Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum: An ER Stress/Defective Unfolded Protein Response Model

Richard T. Waldron; Hsin Yuan Su; Honit Piplani; Joseph Capri; Whitaker Cohn; Julian P. Whitelegge; Kym F. Faull; Sugunadevi Sakkiah; Ravinder Abrol; Wei Yang; Bo Zhou; Michael R. Freeman; Stephen J. Pandol; Aurelia Lugea

doi:10.1016/j.jcmgh.2018.01.001

Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum: An ER Stress/Defective Unfolded Protein Response Model

Richard T. Waldron
, Hsin Yuan Su
, Honit Piplani
, Joseph Capri
, Whitaker Cohn
, Julian P. Whitelegge
, Kym F. Faull
, Sugunadevi Sakkiah
, Ravinder Abrol
, Wei Yang
, Bo Zhou
, Michael R. Freeman
, Stephen J. Pandol
, Aurelia Lugea

Pathology

Cedars-Sinai Medical Center
University of California at Los Angeles

Research output: Contribution to journal › Article › peer-review

25 Scopus citations

Abstract

Background & Aims: Heavy alcohol drinking is associated with pancreatitis, whereas moderate intake lowers the risk. Mice fed ethanol long term show no pancreas damage unless adaptive/protective responses mediating proteostasis are disrupted. Pancreatic acini synthesize digestive enzymes (largely serine hydrolases) in the endoplasmic reticulum (ER), where perturbations (eg, alcohol consumption) activate adaptive unfolded protein responses orchestrated by spliced X-box binding protein 1 (XBP1). Here, we examined ethanol-induced early structural changes in pancreatic ER proteins. Methods: Wild-type and Xbp1+/- mice were fed control and ethanol diets, then tissues were homogenized and fractionated. ER proteins were labeled with a cysteine-reactive probe, isotope-coded affinity tag to obtain a novel pancreatic redox ER proteome. Specific labeling of active serine hydrolases in ER with fluorophosphonate desthiobiotin also was characterized proteomically. Protein structural perturbation by redox changes was evaluated further in molecular dynamic simulations. Results: Ethanol feeding and Xbp1 genetic inhibition altered ER redox balance and destabilized key proteins. Proteomic data and molecular dynamic simulations of Carboxyl ester lipase (Cel), a unique serine hydrolase active within ER, showed an uncoupled disulfide bond involving Cel Cys266, Cel dimerization, ER retention, and complex formation in ethanol-fed, XBP1-deficient mice. Conclusions: Results documented in ethanol-fed mice lacking sufficient spliced XBP1 illustrate consequences of ER stress extended by preventing unfolded protein response from fully restoring pancreatic acinar cell proteostasis during ethanol-induced redox challenge. In this model, orderly protein folding and transport to the secretory pathway were disrupted, and abundant molecules including Cel with perturbed structures were retained in ER, promoting ER stress-related pancreas pathology.

Original language	English
Pages (from-to)	479-497
Number of pages	19
Journal	CMGH
Volume	5
Issue number	4
DOIs	https://doi.org/10.1016/j.jcmgh.2018.01.001
State	Published - 2018

Keywords

Alcohol Pancreatitis
Carboxyl Ester Lipase
Disulfide Bond
Unfolded Protein Response

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10.1016/j.jcmgh.2018.01.001

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Waldron, R. T., Su, H. Y., Piplani, H., Capri, J., Cohn, W., Whitelegge, J. P., Faull, K. F., Sakkiah, S., Abrol, R., Yang, W., Zhou, B., Freeman, M. R., Pandol, S. J., & Lugea, A. (2018). Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum: An ER Stress/Defective Unfolded Protein Response Model. CMGH, 5(4), 479-497. https://doi.org/10.1016/j.jcmgh.2018.01.001

