Literature DB >> 25875859

Rat skeletal muscle glycogen degradation pathways reveal differential association of glycogen-related proteins with glycogen granules.

Hongyang Xu1, David Stapleton, Robyn M Murphy.   

Abstract

Glycogenin, glycogen-debranching enzyme (GDE) and glycogen phosphorylase (GP) are important enzymes that contribute to glycogen particle metabolism. In Long-Evans Hooded rat whole muscle homogenates prepared from extensor digitorum longus (EDL, fast-twitch) and soleus (SOL, oxidative, predominantly slow twitch), it was necessary to include α-amylase, which releases glucosyl units from glycogen, to detect glycogenin but not GDE or GP. Up to ∼12 % of intramuscular glycogen pool was broken down using either in vitro electrical stimulation or leaving muscle at room temperature >3 h (delayed, post-mortem). Electrical stimulation did not reveal glycogenin unless α-amylase was added, although in post-mortem muscle ∼50 and ∼30 % of glycogenin in EDL and SOL muscles, respectively, was detected compared to the amount detected with α-amylase treatment. Single muscle fibres were dissected from fresh or post-mortem EDL muscles, mechanically skinned to remove surface membrane and the presence of glycogenin, GDE and GP as freely diffusible proteins (i.e. cytoplasmic localization) compared by Western blotting. Diffusibility of glycogenin (∼20 %) and GP (∼60 %) was not different between muscles, although GDE increased from ∼15 % diffusible in fresh muscle to ∼60 % in post-mortem muscle. Under physiologically relevant circumstances, in rat muscle and within detection limits: (1) The total cellular pool of glycogenin is always associated with glycogen granules, (2) GDE is associated with glycogen granules with over half the total pool associated with the outer tiers of glycogen, (3) GP is only ever weakly associated with glycogen granules and (4) addition of α-amylase is necessary in order to detect glycogenin, but not GDE or GP.

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Year:  2015        PMID: 25875859     DOI: 10.1007/s13105-015-0407-y

Source DB:  PubMed          Journal:  J Physiol Biochem        ISSN: 1138-7548            Impact factor:   4.158


  31 in total

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2.  Single fiber analyses of glycogen-related proteins reveal their differential association with glycogen in rat skeletal muscle.

Authors:  Robyn M Murphy; Hongyang Xu; Heidy Latchman; Noni T Larkins; Paul R Gooley; David I Stapleton
Journal:  Am J Physiol Cell Physiol       Date:  2012-09-26       Impact factor: 4.249

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Authors:  R Meléndez; E Meléndez-Hevia; M Cascante
Journal:  J Mol Evol       Date:  1997-10       Impact factor: 2.395

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Journal:  Clin Exp Pharmacol Physiol       Date:  2005-09       Impact factor: 2.557

5.  No limiting role for glycogenin in determining maximal attainable glycogen levels in rat skeletal muscle.

Authors:  B F Hansen; W Derave; P Jensen; E A Richter
Journal:  Am J Physiol Endocrinol Metab       Date:  2000-03       Impact factor: 4.310

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7.  AMP-activated protein kinase does not associate with glycogen alpha-particles from rat liver.

Authors:  Glendon J Parker; Ann Koay; Ryan Gilbert-Wilson; Lynne J Waddington; David Stapleton
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Authors:  Janelle P Mollica; Jonathan S Oakhill; Graham D Lamb; Robyn M Murphy
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10.  Comparative structural analyses of purified glycogen particles from rat liver, human skeletal muscle and commercial preparations.

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Journal:  J Muscle Res Cell Motil       Date:  2018-06-15       Impact factor: 2.698

3.  Skeletal muscle cell-specific differences in type 2 diabetes.

Authors:  Noni T Frankenberg; Shaun A Mason; Glenn D Wadley; Robyn M Murphy
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4.  Elevated GLUT4 and glycogenin protein abundance correspond to increased glycogen content in the soleus muscle of mdx mice with no benefit associated with taurine supplementation.

Authors:  Robert G Barker; Barnaby P Frankish; Hongyang Xu; Robyn M Murphy
Journal:  Physiol Rep       Date:  2018-03
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