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Query: EC:3.1.3.9 (
glucose-6-phosphatase
)
3,081
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
A pancreatic
islet-specific glucose-6-phosphatase-related protein
(
IGRP
) was cloned using a subtractive cDNA expression cloning procedure from mouse insulinoma tissue. Two alternatively spliced variants that differed by the presence or absence of a 118-bp exon (exon IV) were detected in normal balb/c mice, diabetic ob/ob mice, and insulinoma tissue. The longer, 1901-bp full-length cDNA encoded a 355-amino acid protein (molecular weight 40,684) structurally related (50% overall identity) to the liver
glucose-6-phosphatase
and exhibited similar predicted transmembrane topology, conservation of catalytically important residues, and the presence of an endoplasmic reticulum retention signal. The shorter transcript encoded two possible open reading frames (ORFs), neither of which possessed His174, a residue thought to be the phosphoryl acceptor (Pan CJ, Lei KJ, Annabi B, Hemrika W, Chou JY: Transmembrane topology of
glucose-6-phosphatase
. J Biol Chem 273:6144-6148, 1998). Northern blot and reverse transcription-polymerase chain reaction analysis showed that the mRNA was highly expressed in pancreatic islets and expressed more in beta-cell lines than in an alpha-cell line. It was notably absent in tissues and cell lines of non-islet neuroendocrine origin, and no other major tissue source of the mRNA was found. During development, it was expressed in parallel with insulin mRNA. The mRNA was efficiently translated and glycosylated in an in vitro translation/membrane translocation system and readily transcribed into COS 1, HIT, and CHO cells using cytomegalovirus or Rous sarcoma virus promoters. Whereas the liver
glucose-6-phosphatase
showed activity in these transfection systems, the
IGRP
failed to show glucose phosphotransferase or phosphatase activity with p-nitrophenol phosphate, inorganic pyrophosphate, or a range of sugar phosphates hydrolyzed by the liver enzyme. While the metabolic function of the enzyme is not resolved, its remarkable tissue-specific expression warrants further investigation, as does its transcriptional regulation in conditions where glucose responsiveness of the pancreatic islet is altered.
...
PMID:Molecular cloning of a pancreatic islet-specific glucose-6-phosphatase catalytic subunit-related protein. 1007 53
Islet-specific
glucose-6-phosphatase
(
G6Pase
) catalytic subunit-related protein (
IGRP
) is a homolog of the catalytic subunit of
G6Pase
, the enzyme that catalyzes the terminal step of the gluconeogenic pathway. Its catalytic activity, however, has not been defined. Since
IGRP
gene expression is restricted to islets, this suggests a possible role in the regulation of islet metabolism and, hence, insulin secretion induced by metabolites. We report here a comparative analysis of the human, mouse, and rat
IGRP
genes. These studies aimed to identify conserved sequences that may be critical for
IGRP
function and that specify its restricted tissue distribution. The single copy human
IGRP
gene has five exons of similar length and coding sequence to the mouse
IGRP
gene and is located on human chromosome 2q28-32 adjacent to the myosin heavy chain 1B gene. In contrast, the rat
IGRP
gene does not appear to encode a protein as a result of a series of deletions and insertions in the coding sequence. Moreover, rat
IGRP
mRNA, unlike mouse and human
IGRP
mRNA, is not expressed in islets or islet-derived cell lines, an observation that was traced by fusion gene analysis to a mutation of the TATA box motif in the mouse/human
IGRP
promoters to TGTA in the rat sequence. The results provide a framework for the further analysis of the molecular basis for the tissue-restricted expression of the
IGRP
gene and the identification of key amino acid sequences that determine its biological activity.
...
