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一种荧光胞苷TNA三磷酸类似物的合成与聚合酶活性

Synthesis and polymerase activity of a fluorescent cytidine TNA triphosphate analogue.

作者信息

Mei Hui, Shi Changhua, Jimenez Randi M, Wang Yajun, Kardouh Miramar, Chaput John C

机构信息

Department of Pharmaceutical Sciences, University of California, Irvine, CA 92697-3958, USA.

出版信息

Nucleic Acids Res. 2017 Jun 2;45(10):5629-5638. doi: 10.1093/nar/gkx368.

Abstract

Threose nucleic acid (TNA) is an artificial genetic polymer capable of undergoing Darwinian evolution to produce aptamers with affinity to specific targets. This property, coupled with a backbone structure that is refractory to nuclease digestion, makes TNA an attractive biopolymer system for diagnostic and therapeutic applications. Expanding the chemical diversity of TNA beyond the natural bases would enable the development of functional TNA molecules with enhanced physiochemical properties. Here, we describe the synthesis and polymerase activity of a fluorescent cytidine TNA triphosphate analogue (1,3-diaza-2-oxo-phenothiazine, tCfTP) that maintains Watson-Crick base pairing with guanine. Polymerase-mediated primer-extension assays reveal that tCfTP is efficiently added to the growing end of a TNA primer. Detailed kinetic assays indicate that tCfTP and tCTP have comparable rates for the first nucleotide incorporation step (kobs1). However, addition of the second nucleotide (kobs2) is 700-fold faster for tCfTP than tCTP due the increased effects of base stacking. Last, we found that TNA replication using tCfTP in place of tCTP exhibits 98.4% overall fidelity for the combined process of TNA transcription and reverse transcription. Together, these results expand the chemical diversity of enzymatically generated TNA molecules to include a hydrophobic base analogue with strong fluorescent properties that is compatible with in vitro selection.

摘要

苏糖核酸(TNA)是一种人工遗传聚合物,能够经历达尔文进化过程以产生对特定靶标具有亲和力的适体。这一特性,再加上对核酸酶消化具有抗性的主链结构,使得TNA成为一种用于诊断和治疗应用的有吸引力的生物聚合物系统。将TNA的化学多样性扩展到天然碱基之外,将能够开发出具有增强理化性质的功能性TNA分子。在此,我们描述了一种荧光胞苷TNA三磷酸类似物(1,3-二氮杂-2-氧代吩噻嗪,tCfTP)的合成及其聚合酶活性,该类似物与鸟嘌呤保持沃森-克里克碱基配对。聚合酶介导的引物延伸试验表明,tCfTP能够有效地添加到TNA引物的生长末端。详细的动力学试验表明,在第一个核苷酸掺入步骤中,tCfTP和tCTP具有相当的速率(kobs1)。然而,由于碱基堆积效应的增加,tCfTP添加第二个核苷酸的速度(kobs2)比tCTP快700倍。最后,我们发现用tCfTP代替tCTP进行TNA复制时,在TNA转录和逆转录的联合过程中总体保真度为98.4%。总之,这些结果扩展了酶促生成的TNA分子的化学多样性,使其包括一种具有强荧光特性且与体外筛选兼容的疏水碱基类似物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3c4e/5449585/33a9b6e42a13/gkx368fig1.jpg

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