Development of a live cell assay for the zinc transporter ZnT8

被引:0
|
作者
Azzollini, Lucia [1 ]
Del Prete, Dolores [1 ]
Wolf, Gernot [2 ]
Klimek, Christoph [2 ]
Saggioro, Mattia [1 ]
Ricci, Fernanda [1 ]
Christodoulaki, Eirini [2 ]
Wiedmer, Tabea [2 ]
Ingles-Prieto, Alvaro [2 ]
Superti-Furga, Giulio [2 ,3 ]
Scarabottolo, Lia [1 ]
机构
[1] Axxam SpA, Openzone, Via Meucci 3, I-20091 Milan, Italy
[2] Austrian Acad Sci, CeMM Res Ctr Mol Med, Vienna, Austria
[3] Med Univ Vienna, Ctr Physiol & Pharmacol, Vienna, Austria
关键词
Type; 2; diabetes; Zinc transporter; SLC30a8; Transport assay; SLC; ZnT; BETA-CELL; INTRACELLULAR ZINC; SLC30A8; RS13266634; DIABETES-MELLITUS; STRUCTURAL BASIS; HUMAN HEALTH; INSULIN; RISK; POLYMORPHISMS; ASSOCIATION;
D O I
10.1016/j.slasd.2024.100166
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Zinc is an essential trace element that is involved in many biological processes and in cellular homeostasis. In pancreatic beta-cells, zinc is crucial for the synthesis, processing, and secretion of insulin, which plays a key role in glucose homeostasis and which deficiency is the cause of diabetes. The accumulation of zinc in pancreatic cells is regulated by the solute carrier transporter SLC30A8 (or Zinc Transporter 8, ZnT8), which transports zinc from cytoplasm in intracellular vesicles. Allelic variants of SLC30A8 gene have been linked to diabetes. Given the physiological intracellular localization of SLC30A8 in pancreatic beta-cells and the ubiquitous endogenous expression of other Zinc transporters in different cell lines that could be used as cellular model for SLC30A8 recombinant over-expression, it is challenging to develop a functional assay to measure SLC30A8 activity. To achieve this goal, we have firstly generated a HEK293 cell line stably overexpressing SLC30A8, where the overexpression favors the partial localization of SLC30A8 on the plasma membrane. Then, we used the combination of this cell model, commercial FluoZin-3 cell permeant zinc dye and live cell imaging approach to follow zinc flux across SLC30A8 over-expressed on plasma membrane, thus developing a novel functional imaging- based assay specific for SLC30A8. Our novel approach can be further explored and optimized, paving the way for future small molecule medium-throughput screening.
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页数:8
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