PMID:Cloning and characterization of the human and rat islet-specific glucose-6-phosphatase catalytic subunit-related protein (IGRP) genes. 1129 55
Islet-specific
glucose-6-phosphatase
(
G6Pase
) catalytic-subunit-related protein (
IGRP
) is a homologue of the catalytic subunit of
G6Pase
, the enzyme that catalyses the final step of the gluconeogenic pathway. The analysis of
IGRP
-chloramphenicol acetyltransferase (CAT) fusion-gene expression through transient transfection of islet-derived beta TC-3 cells revealed that multiple promoter regions, located between -306 and -97, are required for maximal
IGRP
-CAT fusion-gene expression. These regions correlated with trans -acting factor-binding sites in the
IGRP
promoter that were identified in beta TC-3 cells in situ using the ligation-mediated PCR (LMPCR) footprinting technique. However, the LMPCR data also revealed additional trans -acting factor-binding sites located between -97 and +1 that overlap two E-box motifs, even though this region by itself conferred minimal fusion-gene expression. The data presented here show that these E-box motifs are important for
IGRP
promoter activity, but that their action is only manifest in the presence of distal promoter elements. Thus mutation of either E-box motif in the context of the -306 to +3
IGRP
promoter region reduces fusion-gene expression. These two E-box motifs have distinct sequences and preferentially bind NeuroD/BETA2 (neurogenic differentiation/beta-cell E box transactivator 2) and upstream stimulatory factor (USF) in vitro, consistent with the binding of both factors to the
IGRP
promoter in situ, as determined using the chromatin-immunoprecipitation (ChIP) assay. Based on experiments using mutated
IGRP
promoter constructs, we propose a model to explain how the ubiquitously expressed USF could contribute to islet-specific
IGRP
gene expression.
...
PMID:Upstream stimulatory factor (USF) and neurogenic differentiation/beta-cell E box transactivator 2 (NeuroD/BETA2) contribute to islet-specific glucose-6-phosphatase catalytic-subunit-related protein (IGRP) gene expression. 1254 Feb 93
Glucose is the main physiological stimulus for insulin biosynthesis and secretion by pancreatic beta-cells. Glucose-6-phosphatase (G-6-Pase) catalyzes the dephosphorylation of glucose-6-phosphate to glucose, an opposite process to glucose utilization. G-6-Pase activity in pancreatic islets could therefore be an important factor in the control of glucose metabolism and, consequently, of glucose-dependent insulin secretion. While G-6-Pase activity has been shown to be present in pancreatic islets, the gene responsible for this activity has not been conclusively identified. A homolog of liver
glucose-6-phosphatase
(LG-6-Pase) specifically expressed in islets was described earlier; however, the authors could not demonstrate enzymatic activity for this protein. Here we present evidence that the previously identified
islet-specific glucose-6-phosphatase-related protein
(
IGRP
) is indeed the major islet
glucose-6-phosphatase
.
IGRP
overexpressed in insect cells possesses enzymatic activity comparable to the previously described G-6-Pase activity in islets. The K(m) and V(max) values determined using glucose-6-phosphate as the substrate were 0.45 mm and 32 nmol/mg/min by malachite green assay, and 0.29 mm and 77 nmol/mg/min by glucose oxidase/peroxidase coupling assay, respectively. High-throughput screening of a small molecule library led to the identification of an active compound that specifically inhibits
IGRP
enzymatic activity. Interestingly, this inhibitor did not affect LG-6-Pase activity, while conversely LG-6-Pase inhibitors did not affect
IGRP
activity. These data demonstrate that
IGRP
is likely the authentic islet-specific
glucose-6-phosphatase
catalytic subunit, and selective inhibitors to this molecule can be obtained.
IGRP
inhibitors may be an attractive new approach for the treatment of insulin secretion defects in type 2 diabetes.
...
PMID:Enzymatic characterization of the pancreatic islet-specific glucose-6-phosphatase-related protein (IGRP). 1472 2
The
glucose-6-phosphatase
(
G6Pase
) system participates in the regulation of glucose homeostasis by converting glucose-6-phosphate (G6P) into glucose and inorganic phosphates. We have used an RT-PCR-based cloning and sequencing approach to study the expression of components of the
G6Pase
system in the hypothalamus and cortex tissues of the ob/ob mouse. We observed the expression of hepatic
G6Pase
catalytic subunit, G6PC, in both tissues, although increased template inputs were required for its detection. Conversely, expression of both the mouse homologue of the previously-described brain-specific G6P translocase T1 (G6PT1) variant and of the hepatic G6PT1 isoform was easily detectable in hypothalamus and cortex tissues. Of the proposed
G6Pase
catalytic subunit homologues, the expression of murine ubiquitous
G6Pase
catalytic subunit-related protein (UGRP, G6PC3) was also easily detectable in both tissues. However, islet-specific
G6Pase
catalytic subunit-related protein (
IGRP
,
G6PC2
) was expressed in a tissue-specific manner, and was detectable only in hypothalamus tissue at increased template inputs. We conclude that cells within ob/ob mouse hypothalamus and cortex tissues express genes with either established or proposed roles in G6P hydrolysis.
