鉴定大鼠P2X(7)受体细胞外结构域中参与酸性pH功能抑制的氨基酸残基。
Identification of the amino acid residues in the extracellular domain of rat P2X(7) receptor involved in functional inhibition by acidic pH.
作者信息
Liu X, Ma W, Surprenant A, Jiang L-H
机构信息
Institute of Membrane and Systems Biology, Faculty of Biological Sciences, University of Leeds, Leeds, UK.
出版信息
Br J Pharmacol. 2009 Jan;156(1):135-42. doi: 10.1111/j.1476-5381.2008.00002.x.
BACKGROUND AND PURPOSE
P2X(7), receptors are potently inhibited by extracellular acidification. The underlying molecular basis remains unknown. This study aimed to examine the role of extracellular histidine, lysine, aspartic acid and glutamic acid residues in the functional inhibition of rat P2X(7) receptors by acidic pH.
EXPERIMENTAL APPROACH
We introduced point mutations into rat P2X(7) receptor by site-directed mutagenesis, expressed wild type (WT) and mutant receptors in human embryonic kidney (HEK293) cells and, using patch clamp recording, characterized the effects of acidic pH on BzATP [2'-3'O-(4-benzoylbenzoyl) adenosine 5'-triphosphate]-evoked ionic currents.
KEY RESULTS
Reducing extracellular pH, that is, increasing extracellular proton concentrations, inhibited BzATP-evoked currents in cells expressing WT P2X(7) receptors, with IC(50) value (half-maximal antagonist or inhibitor concentration) for protons of 0.2 mumol.L(-1). The major effect of acidification was suppression of the maximal current response without altering the agonist sensitivity. five residues in the receptor extracellular domain (His(85), Lys(110), Lys(137), Asp(197) and His(219)) were mutated to alanine and current inhibition by protons assessed. Compared with WT, the H85A, H219A, K137A mutants were two- to threefold more sensitive, whereas the K110A and D197A mutants were 2.5- and 9-fold less sensitive. Double-alanine substitution of Lys(110) and Asp(197) resulted in 23-fold decreased sensitivity to inhibition by protons. Furthermore, charge neutralization (K110M, K110F, D197N and D197F), but not charge conserving mutation (K110R and D197E), attenuated the inhibition of currents by protons.
CONCLUSIONS AND IMPLICATIONS
Functional inhibition of rat P2X(7) receptors by acidic pH was variably affected by the extra-cellular His(85), Lys(110), Lys(137), Asp(197) and His(219) residues, with the Asp(197) residue being most critical for this inhibition.
背景与目的
P2X(7)受体受到细胞外酸化的强烈抑制。其潜在的分子基础仍不清楚。本研究旨在探讨细胞外组氨酸、赖氨酸、天冬氨酸和谷氨酸残基在酸性pH对大鼠P2X(7)受体功能抑制中的作用。
实验方法
我们通过定点诱变在大鼠P2X(7)受体中引入点突变,在人胚肾(HEK293)细胞中表达野生型(WT)和突变型受体,并使用膜片钳记录法,表征酸性pH对BzATP[2'-3'O-(4-苯甲酰苯甲酰)腺苷5'-三磷酸]诱发的离子电流的影响。
关键结果
降低细胞外pH,即增加细胞外质子浓度,抑制表达WT P2X(7)受体的细胞中BzATP诱发的电流,质子的IC(50)值(半数最大拮抗剂或抑制剂浓度)为0.2μmol.L(-1)。酸化的主要作用是抑制最大电流反应而不改变激动剂敏感性。受体细胞外结构域中的五个残基(His(85)、Lys(110)、Lys(137)、Asp(197)和His(219))突变为丙氨酸,并评估质子对电流的抑制作用。与WT相比,H85A、H219A、K137A突变体的敏感性高2至3倍,而K110A和D197A突变体的敏感性分别低2.5倍和9倍。Lys(110)和Asp(197)的双丙氨酸取代导致对质子抑制的敏感性降低23倍。此外,电荷中和(K110M、K110F、D197N和D197F)而非电荷保守突变(K110R和D197E)减弱了质子对电流的抑制作用。
结论与意义
酸性pH对大鼠P2X(7)受体的功能抑制受到细胞外His(85)、Lys(110)、Lys(137)、Asp(197)和His(219)残基的不同影响,其中Asp(197)残基对这种抑制最为关键。
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