Lo Wei-Jen, Chiou Yu-Ching, Hsu Yu-Ting, Lam Wing See, Chang Ming-Yun, Jao Shu-Chuan, Li Wen-Shan
Department of Chemistry & Biochemistry, National Chung Cheng University, Chia-Yi 621, Taiwan.
Bioconjug Chem. 2007 Jan-Feb;18(1):109-20. doi: 10.1021/bc0601727.
A primary pathway for metabolism of electrophilic compounds in Schistosoma japonicum involves glutathione S-transferase (SjGST)-catalyzed formation of glutathione (GSH) conjugates. As part of a program aimed at gaining a better understanding of the defense system of parasites, a series of aromatic halides (1-8), aliphatic halides (9, 10), epoxides (11-20), alpha,beta-unsaturated esters (21, 22), and alpha,beta-unsaturated amides (23, 24) were prepared, and their participation in glutathione conjugate formation was evaluated. Products from enzymatic and nonenzymatic reactions of these substances with glutathione were characterized and quantified by using reverse-phase high-performance liquid chromatography (HPLC), NMR, and fast atom bombardment mass spectrometry (FAB-MS) analysis. Mechanisms for formation of specific mono(glutathionyl) or bis(glutathionyl) conjugates are proposed. Although the results of this effort indicate that SjGST does not catalyze addition or substitution reactions of 1, 3, 4, 7-9, 11-13, 15-17, 19-21, and 24, they demonstrate that 2, 5, 6, 14, 18, and 23 undergo efficient enzyme-catalyzed conjugation reactions. The kcat values for SjGST with 23 and 18 are about 886-fold and 14-fold, respectively, larger than that for 5. This observation suggests that 23 is a good substrate in comparison to other electrophiles. Furthermore, the initially formed conjugation product, 23a, is also a substrate for SjGST in a process that forms the bis(glutathionyl) conjugate 23b. Products arising by enzymatic and nonenzymatic pathways are generated under the conditions of SjGST-activated GSH conjugation. Interestingly, production of nonenzymatic GSH conjugates with electrophilic substrates often overwhelms the activity of the enzyme. The nonenzymatic GSH conjugates, 9a-11a, 16a, 21a, and 22a, are inhibitors of SjGST with respective IC50 values of 1.95, 75.5, 0.96, 19.0, 152, and 0.36 microM, and they display moderate inhibitory activities against human GSTA2. Direct evidence has been gained for substrate inhibition by 10 toward SjGST and GSTA2 that is more potent than that of its GSH conjugate 10a. The significance of this work is found in the development of a convenient NMR-based technique that can be used to characterize glutathione conjugates derived from small molecule libraries as part of efforts aimed at uncovering specific potent SjGST and GSTA2 inhibitors. This method has potential in applications to the identification of novel inhibitors of other GST targets that are of chemotherapeutic interest.
日本血吸虫中亲电化合物代谢的主要途径涉及谷胱甘肽S-转移酶(SjGST)催化形成谷胱甘肽(GSH)缀合物。作为旨在更好地理解寄生虫防御系统的项目的一部分,制备了一系列芳香族卤化物(1 - 8)、脂肪族卤化物(9, 10)、环氧化物(11 - 20)、α,β-不饱和酯(21, 22)和α,β-不饱和酰胺(23, 24),并评估了它们参与谷胱甘肽缀合物形成的情况。通过反相高效液相色谱(HPLC)、核磁共振(NMR)和快原子轰击质谱(FAB-MS)分析对这些物质与谷胱甘肽的酶促和非酶促反应产物进行了表征和定量。提出了形成特定单(谷胱甘肽基)或双(谷胱甘肽基)缀合物的机制。尽管这项研究的结果表明SjGST不催化1、3、4、7 - 9、11 - 13、15 - 17、19 - 21和24的加成或取代反应,但它们表明2、5、6、14、18和23会发生有效的酶促缀合反应。SjGST与23和18的kcat值分别比与5的kcat值大约大886倍和14倍。这一观察结果表明,与其他亲电试剂相比,23是一种良好的底物。此外,最初形成的缀合产物2-3a也是SjGST的底物,在此过程中形成双(谷胱甘肽基)缀合物23b。在SjGST激活的GSH缀合条件下会产生酶促和非酶促途径产生的产物。有趣的是,亲电底物的非酶促GSH缀合物的产生常常超过酶的活性。非酶促GSH缀合物9a - 11a、16a、21a和22a是SjGST的抑制剂,其IC50值分别为1.95、75.5、0.96、19.0、152和0.36 microM,并且它们对人GSTA2表现出中等抑制活性。已获得直接证据表明10对SjGST和GSTA2的底物抑制作用比其GSH缀合物10a更强。这项工作的意义在于开发了一种基于NMR的便捷技术,该技术可用于表征源自小分子文库的谷胱甘肽缀合物,作为旨在发现特定强效SjGST和GSTA2抑制剂的努力的一部分。该方法在应用于鉴定其他具有化疗意义的GST靶点的新型抑制剂方面具有潜力。