...
PMID:Expression of glucose-6-phosphatase system genes in murine cortex and hypothalamus. 1647 32
Islet-specific glucose-6-phosphatase catalytic subunit-related protein
(
IGRP
) is recognized as a major autoantigen for autoimmune type 1 diabetes (T1D) in the NOD mouse model. This study was undertaken to examine CD4+ T cell responses toward
IGRP
in human subjects. The tetramer-guided epitope mapping approach was used to identify
IGRP
-specific CD4+ T cell epitopes.
IGRP
(23-35) and
IGRP
(247-259) were identified as DRA1*0101/DRB1*0401-restricted epitopes.
IGRP
(13-25) and
IGRP
(226-238) were identified as DRA1*0101/DRB1*0301-restricted epitopes.
IGRP
-specific tetramers were used to evaluate the prevalence of
IGRP
-reactive T cells in healthy and T1D subjects. More than 80% of subjects with either DRB1*0401 or DRB1*0301 haplotype have
IGRP
-specific CD4+ T cell responses for at least one
IGRP
epitope.
IGRP
-specific T cells from both healthy and T1D groups produce both gamma-IFN and IL-10. DRA1*0101/DRB1*0401
IGRP
(247-259)-restricted T cells also show cross-reactivity to an epitope derived from liver/kidney
glucose-6-phosphatase
. The detection of
IGRP
-reactive T cells in both type 1 diabetic subjects and healthy subjects and recent reports of other autoreactive T cells detected in healthy subjects underscore the prevalence of potentially autoreactive T cells in the peripheral immune system of the general population.
...
PMID:Islet-specific glucose-6-phosphatase catalytic subunit-related protein-reactive CD4+ T cells in human subjects. 1649 34
Type 1 diabetes is preceded by a long, protracted period of pancreatic islet inflammation by autoreactive lymphocytes. Noninvasive imaging of islet inflammation prior to the onset of hyperglycemia might have diagnostic and therapeutic implications, but this is not currently possible. Here, MRI is used to track, noninvasively, the accumulation diabetogenic CD8+ T-cells during type 1 diabetes progression in nonobese diabetic (NOD) mice. The contrast agent is an MRI probe (MN-NRP-V7) that specifically labels CD8+ T-cells recognizing residues 206-214 of islet-specific
glucose-6-phosphatase
catalytic subunit related protein (
IGRP
(206-214)) in the context of the major histocompatibility complex (MHC) class I molecule H-2K(d). This probe consists of superparamagnetic iron oxide nanoparticles (MN) coated with K(d) molecules presenting NRP-V7, a high-avidity mimotope of
IGRP
(206-214). NOD mice of different ages (5, 8, 15, and 24 weeks) were imaged by MRI before and after a single intravenous injection of MN-NRP-V7 or unmodified MN nanoparticles. MN-NRP-V7 accumulation, as determined by semiquantitative MRI analysis of pancreas-associated T(2) relaxation time, was antigen-specific, age-dependent, and well correlated with the numbers of MN-NRP-V7-labeled CD8+ T-cells recovered from the pancreata of the treated mice. Antigen/MHC-coupled nanoparticles represent a promising new avenue for noninvasive imaging of lymphocyte inflammation in organ-specific autoimmunity and transplantation.
...
