Martinez-Vaz Betsy M, Xie Yang, Pan Wei, Khodursky Arkady B
Department of Biochemistry, Molecular Biology and Biophysics and Biotechnology Institute, University of Minnesota, Saint Paul, MN 55108, USA.
BMC Genomics. 2005 Jun 1;6:81. doi: 10.1186/1471-2164-6-81.
The distribution and location of insertion elements in a genome is an excellent tool to track the evolution of bacterial strains and a useful molecular marker to distinguish between closely related bacterial isolates. The information about the genomic locations of IS elements is available in public sequence databases. However, the locations of mobile elements may vary from strain to strain and within the population of an individual strain. Tools that allow de novo localization of IS elements and are independent of existing sequence information are essential to map insertion elements and advance our knowledge of the role that such elements play in gene regulation and genome plasticity in bacteria.
In this study, we present an efficient and reliable method for linear mapping of mobile elements using whole-genome DNA microarrays. In addition, we describe an algorithm for analysis of microarray data that can be applied to find DNA sequences physically juxtaposed with a target sequence of interest. This approach was used to map the locations of the IS5 elements in the genome of Escherichia coli K12. All IS5 elements present in the E. coli genome known from GenBank sequence data were identified. Furthermore, previously unknown insertion sites were predicted with high sensitivity and specificity. Two variants of E. coli K-12 MG1655 within a population of this strain were predicted by our analysis. The only significant difference between these two isolates was the presence of an IS5 element upstream of the main flagella regulator, flhDC. Additional experiments confirmed this prediction and showed that these isolates were phenotypically distinct. The effect of IS5 on the transcriptional activity of motility and chemotaxis genes in the genome of E. coli strain MG1655 was examined. Comparative analysis of expression profiles revealed that the presence of IS5 results in a mild enhancement of transcription of the flagellar genes that translates into a slight increase in motility.
In summary, this work presents a case study of an experimental and analytical application of DNA microarrays to map insertion elements in bacteria and gains an insight into biological processes that might otherwise be overlooked by relying solely on the available genome sequence data.
插入元件在基因组中的分布和位置是追踪细菌菌株进化的优良工具,也是区分密切相关细菌分离株的有用分子标记。关于插入序列(IS元件)基因组位置的信息可在公共序列数据库中获取。然而,移动元件的位置可能因菌株而异,且在单个菌株群体内也会有所不同。能够对IS元件进行从头定位且独立于现有序列信息的工具,对于绘制插入元件图谱以及增进我们对这些元件在细菌基因调控和基因组可塑性中所起作用的了解至关重要。
在本研究中,我们提出了一种使用全基因组DNA微阵列对移动元件进行线性图谱绘制的高效且可靠的方法。此外,我们描述了一种用于分析微阵列数据的算法,该算法可用于找到与感兴趣的目标序列物理相邻的DNA序列。此方法用于绘制大肠杆菌K12基因组中IS5元件的位置。从GenBank序列数据中已知的大肠杆菌基因组中存在的所有IS5元件均被识别出来。此外,还以高灵敏度和特异性预测了先前未知的插入位点。我们的分析预测了该菌株群体内大肠杆菌K - 12 MG1655的两个变体。这两个分离株之间唯一显著的差异是在主要鞭毛调节因子flhDC上游存在一个IS5元件。额外的实验证实了这一预测,并表明这些分离株在表型上有所不同。研究了IS5对大肠杆菌MG1655菌株基因组中运动性和趋化性基因转录活性的影响。表达谱的比较分析表明,IS5的存在导致鞭毛基因转录轻度增强,进而转化为运动性略有增加。
总之,这项工作展示了一个将DNA微阵列用于绘制细菌中插入元件的实验和分析应用的案例研究,并深入了解了一些生物过程,否则仅依靠现有的基因组序列数据可能会忽略这些过程。
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