Evaluating the antifibrotic potency of galunisertib in a human ex vivo model of liver fibrosis

Theerut Luangmonkong; Su Suriguga; Emilia Bigaeva; Miriam Boersema; Dorenda Oosterhuis; Koert P de Jong; Detlef Schuppan; Henricus A M Mutsaers; Peter Olinga

doi:10.1111/bph.13945

Evaluating the antifibrotic potency of galunisertib in a human ex vivo model of liver fibrosis

Theerut Luangmonkong, Su Suriguga, Emilia Bigaeva, Miriam Boersema, Dorenda Oosterhuis, Koert P de Jong, Detlef Schuppan, Henricus A M Mutsaers, Peter Olinga^*

^*Corresponding author for this work

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

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Abstract

Background and PurposeLiver fibrosis is a major cause of liver-related mortality and, so far, no effective antifibrotic drug is available. Galunisertib, a TGF- receptor type I kinase inhibitor, is a potential candidate for the treatment of liver fibrosis. Here, we evaluated the potency of galunisertib in a human ex vivo model of liver fibrosis.

Experimental ApproachAntifibrotic potency and associated mechanisms were studied ex vivo, using both healthy and cirrhotic human precision-cut liver slices. Fibrosis-related parameters, both transcriptional and translational level, were assessed after treatment with galunisertib.

Key ResultsGalunisertib showed a prominent antifibrotic potency. Phosphorylation of SMAD2 was inhibited, while that of SMAD1 remained unchanged. In healthy and cirrhotic human livers, spontaneous transcription of numerous genes encoding collagens, including collagen type I, 1, collagen maturation, non-collageneous extracellular matrix (ECM) components, ECM remodelling and selected ECM receptors was significantly decreased. The reduction of fibrosis-related transcription was paralleled by a significant inhibition of procollagen I C-peptide released by both healthy and cirrhotic human liver slices. Moreover, galunisertib showed similar antifibrotic potency in human and rat lives.

Conclusions and ImplicationsGalunisertib is a drug that deserves to be further investigated for the treatment of liver fibrosis. Inhibition of SMAD2 phosphorylation is probably a central mechanism of action. In addition, blocking the production and maturation of collagens and promoting their degradation are related to the antifibrotic action of galunisertib.

Original language	English
Pages (from-to)	3107-3117
Number of pages	11
Journal	British Journal of Pharmacology
Volume	174
Issue number	18
Early online date	10-Jul-2017
DOIs	https://doi.org/10.1111/bph.13945
Publication status	Published - Sept-2017

Keywords

GROWTH-FACTOR-BETA
PRECISION-CUT LIVER
HEPATIC STELLATE CELLS
COLLAGEN TYPE-I
LY2157299 MONOHYDRATE
SIGNALING PATHWAY
HEPATOCELLULAR-CARCINOMA
KINASE INHIBITOR
CONCISE GUIDE
EXPRESSION

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Evaluating the antifibrotic potency of galunisertib in a human ex vivomodel of liver fibrosisFinal publisher's version, 1.36 MBLicence: Taverne

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@article{fb01c8959db146378840afe793cefce3,

title = "Evaluating the antifibrotic potency of galunisertib in a human ex vivo model of liver fibrosis",

abstract = "Background and PurposeLiver fibrosis is a major cause of liver-related mortality and, so far, no effective antifibrotic drug is available. Galunisertib, a TGF- receptor type I kinase inhibitor, is a potential candidate for the treatment of liver fibrosis. Here, we evaluated the potency of galunisertib in a human ex vivo model of liver fibrosis.Experimental ApproachAntifibrotic potency and associated mechanisms were studied ex vivo, using both healthy and cirrhotic human precision-cut liver slices. Fibrosis-related parameters, both transcriptional and translational level, were assessed after treatment with galunisertib.Key ResultsGalunisertib showed a prominent antifibrotic potency. Phosphorylation of SMAD2 was inhibited, while that of SMAD1 remained unchanged. In healthy and cirrhotic human livers, spontaneous transcription of numerous genes encoding collagens, including collagen type I, 1, collagen maturation, non-collageneous extracellular matrix (ECM) components, ECM remodelling and selected ECM receptors was significantly decreased. The reduction of fibrosis-related transcription was paralleled by a significant inhibition of procollagen I C-peptide released by both healthy and cirrhotic human liver slices. Moreover, galunisertib showed similar antifibrotic potency in human and rat lives.Conclusions and ImplicationsGalunisertib is a drug that deserves to be further investigated for the treatment of liver fibrosis. Inhibition of SMAD2 phosphorylation is probably a central mechanism of action. In addition, blocking the production and maturation of collagens and promoting their degradation are related to the antifibrotic action of galunisertib.",

keywords = "GROWTH-FACTOR-BETA, PRECISION-CUT LIVER, HEPATIC STELLATE CELLS, COLLAGEN TYPE-I, LY2157299 MONOHYDRATE, SIGNALING PATHWAY, HEPATOCELLULAR-CARCINOMA, KINASE INHIBITOR, CONCISE GUIDE, EXPRESSION",

