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在体外模拟拥挤的细胞内环境可显著提高逆转录聚合酶链反应(RT-PCR)的性能。

Emulating a crowded intracellular environment in vitro dramatically improves RT-PCR performance.

作者信息

Lareu Ricky R, Harve Karthik S, Raghunath Michael

机构信息

Tissue Modulation Laboratory, Division of Bioengineering, Faculty of Engineering, National University of Singapore, Division Office Block E3A #04-15, 7 Engineering Drive 1, Singapore 117574, Singapore.

出版信息

Biochem Biophys Res Commun. 2007 Nov 9;363(1):171-7. doi: 10.1016/j.bbrc.2007.08.156. Epub 2007 Sep 5.

Abstract

The polymerase chain reaction's (PCR) phenomenal success in advancing fields as diverse as Medicine, Agriculture, Conservation, or Paleontology is based on the ability of using isolated prokaryotic thermostable DNA polymerases in vitro to copy DNA irrespective of origin. This process occurs intracellularly and has evolved to function efficiently under crowded conditions, namely in an environment packed with macromolecules. However, current in vitro practice ignores this important biophysical parameter of life. In order to more closely emulate conditions of intracellular biochemistry in vitro we added inert macromolecules into reverse transcription (RT) and PCR. We show dramatic improvements in all parameters of RT-PCR including 8- to 10-fold greater sensitivity, enhanced polymerase processivity, higher specific amplicon yield, greater primer annealing and specificity, and enhanced DNA polymerase thermal stability. The faster and more efficient reaction kinetics was a consequence of the cumulative molecular and thermodynamic effects of the excluded volume effect created by macromolecular crowding.

摘要

聚合酶链反应(PCR)在医学、农业、保护生物学或古生物学等诸多领域取得了巨大成功,这基于在体外使用分离的原核热稳定DNA聚合酶复制DNA的能力,而不论其来源如何。这个过程在细胞内发生,并且已经进化到在拥挤条件下高效运作,即在充满大分子的环境中。然而,当前的体外实践忽略了生命这一重要的生物物理参数。为了在体外更紧密地模拟细胞内生物化学条件,我们在逆转录(RT)和PCR中添加了惰性大分子。我们展示了RT-PCR所有参数的显著改善,包括灵敏度提高8至10倍、聚合酶持续合成能力增强、特异性扩增产物产量更高、引物退火和特异性增强以及DNA聚合酶热稳定性增强。更快且更高效的反应动力学是大分子拥挤产生的排阻体积效应所带来的累积分子和热力学效应的结果。

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