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嗜热 DNA 聚合酶的进化用于识别和扩增 C2'-修饰的 DNA。

Evolution of thermophilic DNA polymerases for the recognition and amplification of C2'-modified DNA.

机构信息

Department of Chemistry, The Scripps Research Institute, 10550 North Torrey Pines Road, La Jolla, California 92037, USA.

出版信息

Nat Chem. 2016 Jun;8(6):556-62. doi: 10.1038/nchem.2493. Epub 2016 Apr 18.

Abstract

The PCR amplification of oligonucleotides enables the evolution of sequences called aptamers that bind specific targets with antibody-like affinity. However, in many applications the use of these aptamers is limited by nuclease-mediated degradation. In contrast, oligonucleotides that are modified at their sugar C2' positions with methoxy or fluorine substituents are stable to nucleases, but they cannot be synthesized by natural polymerases. Here we report the development of a polymerase-evolution system and its use to evolve thermostable polymerases that efficiently interconvert C2'-OMe-modified oligonucleotides and their DNA counterparts via 'transcription' and 'reverse transcription' or, more importantly, that PCR-amplify partially C2'-OMe- or C2'-F-modified oligonucleotides. A mechanistic analysis demonstrates that the ability to amplify the modified oligonucleotides evolved by optimizing interdomain interactions that stabilize the catalytically competent closed conformation of the polymerase. The evolved polymerases should find practical applications and the developed evolution system should be a powerful tool for tailoring polymerases to have other types of novel function.

摘要

寡核苷酸的 PCR 扩增使能够进化出称为适体的序列,这些序列具有类似于抗体的亲和力,可以结合特定的靶标。然而,在许多应用中,这些适体的使用受到核酶介导的降解的限制。相比之下,在其糖 C2'位置用甲氧基或氟取代的修饰寡核苷酸对核酶稳定,但它们不能被天然聚合酶合成。在这里,我们报告了聚合酶进化系统的开发及其用于进化耐热聚合酶的用途,该聚合酶通过“转录”和“反转录”有效地相互转化 C2'-OMe 修饰的寡核苷酸及其 DNA 对应物,或者更重要的是,能够 PCR 扩增部分 C2'-OMe 或 C2'-F 修饰的寡核苷酸。机理分析表明,通过优化稳定聚合酶催化活性封闭构象的结构域间相互作用,进化出了能够扩增修饰寡核苷酸的能力。进化出的聚合酶应该会有实际的应用,而开发的进化系统应该是定制具有其他新型功能的聚合酶的有力工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5a06/4880425/57ceb17836f9/nihms766025f1.jpg

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