PMID:In vivo imaging of a diabetogenic CD8+ T cell response during type 1 diabetes progression. 1830 24
Several studies have shown that healthy individuals with fasting plasma glucose (FPG) levels at the high end of the normal range have an increased risk of mortality. To identify genetic determinants that contribute to interindividual variation in FPG, we tested 392,935 single-nucleotide polymorphisms (SNPs) in 654 normoglycemic participants for association with FPG, and we replicated the most strongly associated SNP (rs560887, P = 4 x 10(-7)) in 9353 participants. SNP rs560887 maps to intron 3 of the
G6PC2
gene, which encodes
glucose-6-phosphatase
catalytic subunit-related protein (also known as
IGRP
), a protein selectively expressed in pancreatic islets. This SNP was associated with FPG (linear regression coefficient beta = -0.06 millimoles per liter per A allele, combined P = 4 x 10(-23)) and with pancreatic beta cell function (Homa-B model, combined P = 3 x 10(-13)) in three populations; however, it was not associated with type 2 diabetes risk. We speculate that
G6PC2
regulates FPG by modulating the set point for glucose-stimulated insulin secretion in pancreatic beta cells.
...
PMID:A polymorphism within the G6PC2 gene is associated with fasting plasma glucose levels. 1845 Dec 65
Mesenchymal stromal cell (MSC) markers are expressed on brain tumor-initiating cells involved in the development of hypoxic glioblastoma. Given that MSCs can survive hypoxia and that the glucose-6-phosphate transporter (G6PT) provides metabolic control that contributes to MSC mobilization and survival, we investigated the effects of low oxygen (1.2% O(2)) exposure on G6PT gene expression. We found that MSCs significantly expressed G6PT and the
glucose-6-phosphatase
catalytic subunit beta, whereas expression of the
glucose-6-phosphatase
catalytic subunit alpha and the
islet-specific glucose-6-phosphatase catalytic subunit-related protein
was low to undetectable. Analysis of the G6PT promoter sequence revealed potential binding sites for hypoxia inducible factor (HIF)-1alpha and for the aryl hydrocarbon receptor (AhR) and its dimerization partner, the AhR nuclear translocator (ARNT), AhR:ARNT. In agreement with this, hypoxia and the hypoxia mimetic cobalt chloride induced the expression of G6PT, vascular endothelial growth factor (VEGF), and HIF-1alpha. Gene silencing of HIF-1alpha prevented G6PT and VEGF induction in hypoxic MSCs whereas generation of cells stably expressing HIF-1alpha resulted in increased endogenous G6PT gene expression. A semisynthetic analog of the polyketide mumbaistatin, a potent G6PT inhibitor, specifically reduced MSC-HIF-1alpha cell survival. Collectively, our data suggest that G6PT may account for the metabolic flexibility that enables MSCs to survive under conditions characterized by hypoxia and could be specifically targeted within developing tumors.
...
PMID:Evidence for transcriptional regulation of the glucose-6-phosphate transporter by HIF-1alpha: Targeting G6PT with mumbaistatin analogs in hypoxic mesenchymal stromal cells. 1907 14
Elevated fasting blood glucose (FBG) is associated with increased risk for the development of type 2 diabetes and cardiovascular-associated mortality. Genome-wide association studies (GWAS) have linked polymorphisms in
G6PC2
with variations in FBG and body fat, although not insulin sensitivity or glucose tolerance.
G6PC2
encodes an islet-specific, endoplasmic reticulum-resident
glucose-6-phosphatase
catalytic subunit. A combination of in situ perfused pancreas, in vitro isolated islet, and in vivo analyses were used to explore the function of G6pc2 in mice. G6pc2 deletion had little effect on insulin sensitivity and glucose tolerance, whereas body fat was reduced in female G6pc2 knockout (KO) mice on both a chow and high-fat diet, observations that are all consistent with human GWAS data. G6pc2 deletion resulted in a leftward shift in the dose-response curve for glucose-stimulated insulin secretion (GSIS). As a consequence, under fasting conditions in which plasma insulin levels were identical, blood glucose levels were reduced in G6pc2 KO mice, again consistent with human GWAS data. Glucose-6-phosphatase activity was reduced, whereas basal cytoplasmic calcium levels were elevated in islets isolated from G6pc2 KO mice. These data suggest that G6pc2 represents a novel, negative regulator of basal GSIS that acts by hydrolyzing glucose-6-phosphate, thereby reducing glycolytic flux.
...
PMID:G6PC2: a negative regulator of basal glucose-stimulated insulin secretion. 2327 94
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