author = "Theerut Luangmonkong and Su Suriguga and Emilia Bigaeva and Miriam Boersema and Dorenda Oosterhuis and {de Jong}, {Koert P} and Detlef Schuppan and Mutsaers, {Henricus A M} and Peter Olinga",

note = "{\textcopyright} 2017 The British Pharmacological Society.",

year = "2017",

month = sep,

doi = "10.1111/bph.13945",

language = "English",

volume = "174",

pages = "3107--3117",

journal = "British Journal of Pharmacology",

issn = "0007-1188",

publisher = "Wiley-Blackwell",

number = "18",

}

TY - JOUR

T1 - Evaluating the antifibrotic potency of galunisertib in a human ex vivo model of liver fibrosis

AU - Luangmonkong, Theerut

AU - Suriguga, Su

AU - Bigaeva, Emilia

AU - Boersema, Miriam

AU - Oosterhuis, Dorenda

AU - de Jong, Koert P

AU - Schuppan, Detlef

AU - Mutsaers, Henricus A M

AU - Olinga, Peter

PY - 2017/9

Y1 - 2017/9

N2 - Background and PurposeLiver fibrosis is a major cause of liver-related mortality and, so far, no effective antifibrotic drug is available. Galunisertib, a TGF- receptor type I kinase inhibitor, is a potential candidate for the treatment of liver fibrosis. Here, we evaluated the potency of galunisertib in a human ex vivo model of liver fibrosis.Experimental ApproachAntifibrotic potency and associated mechanisms were studied ex vivo, using both healthy and cirrhotic human precision-cut liver slices. Fibrosis-related parameters, both transcriptional and translational level, were assessed after treatment with galunisertib.Key ResultsGalunisertib showed a prominent antifibrotic potency. Phosphorylation of SMAD2 was inhibited, while that of SMAD1 remained unchanged. In healthy and cirrhotic human livers, spontaneous transcription of numerous genes encoding collagens, including collagen type I, 1, collagen maturation, non-collageneous extracellular matrix (ECM) components, ECM remodelling and selected ECM receptors was significantly decreased. The reduction of fibrosis-related transcription was paralleled by a significant inhibition of procollagen I C-peptide released by both healthy and cirrhotic human liver slices. Moreover, galunisertib showed similar antifibrotic potency in human and rat lives.Conclusions and ImplicationsGalunisertib is a drug that deserves to be further investigated for the treatment of liver fibrosis. Inhibition of SMAD2 phosphorylation is probably a central mechanism of action. In addition, blocking the production and maturation of collagens and promoting their degradation are related to the antifibrotic action of galunisertib.

AB - Background and PurposeLiver fibrosis is a major cause of liver-related mortality and, so far, no effective antifibrotic drug is available. Galunisertib, a TGF- receptor type I kinase inhibitor, is a potential candidate for the treatment of liver fibrosis. Here, we evaluated the potency of galunisertib in a human ex vivo model of liver fibrosis.Experimental ApproachAntifibrotic potency and associated mechanisms were studied ex vivo, using both healthy and cirrhotic human precision-cut liver slices. Fibrosis-related parameters, both transcriptional and translational level, were assessed after treatment with galunisertib.Key ResultsGalunisertib showed a prominent antifibrotic potency. Phosphorylation of SMAD2 was inhibited, while that of SMAD1 remained unchanged. In healthy and cirrhotic human livers, spontaneous transcription of numerous genes encoding collagens, including collagen type I, 1, collagen maturation, non-collageneous extracellular matrix (ECM) components, ECM remodelling and selected ECM receptors was significantly decreased. The reduction of fibrosis-related transcription was paralleled by a significant inhibition of procollagen I C-peptide released by both healthy and cirrhotic human liver slices. Moreover, galunisertib showed similar antifibrotic potency in human and rat lives.Conclusions and ImplicationsGalunisertib is a drug that deserves to be further investigated for the treatment of liver fibrosis. Inhibition of SMAD2 phosphorylation is probably a central mechanism of action. In addition, blocking the production and maturation of collagens and promoting their degradation are related to the antifibrotic action of galunisertib.

KW - GROWTH-FACTOR-BETA

KW - PRECISION-CUT LIVER

KW - HEPATIC STELLATE CELLS

KW - COLLAGEN TYPE-I

KW - LY2157299 MONOHYDRATE

KW - SIGNALING PATHWAY

KW - HEPATOCELLULAR-CARCINOMA

KW - KINASE INHIBITOR

KW - CONCISE GUIDE

KW - EXPRESSION

U2 - 10.1111/bph.13945

DO - 10.1111/bph.13945

M3 - Article

C2 - 28691737

SN - 0007-1188

VL - 174

SP - 3107

EP - 3117

JO - British Journal of Pharmacology

JF - British Journal of Pharmacology

IS - 18

ER -

Evaluating the antifibrotic potency of galunisertib in a human ex vivo model of liver fibrosis

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