Transient kinetics reveal the mechanism of competitive inhibition of the neutral amino acid transporter ASCT2

被引:0
|
作者
Dong Y. [1 ]
Wang J. [1 ]
Grewer C. [1 ]
机构
[1] Department of Chemistry, Binghamton University, Binghamton, NY
基金
美国国家卫生研究院;
关键词
ASCT2; electrophysiology; inhibition mechanism; kinetics; membrane protein; neutral amino acid transporter; rapid solution exchange;
D O I
10.1016/j.jbc.2024.107382
中图分类号
学科分类号
摘要
ASCT2 (alanine serine cysteine transporter 2), a member of the solute carrier 1 family, mediates Na+-dependent exchange of small neutral amino acids across cell membranes. ASCT2 was shown to be highly expressed in tumor cells, making it a promising target for anticancer therapies. In this study, we explored the binding mechanism of the high-affinity competitive inhibitor L-cis hydroxyproline biphenyl ester (Lc-BPE) with ASCT2, using electrophysiological and rapid kinetic methods. Our investigations reveal that Lc-BPE binding requires one or two Na+ ions initially bound to the apo-transporter with high affinity, with Na1 site occupancy being more critical for inhibitor binding. In contrast to the amino acid substrate bound form, the final, third Na+ ion cannot bind, due to distortion of its binding site (Na2), thus preventing the formation of a translocation-competent complex. Based on the rapid kinetic analysis, the application of Lc-BPE generated outward transient currents, indicating that despite its net neutral nature, the binding of Lc-BPE in ASCT2 is weakly electrogenic, most likely because of asymmetric charge distribution within the amino acid moiety of the inhibitor. The preincubation with Lc-BPE also led to a decrease of the turnover rate of substrate exchange and a delay in the activation of substrate-induced anion current, indicating relatively slow Lc-BPE dissociation kinetics. Overall, our results provide new insight into the mechanism of binding of a prototypical competitive inhibitor to the ASCT transporters. © 2024 The Authors
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