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Computational identification of cis-acting elements affecting post-transcriptional control of gene expression in Saccharomyces cerevisiae

机译:影响酿酒酵母基因表达转录后控制的顺式作用元件的计算鉴定

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Understanding the regulation of gene expression requires the identification of cis-acting control elements that modulate gene function. The recent availability of complete genome sequences and profiles of mRNA expression has facilitated the development and utilization of computational methods to identify discrete regulatory elements. We have developed an oligomer counting method that identifies sequences that occur significantly more often in a group of interest relative to other genes in the genome. The use of a second parameter, which measures the frequency of oligomers within the group of interest, allows the detection of false positive signals caused by very infrequent oligomers that would otherwise appear as significant. Applying this method to gene groups that have a common expression pattern or shared function should identify oligomers that comprise cis-acting control elements. As a test of this method, we applied this approach to a set of intron-containing yeast genes, where we easily identified the known splicing signals as control elements. We have used this training set to examine how this method is affected by the length of the oligomer examined, as well as the size and composition of the gene group. These simulations allowed us to identify rules for selecting groups of genes to analyze. Finally, application of this method to nuclear genes encoding proteins targeted to the mitochondria identified a new putative cis-acting sequence in the 3′-untranslated region of this family of genes, which may play a role in mRNA localization or the regulation of mRNA stability or translation.
机译:要了解基因表达的调控,就需要鉴定调节基因功能的顺式作用调控元件。完整基因组序列和mRNA表达谱的最新可用性促进了计算方法的发展和利用,以鉴定离散的调控元件。我们已经开发出一种寡聚体计数方法,该方法可识别相对于基因组中其他基因在感兴趣的一组中出现频率更高的序列。使用第二参数来测量目标组中寡聚物的频率,可以检测由极少出现的寡聚物引起的假阳性信号,否则这些假阳性信号会显得很重要。将此方法应用于具有共同表达模式或共有功能的基因组,应鉴定出包含顺式作用控制元件的寡聚体。作为对该方法的测试,我们将该方法应用于一组含内含子的酵母基因,在其中我们容易地将已知的剪接信号识别为控制元件。我们已经使用该训练集来检查这种方法如何受到所检查的寡聚物的长度以及基因组的大小和组成的影响。这些模拟使我们能够确定选择基因组进行分析的规则。最后,该方法在编码靶向线粒体蛋白的核基因中的应用在该基因家族的3'-非翻译区中发现了一个新的假定的顺式作用序列,这可能在mRNA定位或mRNA稳定性调节中起作用或翻译。

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