Exendin-4 Stimulation of Cyclin A2 in β-Cell Proliferation

Song, Wonkyong; Schreiber, Weston E.; Zhong, Enhong; Liu, Fei‐Fei; Kornfeld, Benjamin; Wondisford, Fredric E.; Hussain, Mehboob A.

doi:10.2337/db07-1541

Cited by 86 publications

(64 citation statements)

References 42 publications

(74 reference statements)

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“…To further improve differentiation conditions from pancreatic progenitor to β cells, exendin-4, a glucagon-like peptide-1 agonist, and SB431542, a TGF-β signaling inhibitor, were added to stage 3 progenitor cells. Both of these additions enhanced the differentiation efficiency of β cells to 4.6% and 8.2% (C-peptide + ), respectively, consistent with previous observations (21)(22)(23). A combination of exendin-4 and SB431542 treatment from day 9 to day 12 produced the highest percentage of β cells (15%) ( Figure 2D).…”

Section: Gck Mutations Specifically Affect Glucose-mediated Insulin Ssupporting

confidence: 90%

iPSC-derived β cells model diabetes due to glucokinase deficiency

Hua¹,

Shang²,

Martínez³

et al. 2013

J. Clin. Invest.

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Diabetes is a disorder characterized by loss of β cell mass and/or β cell function, leading to deficiency of insulin relative to metabolic need. To determine whether stem cell-derived β cells recapitulate molecular-physiological phenotypes of a diabetic subject, we generated induced pluripotent stem cells (iPSCs) from subjects with maturity-onset diabetes of the young type 2 (MODY2), which is characterized by heterozygous loss of function of the gene encoding glucokinase (GCK). These stem cells differentiated into β cells with efficiency comparable to that of controls and expressed markers of mature β cells, including urocortin-3 and zinc transporter 8, upon transplantation into mice. While insulin secretion in response to arginine or other secretagogues was identical to that in cells from healthy controls, GCK mutant β cells required higher glucose levels to stimulate insulin secretion. Importantly, this glucose-specific phenotype was fully reverted upon gene sequence correction by homologous recombination. Our results demonstrate that iPSC-derived β cells reflect β cell-autonomous phenotypes of MODY2 subjects, providing a platform for mechanistic analysis of specific genotypes on β cell function.

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Section: Gck Mutations Specifically Affect Glucose-mediated Insulin Ssupporting

confidence: 90%

iPSC-derived β cells model diabetes due to glucokinase deficiency

Hua¹,

Shang²,

Martínez³

et al. 2013

J. Clin. Invest.

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“…This conclusion is further supported by our demonstration that transient overexpression of NUPR1 reduced the rate of MIN6 beta cell proliferation in parallel with inhibiting expression of the cell cycle regulators Ccna2 and Tcf19 through effects to suppress their promoter activities in beta cells. The Ccna2 gene regulates progression at both the G1/S and G2/M checkpoints of the cell cycle [27,28] and lentiviral-mediated infection of islets to overexpress Ccna2 stimulates beta cell self-replication [20]. The TCF19 protein contains a sequence exhibiting characteristics of transcription factors and its expression is regulated in the late stages of the cell cycle [21], consistent with it playing a regulatory role in the expression of genes necessary for cell cycle progression.…”

Section: Discussionmentioning

confidence: 99%

“…Given the increased islet mass with Nupr1 deletion, attention was focused on genes known to regulate the cell cycle. Messenger RNAs for cyclin A2, which has been identified as a target in the regulation of beta cell mass [20], and TCF19, which has been implicated in regulating genes involved in the later stages of cell cycle progression [21], emerged as possible candidates. Our array analysis indicated that Ccna2 and Tcf19 mRNAs were increased by 1.6-fold (p <0.0004) and 1.9-fold (p =0.00002), respectively, in Nupr1 −/− islets.…”

