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Aspects of protein–DNA interactions: a review of quantitative thermodynamic theory for modelling synthetic circuits utilising LacI and CI repressors, IPTG and the reporter gene lacZ

机译:蛋白质与DNA相互作用的方面:使用LacI和CI阻遏物,IPTG和报告基因lacZ对合成电路建模的定量热力学理论综述

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摘要

Protein–DNA interactions are central to the control of gene expression across all forms of life. The development of approaches to rigorously model such interactions has often been hindered both by a lack of quantitative binding data and by the difficulty in accounting for parameters relevant to the intracellular situation, such as DNA looping and thermodynamic non-ideality. Here, we review these considerations by developing a thermodynamically based mathematical model that attempts to simulate the functioning of an Escherichia coli expression system incorporating two of the best characterised prokaryotic DNA binding proteins, Lac repressor and lambda CI repressor. The key aim was to reproduce experimentally observed reporter gene activities arising from the expression of either wild-type CI repressor or one of three positive-control CI mutants. The model considers the role of several potentially important, but sometimes neglected, biochemical features, including DNA looping, macromolecular crowding and non-specific binding, and allowed us to obtain association constants for the binding of CI and its variants to a specific operator sequence.
机译:蛋白质与DNA的相互作用对于控制所有生命形式的基因表达至关重要。由于缺乏定量结合数据和难以解释与细胞内情况相关的参数(例如DNA环化和热力学非理想性),常常阻碍了对此类相互作用进行严格建模的方法的开发。在这里,我们通过开发基于热力学的数学模型来回顾这些考虑,该数学模型试图模拟结合了两种最典型的原核DNA结合蛋白Lac阻遏物和lambda CI阻遏物的大肠杆菌表达系统的功能。关键目的是重现通过实验观察到的报道基因活性,该活性由野生型CI阻遏物或三个阳性对照CI突变体之一的表达引起。该模型考虑了几个潜在的重要但有时被忽略的生化特征的作用,包括DNA环化,大分子拥挤和非特异性结合,并允许我们获得CI及其变体与特定操纵基因序列结合的缔合常数。

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