Development of a Method for the Determination of Pulsatile Growth Hormone Secretion in Mice

Steyn, Frederik J.; Huang, Lili; Ngo, Shyuan T.; Leong, Jcy; Tan, Haihan; Xie, Teresa; Parlow, Albert F.; Veldhuis, Johannes D.; Waters, Michael J.; Chen, Chen

doi:10.1210/en.2011-0253

Cited by 118 publications

(157 citation statements)

References 19 publications

(27 reference statements)

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“…1B). These data indicate that GH is able to induce directed macrophage movement (chemotaxis) at concentrations of GH well within the physiological range for rodent plasma GH [pulsatile peak levels of 200-300 ng/ml (Edén, 1979;Steyn et al, 2011) and ghrelin-stimulated levels of GH up to 600 ng/ml (Morozumi et al, 2011)]. Based on these results, GH was added only to the lower chamber of the transwell plate for subsequent migration assays.…”

Section: Gh Acts As a Chemoattractant For Macrophagesmentioning

confidence: 75%

Phosphorylation of the adaptor protein SH2B1βregulates its ability to enhance growth hormone (GH)-dependent macrophage motility

Lanning

Morris

et al. 2013

Journal of Cell Science

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SummaryPrevious studies have shown that growth hormone (GH) recruits the adapter protein SH2B1b to the GH-activated, GH receptorassociated tyrosine kinase JAK2, implicating SH2B1b in GH-dependent actin cytoskeleton remodeling, and suggesting that phosphorylation at serines 161 and 165 in SH2B1b releases SH2B1b from the plasma membrane. Here, we examined the role of SH2B1b in GH regulation of macrophage migration. We show that GH stimulates migration of cultured RAW264.7 macrophages, and primary cultures of peritoneal and bone marrow-derived macrophages. SH2B1b overexpression enhances, whereas SH2B1 knockdown inhibits, GH-dependent motility of RAW macrophages. At least two independent mechanisms regulate the SH2B1b-mediated changes in motility. In response to GH, tyrosines 439 and 494 in SH2B1b are phosphorylated. Mutating these tyrosines in SH2B1b decreases both basal and GH-stimulated macrophage migration. In addition, mutating the polybasic nuclear localization sequence (NLS) in SH2B1b or creating the phosphomimetics SH2B1b(S161E) or SH2B1b(S165E), all of which release SH2B1b from the plasma membrane, enhances macrophage motility. Conversely, SH2B1b(S161/165A) exhibits increased localization at the plasma membrane and decreased macrophage migration. Mutating the NLS or the nearby serine residues does not alter GH-dependent phosphorylation on tyrosines 439 and 494 in SH2B1b. Mutating tyrosines 439 and 494 does not affect localization of SH2B1b at the plasma membrane or movement of SH2B1b into focal adhesions. Taken together, these results suggest that SH2B1b enhances GH-stimulated macrophage motility via mechanisms involving phosphorylation of SH2B1b on tyrosines 439 and 494 and movement of SH2B1b out of the plasma membrane (e.g. as a result of phosphorylation of serines 161 and 165).

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Section: Gh Acts As a Chemoattractant For Macrophagesmentioning

confidence: 75%

Phosphorylation of the adaptor protein SH2B1βregulates its ability to enhance growth hormone (GH)-dependent macrophage motility

Lanning

Morris

et al. 2013

Journal of Cell Science

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“…After centrifugation, plasma was acidified with HCl (0.1 M final) and stored at −80°C. Plasma GH concentrations were determined by a double antibody EIA assay using materials supplied by the National Hormone and Peptide Program (NHPP) as 20 previously described (49). Insulin concentrations were determined by ELISA (Mercodia) and rat acyl ghrelin and des-acyl ghrelin concentrations were measured with ELISA kits (Bertin Pharma).…”

Section: Blood Glucose and Hormone Measurementsmentioning

confidence: 99%

Enhanced responsiveness of Ghsr ^Q343X rats to ghrelin results in enhanced adiposity without increased appetite

et al. 2016

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The ability of the gut hormone ghrelin to promote positive energy balance is mediated by the growth hormone secretagogue receptor (GHSR). GHSR is a G protein-coupled receptor (GPCR) that is found centrally and peripherally and that can signal in a ligand-independent manner basally or when heterodimerized with other GPCRs. However, current Ghsr knockout models cannot dissect ghrelindependent and -independent signaling, precluding assessment of the physiological importance of these signaling pathways. An animal model carrying a Ghsr mutation that preserves GHSR cell surface abundance, but selectively alters GHSR signaling, would be a useful tool to decipher GHSR signaling in vivo. We used rats with the Ghsr Q343X mutation (Ghsr M/M ), which is predicted to delete the distal part of the GHSR C-terminus tail, a domain critical for the signal termination processes of receptor internalization and -arrestin recruitment. In cells, the Q343X GHSR mutant showed enhanced ligandinduced G protein-dependent signaling and blunted activity of processes involved in GPCR signal termination. Ghsr M/M rats displayed enhanced responses to submaximal doses of ghrelin or GHSR agonist. Moreover, Ghsr M/M rats had a more stable body weight under caloric restriction, a condition that increases endogenous ghrelin tone, whereas under standard housing conditions, Ghsr M/M rats showed increased body weight, adiposity and reduced glucose tolerance. Overall, our data stresses the physiological role of the distal domain of GHSR C-terminus as a suppressor of ghrelin sensitivity and we propose using the Ghsr M/M rat as a physiological model of gain-of-function in Ghsr to identify treatments for obesity-related conditions.3

