Trans-11 vaccenic acid improves insulin secretion in models of type 2 diabetes in vivo and in vitro

被引:29
|
作者
Wang, Xiaofeng [1 ]
Gupta, Joel [1 ]
Kerslake, Matthew [1 ]
Rayat, Gina [2 ]
Proctor, Spencer D. [1 ]
Chan, Catherine B. [1 ,3 ]
机构
[1] Univ Alberta, Dept Agr Food & Nutr Sci, Edmonton, AB, Canada
[2] Univ Alberta, Fac Med & Dent, Dept Surg, Alberta Diabet Inst,Surg Med Res Inst, Edmonton, AB, Canada
[3] Univ Alberta, Dept Physiol, Edmonton, AB, Canada
关键词
Insulin secretion; Islets; Ruminant trans-fatty acids; Trans-11 vaccenic acid; Type; 2; diabetes; CONJUGATED LINOLEIC-ACID; PANCREATIC BETA-CELLS; MONOUNSATURATED FATTY-ACIDS; REGENERATING GENE PROTEIN; DIETARY SUPPLEMENTATION; RECEPTOR; ACTIVATION; RISK; GPR40; ASSOCIATION;
D O I
10.1002/mnfr.201500783
中图分类号
TS2 [食品工业];
学科分类号
0832 ;
摘要
ScopeTrans-11 vaccenic acid (VA) is a fatty acid produced by ruminants entering the human food supply through meat and dairy products, which appears not to have the health risks associated with industrially produced trans-fatty acids. In this study, we investigated the effect of VA on insulin secretion in vivo in rats and in vitro in human and rat islets after diabetogenic insult. Methods and resultsHyperglycemic clamp showed that VA dietary supplementation for 8 weeks significantly increased glucose turnover in rats with type 2 diabetes (T2D), accompanied by an elevated plasma C-peptide concentration, indicating improved insulin secretion. The -cell area and proliferation rate were higher in T2D+VA than T2D group. Isolated islets from T2D+VA rats had higher glucose-stimulated insulin secretion (GSIS) than T2D group. In vitro, VA treatment for 24 and 48 h significantly enhanced GSIS in rat and human islets after diabetogenic challenges. The mRNA expression of G-protein-coupled receptor 40 (GPR40) and regenerating islet-derived 1 (REG-1) were consistently increased by VA in both rat and human islets. ConclusionThese results indicate that VA may improve insulin secretion and growth of islets in T2D, at least partly by altering GPR40 and REG-1 mRNA expression.
引用
收藏
页码:846 / 857
页数:12
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