli Using a Novel Transposon-mediated Approach.

作者信息

Frimodt-Møller Jakob, Charbon Godefroid, Krogfelt Karen A, Løbner-Olesen Anders

机构信息

Department of Biology, Section for Functional Genomics and Center for Bacterial Stress Response and Persistence (BASP), University of Copenhagen.

Department of Microbiology and Infection Control, Statens Serum Institut.

出版信息

J Vis Exp. 2017 Sep 11(127):55946. doi: 10.3791/55946.

Abstract

The optimal chromosomal position(s) of a given DNA element was/were determined by transposon-mediated random insertion followed by fitness selection. In bacteria, the impact of the genetic context on the function of a genetic element can be difficult to assess. Several mechanisms, including topological effects, transcriptional interference from neighboring genes, and/or replication-associated gene dosage, may affect the function of a given genetic element. Here, we describe a method that permits the random integration of a DNA element into the chromosome of Escherichia coli and select the most favorable locations using a simple growth competition experiment. The method takes advantage of a well-described transposon-based system of random insertion, coupled with a selection of the fittest clone(s) by growth advantage, a procedure that is easily adjustable to experimental needs. The nature of the fittest clone(s) can be determined by whole-genome sequencing on a complex multi-clonal population or by easy gene walking for the rapid identification of selected clones. Here, the non-coding DNA region DARS2, which controls the initiation of chromosome replication in E. coli, was used as an example. The function of DARS2 is known to be affected by replication-associated gene dosage; the closer DARS2 gets to the origin of DNA replication, the more active it becomes. DARS2 was randomly inserted into the chromosome of a DARS2-deleted strain. The resultant clones containing individual insertions were pooled and competed against one another for hundreds of generations. Finally, the fittest clones were characterized and found to contain DARS2 inserted in close proximity to the original DARS2 location.

摘要

通过转座子介导的随机插入并随后进行适应性选择,确定给定DNA元件的最佳染色体位置。在细菌中,遗传背景对遗传元件功能的影响可能难以评估。包括拓扑效应、来自相邻基因的转录干扰和/或与复制相关的基因剂量等几种机制,可能会影响给定遗传元件的功能。在这里,我们描述了一种方法,该方法允许将DNA元件随机整合到大肠杆菌染色体中,并通过简单的生长竞争实验选择最有利的位置。该方法利用了一个描述详尽的基于转座子的随机插入系统,再加上通过生长优势选择最适合的克隆,这一过程很容易根据实验需求进行调整。最适合的克隆的性质可以通过对复杂多克隆群体进行全基因组测序来确定,或者通过简单的基因步移来快速鉴定所选克隆。在这里,以控制大肠杆菌染色体复制起始的非编码DNA区域DARS2为例。已知DARS2的功能受与复制相关的基因剂量影响;DARS2距离DNA复制起点越近,其活性就越高。将DARS2随机插入到缺失DARS2的菌株的染色体中。将得到的含有单个插入片段的克隆混合在一起,并相互竞争数百代。最后,对最适合的克隆进行表征,发现其含有插入到与原始DARS2位置紧邻处的DARS2。

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