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分支迁移介导的DNA标记与克隆

Branch migration mediated DNA labeling and cloning.

作者信息

Quartin R S, Plewinska M, Wetmur J G

机构信息

Department of Microbiology, Mount Sinai School of Medicine, New York, New York 10029.

出版信息

Biochemistry. 1989 Oct 31;28(22):8676-82. doi: 10.1021/bi00448a002.

Abstract

The sequence-dependent attachment (capture) of an oligodeoxynucleotide duplex containing a single-stranded tail can be mediated by branch migration into the end of a DNA molecule. Substitution of bromodeoxycytidine (BrdC) for deoxycytidine (dC) increased DNA-DNA hybrid stability. BrdC-containing oligodeoxynucleotides displaced dC-containing strands from duplexes with blunt ends or 3'-overhangs. In the later case the rate of displacement was of the same order of magnitude as DNA reassociation. A BrdC-containing displacer oligodeoxynucleotide was used for transient sequence-specific invasion at a particular PstI site. The product was captured by use of T4 DNA ligase and a linker oligodeoxynucleotide. The capture rate was more than 300 times the rate observed for an unrelated PstI site. This high degree of specificity required BrdC substitution. In addition, deliberate incorporation of an incorrect nucleotide into a displacer strand demonstrated that branch migration was terminated at a mismatch. A branched, BrdC-containing ligated product of a capture reaction was cloned and sequenced. The specific capture reaction may be used to label a particular DNA fragment prior to electrophoresis, to mark the specific fragment for affinity chromatography, or to facilitate cloning by introducing a new overhanging sequence compatible with a restriction endonuclease site in a cloning vector.

摘要

含有单链尾巴的寡脱氧核苷酸双链体的序列依赖性附着(捕获)可通过分支迁移到DNA分子末端来介导。用溴脱氧胞苷(BrdC)取代脱氧胞苷(dC)可提高DNA-DNA杂交稳定性。含BrdC的寡脱氧核苷酸从具有平端或3'突出端的双链体中取代含dC的链。在后一种情况下,取代速率与DNA重新缔合处于同一数量级。一种含BrdC的置换寡脱氧核苷酸用于在特定的PstI位点进行瞬时序列特异性侵入。产物通过使用T4 DNA连接酶和连接寡脱氧核苷酸进行捕获。捕获率比在不相关的PstI位点观察到的速率高出300多倍。这种高度的特异性需要BrdC取代。此外,故意将一个错误的核苷酸掺入置换链中表明分支迁移在错配处终止。捕获反应的一个含BrdC的分支连接产物被克隆并测序。特异性捕获反应可用于在电泳前标记特定的DNA片段,为亲和色谱标记特定片段,或通过引入与克隆载体中的限制性内切酶位点兼容的新突出序列来促进克隆。

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