Excessive Iron Induces Oxidative Stress Promoting Cellular Perturbations and Insulin Secretory Dysfunction in MIN6 Beta Cells

被引:24
作者
Blesia, Voni [1 ]
Patel, Vinood B. [1 ]
Al-Obaidi, Hisham [2 ]
Renshaw, Derek [3 ]
Zariwala, Mohammed Gulrez [1 ]
机构
[1] Univ Westminster, Sch Life Sci, Ctr Nutraceut, 115 New Cavendish St, London W1W 6UW, England
[2] Univ Reading, Sch Pharm, POB 226, Reading RG6 6AP, Berks, England
[3] Coventry Univ, Inst Hlth & Wellbeing, Ctr Sport Exercise & Life Sci, Priory St, Coventry CV1 5FB, W Midlands, England
关键词
excess iron; oxidative stress; impaired insulin secretion; type 2 diabetes mellitus; β -cell; FERRITIN; RISK; MITOCHONDRIA; PROJECTIONS; PREVALENCE; RESISTANCE; APOPTOSIS; PROTEINS; RADICALS; STORES;
D O I
10.3390/cells10051141
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Exposure to high levels of glucose and iron are co-related to reactive oxygen species (ROS) generation and dysregulation of insulin synthesis and secretion, although the precise mechanisms are not well clarified. The focus of this study was to examine the consequences of exposure to high iron levels on MIN6 beta-cells. MIN6 pseudoislets were exposed to 20 mu M (control) or 100 mu M (high) iron at predefined glucose levels (5.5 mM and 11 mM) at various time points (3, 24, 48, and 72 h). Total iron content was estimated by a colourimetric FerroZine (TM) assay in presence or absence of transferrin-bound iron. Cell viability was assessed by a resazurin dye-based assay, and ROS-mediated cellular oxidative stress was assessed by estimating malondialdehyde levels. beta-cell iron absorption was determined by a ferritin immunoassay. Cellular insulin release and content was measured by an insulin immunoassay. Expression of SNAP-25, a key protein in the core SNARE complex that modulates vesicle exocytosis, was measured by immunoblotting. Our results demonstrate that exposure to high iron levels resulted in a 15-fold (48 h) and 4-fold (72 h) increase in cellular iron accumulation. These observations were consistent with data from oxidative stress analysis which demonstrated 2.7-fold higher levels of lipid peroxidation. Furthermore, exposure to supraphysiological (11 mM) levels of glucose and high iron (100 mu M) at 72 h exerted the most detrimental effect on the MIN6 beta-cell viability. The effect of high iron exposure on total cellular iron content was identical in the presence or absence of transferrin. High iron exposure (100 mu M) resulted in a decrease of MIN6 insulin secretion (64% reduction) as well as cellular insulin content (10% reduction). Finally, a significant reduction in MIN6 beta-cell SNAP-25 protein expression was evident at 48 h upon exposure to 100 mu M iron. Our data suggest that exposure to high iron and glucose concentrations results in cellular oxidative damage and may initiate insulin secretory dysfunction in pancreatic beta-cells by modulation of the exocytotic machinery.
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页数:20
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