针对谷胱甘肽结合域的肽类抗体抑制由线粒体复合物 I 介导的超氧化物产生。
Peptide-based antibodies against glutathione-binding domains suppress superoxide production mediated by mitochondrial complex I.
机构信息
Division of Cardiovascular Medicine, Department of Internal Medicine, Davis Heart & Lung Research Institute, College of Medicine, The Ohio State University, Columbus, Ohio 43210, USA.
出版信息
J Biol Chem. 2010 Jan 29;285(5):3168-80. doi: 10.1074/jbc.M109.056846. Epub 2009 Nov 23.
Complex I (NQR) is a critical site of superoxide (O2-) production and the major host of redox protein thiols in mitochondria. In response to oxidative stress, NQR-derived protein thiols at the 51- and 75-kDa subunits are known to be reversibly S-glutathionylated. Although several glutathionylated domains from NQR 51 and 75 kDa have been identified, their roles in the regulatory functions remain to be explored. To gain further insights into protein S-glutathionylation of complex I, we used two peptides of S-glutathionylated domain ((200)GAGAYICGEETALIESIEGK(219) of 51-kDa protein and (361)VDSDTLCTEEVFPTAGAGTDLR(382) of 75-kDa protein) as chimeric epitopes incorporating a "promiscuous" T-cell epitope to generate two polyclonal antibodies, AbGSCA206 and AbGSCB367. Binding of AbGSCA206 and AbGSCB367 inhibited NQR-mediated O2- generation by 37 and 57%, as measured by EPR spin-trapping. To further provide an appropriate control, two peptides of non-glutathionylated domain ((21)SGDTTAPKKTSFGSLKDFDR(40) of 51-kDa peptide and (100)WNILTNSEKTKKAREGVMEFL(120) of 75-kDa peptide) were synthesized as chimeric epitopes to generate two polyclonal antibodies, Ab51 and Ab75. Binding of A51 did not affect NQR-mediated generation to a significant level. However, binding of Ab75 inhibited NQR-mediated O2-*generation by 35%. None of AbGSCA206, AbGSCB367, Ab51, or Ab75 showed an inhibitory effect on the electron transfer activity of NQR, suggesting that antibody binding to the glutathione-binding domain decreased electron leakage from the hydrophilic domain of NQR. When heart tissue homogenates were immunoprecipitated with Ab51 or Ab75 and probed with an antibody against glutathione, protein S-glutathionylation was enhanced in post-ischemic myocardium at the NQR 51-kDa subunit, but not at the 75-kDa subunit, indicating that the 51-kDa subunit of flavin subcomplex is more sensitive to oxidative stress resulting from myocardial infarction.
复合体 I(NQR)是超氧化物(O2-*)产生的关键部位,也是线粒体中氧化还原蛋白巯基的主要宿主。在氧化应激反应中,已知 NQR 的 51 和 75 kDa 亚基上的 NQR 衍生蛋白巯基可被可逆地 S-谷胱甘肽化。尽管已经鉴定出来自 NQR 51 和 75 kDa 的几个谷胱甘肽化结构域,但它们在调节功能中的作用仍有待探索。为了更深入地了解复合体 I 的蛋白质 S-谷胱甘肽化,我们使用两个 S-谷胱甘肽化结构域的肽(51 kDa 蛋白的(200)GAGAYICGEETALIESIEGK(219)和 75 kDa 蛋白的(361)VDSDTLCTEEVFPTAGAGTDLR(382))作为包含“混杂”T 细胞表位的嵌合表位,生成两种多克隆抗体,AbGSCA206 和 AbGSCB367。AbGSCA206 和 AbGSCB367 的结合抑制了 NQR 介导的 O2-*生成,抑制率分别为 37%和 57%,通过 EPR 自旋捕获法测量。为了提供适当的对照,我们合成了两个非谷胱甘肽化结构域的肽(51 kDa 肽的(21)SGDTTAPKKTSFGSLKDFDR(40)和 75 kDa 肽的(100)WNILTNSEKTKKAREGVMEFL(120))作为嵌合表位,生成两种多克隆抗体,Ab51 和 Ab75。Ab51 的结合未对 NQR 介导的生成产生显著抑制作用。然而,Ab75 的结合抑制了 NQR 介导的 O2-*生成,抑制率为 35%。AbGSCA206、AbGSCB367、Ab51 或 Ab75 均未显示出对 NQR 电子转移活性的抑制作用,表明抗体与谷胱甘肽结合域的结合降低了 NQR 亲水性结构域的电子泄漏。当用 Ab51 或 Ab75 免疫沉淀心脏组织匀浆并用针对谷胱甘肽的抗体进行探测时,在缺血后心肌的 NQR 51 kDa 亚基中增强了蛋白质 S-谷胱甘肽化,但在 75 kDa 亚基中没有,表明黄素亚复合物的 51 kDa 亚基对心肌梗死引起的氧化应激更敏感。
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