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MAPCap allows high-resolution detection and differential expression analysis of transcription start sites

机译:MAPCap允许对转录起始位点进行高分辨率检测和差异表达分析

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摘要

The position, shape and number of transcription start sites (TSS) are critical determinants of gene regulation. Most methods developed to detect TSSs and study promoter usage are, however, of limited use in studies that demand quantification of expression changes between two or more groups. In this study, we combine high-resolution detection of transcription start sites and differential expression analysis using a simplified TSS quantification protocol, MAPCap (Multiplexed Affinity Purification of Capped RNA) along with the software . Applying MAPCap on developing Drosophila melanogaster embryos and larvae, we detected stage and sex-specific promoter and enhancer activity and quantify the effect of mutants of maleless (MLE) helicase at X-chromosomal promoters. We observe that MLE mutation leads to a median 1.9 fold drop in expression of X-chromosome promoters and affects the expression of several TSSs with a sexually dimorphic expression on autosomes. Our results provide quantitative insights into promoter activity during dosage compensation.
机译:转录起始位点(TSS)的位置,形状和数量是基因调控的关键决定因素。然而,大多数开发的检测TSS和研究启动子使用的方法在需要量化两个或多个组之间表达变化的研究中使用有限。在这项研究中,我们将高分辨率的转录起始位点检测与差异表达分析相结合,使用简化的TSS定量方案MAPCap(加帽RNA的多路亲和纯化)以及该软件。将MAPCap应用于发育中的果蝇胚胎和幼虫,我们检测了阶段和性别特异性启动子和增强子活性,并定量了无雄性(MLE)解旋酶突变体在X染色体启动子上的作用。我们观察到,MLE突变导致X染色体启动子表达中位数下降1.9倍,并影响常染色体上具有性双态表达的几种TSS的表达。我们的结果提供了剂量补偿过程中启动子活性的定量见解。

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