Abstract
Aims/hypothesisThe adipose tissue-derived hormone leptin plays an important role in the maintenance of body weight and glucose homeostasis. Leptin mediates its effects by interaction with leptin receptors (LepRb), which are highly expressed in the hypothalamus and other brain centres, and at lower levels in the periphery. Previous studies have used relatively promiscuous or inefficient Cre deleter strains, respectively, to explore the roles of LepR in pancreatic β and α cells. Here, we use two newly-developed Cre lines to explore the role of leptin signalling in insulin and proglucagon-expressing cells.MethodsLeptin receptor expression was measured in isolated mouse islets and highly-purified islet cells by RNASeq and quantitative RT-PCR. Mice lacking leptin signalling in pancreatic β, or in α and other proglucagon-expressing cells, were generated using Ins1Cre- or iGluCre-mediated recombination respectively of flox'd leptin receptor alleles. In vivo glucose homeostasis, changes in body weight, pancreatic histology and hormone secretion from isolated islets were assessed using standard techniques.ResultsLeptin receptor mRNA levels were at or below the level of detection in wild-type adult mouse isolated islets and purified cells, and leptin signalling to Stat3 phosphorylation was undetectable. Whereas male mice further deleted for leptin receptors in β cells exhibited no abnormalities in glucose tolerance up to 16 weeks of age, females transiently displayed improved glucose tolerance at 8 weeks (11.2 ± 3.2% decrease in area under curve; p < 0.05), and improved (39.0 ± 13.0%, P < 0.05) glucose-stimulated insulin secretion in vitro. No differences were seen between genotypes in body weight, fasting glucose or β/α cell ratio. Deletion of LepR from α-cells, a minority of β cells, and a subset of proglucagon-expressing cells in the brain, exerted no effects on body weight, glucose or insulin tolerance, nor on pancreatic hormone secretion assessed in vivo and in vitro.Conclusions/interpretationThe use here of a highly selective Cre recombinase indicates that leptin signalling plays a relatively minor, age- and sex-dependent role in the control of β cell function in the mouse. No in vivo role for leptin receptors on α cells, nor in other proglucagon-expressing cells, was detected in this study.
Highlights
Type 2 Diabetes mellitus (T2D) currently affects approximately 380 million individuals worldwide [1] and is characterized by elevated blood glucose levels
LepR mRNA levels are low in isolated mouse islets and in purified islet cells We first assessed expression of leptin receptors in isolated islets and highly purified preparations of islet cells from wild-type mice (Materials and Methods) using RNASeq and quantitative RT-PCR
LepR mRNA was detected at 0.2 RPKM in whole islets [27], at the lower 39th centile of all messages, and 0.23, 0.036 and 0 RPKM in purified b, d and a and cells, respectively (n 1⁄4 3, 2 and 4 separate preparations, respectively)
Summary
Type 2 Diabetes mellitus (T2D) currently affects approximately 380 million individuals worldwide [1] and is characterized by elevated blood glucose levels. Whilst insulin, secreted from pancreatic islet b cells, acts to lower blood glucose levels, glucagon, secreted by pancreatic a cells, increases glycaemia. Obesity, which affects w1 in 4 adults in the UK (www.hscic.gov.uk/ catalogue/PUB10364), is an important risk factor for T2D and promotes both insulin resistance and b cell failure [4]. The adipose tissuederived hormone leptin is an important satiety factor which acts on the feeding centres in the brain to suppress appetite [5]. Demonstrating a conserved role for the hormone across mammalian species, mice carrying mutations in the homologous genes (ob/ob [9] or db/db) [10] display severe hyperphagia, obesity and disturbed glucose homeostasis
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