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通过RecA辅助限制性内切酶(RARE)切割对酵母人工染色体重叠群图谱进行物理校准。

Physical calibration of yeast artificial chromosome contig maps by RecA-assisted restriction endonuclease (RARE) cleavage.

作者信息

Gnirke A, Iadonato S P, Kwok P Y, Olson M V

机构信息

Department of Molecular Biotechnology, University of Washington, Seattle 98195.

出版信息

Genomics. 1994 Nov 15;24(2):199-210. doi: 10.1006/geno.1994.1607.

Abstract

Clone-based genome maps can be constructed by determining the presence or absence of sequence-tagged sites (STSs) in a redundant collection of yeast artificial chromosome clones (YACs). While STS-content mapping has proven to be an effective means of ordering clone ends and STSs along chromosomes, the exact physical map positions of these landmarks are not determined. This fundamental weakness can be overcome by RecA-assisted restriction endonuclease (RARE) cleavage, a method that exploits the binding specificity on duplex DNA of a RecA-protein-oligodeoxynucleotide complex to enhance the cleavage specificity of a restriction endonuclease. This technique allows selective cleavage at individual members of a large set of restriction sites. RARE-cleavage mapping was applied to a contig comprising 5 overlapping YACs spanning 580 kb on human chromosome 14. An STS-content map comprising 10 YAC-end specific STSs and one internal STS was constructed. RARE cleavage was performed on 2 YACs that span the entire contig at the EcoRI sites defining the vector-insert junctions of all 5 YACs, as well as at a HhaI site within the STS that was initially used to screen the YAC library for the clones in the contig. The sizes of the RARE-cleavage fragments were measured by pulsed-field gel electrophoresis and used to convert the STS-content map into a true physical map that indicates precise positions of clone ends and STSs.

摘要

基于克隆的基因组图谱可以通过确定酵母人工染色体克隆(YAC)的冗余集合中序列标签位点(STS)的有无来构建。虽然STS含量图谱已被证明是沿染色体排列克隆末端和STS的有效方法,但这些标志物的确切物理图谱位置尚未确定。这种基本缺陷可以通过RecA辅助限制性内切酶(RARE)切割来克服,该方法利用RecA蛋白 - 寡脱氧核苷酸复合物对双链DNA 的结合特异性来增强限制性内切酶的切割特异性。该技术允许在一大组限制性位点的单个成员处进行选择性切割。RARE切割图谱应用于一个重叠群,该重叠群由跨越人类14号染色体上580 kb的5个重叠YAC组成。构建了一个包含10个YAC末端特异性STS和一个内部STS的STS含量图谱。在定义所有5个YAC的载体 - 插入连接的EcoRI位点以及最初用于筛选重叠群中克隆的YAC文库的STS内的HhaI位点上,对跨越整个重叠群的2个YAC进行了RARE切割。通过脉冲场凝胶电泳测量RARE切割片段的大小,并用于将STS含量图谱转换为指示克隆末端和STS精确位置的真实物理图谱。

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