Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation

Volker M. Lauschke; Sabine U. Vorrink; Sabrina M.L. Moro; Fatemah Rezayee; Åsa Nordling; Delilah F.G. Hendriks; Catherine C. Bell; Rowena Sison-Young; B. Kevin Park; Christopher E. Goldring; Ewa Ellis; Inger Johansson; Souren Mkrtchian; Tommy B. Andersson; Magnus Ingelman-Sundberg

doi:10.1002/hep.28780

Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation

Volker M. Lauschke
, Sabine U. Vorrink
, Sabrina M.L. Moro
, Fatemah Rezayee
, Åsa Nordling
, Delilah F.G. Hendriks
, Catherine C. Bell
, Rowena Sison-Young
, B. Kevin Park
, Christopher E. Goldring
, Ewa Ellis
, Inger Johansson
, Souren Mkrtchian
, Tommy B. Andersson
, Magnus Ingelman-Sundberg

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

108 Citations (Scopus)

Abstract

Hepatocytes are dynamic cells that, upon injury, can alternate between nondividing differentiated and dedifferentiated proliferating states in vivo. However, in two-dimensional cultures, primary human hepatocytes (PHHs) rapidly dedifferentiate, resulting in loss of hepatic functions that significantly limits their usefulness as an in vitro model of liver biology, liver diseases, as well as drug metabolism and toxicity. Thus, understanding the underlying mechanisms and stalling of the dedifferentiation process would be highly beneficial to establish more-accurate and relevant long-term in vitro hepatocyte models. Here, we present comprehensive analyses of whole proteome and transcriptome dynamics during the initiation of dedifferentiation during the first 24 hours of culture. We report that early major rearrangements of the noncoding transcriptome, hallmarked by increased expression of small nucleolar RNAs, long noncoding RNAs, microRNAs (miRNAs), and ribosomal genes, precede most changes in coding genes during dedifferentiation of PHHs, and we speculated that these modulations could drive the hepatic dedifferentiation process. To functionally test this hypothesis, we globally inhibited the miRNA machinery using two established chemically distinct compounds, acriflavine and poly-l-lysine. These inhibition experiments resulted in a significantly impaired miRNA response and, most important, in a pronounced reduction in the down-regulation of hepatic genes with importance for liver function. Thus, we provide strong evidence for the importance of noncoding RNAs, in particular, miRNAs, in hepatic dedifferentiation, which can aid the development of more-efficient differentiation protocols for stem-cell-derived hepatocytes and broaden our understanding of the dynamic properties of hepatocytes with respect to liver regeneration. Conclusion: miRNAs are important drivers of hepatic dedifferentiation, and our results provide valuable information regarding the mechanisms behind liver regeneration and possibilities to inhibit dedifferentiation in vitro. (Hepatology 2016;64:1743-1756).

Original language	English
Pages (from-to)	1743-1756
Number of pages	14
Journal	Hepatology
Volume	64
Issue number	5
DOIs	https://doi.org/10.1002/hep.28780
Publication status	Published - 1 Nov 2016
Externally published	Yes

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10.1002/hep.28780

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Lauschke, V. M., Vorrink, S. U., Moro, S. M. L., Rezayee, F., Nordling, Å., Hendriks, D. F. G., Bell, C. C., Sison-Young, R., Park, B. K., Goldring, C. E., Ellis, E., Johansson, I., Mkrtchian, S., Andersson, T. B., & Ingelman-Sundberg, M. (2016). Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation. Hepatology, 64(5), 1743-1756. https://doi.org/10.1002/hep.28780

