Literature DB >> 15025560

Increased levels of insulin and insulin-like growth factor-1 hybrid receptors and decreased glycosylation of the insulin receptor alpha- and beta-subunits in scrapie-infected neuroblastoma N2a cells.

Daniel Nielsen1, Hanna Gyllberg, Pernilla Ostlund, Tomas Bergman, Katarina Bedecs.   

Abstract

We have previously shown that ScN2a cells (scrapie-infected neuroblastoma N2a cells) express 2-fold- and 4-fold-increased levels of IR (insulin receptor) and IGF-1R (insulin-like growth factor-1 receptor) respectively. In addition, the IR alpha- and beta-subunits are aberrantly processed, with apparent molecular masses of 128 and 85 kDa respectively, as compared with 136 and 95 kDa in uninfected N2a cells. Despite the 2-fold increase in IR protein, the number of (125)I-insulin-binding sites was slightly decreased in ScN2a cells [Ostlund, Lindegren, Pettersson and Bedecs (2001) Brain Res. 97, 161-170]. In order to determine the cellular localization of IR in ScN2a cells, surface biotinylation was performed, showing a correct IR trafficking and localization to the cell surface. The present study shows for the first time that neuroblastoma N2a cells express significant levels of IR-IGF-1R hybrid receptors, and in ScN2a cells the number of hybrid receptors was 2-fold higher than that found in N2a cells, potentially explaining the apparent loss of insulin-binding sites due to a lower affinity for insulin compared with the homotypic IR. Furthermore, the decreased molecular mass of IR subunits in ScN2a cells is not caused by altered phosphorylation or proteolytic processing, but rather by altered glycosylation. Enzymic deglycosylation of immunoprecipitated IR from N2a and ScN2a cells with endoglycosidase H, peptide N-glycosidase F and neuraminidase all resulted in subunits with increased electrophoretic mobility; however, the 8-10 kDa shift remained. Combined enzymic or chemical deglycosylation using anhydrous trifluoromethane sulphonic acid treatment ultimately showed that the IR alpha- and beta-subunits from ScN2a cells are aberrantly glycosylated. The increased formation of IR-IGF-1R hybrids in ScN2a cells may be part of a neuroprotective response to prion infection. The degree and functional significance of aberrantly glycosylated proteins in ScN2a cells remain to be determined.

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Year:  2004        PMID: 15025560      PMCID: PMC1224193          DOI: 10.1042/BJ20040010

Source DB:  PubMed          Journal:  Biochem J        ISSN: 0264-6021            Impact factor:   3.857


  44 in total

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2.  Mutational analysis of the NH2-terminal glycosylation sites of the insulin receptor alpha-subunit.

Authors:  L H Caro; A Ohali; P Gorden; E Collier
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3.  The functions of the human insulin receptor are affected in different ways by mutation of each of the four N-glycosylation sites in the beta subunit.

Authors:  I Leconte; J L Carpentier; E Clauser
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4.  Insulin receptor/IGF-I receptor hybrids are widely distributed in mammalian tissues: quantification of individual receptor species by selective immunoprecipitation and immunoblotting.

Authors:  E M Bailyes; B T Navé; M A Soos; S R Orr; A C Hayward; K Siddle
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9.  Characterization of human placental insulin-like growth factor-I/insulin hybrid receptors by protein microsequencing and purification.

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10.  Loss of insulin receptor immunoreactivity from the substantia nigra pars compacta neurons in Parkinson's disease.

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2.  Protein Mobility Shifts Contribute to Gel Electrophoresis Liquid Chromatography Analysis.

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3.  Altered glycosylation of acetylcholinesterase in the Creutzfeldt-Jakob cerebrospinal fluid.

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Review 7.  How independent are TSE agents from their hosts?

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8.  Unaltered Prion Pathogenesis in a Mouse Model of High-Fat Diet-Induced Insulin Resistance.

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9.  Species and strain glycosylation patterns of PrPSc.

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10.  Glimepiride reduces the expression of PrPc, prevents PrPSc formation and protects against prion mediated neurotoxicity in cell lines.

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