@article{2fac2162b30a40e483ba93872b559d2b,

title = "Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum: An ER Stress/Defective Unfolded Protein Response Model",

abstract = "Background \& Aims: Heavy alcohol drinking is associated with pancreatitis, whereas moderate intake lowers the risk. Mice fed ethanol long term show no pancreas damage unless adaptive/protective responses mediating proteostasis are disrupted. Pancreatic acini synthesize digestive enzymes (largely serine hydrolases) in the endoplasmic reticulum (ER), where perturbations (eg, alcohol consumption) activate adaptive unfolded protein responses orchestrated by spliced X-box binding protein 1 (XBP1). Here, we examined ethanol-induced early structural changes in pancreatic ER proteins. Methods: Wild-type and Xbp1+/- mice were fed control and ethanol diets, then tissues were homogenized and fractionated. ER proteins were labeled with a cysteine-reactive probe, isotope-coded affinity tag to obtain a novel pancreatic redox ER proteome. Specific labeling of active serine hydrolases in ER with fluorophosphonate desthiobiotin also was characterized proteomically. Protein structural perturbation by redox changes was evaluated further in molecular dynamic simulations. Results: Ethanol feeding and Xbp1 genetic inhibition altered ER redox balance and destabilized key proteins. Proteomic data and molecular dynamic simulations of Carboxyl ester lipase (Cel), a unique serine hydrolase active within ER, showed an uncoupled disulfide bond involving Cel Cys266, Cel dimerization, ER retention, and complex formation in ethanol-fed, XBP1-deficient mice. Conclusions: Results documented in ethanol-fed mice lacking sufficient spliced XBP1 illustrate consequences of ER stress extended by preventing unfolded protein response from fully restoring pancreatic acinar cell proteostasis during ethanol-induced redox challenge. In this model, orderly protein folding and transport to the secretory pathway were disrupted, and abundant molecules including Cel with perturbed structures were retained in ER, promoting ER stress-related pancreas pathology.",

keywords = "Alcohol Pancreatitis, Carboxyl Ester Lipase, Disulfide Bond, Unfolded Protein Response",

author = "Waldron, \{Richard T.\} and Su, \{Hsin Yuan\} and Honit Piplani and Joseph Capri and Whitaker Cohn and Whitelegge, \{Julian P.\} and Faull, \{Kym F.\} and Sugunadevi Sakkiah and Ravinder Abrol and Wei Yang and Bo Zhou and Freeman, \{Michael R.\} and Pandol, \{Stephen J.\} and Aurelia Lugea",

note = "Publisher Copyright: {\textcopyright} 2018 The Authors",

year = "2018",

doi = "10.1016/j.jcmgh.2018.01.001",

language = "English",

volume = "5",

pages = "479--497",

journal = "CMGH",

issn = "2352-345X",

number = "4",

}

Waldron, RT, Su, HY, Piplani, H, Capri, J, Cohn, W, Whitelegge, JP, Faull, KF, Sakkiah, S, Abrol, R, Yang, W, Zhou, B, Freeman, MR, Pandol, SJ & Lugea, A 2018, 'Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum: An ER Stress/Defective Unfolded Protein Response Model', CMGH, vol. 5, no. 4, pp. 479-497. https://doi.org/10.1016/j.jcmgh.2018.01.001

TY - JOUR

T1 - Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum

T2 - An ER Stress/Defective Unfolded Protein Response Model

AU - Waldron, Richard T.

AU - Su, Hsin Yuan

AU - Piplani, Honit

AU - Capri, Joseph

AU - Cohn, Whitaker

AU - Whitelegge, Julian P.

AU - Faull, Kym F.

AU - Sakkiah, Sugunadevi

AU - Abrol, Ravinder

AU - Yang, Wei

AU - Zhou, Bo

AU - Freeman, Michael R.

AU - Pandol, Stephen J.