@article{3bd9362466dc42d698396ef9e3ed8e78,

title = "Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation",

abstract = "Hepatocytes are dynamic cells that, upon injury, can alternate between nondividing differentiated and dedifferentiated proliferating states in vivo. However, in two-dimensional cultures, primary human hepatocytes (PHHs) rapidly dedifferentiate, resulting in loss of hepatic functions that significantly limits their usefulness as an in vitro model of liver biology, liver diseases, as well as drug metabolism and toxicity. Thus, understanding the underlying mechanisms and stalling of the dedifferentiation process would be highly beneficial to establish more-accurate and relevant long-term in vitro hepatocyte models. Here, we present comprehensive analyses of whole proteome and transcriptome dynamics during the initiation of dedifferentiation during the first 24 hours of culture. We report that early major rearrangements of the noncoding transcriptome, hallmarked by increased expression of small nucleolar RNAs, long noncoding RNAs, microRNAs (miRNAs), and ribosomal genes, precede most changes in coding genes during dedifferentiation of PHHs, and we speculated that these modulations could drive the hepatic dedifferentiation process. To functionally test this hypothesis, we globally inhibited the miRNA machinery using two established chemically distinct compounds, acriflavine and poly-l-lysine. These inhibition experiments resulted in a significantly impaired miRNA response and, most important, in a pronounced reduction in the down-regulation of hepatic genes with importance for liver function. Thus, we provide strong evidence for the importance of noncoding RNAs, in particular, miRNAs, in hepatic dedifferentiation, which can aid the development of more-efficient differentiation protocols for stem-cell-derived hepatocytes and broaden our understanding of the dynamic properties of hepatocytes with respect to liver regeneration. Conclusion: miRNAs are important drivers of hepatic dedifferentiation, and our results provide valuable information regarding the mechanisms behind liver regeneration and possibilities to inhibit dedifferentiation in vitro. (Hepatology 2016;64:1743-1756).",

author = "Lauschke, \{Volker M.\} and Vorrink, \{Sabine U.\} and Moro, \{Sabrina M.L.\} and Fatemah Rezayee and {\AA}sa Nordling and Hendriks, \{Delilah F.G.\} and Bell, \{Catherine C.\} and Rowena Sison-Young and Park, \{B. Kevin\} and Goldring, \{Christopher E.\} and Ewa Ellis and Inger Johansson and Souren Mkrtchian and Andersson, \{Tommy B.\} and Magnus Ingelman-Sundberg",

note = "Publisher Copyright: {\textcopyright} 2016 by the American Association for the Study of Liver Diseases",

year = "2016",

month = nov,

day = "1",

doi = "10.1002/hep.28780",

language = "English",

volume = "64",

pages = "1743--1756",

journal = "Hepatology",

issn = "0270-9139",

publisher = "Lippincott Williams and Wilkins",

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}

Lauschke, VM, Vorrink, SU, Moro, SML, Rezayee, F, Nordling, Å, Hendriks, DFG, Bell, CC, Sison-Young, R, Park, BK, Goldring, CE, Ellis, E, Johansson, I, Mkrtchian, S, Andersson, TB & Ingelman-Sundberg, M 2016, 'Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation', Hepatology, vol. 64, no. 5, pp. 1743-1756. https://doi.org/10.1002/hep.28780

TY - JOUR

T1 - Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation

AU - Lauschke, Volker M.

AU - Vorrink, Sabine U.

AU - Moro, Sabrina M.L.

AU - Rezayee, Fatemah

AU - Nordling, Åsa

AU - Hendriks, Delilah F.G.

AU - Bell, Catherine C.

AU - Sison-Young, Rowena

AU - Park, B. Kevin

AU - Goldring, Christopher E.

AU - Ellis, Ewa

AU - Johansson, Inger

AU - Mkrtchian, Souren

AU - Andersson, Tommy B.

