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Development and characterization of a UV-violet/Green photoreversible transcriptional regulator in E.coli.

机译:紫外线-绿色/绿色光可逆转录调节因子在大肠杆菌中的开发和表征。

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摘要

Genetically encoded photoreceptors, or optogenetic tools, have been used to leverage the tractability of light as an input signal to control biological processes in vivo with unrivaled spatiotemporal precision. The Tabor lab has previously engineered green/red and red/far-red photoreversible two-component systems (TCS) for quantitative, programmable control of transcription dynamics. A photoreversible optogenetic tool with spectral sensitivity in the UV-blue region of the visible spectrum would enable new optogenetic applications in single-cell microscopy, and could be combined with existing tools for dynamic control of multiple genes.;In this work, we engineer a photoreversible UV-violet/Green transcriptional regulator in E.coli by repurposing the light-switchable cyanobacteriochrome TCS UirS-UirR from Synechocystis PCC 6803. We demonstrate that UirS-UirR regulates the promoter of the low carbon stress-induced small RNA csiR1 (PcsiR1) ∼6-fold in response to UV-light. Using a combination of mutations, dose-response experiments, and in vivo phosphorylation measurements, we show that UirS phosphorylates UirR to activate transcription from PcsiR1 in a UV-light dependent manner. This result is in contrast to a proposed sequestration model for UirS-UirR.;By measuring the action spectra of UirS-UirR, we show that it responds specifically in the narrow (380-420nm) UV-violet region of the visible spectrum. We show that the gene expression response to input light occurs in minutes and exploit these rapid dynamics to predictably program gene expression signals. By truncating N-terminal protein domains in UirS, we identify an improved sensor with >15-fold light-induced dynamic range but similar response characteristics as UirS.;UirS-UirR is the first photoreversible optogenetic tool that responds in the UV-violet region of the visible spectrum, and could be combined with our previously engineered green/red and red/far-red sensors for precise three-input, three-output optogenetic control of transcription, enabling new modes of characterization and control in systems and synthetic biology and metabolic engineering studies.;UirS contains a functional ethylene-binding domain similar to the Arabidopsis thaliana ethylene receptors, but is not known have an ethylene response. We have used the E. coli UirS-UirR system for studying the putative ethylene response of UirS heterologously, free of the cross-regulatory networks present in Synechocystis PCC6803. This work provides preliminary evidence that at least in E.coli, UirS does not have a signalling response to ethylene, or that the ethylene response is not transduced through UirR. The UirS-UirR E.coli system provides a test-bed to study the remarkable spectral diversity of the 'DXCF cyanobacteriochrome' family of photoreceptors, and the signaling properties of TCSs containing AraC-family DNA binding domains, which are involved in pathogenesis but are poorly understood.
机译:遗传编码的感光体或光遗传学工具已被用来利用光的可牵引性作为输入信号,以无与伦比的时空精度控制体内的生物过程。 Tabor实验室以前设计了绿色/红色和红色/远红色的光可逆两组分系统(TCS),用于定量,可编程地控制转录动力学。在可见光谱的紫外蓝色区域具有光谱敏感性的光可逆光遗传学工具将使单细胞显微镜能够实现新的光遗传学应用,并且可以与用于动态控制多个基因的现有工具相结合;在这项工作中,我们设计了一个通过重新利用来自集胞藻PCC 6803的可光转换的蓝细菌色素TCS UirS-UirR,来在大肠杆菌中建立光可逆的紫外线/绿色转录调节因子。我们证明了UirS-UirR调节低碳胁迫诱导的小RNA csiR1(PcsiR1)的启动子响应紫外线约6倍。使用突变,剂量反应实验和体内磷酸化测量的组合,我们显示UirS磷酸化UirR以激活依赖于UV-光的方式从PcsiR1转录。该结果与为UirS-UirR提出的隔离模型相反;通过测量UirS-UirR的作用光谱,我们显示出它在可见光谱的狭窄(380-420nm)紫外线-紫色区域中有特殊反应。我们表明,对输入光的基因表达响应在几分钟内发生,并利用这些快速动力学来可预测地编程基因表达信号。通过截断UirS中的N末端蛋白结构域,我们确定了一种改进的传感器,其光诱导动态范围> 15倍,但响应特性与UirS相似。; UirS-UirR是第一个在紫外线-紫光区域做出响应的光可逆光遗传学工具可以与我们以前设计的绿色/红色和红色/远红色传感器组合使用,以实现精确的三输入,三输出转录的光遗传学控制,从而实现系统和合成生物学以及代谢工程学研究; UirS包含一个与拟南芥乙烯受体相似的功能性乙烯结合域,但尚不知道其具有乙烯反应。我们已经使用大肠杆菌UirS-UirR系统来异源地研究UirS的假定乙烯反应,而没有Synechocystis PCC6803中存在的交叉调节网络。这项工作提供了初步的证据,即至少在大肠杆菌中,UirS没有对乙烯的信号传导应答,或者乙烯应答没有通过UirR进行转导。 UirS-UirR大肠杆菌系统提供了一个试验台,用于研究“ DXCF蓝细菌色素”家族光感受器的显着光谱多样性,以及含有AraC家族DNA结合域的TCS的信号传导特性,这些参与了发病机制,但知之甚少。

著录项

  • 作者

    Ramakrishnan, Prabha.;

  • 作者单位

    Rice University.;

  • 授予单位 Rice University.;
  • 学科 Biomedical engineering.;Molecular biology.;Microbiology.
  • 学位 Ph.D.
  • 年度 2017
  • 页码 145 p.
  • 总页数 145
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

  • 入库时间 2022-08-17 11:38:47

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