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用于基因组SELEX的文库。

Libraries for genomic SELEX.

作者信息

Singer B S, Shtatland T, Brown D, Gold L

机构信息

Department of Molecular Biology, University of Colorado, Boulder 80309-0347, USA.

出版信息

Nucleic Acids Res. 1997 Feb 15;25(4):781-6. doi: 10.1093/nar/25.4.781.

Abstract

An increasing number of proteins are being identified that regulate gene expression by binding specific nucleic acidsin vivo. A method termed genomic SELEX facilitates the rapid identification of networks of protein-nucleic acid interactions by identifying within the genomic sequences of an organism the highest affinity sites for any protein of the organism. As with its progenitor, SELEX of random-sequence nucleic acids, genomic SELEX involves iterative binding, partitioning, and amplification of nucleic acids. The two methods differ in that the variable region of the nucleic acid library for genomic SELEX is derived from the genome of an organism. We have used a quick and simple method to construct Escherichia coli, Saccharomyces cerevisiae, and human genomic DNA PCR libraries that can be transcribed with T7 RNA polymerase. We present evidence that the libraries contain overlapping inserts starting at most of the positions within the genome, making these libraries suitable for genomic SELEX.

摘要

越来越多的蛋白质被鉴定出可在体内通过结合特定核酸来调控基因表达。一种称为基因组SELEX的方法,通过在生物体的基因组序列中识别该生物体任何蛋白质的最高亲和力位点,促进了蛋白质 - 核酸相互作用网络的快速鉴定。与其前身——随机序列核酸的SELEX一样,基因组SELEX涉及核酸的迭代结合、分区和扩增。这两种方法的不同之处在于,用于基因组SELEX的核酸文库的可变区来自生物体的基因组。我们使用了一种快速简单的方法来构建可被T7 RNA聚合酶转录的大肠杆菌、酿酒酵母和人类基因组DNA PCR文库。我们提供的证据表明,这些文库包含从基因组内大多数位置起始的重叠插入片段,使得这些文库适用于基因组SELEX。

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