Section: Metabolic Characterisation Of Nupr1mentioning

confidence: 99%

Nupr1 deletion protects against glucose intolerance by increasing beta cell mass

et al. 2013

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Aims/hypothesis The stress-activated nuclear protein transcription regulator 1 (NUPR1) is induced in response to glucose and TNF-α, both of which are elevated in type 2 diabetes, and Nupr1 has been implicated in cell proliferation and apoptosis cascades. We used Nupr1 −/− mice to study the role of Nupr1 in glucose homeostasis under normal conditions and following maintenance on a high-fat diet (HFD). Methods Glucose homeostasis in vivo was determined by measuring glucose tolerance, insulin sensitivity and insulin secretion. Islet number, morphology and beta cell area were assessed by immunofluorescence and morphometric analysis, and islet cell proliferation was quantified by analysis of BrdU incorporation. Islet gene expression was measured by gene arrays and quantitative RT-PCR, and gene promoter activities were monitored by measuring luciferase activity. Results Nupr1 −/− mice had increased beta cell mass as a consequence of enhanced islet cell proliferation. Nupr1-dependent suppression of beta cell Ccna2 and Tcf19 promoter activities was identified as a mechanism through which Nupr1 may regulate beta cell cycle progression. Nupr1 −/− mice maintained on a normal diet were mildly insulin resistant, but were normoglycaemic with normal glucose tolerance because of compensatory increases in basal and glucose-induced insulin secretion. Nupr1 deletion was protective against HFD-induced obesity, insulin resistance and glucose intolerance. Conclusions/interpretation Inhibition of NUPR1 expression or activity has the potential to protect against the metabolic defects associated with obesity and type 2 diabetes.

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“…Previous studies have implicated both cAMP- (Buteau et al 2003, Song et al 2008) and b-arrestin (Talbot et al 2012)-dependent mechanisms in the proliferative effects of GLP1 on pancreatic b-cells. In addition, it has been reported that the proliferative action of GLP1 is mediated by the transactivation of epidermal growth factor receptor (EGFR; Buteau et al 2003) or the increased expression and activation of the insulin-like growth factor 1 receptor (IGF1R) (Cornu et al 2010) both of which result in the activation of the PI3K/protein kinase B (PKB) pathway.…”

Section: Introductionmentioning

confidence: 99%

Exendin-4 stimulates islet cell replication via the IGF1 receptor activation of mTORC1/S6K1

Xie¹,

El-Sayed²,

Cheng³

et al. 2014

Journal of Molecular Endocrinology

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Glucagon-like peptide 1 receptor (GLP1R) agonists, such as exendin-4, potentiate glucosestimulated insulin secretion and are currently used in the management of type 2 diabetes. Interestingly, GLP1R agonists also have the ability to augment b-cell mass. In this report, we provide evidence that in the presence of glucose, exendin-4 stimulates rodent islet cell DNA replication via the activation of ribosomal protein S6 kinase 1 (S6K1) and that this is mediated by the protein kinase B (PKB)-dependent activation of mTOR complex 1 (mTORC1). We show that activation of this pathway is caused by the autocrine or paracrine activation of the IGF1 receptor (IGF1R), as siRNA-mediated knockdown of the IGF1R effectively blocked exendin-4-stimulated PKB and mTORC1 activation. In contrast, pharmacological inactivation of the epidermal growth factor receptor has no discernible effect on exendin-4-stimulated PKB or mTORC1 activation. Therefore, we conclude that GLP1R agonists stimulate b-cell proliferation via the PKB-dependent stimulation of mTORC1/S6K1 whose activation is mediated through the autocrine/paracrine activation of the IGF1R. This work provides a better understanding of the molecular basis of GLP1 agonist-induced b-cell proliferation which could potentially be exploited in the identification of novel drug targets that increase b-cell mass.

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Exendin-4 Stimulation of Cyclin A2 in β-Cell Proliferation

Cited by 86 publications

References 42 publications

iPSC-derived β cells model diabetes due to glucokinase deficiency

iPSC-derived β cells model diabetes due to glucokinase deficiency

Nupr1 deletion protects against glucose intolerance by increasing beta cell mass

Exendin-4 stimulates islet cell replication via the IGF1 receptor activation of mTORC1/S6K1

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