ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes

The unfolded protein response in the endoplasmic reticulum (UPR(ER)) is involved in a number of metabolic diseases. Here, we characterize UPR(ER)-induced metabolic changes in mouse livers in vivo through metabolic labeling and mass spectrometric analysis of lipid and proteome-wide fluxes. We induced...

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Autores principales: Ward, Catherine P., Peng, Lucy, Yuen, Samuel, Chang, Michael, Karapetyan, Rozalina, Nyangau, Edna, Mohammed, Hussein, Palacios, Hector, Ziari, Naveed, Joe, Larry K., Frakes, Ashley E., Dandan, Mohamad, Dillin, Andrew, Hellerstein, Marc K.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2022
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Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8835023/
https://www.ncbi.nlm.nih.gov/pubmed/35162995
http://dx.doi.org/10.3390/ijms23031073
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author Ward, Catherine P.
Peng, Lucy
Yuen, Samuel
Chang, Michael
Karapetyan, Rozalina
Nyangau, Edna
Mohammed, Hussein
Palacios, Hector
Ziari, Naveed
Joe, Larry K.
Frakes, Ashley E.
Dandan, Mohamad
Dillin, Andrew
Hellerstein, Marc K.
author_facet Ward, Catherine P.
Peng, Lucy
Yuen, Samuel
Chang, Michael
Karapetyan, Rozalina
Nyangau, Edna
Mohammed, Hussein
Palacios, Hector
Ziari, Naveed
Joe, Larry K.
Frakes, Ashley E.
Dandan, Mohamad
Dillin, Andrew
Hellerstein, Marc K.
author_sort Ward, Catherine P.
collection PubMed
description The unfolded protein response in the endoplasmic reticulum (UPR(ER)) is involved in a number of metabolic diseases. Here, we characterize UPR(ER)-induced metabolic changes in mouse livers in vivo through metabolic labeling and mass spectrometric analysis of lipid and proteome-wide fluxes. We induced UPR(ER) by tunicamycin administration and measured synthesis rates of proteins, fatty acids and cholesterol, as well as RNA-seq. Contrary to reports in isolated cells, hepatic de novo lipogenesis and cholesterogenesis were markedly reduced, as were mRNA levels and synthesis rates of lipogenic proteins. H&E staining showed enrichment with lipid droplets while electron microscopy revealed ER morphological changes. Interestingly, the pre-labeling of adipose tissue prior to UPR(ER) induction resulted in the redistribution of labeled fatty acids from adipose tissue to the liver, with replacement by unlabeled glycerol in the liver acylglycerides, indicating that the liver uptake was of free fatty acids, not whole glycerolipids. The redistribution of adipose fatty acids to the liver was not explicable by altered plasma insulin, increased fatty acid levels (lipolysis) or by reduced food intake. Synthesis of most liver proteins was suppressed under UPR(ER) conditions, with the exception of BiP, other chaperones, protein disulfide isomerases, and proteins of ribosomal biogenesis. Protein synthesis rates generally, but not always, paralleled changes in mRNA. In summary, this combined approach, linking static changes with fluxes, revealed an integrated reduction of lipid and cholesterol synthesis pathways, from gene expression to translation and metabolic flux rates, under UPR(ER) conditions. The reduced lipogenesis does not parallel human fatty liver disease. This approach provides powerful tools to characterize metabolic processes underlying hepatic UPR(ER) in vivo.
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spelling pubmed-88350232022-02-12 ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes Ward, Catherine P. Peng, Lucy Yuen, Samuel Chang, Michael Karapetyan, Rozalina Nyangau, Edna Mohammed, Hussein Palacios, Hector Ziari, Naveed Joe, Larry K. Frakes, Ashley E. Dandan, Mohamad Dillin, Andrew Hellerstein, Marc K. Int J Mol Sci Article The unfolded protein response in the endoplasmic reticulum (UPR(ER)) is involved in a number of metabolic diseases. Here, we characterize UPR(ER)-induced metabolic changes in mouse livers in vivo through metabolic labeling and mass spectrometric analysis of lipid and proteome-wide fluxes. We induced UPR(ER) by tunicamycin administration and measured synthesis rates of proteins, fatty acids and cholesterol, as well as RNA-seq. Contrary to reports in isolated cells, hepatic de novo lipogenesis and cholesterogenesis were markedly reduced, as were mRNA levels and synthesis rates of lipogenic proteins. H&E staining showed enrichment with lipid droplets while electron microscopy revealed ER morphological changes. Interestingly, the pre-labeling of adipose tissue prior to UPR(ER) induction resulted in the redistribution of labeled fatty acids from adipose tissue to the liver, with replacement by unlabeled glycerol in the liver acylglycerides, indicating that the liver uptake was of free fatty acids, not whole glycerolipids. The redistribution of adipose fatty acids to the liver was not explicable by altered plasma insulin, increased fatty acid levels (lipolysis) or by reduced food intake. Synthesis of most liver proteins was suppressed under UPR(ER) conditions, with the exception of BiP, other chaperones, protein disulfide isomerases, and proteins of ribosomal biogenesis. Protein synthesis rates generally, but not always, paralleled changes in mRNA. In summary, this combined approach, linking static changes with fluxes, revealed an integrated reduction of lipid and cholesterol synthesis pathways, from gene expression to translation and metabolic flux rates, under UPR(ER) conditions. The reduced lipogenesis does not parallel human fatty liver disease. This approach provides powerful tools to characterize metabolic processes underlying hepatic UPR(ER) in vivo. MDPI 2022-01-19 /pmc/articles/PMC8835023/ /pubmed/35162995 http://dx.doi.org/10.3390/ijms23031073 Text en © 2022 by the authors. https://creativecommons.org/licenses/by/4.0/Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Ward, Catherine P.
Peng, Lucy
Yuen, Samuel
Chang, Michael
Karapetyan, Rozalina
Nyangau, Edna
Mohammed, Hussein
Palacios, Hector
Ziari, Naveed
Joe, Larry K.
Frakes, Ashley E.
Dandan, Mohamad
Dillin, Andrew
Hellerstein, Marc K.
ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes
title ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes
title_full ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes
title_fullStr ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes
title_full_unstemmed ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes
title_short ER Unfolded Protein Response in Liver In Vivo Is Characterized by Reduced, Not Increased, De Novo Lipogenesis and Cholesterol Synthesis Rates with Uptake of Fatty Acids from Adipose Tissue: Integrated Gene Expression, Translation Rates and Metabolic Fluxes
title_sort er unfolded protein response in liver in vivo is characterized by reduced, not increased, de novo lipogenesis and cholesterol synthesis rates with uptake of fatty acids from adipose tissue: integrated gene expression, translation rates and metabolic fluxes
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8835023/
https://www.ncbi.nlm.nih.gov/pubmed/35162995
http://dx.doi.org/10.3390/ijms23031073
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