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通过亲和捕获选择性富集大尺寸基因组DNA片段:一种基因组图谱绘制方法。

Selective enrichment of a large size genomic DNA fragment by affinity capture: an approach for genome mapping.

作者信息

Kandpal R P, Ward D C, Weissman S M

机构信息

Department of Human Genetics, Yale University School of Medicine, New Haven, CT 06510.

出版信息

Nucleic Acids Res. 1990 Apr 11;18(7):1789-95. doi: 10.1093/nar/18.7.1789.

Abstract

A method to enrich large size DNA fragments obtained by digestion with rare cutting restriction endonucleases was developed and applied for the isolation of a 150 kb SfiI fragment containing the beta-globin gene cluster. The digested DNA is rendered single stranded at the ends by diffusing a strand specific exonuclease into an agarose plug containing DNA. The plug is melted and solution hybridization is then performed with a bridge RNA containing specific sequences from the end of a desired fragment linked to a common probe sequence. The common probe sequence is annealed to a biotinylated RNA and the resulting tripartite hybrid is retained onto a solid matrix containing avidin and specifically released by ribonuclease action. Enrichments of greater than 350 fold have been achieved consistently. Such directed purification of large DNA fragments without cloning can considerably expedite mapping and gene localization in a complex genome and facilitate the construction of sublibraries from defined regions of the genome.

摘要

开发了一种富集用稀有切割限制内切酶消化获得的大尺寸DNA片段的方法,并将其应用于分离包含β-珠蛋白基因簇的150 kb SfiI片段。通过将链特异性核酸外切酶扩散到含有DNA的琼脂糖凝胶块中,使消化后的DNA末端变为单链。将凝胶块融化,然后用含有与共同探针序列相连的所需片段末端特定序列的桥接RNA进行溶液杂交。共同探针序列与生物素化RNA退火,产生的三方杂交体保留在含有抗生物素蛋白的固体基质上,并通过核糖核酸酶作用特异性释放。始终实现了超过350倍的富集。这种无需克隆的大DNA片段定向纯化可大大加快复杂基因组中的图谱绘制和基因定位,并有助于从基因组的特定区域构建亚文库。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c50a/330597/487b55f13510/nar00191-0112-a.jpg

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