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Identifying gene regulatory elements by genomic microarray mapping of DNaseI hypersensitive sites

机译:通过基因组微阵列定位DNaseI超敏位点鉴定基因调控元件

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摘要

The identification of cis-regulatory elements is central to understanding gene transcription. Hypersensitivity of cis-regulatory elements to digestion with DNaseI remains the gold-standard approach to locating such elements. Traditional methods used to identify DNaseI hypersensitive sites are cumbersome and can only be applied to short stretches of DNA at defined locations. Here we report the development of a novel genomic array-based approach to DNaseI hypersensitive site mapping (ADHM) that permits precise, large-scale identification of such sites from as few as 5 million cells. Using ADHM we identified all previously recognized hematopoietic regulatory elements across 200 kb of the mouse T-cell acute lymphocytic leukemia-1 (Tal1) locus, and, in addition, identified two novel elements within the locus, which show transcriptional regulatory activity. We further validated the ADHM protocol by mapping the DNaseI hypersensitive sites across 250 kb of the human TAL1 locus in CD34+ primary stem/progenitor cells and K562 cells and by mapping the previously known DNaseI hypersensitive sites across 240 kb of the human α-globin locus in K562 cells. ADHM provides a powerful approach to identifying DNaseI hypersensitive sites across large genomic regions.
机译:顺式调控元件的识别对于理解基因转录至关重要。顺式调控元件对用DNaseI消化的超敏性仍然是定位此类元件的金标准方法。用于识别DNaseI超敏位点的传统方法比较麻烦,并且只能应用于限定位置的短片段DNA。在这里,我们报道了一种新的基于基因组阵列的方法对DNaseI超敏位点作图(ADHM)的开发,该方法允许从少至500万个细胞中进行精确,大规模的鉴定。使用ADHM,我们在200 kb的小鼠T细胞急性淋巴细胞白血病1(Tal1)基因座中鉴定了所有先前公认的造血调控元件,此外,在该基因座中鉴定了两个新元件,它们显示了转录调控活性。我们通过在CD34 +主要干细胞/祖细胞和K562细胞中的TALase基因座250 kb上绘制DNaseI超敏位点,并在240 kb的人α-珠蛋白基因座中绘制先前已知的DNaseI超敏位点,进一步验证了ADHM协议。 K562细胞。 ADHM提供了一种强大的方法来识别大基因组区域中的DNaseI超敏位点。

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