Early diabetes and abnormal postnatal pancreatic islet development in mice lacking Glut-2

Guillam, Marie-Thérèse; Hummler, Edith; Schaerer, E; Yeh, Jih‐I; Birnbaum, Morris J.; Beermann, Friedrich; Schmidt, Alejandro Raúl; Dériaz, Nathalie; Thorens, Bernard

doi:10.1038/ng1197-327

Cited by 392 publications

(311 citation statements)

References 27 publications

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“…GLUT2 is required for glucose sensing, normal glucose homeostasis and insulin secretion [44]. Glut2 was one of the most highly regulated candidate genes in activin A-or follistatin-treated islets and MIN6 cells.…”

Section: Discussionmentioning

confidence: 99%

Reciprocal modulation of adult beta cell maturity by activin A and follistatin

2010

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Aims/hypothesis The functional maturity of pancreatic beta cells is impaired in diabetes mellitus. We sought to define factors that can influence adult beta cell maturation status and function. Methods MIN6 cells labelled with a Pdx1 monomeric red fluorescent protein-Ins1 enhanced green fluorescent protein dual reporter lentivirus were used to screen candidate growth and/or differentiation factors using image-based approaches with confirmation by real-time RT-PCR and assays of beta cell function using primary mouse islets.Results Activin A strikingly decreased the number of mature beta cells and increased the number of immature beta cells. While activins are critical for pancreatic morphogenesis, their role in adult beta cells remains controversial. In primary islets and MIN6 cells, activin A significantly decreased the expression of insulin and several genes associated with beta cell maturity (e.g. Pdx1, Mafa, Glut2 [also known as Slc2a2]). Genes found in immature beta cells (e.g. Mafb) tended to be upregulated by activin A. Insulin secretion was also reduced by activin A. In addition, activin A-treated MIN6 cells proliferated faster than non-treated cells. The effects of endogenous activin A on beta cells were completely reversed by exogenous follistatin. Conclusions/interpretation These results suggest that autocrine and/or paracrine activin A signalling exerts a suppressive effect on adult beta cell maturation and function. Thus, the maturation state of adult beta cells can be modulated by external factors in culture. Interventions inhibiting activin or its signalling pathways may improve beta cell function. Understanding of maturation and plasticity of adult pancreatic tissue has significant implications for islet regeneration and for in vitro generation of functional beta cells.

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Section: Discussionmentioning

confidence: 99%

Reciprocal modulation of adult beta cell maturity by activin A and follistatin

2010

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“…Before we began this study, we considered that, because Glut2 −/− pups are viable until weaning [26], GLUT2 is not necessary for embryonic or fetal development. Therefore, as explained above, its presence or absence would appear to have little consequence during non-diabetic pregnancy, and so the expression of Glut2 may be vestigial.…”

Section: Discussionmentioning

confidence: 99%

“…Mice carrying a Glut2 knockout allele [26] on a 129/SvJ background were used to generate embryos that were GLUT2-deficient. The Glut2 knockout strain was originally generated on a mixed C57Bl/6J×129/Sv background.…”

Section: Methodsmentioning

confidence: 99%

“…Postnatally, GLUT2 is produced by pancreatic beta cells, hepatocytes, intestine and kidney-tissues that must transport glucose with high efficiency when its concentration is high, for example after intestinal absorption of nutrients following feeding [11,25]. GLUT2 is essential for glucose-stimulated insulin release, and also regulates glucose sensing by extrapancreatic tissues [26,27]. However, the early embryo is not normally exposed to glucose concentrations approaching the K m of the GLUT2 transporter.…”

Section: Introductionmentioning

confidence: 99%

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Expression of the gene encoding the high-K m glucose transporter 2 by the early postimplantation mouse embryo is essential for neural tube defects associated with diabetic embryopathy

