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蓝光调控的双组分系统:光-氧-电压(LOV)-组氨酸激酶和下游响应调节剂的酶学和功能分析。

Blue light regulated two-component systems: enzymatic and functional analyses of light-oxygen-voltage (LOV)-histidine kinases and downstream response regulators.

机构信息

Departments of Biophysics and Biochemistry, University of Texas Southwestern Medical Center , Dallas, Texas 75390, United States.

出版信息

Biochemistry. 2013 Jul 9;52(27):4656-66. doi: 10.1021/bi400617y. Epub 2013 Jun 27.

Abstract

Light is an essential environmental cue for diverse organisms. Many prokaryotic blue light photoreceptors use light, oxygen, voltage (LOV) sensory domains to control the activities of diverse output domains, including histidine kinases (HK). Upon activation, these proteins autophosphorylate a histidine residue before subsequently transferring the phosphate to an aspartate residue in the receiver domain of a cognate response regulator (RR). Such phosphorylation activates the output domain of the RR, leading to changes in gene expression, protein-protein interactions, or enzymatic activities. Here, we focus on one such light sensing LOV-HK from the marine bacterium Erythrobacter litoralis HTCC2594 (EL368), seeking to understand how kinase activity and subsequent downstream effects are regulated by light. We found that photoactivation of EL368 led to a significant enhancement in the incorporation of phosphate within the HK domain. Further enzymatic studies showed that the LOV domain affected both the LOV-HK turnover rate (kcat) and Km in a light-dependent manner. Using in vitro phosphotransfer profiling, we identified two target RRs for EL368 and two additional LOV-HKs (EL346 and EL362) encoded within the host genome. The two RRs include a PhyR-type transcriptional regulator (EL_PhyR) and a receiver-only protein (EL_LovR), reminiscent of stress-triggered systems in other bacteria. Taken together, our data provide a biochemical foundation for this light-regulated signaling module of sensors, effectors, and regulators that control bacterial responses to environmental conditions.

摘要

光是许多原核生物蓝光光感受器控制各种输出域活性的必需环境线索,这些输出域包括组氨酸激酶(HK)。这些蛋白在被激活后,会在随后将磷酸基团转移到同源响应调节蛋白(RR)的受体域中的天冬氨酸残基之前,先将组氨酸残基自身磷酸化。这种磷酸化激活 RR 的输出域,导致基因表达、蛋白质-蛋白质相互作用或酶活性的变化。在这里,我们关注的是来自海洋细菌 Erythrobacter litoralis HTCC2594(EL368)的一种这样的光感应 LOV-HK,试图了解激酶活性和随后的下游效应是如何被光调节的。我们发现,EL368 的光激活导致 HK 域内磷酸化的显著增强。进一步的酶学研究表明,LOV 域以光依赖性的方式影响 LOV-HK 的周转率(kcat)和 Km。使用体外磷酸转移分析,我们确定了 EL368 的两个靶 RR 和宿主基因组中编码的另外两个 LOV-HK(EL346 和 EL362)。这两个 RR 包括一个 PhyR 型转录调节蛋白(EL_PhyR)和一个仅受体蛋白(EL_LovR),这让人联想到其他细菌中应激触发系统。总之,我们的数据为这个光调控的传感器、效应器和调节剂信号模块提供了生化基础,该模块控制着细菌对环境条件的反应。

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