Molecular and Environmental Toxicology Center, University of Wisconsin-Madison, Madison, Wisconsin 53706, USA.
Chem Res Toxicol. 2011 Nov 21;24(11):1915-23. doi: 10.1021/tx200263n. Epub 2011 Oct 25.
S-(1,2-Dichlorovinyl)-L-cysteine sulfoxide (DCVCS) is a reactive and potent nephrotoxic metabolite of the human trichloroethylene metabolite S-(1,2-dichlorovinyl)-L-cysteine (DCVC). Because DCVCS covalent binding to kidney proteins likely plays a role in its nephrotoxicity, in this study biotin-tagged DCVCS, N-biotinyl-DCVCS (NB-DCVCS), was synthesized, and its stability in buffer alone and in the presence of rat blood or plasma was characterized in vitro. In addition, reactivity toward GSH and covalent binding to selected model enzymes and isolated kidney proteins were characterized. The half-lives of NB-DCVCS (39.6 min) and the DCVCS (diastereomer 1, 14.4 min; diastereomer 2, 6 min) in the presence of GSH were comparable. Incubating the model enzymes glutathione reductase and malate dehydrogenase with 10 μM NB-DCVCS for 3 h at 37 °C followed by immunoblotting using antibiotin antibodies demonstrated that glutathione reductase and malate dehydrogenase were extensively modified by NB-DCVCS. When rat kidney cytosol (6 μg/μL) was incubated with NB-DCVCS (312.5 nM to 5 μM) for 3 h at 37 °C followed by immunoblotting, a concentration-dependent increase in signal with multiple proteins with different molecular weights was observed, suggesting that NB-DCVCS binds to multiple kidney proteins with different selectivity. Incubating rat kidney cytosol with DCVCS (10-100 μM) prior to the addition of NB-DCVCS (2.5 μM) reduced the immunoblotting signal, suggesting that NB-DCVCS and DCVCS compete for the same binding sites. A comparison of the stability of NB-DCVCS and DCVCS in rat blood and plasma was determined in vitro, and NB-DCVCS exhibited higher stability than DCVCS in both media. Collectively, these results suggest that NB-DCVCS shows sufficient stability, reactivity, and selectivity to warrant further investigations into its possible use as a tool for future characterization of the role of covalent modification of renal proteins by DCVCS in nephrotoxicity.
S-(1,2-二氯乙烯基)-L-半胱氨酸亚砜 (DCVCS) 是人类三氯乙烯代谢物 S-(1,2-二氯乙烯基)-L-半胱氨酸 (DCVC) 的一种反应性和强效肾毒性代谢物。由于 DCVCS 与肾脏蛋白的共价结合可能在其肾毒性中起作用,因此在这项研究中,合成了生物素标记的 DCVCS,即 N-生物素基-DCVCS (NB-DCVCS),并在体外研究了其在缓冲液中以及在大鼠血液或血浆中的稳定性。此外,还研究了其与 GSH 的反应性以及与选定的模型酶和分离的肾脏蛋白的共价结合。在 GSH 存在下,NB-DCVCS(diastereomer 1,14.4 min;diastereomer 2,6 min)的半衰期(39.6 min)与 DCVCS 的半衰期相当。将模型酶谷胱甘肽还原酶和苹果酸脱氢酶与 10 μM NB-DCVCS 在 37°C 下孵育 3 小时,然后用抗生物素抗体进行免疫印迹,结果表明谷胱甘肽还原酶和苹果酸脱氢酶被 NB-DCVCS 广泛修饰。当大鼠肾细胞质(6 μg/μL)与 NB-DCVCS(312.5 nM 至 5 μM)在 37°C 下孵育 3 小时,然后进行免疫印迹时,观察到信号随多种不同分子量的蛋白质呈浓度依赖性增加,这表明 NB-DCVCS 与多种具有不同选择性的肾脏蛋白结合。在加入 NB-DCVCS(2.5 μM)之前,将大鼠肾细胞质与 DCVCS(10-100 μM)孵育,可降低免疫印迹信号,这表明 NB-DCVCS 和 DCVCS 竞争相同的结合位点。在体外比较了 NB-DCVCS 和 DCVCS 在大鼠血液和血浆中的稳定性,结果表明 NB-DCVCS 在这两种介质中的稳定性均高于 DCVCS。总的来说,这些结果表明 NB-DCVCS 具有足够的稳定性、反应性和选择性,这使其有理由进一步研究其作为未来表征 DCVCS 对肾脏蛋白共价修饰在肾毒性中作用的工具的可能性。