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从头设计一种孕激素生物传感器的转录因子。

De novo design of a transcription factor for a progesterone biosensor.

机构信息

State Key Laboratory of Bioreactor Engineering, Newworld Institute of Biotechnology, East China University of Science and Technology, 130 Meilong Road, Shanghai, 200237, China.

School of Ethnic Medicine, Chengdu University of Traditional Chinese Medicine, Chengdu, 611137, China.

出版信息

Biosens Bioelectron. 2022 May 1;203:113897. doi: 10.1016/j.bios.2021.113897. Epub 2021 Dec 20.

DOI:10.1016/j.bios.2021.113897
PMID:35134684
Abstract

Identifying, isolating, and obtaining naturally occurring transcription factors (TFs) is crucial for developing transcription-dependent biosensors. However, identifying and optimizing TFs for given molecules requires extensive time and effort. Accordingly, here, we report a strategy for the de novo design of a nonnatural TF, DLA, on the basis of a subtle conformational change of the ligand-binding domain (LBD) after the binding of a target molecule with its receptor. For the de novo design of DLA, we applied molecular dynamics to simulate different conformational states of DLA in order to understand the complete activity of DLA, which involves shortening of the distance between the DNA-binding domain (DBD) and the activation domain (AD) after progesterone binds to its LBD within DLA. The simulated results suggested that prokaryotic LexA, a truncated LBD from the progesterone receptor, and prokaryotic B42 together constitute DLA with a TF function. As a proof of concept, DLA was used as a transcription activator controlling the transcription of green fluorescent protein to construct an S. cerevisiae biosensor for progesterone detection. The progesterone-specific biosensor was successfully constructed with a sensitivity index EC of 27 μg/L, working range (0.16-60 μg/L), and time-to-detection (2.5 h). Ultimately, a low-cost, user-friendly kit was developed for the rapid detection of progesterone in the clinic. Theoretically, this work can also be used to develop a variety of other biosensors by employing the same strategy.

摘要

鉴定、分离和获取天然存在的转录因子(TFs)对于开发依赖转录的生物传感器至关重要。然而,确定和优化给定分子的 TFs 需要大量的时间和精力。因此,在这里,我们报告了一种基于目标分子与其受体结合后配体结合域(LBD)细微构象变化来从头设计非天然 TF 的策略,即 DLA。为了从头设计 DLA,我们应用分子动力学模拟 DLA 的不同构象状态,以了解 DLA 的完整活性,其中包括 DLA 中的孕激素结合其 LBD 后 DNA 结合域(DBD)和激活域(AD)之间距离的缩短。模拟结果表明,原核 LexA(孕激素受体中截断的 LBD)和原核 B42 一起构成了具有 TF 功能的 DLA。作为概念验证,我们将 DLA 用作转录激活剂来控制绿色荧光蛋白的转录,以构建用于检测孕激素的 S. cerevisiae 生物传感器。成功构建了孕激素特异性生物传感器,其灵敏度指数 EC 为 27μg/L,工作范围(0.16-60μg/L),检测时间(2.5h)。最终,开发了一种低成本、用户友好的试剂盒,用于临床快速检测孕激素。从理论上讲,通过采用相同的策略,这项工作也可用于开发各种其他生物传感器。

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