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通过乳液聚合酶链反应及后续链分离制备修饰的组合DNA文库

[Preparation of Modified Combinatorial DNA Libraries via Emulsion PCR with Subsequent Strand Separation].

作者信息

Lapa S A, Romashova K S, Spitsyn M A, Shershov V E, Kuznetsova V E, Guseinov T O, Zasedateleva O A, Radko S P, Timofeev E N, Lisitsa A V, Chudinov A V

机构信息

Engelhardt Institute of Molecular Biology, Russian Academy of Sciences, Moscow, 119991 Russia.

IBMC-EcoBioPharm Ltd., Moscow, 119121 Russia.

出版信息

Mol Biol (Mosk). 2018 Nov-Dec;52(6):984-996. doi: 10.1134/S0026898418060113.

Abstract

A modification of the enzymatic method for the preparation of combinatorial random DNA libraries, which combines amplification in isolated microvolumes with the simultaneous incorporation of modified nucleotides and subsequent separation of DNA strands, was developed. Deoxyuridine triphosphate with hydrophobic substituents such as structural analogues of amino acid side chains in the C5 position of the pyrimidine ring was used to introduce modifications into DNA. To prevent competitive amplification, which reduces the representativeness of combinatorial libraries, PCR in inverse emulsion was used. The separation of the strands of PCR products was carried out. There were six single-stranded DNA libraries with complete substitution of deoxythymidine via modified analogues with various functional groups. These DNA libraries are suitable for generating aptamers to protein targets through additional hydrophobic interactions from the introductions of appropriate modifications, and are completely compatible with the SELEX aptamer selection methodology.

摘要

开发了一种用于制备组合随机DNA文库的酶法改进方法,该方法将在分离的微体积中进行扩增与同时掺入修饰核苷酸以及随后分离DNA链相结合。使用在嘧啶环C5位置带有疏水取代基(如氨基酸侧链结构类似物)的三磷酸脱氧尿苷将修饰引入DNA。为防止竞争性扩增(这会降低组合文库的代表性),采用了反相乳液PCR。对PCR产物的链进行了分离。有六个单链DNA文库,其中脱氧胸苷通过具有各种官能团的修饰类似物完全被取代。这些DNA文库适用于通过引入适当修饰产生的额外疏水相互作用来生成针对蛋白质靶标的适配体,并且与SELEX适配体筛选方法完全兼容。

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