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Inferring gene regulatory logic from high-throughput measurements of thousands of systematically designed promoters

机译:从数千个系统设计启动子的高通量测量中推断基因调控逻辑

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摘要

Despite extensive research, our understanding of the rules according to which cis-regulatory sequences are converted into gene expression is limited. We devised a method for obtaining parallel, highly accurate gene expression measurements from thousands of designed promoters and applied it to measure the effect of systematic changes in the location, number, orientation, affinity and organization of transcription-factor binding sites and nucleosome-disfavoring sequences. Our analyses reveal a clear relationship between expression and binding-site multiplicity, as well as dependencies of expression on the distance between transcription-factor binding sites and gene starts which are transcription-factor specific, including a striking similar to 10-bp periodic relationship between gene expression and binding-site location. We show how this approach can measure transcription-factor sequence specificities and the sensitivity of transcription-factor sites to the surrounding sequence context, and compare the activity of 75 yeast transcription factors. Our method can be used to study both cis and trans effects of genotype on transcriptional, post-transcriptional and translational control.
机译:尽管进行了广泛的研究,但我们对将顺式调控序列转化为基因表达的规则的理解仍然有限。我们设计了一种方法,该方法可从数千个设计的启动子中获取平行,高精度的基因表达测量值,并将其应用于测量转录因子结合位点和不利于核小体的序列的位置,数量,方向,亲和力和组织的系统变化的影响。我们的分析揭示了表达与结合位点多重性之间的明确关系,以及表达对转录因子特异性位点与转录起始因子之间的距离的依赖性,这些转录因子是转录因子特异性的,包括与基因表达和结合位点定位。我们展示了这种方法如何可以测量转录因子序列的特异性和转录因子位点对周围序列上下文的敏感性,并比较75种酵母转录因子的活性。我们的方法可用于研究基因型对转录,转录后和翻译控制的顺式和反式作用。

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