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首页> 美国卫生研究院文献>Molecular and Cellular Biology >Correlation between patterns of DNase I-hypersensitive sites and upstream promoter activity of the human epsilon-globin gene at different stages of erythroid development.
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Correlation between patterns of DNase I-hypersensitive sites and upstream promoter activity of the human epsilon-globin gene at different stages of erythroid development.

机译:DNase I超敏性位点的模式与人类ε-珠蛋白基因在红系发育不同阶段的上游启动子活性之间的相关性。

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DNA 5' to the human epsilon-globin gene exhibits unique patterns of DNase I-hypersensitive sites (DHS) in three human erythroleukemic cell lines which represent the embryonic (K562), fetal (HEL), and adult (KMOE) stages of erythroid development. We have mapped 10 epsilon-globin DHS in K562 cells, in which the epsilon-globin gene is maximally active. Major sites are located -11.7, -10.5, -6.5, -2.2 kilobase pairs (kbp) and -200 base pairs (bp) upstream of the gene and directly over the major cap site. Minor sites are located -5.5, -4.5, and -1.48 kbp and -900 bp upstream of the cap site. In HEL cells, in which the epsilon-globin gene is expressed at extremely low levels, the -11.7-, -10.5-, -5.5-, -4.5-, and -2.2-kbp DHS are no longer detectable; the -200-bp site is approximately 300-fold less sensitive to DNase I; and the -1.48-kbp, -900-bp, and major cap site DHS are 3- to 4-fold less sensitive. Only the DHS located -6.5 kbp relative to the major cap site is detectable at all three stages of erythroid development, including KMOE cells in which epsilon-globin synthesis is undetectable. We suggest that this site may be implicated in maintaining the entire beta-globin cluster in an active chromatin conformation. The five DHS downstream of the -6.5-kbp element possess associated promoters. Thus two distinct types of DHS exist--promoter positive and promoter negative. In HEL cells, all the upstream promoters are inactivated, although the -1.48-kbp and -900- and -200-bp DHS are still present. This suggests that the maintenance of DHS and regulation of their associated promoters occur by independent mechanisms. The inactivation of the upstream promoters in HEL cells while the major cap site remains active represents a unique pattern of expression and suggests that HEL cells possess regulatory factors which specifically down regulate the epsilon-globin upstream promoters.
机译:人类ε-珠蛋白基因的DNA 5'在三种人类红白血病细胞系中表现出独特的DNase I超敏性位点(DHS)模式,这三种细胞系代表类红细胞发育的胚胎(K562),胎儿(HEL)和成年(KMOE)阶段。我们在K562细胞中绘制了10个ε-珠蛋白DHS,其中ε-珠蛋白基因具有最大活性。主要位点位于基因上游且直接在主要帽位点上方的-11.7,-10.5,-6.5,-2.2碱基对(kbp)和-200碱基对(bp)。次要站点位于上限站点的上游-5.5,-4.5和-1.48 kbp和-900 bp。在ε-珠蛋白基因以极低水平表达的HEL细胞中,不再检测到-11.7-,-10.5-,-5.5-,-4.5-和-2.2-kbp DHS。 -200-bp位点对DNase I的敏感性降低约300倍;而-1.48-kbp,-900-bp和主要帽位DHS的敏感性降低了3到4倍。在红系发育的所有三个阶段(包括其中无法检测到ε-珠蛋白合成的KMOE细胞),仅相对于主要帽状位点位于-6.5 kbp的DHS是可检测到的。我们建议该位点可能与维持整个β-珠蛋白簇处于活性染色质构象有关。 -6.5-kbp元件下游的五个DHS具有相关的启动子。因此,存在两种不同类型的DHS:启动子阳性和启动子阴性。在HEL细胞中,尽管-1.48-kbp和-900-和-200-bp DHS仍然存在,但所有上游启动子均被灭活。这表明,DHS的维持及其相关启动子的调节是通过独立的机制进行的。 HEL细胞中上游启动子的失活,而主要帽状位点仍处于活跃状态,代表了一种独特的表达方式,这表明HEL细胞具有调节因子,这些调节因子特别下调了ε-珠蛋白的上游启动子。

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