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“…The method has been previously described [253]. Animals had free access to food and water through blood collection.…”

Section: Blood Collectionmentioning

confidence: 99%

“…To determine GH concentration, a sensitive sandwich ELISA had been developed and validated (as shown in Figure 2.1) [253]. In general, a 96-well plate was coated by monkey anti-rat antibody …”

Section: Analysis Of Pulsatile Growth Hormone Secretion By Sensitive mentioning

confidence: 99%

The effect of hexarelin in streptozotocin (STZ)-induced rat model through protective actions on islet beta cells and cardiomyocytes

Zhang¹

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Diabetes mellitus (DM) is a major chronic disease, affecting over 300 million people worldwide.Pancreatic islet β-cell dysfunction is known as the major cause of glucose metabolism disorder, which leads to hyperglycemia and eventually DM. Inside the cell, mitochondria perform a crucial role in coupling glucose metabolism to insulin secretion by the β-cell and on other cell functions requiring normal energy balance. Abnormal activity of mitochondria, such as increased apoptosis, contributes to β-cell dysfunction and diabetes related pathological changes in other cell types, for example, depressed growth hormone (GH) secretion was observed in the diabetic state. Cardiac complications of diabetes, also named diabetic cardiomyopathy, account for over 70% of the mortality among diabetic patients, which is characterized as cardiac systolic and diastolic dysfunctions. There are currently no effective targeted treatments. GH secretagogues (GHS) stimulate insulin secretion and GH release in the diabetic rodent model, and protect cardiomyocytes from ischemia/reperfusion injury. To further clarify the mechanism of GHS on diabetes and its cardiovascular complications, the present study employed mouse a β-cell line (MIN6) and streptozotocin (STZ)-induced diabetic rat model treated with the synthetic GHS, hexarelin (Hex), to investigate β-cell function, pulsatile GH secretion and cardiomyocyte contractility.Diabetes was induced by a single dosage of STZ (65mg/kg) IP injection in male Wistar rats with vehicle control group. After 4 weeks of disease development, animals received Hex (100μg/kg) treatment for 2 weeks. In vitro cell study mimicked the in vivo treatment regime; MIN6 cells were exposed to STZ (1mM) for 4 hours followed by a 2 hour Hex (1μM) incubation. Cell viability and mitochondrial function were measured by MTS and Rhodamine assay. Immunohistochemistry of rat pancreas sections was performed to determine islet morphology and apoptosis signaling pathways.ELISA was conducted to examine pulsatile GH and circulating levels of insulin, insulin-like growth factor-1 (IGF-1) and free fatty acids (FFA). Rat cardiomyocyte contractility and intracellular Ca 2+ concentration were investigated by cell shortening and Ca 2+ transient measurement after cardiomyocyte isolation. Whole-cell patch clamp was performed to study membrane potential and transient outward potassium current (I to ). The expression of the GHS receptor, GHS-R, was determined by Western blot. Apoptotic markers were also assessed by protein expression determination in both MIN6 cells and rat cardiomyocytes.II STZ-treated MIN6 cells showed a decrease in cell proliferation and impaired mitochondrial function with increased expression of apoptotic markers, such as caspase-3, caspase-9 and the ratio of Bax/Bcl-2, while incubation of Hex recovered these parameters towards control levels.STZ-induced diabetic rats showed evidence of symptoms of clinical diabetes such as hyperglycemia, polyphagia, polydipsia and polyuria. Body weight gain was decreased in STZ-t...

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Development of a Method for the Determination of Pulsatile Growth Hormone Secretion in Mice

Cited by 118 publications

References 19 publications

Phosphorylation of the adaptor protein SH2B1βregulates its ability to enhance growth hormone (GH)-dependent macrophage motility

Phosphorylation of the adaptor protein SH2B1βregulates its ability to enhance growth hormone (GH)-dependent macrophage motility

Enhanced responsiveness of Ghsr ^Q343X rats to ghrelin results in enhanced adiposity without increased appetite

The effect of hexarelin in streptozotocin (STZ)-induced rat model through protective actions on islet beta cells and cardiomyocytes

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Development of a Method for the Determination of Pulsatile Growth Hormone Secretion in Mice

Cited by 118 publications

References 19 publications

Phosphorylation of the adaptor protein SH2B1βregulates its ability to enhance growth hormone (GH)-dependent macrophage motility

Phosphorylation of the adaptor protein SH2B1βregulates its ability to enhance growth hormone (GH)-dependent macrophage motility

Enhanced responsiveness of Ghsr Q343X rats to ghrelin results in enhanced adiposity without increased appetite

The effect of hexarelin in streptozotocin (STZ)-induced rat model through protective actions on islet beta cells and cardiomyocytes

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Enhanced responsiveness of Ghsr ^Q343X rats to ghrelin results in enhanced adiposity without increased appetite