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硝酸盐传感器 NarX 揭示了传感器磷酸酶控制双组分信号的保守机制。

Conserved mechanism for sensor phosphatase control of two-component signaling revealed in the nitrate sensor NarX.

机构信息

Department of Microbiology, University of California, Davis, CA 95616-8665, USA.

出版信息

Proc Natl Acad Sci U S A. 2010 Dec 7;107(49):21140-5. doi: 10.1073/pnas.1013081107. Epub 2010 Nov 15.

Abstract

Two-component signal transduction mediates a wide range of phenotypes in microbes and plants. The sensor transmitter module controls the phosphorylation state of the cognate-response-regulator receiver domain. Whereas the two-component autokinase and phosphotransfer reactions are well-understood, the mechanism by which sensors accelerate the rate of phospho-response regulator dephosphorylation, termed "transmitter phosphatase activity," is unknown. We identified a conserved DxxxQ motif adjacent to the phospho-accepting His residue in the HisKA_3 subfamily of two-component sensors. We used site-specific mutagenesis to make substitutions for these conserved Gln and Asp residues in the nitrate-responsive NarX sensor and analyzed function both in vivo and in vitro. Results show that the Gln residue is critical for transmitter phosphatase activity, but is not essential for autokinase or phosphotransfer activities. The documented role of an amide moiety in phosphoryl group hydrolysis suggests an analogous catalytic function for this Gln residue in HisKA_3 members. Results also indicate that the Asp residue is important for both autokinase and transmitter phosphatase activities. Furthermore, we noted that sensors of the HisKA subfamily exhibit an analogous E/DxxT/N motif, the conserved Thr residue of which is critical for transmitter phosphatase activity of the EnvZ sensor. Thus, two-component sensors likely use similar mechanisms for receiver domain dephosphorylation.

摘要

双组分信号转导介导了微生物和植物中广泛的表型。传感器发射器模块控制同源反应调节剂接收器结构域的磷酸化状态。虽然双组分自激酶和磷酸转移反应已经得到很好的理解,但传感器加速磷酸化反应调节蛋白去磷酸化的机制,即“发射器磷酸酶活性”,尚不清楚。我们在双组分传感器的 HisKA_3 亚家族中发现了一个紧邻磷酸接受 His 残基的保守 DxxxQ 模体。我们使用定点突变技术对硝酸盐响应的 NarX 传感器中的这些保守 Gln 和 Asp 残基进行了取代,并在体内和体外分析了它们的功能。结果表明,Gln 残基对于发射器磷酸酶活性至关重要,但对于自激酶或磷酸转移活性并非必需。酰胺部分在磷酸基团水解中的作用表明,HisKA_3 成员中的这个 Gln 残基具有类似的催化功能。结果还表明,Asp 残基对于自激酶和发射器磷酸酶活性都很重要。此外,我们注意到 HisKA 亚家族的传感器表现出类似的 E/DxxT/N 模体,其中保守的 Thr 残基对于 EnvZ 传感器的发射器磷酸酶活性至关重要。因此,双组分传感器可能使用类似的机制进行受体结构域去磷酸化。

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