Kern András, Szentpétery Zsófia, Liliom Károly, Bakos Eva, Sarkadi Balázs, Váradi András
Institute of Enzymology, Hungarian Academy of Sciences, 29 Karolina út, 1113 Budapest, Hungary.
Biochem J. 2004 Jun 1;380(Pt 2):549-60. doi: 10.1042/BJ20031607.
The human ABC (ATP-binding cassette) transporter MRP1 (human multidrug-resistance-associated protein 1; ABCC1) is involved in the cellular extrusion of conjugated metabolites and causes multidrug resistance in tumour cells. The transport of substrate molecules by ABC proteins is energized by ATP hydrolysis, performed by two co-operating ABC units. Orthovanadate (Vi), a non-covalent inhibitor of the ABC ATPases, was found to catalyse a photo-oxidative cleavage of various ATP-binding proteins. In the present study, we have identified three Vi-cleavage sites within MRP1, and found that the cleavage reactions were variably modulated by the presence of nucleotides and by transported substrates. We concluded that Vi cleavage of MRP1 at Site I detects conformational changes due to the binding of MgATP. In contrast, Site II could be identified as part of the substrate-modulated catalytic cycle, probably containing an MRP1.MgADP.Vi transition-state-like complex. Cleavage at Site III was modulated by both the binding and hydrolysis of MgATP, in a biphasic pattern, which was also affected by the presence of transported substrates. We detected two different allosteric effects and found that they control two consecutive steps of the MRP1 ATPase catalytic cycle. Nucleotide binding to the low-affinity site accelerated the formation of the pre-hydrolytic intermediate in the other catalytic centre. Interaction of the transporter with its transported substrates stimulated a later reaction of the hydrolytic cycle, the formation of the post-hydrolytic intermediate, which could be detected in both catalytic sites by the experimental strategy used.
人类ABC(ATP结合盒)转运蛋白MRP1(人类多药耐药相关蛋白1;ABCC1)参与结合代谢物的细胞外排,并导致肿瘤细胞产生多药耐药性。ABC蛋白对底物分子的转运由ATP水解提供能量,这一过程由两个协同作用的ABC单元完成。原钒酸盐(Vi)是ABC ATP酶的一种非共价抑制剂,被发现可催化多种ATP结合蛋白的光氧化裂解。在本研究中,我们在MRP1中鉴定出三个Vi裂解位点,并发现裂解反应受核苷酸和转运底物的存在情况的不同调节。我们得出结论,MRP1在I位点的Vi裂解检测到由于MgATP结合而引起的构象变化。相比之下,II位点可被确定为底物调节催化循环的一部分,可能包含一个MRP1.MgADP.Vi过渡态样复合物。III位点的裂解受MgATP的结合和水解的双相调节,这也受到转运底物存在的影响。我们检测到两种不同的变构效应,并发现它们控制着MRP1 ATP酶催化循环的两个连续步骤。核苷酸与低亲和力位点的结合加速了另一个催化中心中水解前中间体的形成。转运蛋白与其转运底物的相互作用刺激了水解循环的后期反应,即水解后中间体的形成,通过所采用的实验策略可在两个催化位点检测到这一中间体。