Shemon Anne N, Sluyter Ronald, Fernando Suran L, Clarke Alison L, Dao-Ung Lan-Phuong, Skarratt Kristen K, Saunders Bernadette M, Tan Khai See, Gu Ben J, Fuller Stephen J, Britton Warwick J, Petrou Steven, Wiley James S
Department of Medicine, University of Sydney, Level 5, Spurrett Building, Nepean Hospital, Penrith, New South Wales 2750, Australia.
J Biol Chem. 2006 Jan 27;281(4):2079-86. doi: 10.1074/jbc.M507816200. Epub 2005 Nov 1.
The P2X(7) receptor is a ligand-gated cation channel that is highly expressed on mononuclear leukocytes and that mediates ATP-induced apoptosis and killing of intracellular pathogens. There is a wide variation in P2X(7) receptor function between subjects, explained in part by four loss-of-function polymorphisms (R307Q, E496A, I568N, and a 5'-intronic splice site polymorphism), as well as rare mutations. In this study, we report the allele frequencies of 11 non-synonymous P2X(7) polymorphisms and describe a fifth loss-of-function polymorphism in the gene (1096C --> G), which changes Thr(357) to Ser (T357S) with an allele frequency of 0.08 in the Caucasian population. P2X(7) function was measured by ATP-induced ethidium(+) influx into peripheral blood lymphocytes and monocytes and, when compared with wild-type subjects, was reduced to 10-65% in heterozygotes, 1-18% in homozygotes, and 0-10% in compound heterozygotes carrying T357S and a second loss-of-function polymorphism. Overexpression of the T357S mutant P2X(7) in either HEK-293 cells or Xenopus oocytes gave P2X(7) function of approximately 50% that of wild-type constructs. Differentiation of monocytes to macrophages, which also up-regulates P2X(7), restored P2X(7) function to near normal in cells heterozygous for T357S and to a value 50-65% of wild-type in cells homozygous for T357S or compound heterozygous for T357S/E496A. However, macrophages from subjects that are compound heterozygous for either T357S/R307Q or T357S/stop codon had near-to-absent P2X(7) function. These functional deficits induced by T357S were paralleled by impaired ATP-induced apoptosis and mycobacteria killing in macrophages from these subjects. Lymphocytes, monocytes, and macrophages from subjects homozygous for T357S or compound heterozygous for T357S and a second loss-of-function allele have reduced or absent P2X(7) receptor function.
P2X(7)受体是一种配体门控阳离子通道,在单核白细胞上高度表达,介导ATP诱导的细胞凋亡以及细胞内病原体的杀伤。个体之间P2X(7)受体功能存在很大差异,部分原因是4种功能丧失多态性(R307Q、E496A、I568N以及一个5'-内含子剪接位点多态性),还有罕见突变。在本研究中,我们报告了11种非同义P2X(7)多态性的等位基因频率,并描述了该基因中的第五种功能丧失多态性(1096C→G),该多态性将苏氨酸(Thr(357))变为丝氨酸(T357S),在白种人群体中的等位基因频率为0.08。通过ATP诱导溴化乙锭(+)流入外周血淋巴细胞和单核细胞来测量P2X(7)功能,与野生型个体相比,携带T357S和另一种功能丧失多态性的杂合子中P2X(7)功能降低至10 - 65%,纯合子中降低至1 - 18%,复合杂合子中降低至0 - 10%。在HEK - 293细胞或非洲爪蟾卵母细胞中过表达T357S突变型P2X(7),其功能约为野生型构建体的50%。单核细胞向巨噬细胞的分化(这也会上调P2X(7))使T357S杂合细胞中的P2X(7)功能恢复至接近正常,使T357S纯合细胞或T357S/E496A复合杂合细胞中的P2X(7)功能恢复至野生型的50 - 65%。然而,对于T357S/R307Q或T357S/终止密码子复合杂合的个体,其巨噬细胞中的P2X(7)功能几乎完全丧失。T357S诱导的这些功能缺陷与这些个体巨噬细胞中ATP诱导的细胞凋亡受损以及分枝杆菌杀伤受损同时出现。T357S纯合个体或T357S与另一种功能丧失等位基因复合杂合个体的淋巴细胞、单核细胞和巨噬细胞具有降低或缺失的P2X(7)受体功能。
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