2016
DOI: 10.1007/s00204-016-1761-4
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Gene network activity in cultivated primary hepatocytes is highly similar to diseased mammalian liver tissue

Abstract: It is well known that isolation and cultivation of primary hepatocytes cause major gene expression alterations. In the present genome-wide, time-resolved study of cultivated human and mouse hepatocytes, we made the observation that expression changes in culture strongly resemble alterations in liver diseases. Hepatocytes of both species were cultivated in collagen sandwich and in monolayer conditions. Genome-wide data were also obtained from human NAFLD, cirrhosis, HCC and hepatitis B virus-infected tissue as … Show more

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Cited by 92 publications
(66 citation statements)
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References 30 publications
(44 reference statements)
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“…Microarray pre-processing and data analysis. Affymetrix gene expression data were pre-processed using 'affyPLM' packages of the Bioconductor Software 73 . Genes with the strongest evidence of differential expression were obtained using a linear model fit.…”
Section: Methodsmentioning
confidence: 99%
“…Microarray pre-processing and data analysis. Affymetrix gene expression data were pre-processed using 'affyPLM' packages of the Bioconductor Software 73 . Genes with the strongest evidence of differential expression were obtained using a linear model fit.…”
Section: Methodsmentioning
confidence: 99%
“…31) In addition, Ad vectors generally showed more rapid expression of cargo genes than AAV vectors, that would be critical for genome manipulation of hepatocytes since cultured primary human hepatocytes rapidly lose hepatocytic functions such as cytochrome P-450 activity 32) and expression of hepatocyte nuclear factor 4α. 33) Moreover, several types of improved Ad vectors with reduced immunogenicity have been developed. 30,34,35) Therefore, generation of Ad vector-mediated CRISPR/Cpf1 system could provide more options for delivery tools of genome editing in primary cells.…”
Section: Discussionmentioning
confidence: 99%
“…Even though the important information recovered from the whole organ, additional data required the isolation of viable hepatocytes . Despite their use as a cell source for in vivo transplantation studies, isolated primary hepatocytes cannot be cultivated in vitro for more than 24 h causing alterations in cell physiology and major gene expression, comparable to those observed in inflammatory liver diseases . Thus, a growing enthusiasm has favored the discovery of new cell sources used instead of primary hepatocytes and able to proliferate or self‐renew.…”
Section: Introductionmentioning
confidence: 99%