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Glycogenin-2 is dispensable for liver glycogen synthesis and glucagon-stimulated glucose release.

作者信息

Irgens Henrik U, Fjeld Karianne, Johansson Bente B, Ringdal Monika, Immervoll Heike, Leh Sabine, Søvik Oddmund, Johansson Stefan, Molven Anders, Njølstad Pål R

机构信息

KG Jebsen Center for Diabetes Research, Department of Clinical Science (H.U.I., K.F., B.B.J., M.R., O.S., S.J., A.M., P.R.N.), Gade Laboratory for Pathology, Department of Clinical Medicine (H.I., S.L., A.M.), University of Bergen, 5020 Bergen, Norway; and Department of Pediatrics (H.U.I., P.R.N.), Department of Pathology (H.I., S.L, A.M.), and Center for Medical Genetics and Molecular Medicine (K.F., B.B.J., M.R., S.J.), Haukeland University Hospital, 5021 Bergen, Norway.

出版信息

J Clin Endocrinol Metab. 2015 May;100(5):E767-75. doi: 10.1210/jc.2014-4337. Epub 2015 Mar 9.

Abstract

CONTEXT

The synthesis of glycogen is initiated by glycogenin. In humans, glycogenin-1 is expressed ubiquitously, whereas glycogenin-2 (GN2) is highly expressed in liver. It has therefore been suggested that GN2 is a liver isoform of glycogenin. In a search for possible copy number variations associated with monogenic diabetes, we identified a 102-kb deletion of the X chromosome involving the entire GYG2 gene (encoding GN2) in 2 families.

OBJECTIVE

The purpose of this study was to test whether male GYG2 deletion carriers had abnormal glucose metabolism and/or glycogen synthesis.

DESIGN, SETTING, AND PATIENTS: Two families with diabetes and a GYG2 deletion were investigated with medical history and examination, glucagon stimulation tests, and liver biopsies.

RESULTS

We identified a GYG2 deletion in 3 members of family 1, 8 members of family 2, and 1 blood donor. The deletion showed no clear cosegregation with diabetes. Deletion carriers reported no symptoms related to fasting. Results of cardiac examination and abdominal ultrasound imaging were normal. A glucagon stimulation test in 4 male deletion carriers showed a mean rise in plasma glucose of 3.6 mmol/L (95% confidence interval, 2.9-4.2) compared with 2.8 mmol/L (95% confidence interval, 2.2-3.4) in control subjects. Liver biopsy specimens did not show clear morphologic changes by light microscopy and showed the presence of both α- and β-glycogen by electron microscopy. We detected GYG1 but not GYG2 mRNA expression in the liver biopsy specimens.

CONCLUSIONS

This is the first evaluation of humans without GN2 expression. Our data indicate that GN2 is not required for liver glycogen synthesis and glucagon-stimulated glucose release.

摘要

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