AU - Ingelman-Sundberg, Magnus

PY - 2016/11/1

Y1 - 2016/11/1

N2 - Hepatocytes are dynamic cells that, upon injury, can alternate between nondividing differentiated and dedifferentiated proliferating states in vivo. However, in two-dimensional cultures, primary human hepatocytes (PHHs) rapidly dedifferentiate, resulting in loss of hepatic functions that significantly limits their usefulness as an in vitro model of liver biology, liver diseases, as well as drug metabolism and toxicity. Thus, understanding the underlying mechanisms and stalling of the dedifferentiation process would be highly beneficial to establish more-accurate and relevant long-term in vitro hepatocyte models. Here, we present comprehensive analyses of whole proteome and transcriptome dynamics during the initiation of dedifferentiation during the first 24 hours of culture. We report that early major rearrangements of the noncoding transcriptome, hallmarked by increased expression of small nucleolar RNAs, long noncoding RNAs, microRNAs (miRNAs), and ribosomal genes, precede most changes in coding genes during dedifferentiation of PHHs, and we speculated that these modulations could drive the hepatic dedifferentiation process. To functionally test this hypothesis, we globally inhibited the miRNA machinery using two established chemically distinct compounds, acriflavine and poly-l-lysine. These inhibition experiments resulted in a significantly impaired miRNA response and, most important, in a pronounced reduction in the down-regulation of hepatic genes with importance for liver function. Thus, we provide strong evidence for the importance of noncoding RNAs, in particular, miRNAs, in hepatic dedifferentiation, which can aid the development of more-efficient differentiation protocols for stem-cell-derived hepatocytes and broaden our understanding of the dynamic properties of hepatocytes with respect to liver regeneration. Conclusion: miRNAs are important drivers of hepatic dedifferentiation, and our results provide valuable information regarding the mechanisms behind liver regeneration and possibilities to inhibit dedifferentiation in vitro. (Hepatology 2016;64:1743-1756).

AB - Hepatocytes are dynamic cells that, upon injury, can alternate between nondividing differentiated and dedifferentiated proliferating states in vivo. However, in two-dimensional cultures, primary human hepatocytes (PHHs) rapidly dedifferentiate, resulting in loss of hepatic functions that significantly limits their usefulness as an in vitro model of liver biology, liver diseases, as well as drug metabolism and toxicity. Thus, understanding the underlying mechanisms and stalling of the dedifferentiation process would be highly beneficial to establish more-accurate and relevant long-term in vitro hepatocyte models. Here, we present comprehensive analyses of whole proteome and transcriptome dynamics during the initiation of dedifferentiation during the first 24 hours of culture. We report that early major rearrangements of the noncoding transcriptome, hallmarked by increased expression of small nucleolar RNAs, long noncoding RNAs, microRNAs (miRNAs), and ribosomal genes, precede most changes in coding genes during dedifferentiation of PHHs, and we speculated that these modulations could drive the hepatic dedifferentiation process. To functionally test this hypothesis, we globally inhibited the miRNA machinery using two established chemically distinct compounds, acriflavine and poly-l-lysine. These inhibition experiments resulted in a significantly impaired miRNA response and, most important, in a pronounced reduction in the down-regulation of hepatic genes with importance for liver function. Thus, we provide strong evidence for the importance of noncoding RNAs, in particular, miRNAs, in hepatic dedifferentiation, which can aid the development of more-efficient differentiation protocols for stem-cell-derived hepatocytes and broaden our understanding of the dynamic properties of hepatocytes with respect to liver regeneration. Conclusion: miRNAs are important drivers of hepatic dedifferentiation, and our results provide valuable information regarding the mechanisms behind liver regeneration and possibilities to inhibit dedifferentiation in vitro. (Hepatology 2016;64:1743-1756).

UR - https://www.scopus.com/pages/publications/84990068703

U2 - 10.1002/hep.28780

DO - 10.1002/hep.28780

M3 - Article

C2 - 27532775

AN - SCOPUS:84990068703

SN - 0270-9139

VL - 64

SP - 1743

EP - 1756

JO - Hepatology

JF - Hepatology

IS - 5

ER -

Massive rearrangements of cellular MicroRNA signatures are key drivers of hepatocyte dedifferentiation

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