Department of Microbiology and Immunology, University of North Carolina, Chapel Hill, North Carolina, USA.
Department of Microbiology and Immunology, University of North Carolina, Chapel Hill, North Carolina, USA
J Bacteriol. 2020 Jul 9;202(15). doi: 10.1128/JB.00089-20.
Microorganisms and plants utilize two-component systems to regulate adaptive responses to changing environmental conditions. Sensor kinases detect stimuli and alter their autophosphorylation activity accordingly. Signal propagation occurs via the transfer of phosphoryl groups from upstream kinases to downstream response regulator proteins. Removal of phosphoryl groups from the response regulator typically resets the system. Members of the same protein family may catalyze phosphorylation and dephosphorylation reactions with different efficiencies, exhibiting rate constants spanning many orders of magnitude to accommodate response time scales from milliseconds to days. We previously found that variable positions one or two residues to the C-terminal side of the conserved Asp phosphorylation site (D+2) or Thr/Ser (T+1/T+2) in response regulators alter reaction kinetics by direct interaction with phosphodonor or phosphoacceptor molecules. Here, we explore the kinetic effects of amino acid substitutions at the two positions immediately C-terminal to the conserved Lys (K+1/K+2) in the model response regulator CheY. We measured CheY autophosphorylation and autodephosphorylation rate constants for 27 pairs of K+1/K+2 residues that represent 84% of naturally occurring response regulators. Effects on autodephosphorylation were modest, but autophosphorylation rate constants varied by 2 orders of magnitude, suggesting that the K+1/K+2 positions influence reaction kinetics by altering the conformational spectrum sampled by CheY at equilibrium. Additional evidence supporting this indirect mechanism includes the following: the effect on autophosphorylation rate constants is independent of the phosphodonor, the autophosphorylation rate constants and dissociation constants for the phosphoryl group analog BeF are inversely correlated, and the K+1/K+2 positions are distant from the phosphorylation site. We have identified five variable positions in response regulators that allow the rate constants of autophosphorylation and autodephosporylation reactions each to be altered over 3 orders of magnitude in CheY. The distributions of variable residue combinations across response regulator subfamilies suggest that distinct mechanisms associated with different variable positions allow reaction rates to be tuned independently during evolution for diverse biological purposes. This knowledge could be used in synthetic-biology applications to adjust the properties (e.g., background noise and response duration) of biosensors and may allow prediction of response regulator reaction kinetics from the primary amino acid sequence.
微生物和植物利用双组分系统来调节对环境条件变化的适应性反应。传感器激酶检测刺激并相应地改变其自磷酸化活性。信号通过磷酸基团从上游激酶转移到下游响应调节蛋白来传递。从响应调节剂上去除磷酸基团通常会重置系统。同一蛋白家族的成员可能以不同的效率催化磷酸化和去磷酸化反应,表现出跨越多个数量级的速率常数,以适应从毫秒到几天的响应时间尺度。我们之前发现,在响应调节剂中保守的 Asp 磷酸化位点(D+2)或 Thr/Ser(T+1/T+2)的 C 端侧一个或两个残基的位置变化会通过与磷酸供体或磷酸受体分子的直接相互作用改变反应动力学。在这里,我们探索了模型响应调节剂 CheY 中保守 Lys(K+1/K+2)的两个 C 端位置的氨基酸取代对动力学的影响。我们测量了 27 对 K+1/K+2 残基的 CheY 自动磷酸化和自动去磷酸化速率常数,这些残基代表了 84%的天然存在的响应调节剂。对自动去磷酸化的影响较小,但自动磷酸化速率常数变化了 2 个数量级,这表明 K+1/K+2 位置通过改变 CheY 在平衡时采样的构象谱来影响反应动力学。支持这种间接机制的其他证据包括:对自动磷酸化速率常数的影响独立于磷酸供体,自动磷酸化速率常数和磷酸基团类似物 BeF 的解离常数呈反比关系,并且 K+1/K+2 位置远离磷酸化位点。我们已经确定了响应调节剂中的五个可变位置,使 CheY 中的自动磷酸化和自动去磷酸化反应的速率常数都可以改变 3 个数量级。可变残基组合在响应调节剂亚家族中的分布表明,与不同可变位置相关的不同机制允许在进化过程中针对不同的生物学目的独立地调整反应速率。这些知识可用于合成生物学应用,以调整生物传感器的特性(例如,背景噪声和响应持续时间),并且可以根据初级氨基酸序列预测响应调节剂的反应动力学。
