Hyperammonemia-mediated autophagy in skeletal muscle contributes to sarcopenia of cirrhosis | Health & Environmental Research Online (HERO)

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Citation
Tags

HERO ID

2997235

Reference Type

Journal Article

Title

Hyperammonemia-mediated autophagy in skeletal muscle contributes to sarcopenia of cirrhosis

Author(s)

Qiu, Jia; Tsien, C; Thapalaya, S; Narayanan, A; Weihl, CC; Ching, JK; Eghtesad, B; Singh, K; Fu, X; Dubyak, G; McDonald, C; Almasan, A; Hazen, SL; Prasad, SVN; Dasarathy, S

Year

2012

Is Peer Reviewed?

Yes

Journal

American Journal of Physiology: Endocrinology And Metabolism
ISSN: 0193-1849
EISSN: 1522-1555

Volume

303

Issue

Page Numbers

E983-E993

Language

English

PMID

22895779

DOI

10.1152/ajpendo.00183.2012

Web of Science Id

WOS:000309982000005

Abstract

Hyperammonemia and sarcopenia (loss of skeletal muscle) are consistent abnormalities in cirrhosis and portosystemic shunting. We have shown that muscle ubiquitin-proteasome components are not increased with hyperammonemia despite sarcopenia. This suggests that an alternative mechanism of proteolysis contributes to sarcopenia in cirrhosis. We hypothesized that autophagy could be this alternative pathway since we observed increases in classic autophagy markers, increased LC3 lipidation, beclin-1 expression, and p62 degradation in immunoblots of skeletal muscle protein in cirrhotic patients. We observed similar changes in these autophagy markers in the portacaval anastamosis (PCA) rat model. To determine the mechanistic relationship between hyperammonemia and autophagy, we exposed murine C(2)C(12) myotubes to ammonium acetate. Significant increases in LC3 lipidation, beclin-1 expression, and p62 degradation occurred by 1 h, whereas autophagy gene expression (LC3, Atg5, Atg7, beclin-1) increased at 24 h. C(2)C(12) cells stably expressing GFP-LC3 or GFP-mCherry-LC3 constructs showed increased formation of mature autophagosomes supported by electron microscopic studies. Hyperammonemia also increased autophagic flux in mice, as quantified by an in vivo autophagometer. Because hyperammonemia induces nitration of proteins in astrocytes, we quantified global muscle protein nitration in cirrhotic patients, in the PCA rat, and in C(2)C(12) cells treated with ammonium acetate. Increased protein nitration was observed in all of these systems. Furthermore, colocalization of nitrated proteins with GFP-LC3-positive puncta in hyperammonemic C(2)C(12) cells suggested that autophagy is involved in degradation of nitrated proteins. These observations show that increased skeletal muscle autophagy in cirrhosis is mediated by hyperammonemia and may contribute to sarcopenia of cirrhosis.

Keywords

autophagometer; human; tyrosine nitration