Department of Clinical Pharmacology and Pharmacoepidemiology, Heidelberg University Hospital, Im Neuenheimer Feld 410, 69120 Heidelberg, Germany.
Int J Mol Sci. 2022 Mar 26;23(7):3637. doi: 10.3390/ijms23073637.
The solute carrier L-type amino acid transporter 1 (LAT-1/SLC7A5) is a viable target for drug delivery to the central nervous system (CNS) and tumors due to its high abundance at the blood-brain barrier and in tumor tissue. LAT-1 is only localized on the cell surface as a heterodimer with CD98, which is not required for transporter function. To support future CNS drug-delivery development based on LAT-1 targeting, we established an ultra-performance liquid chromatography-tandem mass spectrometry (UPLC-MS/MS) assay for stable isotopically labeled leucine ([C, N]-L-leucine), with a dynamic range of 0.1-1000 ng/mL that can be applied for the functional testing of LAT-1 activity when combined with specific inhibitors and, consequently, the LAT-1 inhibition capacity of new compounds. The assay was established in a 96-well format, facilitating high-throughput experiments, and, hence, can support the screening for novel inhibitors. Applicable recommendations of the US Food and Drug Administration and European Medicines Agency for bioanalytical method validation were followed to validate the assay. The assay was applied to investigate the IC of two well-known LAT-1 inhibitors on hCMEC/D3 cells: the highly specific LAT-1 inhibitor JPH203, which was also used to demonstrate LAT-1 specific uptake, and the general system L inhibitor BCH. In addition, the [C, N]-L-leucine uptake was determined on two human brain capillary endothelial cell lines (NKIM-6 and hCMEC/D3), which were characterized for their expressional differences of LAT-1 at the protein and mRNA level and the surface amount of CD98. The IC values of the inhibitors were in concordance with previously reported values. Furthermore, the [C, N]-L-leucine uptake was significantly higher in hCMEC/D3 cells compared to NKIM-6 cells, which correlated with higher expression of LAT-1 and a higher surface amount of CD98. Therefore, the UPLC-MS/MS quantification of ([C, N]-L-leucine is a feasible strategy for the functional characterization of LAT-1 activity in cells or tissue.
溶质载体 L 型氨基酸转运蛋白 1(LAT-1/SLC7A5)在血脑屏障和肿瘤组织中丰富度高,因此是向中枢神经系统(CNS)和肿瘤递药的可行靶点。LAT-1 仅作为与 CD98 形成的异二聚体存在于细胞表面,而 CD98 对于转运蛋白功能并非必需。为了支持基于 LAT-1 靶向的未来 CNS 递药开发,我们建立了一种超高效液相色谱-串联质谱(UPLC-MS/MS)测定法,用于稳定同位素标记亮氨酸([C, N]-L-亮氨酸),其动态范围为 0.1-1000ng/mL,可与特定抑制剂结合用于 LAT-1 活性的功能测试,从而测定新化合物的 LAT-1 抑制能力。该测定法以 96 孔板格式建立,便于高通量实验,因此可支持新型抑制剂的筛选。遵循美国食品和药物管理局和欧洲药品管理局关于生物分析方法验证的适用建议对测定法进行验证。该测定法应用于研究两种知名 LAT-1 抑制剂对 hCMEC/D3 细胞的 IC:高特异性 LAT-1 抑制剂 JPH203,其也用于证明 LAT-1 特异性摄取;以及一般系统 L 抑制剂 BCH。此外,还在两种人脑血管内皮细胞系(NKIM-6 和 hCMEC/D3)上测定了[C, N]-L-亮氨酸摄取,这些细胞系在蛋白质和 mRNA 水平以及 CD98 表面数量上表现出 LAT-1 的表达差异。抑制剂的 IC 值与先前报道的值一致。此外,hCMEC/D3 细胞中的[C, N]-L-亮氨酸摄取明显高于 NKIM-6 细胞,这与 LAT-1 表达较高和 CD98 表面数量较高相关。因此,[C, N]-L-亮氨酸的 UPLC-MS/MS 定量分析是细胞或组织中 LAT-1 活性功能特征分析的可行策略。
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