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模块化蛋白质-寡核苷酸信号交换

Modular protein-oligonucleotide signal exchange.

作者信息

Agrawal Deepak K, Schulman Rebecca

机构信息

Department of Chemical and Biomolecular Engineering, Johns Hopkins University, 3400 N Charles St, Baltimore, MD 21218, USA.

Department of Bioengineering, University of Colorado Medicine, Aurora, CO 80045, USA.

出版信息

Nucleic Acids Res. 2020 Jul 9;48(12):6431-6444. doi: 10.1093/nar/gkaa405.

Abstract

While many methods are available to measure the concentrations of proteins in solution, the development of a method to quantitatively report both increases and decreases in different protein concentrations in real-time using changes in the concentrations of other molecules, such as DNA outputs, has remained a challenge. Here, we present a biomolecular reaction process that reports the concentration of an input protein in situ as the concentration of an output DNA oligonucleotide strand. This method uses DNA oligonucleotide aptamers that bind either to a specific protein selectively or to a complementary DNA oligonucleotide reversibly using toehold-mediated DNA strand-displacement. It is possible to choose the sequence of output strand almost independent of the sensing protein. Using this strategy, we implemented four different exchange processes to report the concentrations of clinically relevant human α-thrombin and vascular endothelial growth factor using changes in concentrations of DNA oligonucleotide outputs. These exchange processes can operate in tandem such that the same or different output signals can indicate changes in concentration of distinct or identical input proteins. The simplicity of our approach suggests a pathway to build devices that can direct diverse output responses in response to changes in concentrations of specific proteins.

摘要

虽然有许多方法可用于测量溶液中蛋白质的浓度,但开发一种利用其他分子(如DNA输出)浓度变化实时定量报告不同蛋白质浓度增减的方法仍然是一个挑战。在此,我们展示了一种生物分子反应过程,该过程可将输入蛋白质的浓度原位报告为输出DNA寡核苷酸链的浓度。此方法使用DNA寡核苷酸适配体,这些适配体要么选择性地与特定蛋白质结合,要么通过链置换介导的DNA链置换可逆地与互补DNA寡核苷酸结合。几乎可以独立于传感蛋白来选择输出链的序列。利用这一策略,我们实施了四种不同的交换过程,通过DNA寡核苷酸输出浓度的变化来报告临床相关的人α-凝血酶和血管内皮生长因子的浓度。这些交换过程可以串联运行,这样相同或不同的输出信号可以指示不同或相同输入蛋白质浓度的变化。我们方法的简单性为构建能够响应特定蛋白质浓度变化而产生不同输出响应的装置提供了一条途径。

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