AU - Lugea, Aurelia

PY - 2018

Y1 - 2018

N2 - Background & Aims: Heavy alcohol drinking is associated with pancreatitis, whereas moderate intake lowers the risk. Mice fed ethanol long term show no pancreas damage unless adaptive/protective responses mediating proteostasis are disrupted. Pancreatic acini synthesize digestive enzymes (largely serine hydrolases) in the endoplasmic reticulum (ER), where perturbations (eg, alcohol consumption) activate adaptive unfolded protein responses orchestrated by spliced X-box binding protein 1 (XBP1). Here, we examined ethanol-induced early structural changes in pancreatic ER proteins. Methods: Wild-type and Xbp1+/- mice were fed control and ethanol diets, then tissues were homogenized and fractionated. ER proteins were labeled with a cysteine-reactive probe, isotope-coded affinity tag to obtain a novel pancreatic redox ER proteome. Specific labeling of active serine hydrolases in ER with fluorophosphonate desthiobiotin also was characterized proteomically. Protein structural perturbation by redox changes was evaluated further in molecular dynamic simulations. Results: Ethanol feeding and Xbp1 genetic inhibition altered ER redox balance and destabilized key proteins. Proteomic data and molecular dynamic simulations of Carboxyl ester lipase (Cel), a unique serine hydrolase active within ER, showed an uncoupled disulfide bond involving Cel Cys266, Cel dimerization, ER retention, and complex formation in ethanol-fed, XBP1-deficient mice. Conclusions: Results documented in ethanol-fed mice lacking sufficient spliced XBP1 illustrate consequences of ER stress extended by preventing unfolded protein response from fully restoring pancreatic acinar cell proteostasis during ethanol-induced redox challenge. In this model, orderly protein folding and transport to the secretory pathway were disrupted, and abundant molecules including Cel with perturbed structures were retained in ER, promoting ER stress-related pancreas pathology.

AB - Background & Aims: Heavy alcohol drinking is associated with pancreatitis, whereas moderate intake lowers the risk. Mice fed ethanol long term show no pancreas damage unless adaptive/protective responses mediating proteostasis are disrupted. Pancreatic acini synthesize digestive enzymes (largely serine hydrolases) in the endoplasmic reticulum (ER), where perturbations (eg, alcohol consumption) activate adaptive unfolded protein responses orchestrated by spliced X-box binding protein 1 (XBP1). Here, we examined ethanol-induced early structural changes in pancreatic ER proteins. Methods: Wild-type and Xbp1+/- mice were fed control and ethanol diets, then tissues were homogenized and fractionated. ER proteins were labeled with a cysteine-reactive probe, isotope-coded affinity tag to obtain a novel pancreatic redox ER proteome. Specific labeling of active serine hydrolases in ER with fluorophosphonate desthiobiotin also was characterized proteomically. Protein structural perturbation by redox changes was evaluated further in molecular dynamic simulations. Results: Ethanol feeding and Xbp1 genetic inhibition altered ER redox balance and destabilized key proteins. Proteomic data and molecular dynamic simulations of Carboxyl ester lipase (Cel), a unique serine hydrolase active within ER, showed an uncoupled disulfide bond involving Cel Cys266, Cel dimerization, ER retention, and complex formation in ethanol-fed, XBP1-deficient mice. Conclusions: Results documented in ethanol-fed mice lacking sufficient spliced XBP1 illustrate consequences of ER stress extended by preventing unfolded protein response from fully restoring pancreatic acinar cell proteostasis during ethanol-induced redox challenge. In this model, orderly protein folding and transport to the secretory pathway were disrupted, and abundant molecules including Cel with perturbed structures were retained in ER, promoting ER stress-related pancreas pathology.

KW - Alcohol Pancreatitis

KW - Carboxyl Ester Lipase

KW - Disulfide Bond

KW - Unfolded Protein Response

UR - https://www.scopus.com/pages/publications/85044604538

U2 - 10.1016/j.jcmgh.2018.01.001

DO - 10.1016/j.jcmgh.2018.01.001

M3 - Article

AN - SCOPUS:85044604538

SN - 2352-345X

VL - 5

SP - 479

EP - 497

JO - CMGH

JF - CMGH

IS - 4

ER -

Ethanol Induced Disordering of Pancreatic Acinar Cell Endoplasmic Reticulum: An ER Stress/Defective Unfolded Protein Response Model

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Keywords

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