Thorens

Loeken

2007

Diabetologia

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Aims/hypothesis Excess glucose transport to embryos during diabetic pregnancy causes congenital malformations. The early postimplantation embryo expresses the gene encoding the high-K m GLUT2 (also known as SLC2A2) glucose transporter. The hypothesis tested here is that high-K m glucose transport by GLUT2 causes malformations resulting from maternal hyperglycaemia during diabetic pregnancy. Materials and methods Glut2 mRNA was assayed by RT-PCR. The K m of embryo glucose transport was determined by measuring 0.5-20 mmol/l 2-deoxy[ 3 H]glucose transport. To test whether the GLUT2 transporter is required for neural tube defects resulting from maternal hyperglycaemia, Glut2 +/− mice were crossed and transient hyperglycaemia was induced by glucose injection on day 7.5 of pregnancy. Embryos were recovered on day 10.5, and the incidence of neural tube defects in wild-type, Glut2 +/− and Glut2 −/− embryos was scored. Results Early postimplantation embryos expressed Glut2, and expression was unaffected by maternal diabetes. Moreover, glucose transport by these embryos showed Michaelis-Menten kinetics of 16.19 mmol/l, consistent with transport mediated by GLUT2. In pregnancies made hyperglycaemic on day 7.5, neural tube defects were significantly increased in wild-type embryos, but Glut2 +/− embryos were partially protected from neural tube defects, and Glut2 −/− embryos were completely protected from these defects. The frequency of occurrence of wild-type, Glut2 +/− and Glut2 −/− embryos suggests that the presence of Glut2 alleles confers a survival advantage in embryos before day 10.5. Conclusions/interpretations High-K m glucose transport by the GLUT2 glucose transporter during organogenesis is responsible for the embryopathic effects of maternal diabetes.

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“…GLUT2 is also the major glucose transporter in pancreatic ß‐cells, where its genetic inactivation impairs glucose uptake and suppresses glucose‐stimulated insulin secretion. GLUT2 −/− mice die at around the weaning period, and transgenic expression of another glucose transporter, GLUT1, in β‐cells (RIPGlut1;GLUT2 −/− ) restores normal glucose‐stimulated insulin biosynthesis (Bady et al, 2006; Guillam et al, 1997; Thorens et al, 2000). …”

Section: Introductionmentioning

confidence: 99%

Glial hypothalamic inhibition of GLUT2 expression alters satiety, impacting eating behavior

Barahona

Llanos

Recabal

et al. 2017

Glia

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Glucose is a key modulator of feeding behavior. By acting in peripheral tissues and in the central nervous system, it directly controls the secretion of hormones and neuropeptides and modulates the activity of the autonomic nervous system. GLUT2 is required for several glucoregulatory responses in the brain, including feeding behavior, and is localized in the hypothalamus and brainstem, which are the main centers that control this behavior. In the hypothalamus, GLUT2 has been detected in glial cells, known as tanycytes, which line the basal walls of the third ventricle (3V). This study aimed to clarify the role of GLUT2 expression in tanycytes in feeding behavior using 3V injections of an adenovirus encoding a shRNA against GLUT2 and the reporter EGFP (Ad‐shGLUT2). Efficient in vivo GLUT2 knockdown in rat hypothalamic tissue was demonstrated by qPCR and Western blot analyses. Specificity of cell transduction in the hypothalamus and brainstem was evaluated by EGFP‐fluorescence and immunohistochemistry, which showed EGFP expression specifically in ependymal cells, including tanycytes. The altered mRNA levels of both orexigenic and anorexigenic neuropeptides suggested a loss of response to increased glucose in the 3V. Feeding behavior analysis in the fasting‐feeding transition revealed that GLUT2‐knockdown rats had increased food intake and body weight, suggesting an inhibitory effect on satiety. Taken together, suppression of GLUT2 expression in tanycytes disrupted the hypothalamic glucosensing mechanism, which altered the feeding behavior.

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Early diabetes and abnormal postnatal pancreatic islet development in mice lacking Glut-2

Cited by 392 publications

References 27 publications

Reciprocal modulation of adult beta cell maturity by activin A and follistatin

Reciprocal modulation of adult beta cell maturity by activin A and follistatin

Expression of the gene encoding the high-K m glucose transporter 2 by the early postimplantation mouse embryo is essential for neural tube defects associated with diabetic embryopathy

Glial hypothalamic inhibition of GLUT2 expression alters satiety, impacting eating behavior

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