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Screening regulatory sequences from bacterial artificial chromosome DNA of alpha- and beta-globin gene clusters.

机译:从α-和β-珠蛋白基因簇的细菌人工染色体DNA筛选调控序列。

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In the forthcoming postgenomic era, identification of regulatory DNA sequences is becoming increasingly important for characterizing DNA-binding proteins and for elucidating the regulatory mechanisms of gene expression. Presently, there lack efficient methods to broadly screen and identify DNA regulatory elements on a large scale. We established herein an efficient strategy to screen regulatory sequences from bacterial artificial chromosome (BAC) DNAs containing human alpha- and beta-globin gene clusters based on polymerase chain reaction and electrophoretic mobility shift assay (EMSA) techniques without purified transcription factors. Twenty-three subclones derived from alpha-BAC DNA by bulk EMSA selection retained the ability to bind nuclear proteins of K562 cells when retested by EMSA. In 19 clones sequenced, 14 are identical to those registered in GenBank and five have one base difference. All of the 24 randomly picked beta-BAC clones showed specific binding with nuclear proteins of K562 cells. In 11 clones sequenced, eight are identical to those registered in GenBank and three have one base difference. This approach could be particularly powerful if combined with other systematic methods for identifying cis-regulatory DNA elements.
机译:在即将到来的后基因组时代,调节DNA序列的鉴定对于表征DNA结合蛋白和阐明基因表达的调节机制变得越来越重要。当前,缺乏有效的方法来大规模地大规模筛选和鉴定DNA调控元件。我们在这里建立了一种有效的策略,可基于聚合酶链反应和电泳迁移率变动分析(EMSA)技术,从不含人转录因子的人类人工染色体(BAC)DNA中筛选包含人α-和β-珠蛋白基因簇的调控序列。当通过EMSA重新测试时,通过批量EMSA选择衍生自alpha-BAC DNA的23个亚克隆保留了结合K562细胞核蛋白的能力。在测序的19个克隆中,有14个与GenBank中注册的克隆相同,而五个则有一个碱基差异。 24个随机选择的β-BAC克隆均显示出与K562细胞核蛋白的特异性结合。在测序的11个克隆中,有8个与GenBank中注册的克隆相同,其中3个具有一个碱基差异。如果与其他用于鉴定顺式调节性DNA元素的系统方法结合使用,该方法可能会特别有效。

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