Single-Cell Gene Expression Analysis Identifies Chronic Alcohol-Mediated Shift in Hepatocyte Molecular States After Partial Hepatectomy

Achanta, Sirisha; Verma, Aalap; Srivastava, Ankita; Nilakantan, Harshavardhan; Hoek, Jan B.; Vadigepalli, Rajanikanth

doi:10.3727/105221618x15361728786767

Cited by 13 publications

(7 citation statements)

References 56 publications

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“…Lately, single-cell transcriptomic methods are being employed to probe cellular heterogeneities of tissues and reconstruct developmental trajectories of individual organs (Haghverdi et al, 2016;Saelens et al, 2019;Schiebinger et al, 2019). In the case of the liver, this has led to the identification of previously unknown subpopulations of hepatocytes, cholangiocytes, endothelial cells, scar-associated macrophages, stellate cells, and myofibroblasts from healthy and diseased conditions (Aizarani et al, 2019;Dobie et al, 2019;Hyun et al, 2019;MacParland et al, 2018;Pepe-Mooney et al, 2019;Ramachandran et al, 2019;Xiong et al, 2019;Achanta et al, 2019;Cook et al, 2018). The studies revealed that more than 50% of hepatocyte genes follow a discrete zonated expression pattern in a liver lobule, and surprisingly, similar metabolic zonation exists for LSECs and stellate cells Halpern et al, 2018;2017).…”

Section: Discussionmentioning

confidence: 99%

Cellular plasticity balances the metabolic and proliferation dynamics of a regenerating liver

et al. 2021

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The adult liver has exceptional ability to regenerate, but how it sustains normal metabolic activities during regeneration remains unclear. Here, we use partial hepatectomy (PHx) in tandem with single-cell transcriptomics to track cellular transitions and heterogeneities of ~22,000 liver cells through the initiation, progression, and termination phases of mouse liver regeneration. Our results reveal that following PHx, a subset of hepatocytes transiently reactivates an early-postnatal-like gene expression program to proliferate, while a distinct population of metabolically hyperactive cells appears to compensate for any temporary deficits in liver function. Importantly, through combined analysis of gene regulatory networks and cellcell interaction maps, we find that regenerating hepatocytes redeploy key developmental gene regulons, which are guided by extensive ligand-receptor mediated signaling events between hepatocytes and non-parenchymal cells. Altogether, our study offers a detailed blueprint of the intercellular crosstalk and cellular reprogramming that balances the metabolic and proliferation requirements of a regenerating liver..

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Section: Discussionmentioning

confidence: 99%

Cellular plasticity balances the metabolic and proliferation dynamics of a regenerating liver

et al. 2021

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“…is inactivated in some individuals with alcohol-induced liver injury, causing extensive repopulation of SAH livers with immature, fetal-like cells. The results identify the mechanism for liver failure in SAH by revealing that TNF-α and IL-1β ( 19), proinflamma-prevented maturation of hepatocytes (8), which explains why liver regeneration is inhibited by alcohol (17,18). However, the mechanisms involved were not defined.…”

Section: Introductionmentioning

confidence: 98%

“…Single-cell gene expression analysis recently demonstrated that feeding alcohol to adult rats increased the proportion of hepatocytes that are either becoming proliferative or proliferat-ing (8), suggesting that excessive alcohol drinking might promote some degree of hepatocyte dedifferentiation. Maintaining hepatocytes in a differentiated state is a critical function of the Hippo/ YAP signaling pathway (9).…”

Section: Introductionmentioning

confidence: 99%

Epithelial splicing regulatory protein 2–mediated alternative splicing reprograms hepatocytes in severe alcoholic hepatitis

Hyun

Sun

Ahmadi

et al. 2020

Journal of Clinical Investigation

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“…This protocol has been developed over the past decade in our lab to enable reliable high-throughput detection of gene expression by qRT-PCR in low input samples starting from 10 pg total RNA (single cells). We have used this protocol to measure gene expression in a wide variety of samples types, tissue treatments and disease contexts (1)(2)(3)(4)(5)(6)(7)(8)(9)(10)(11)(12). The present version of this protocol was developed as part of the National Institutes of Health SPARC project efforts to construct a comprehensive anatomical, molecular and functional map of the peripheral nervous system at the visceral organs.…”

Section: Introductionmentioning

confidence: 99%

Single cell high-throughput qRT-PCR protocol

Achanta

Vadigepalli

2021

Preprint

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Single cell high-throughput qRT-PCR protocol combines high sensitivity technique of single cell qPCR with high-throughput qPCR technology that can generate data from 96 samples and 96 genes in a single experiment. It can be adapted for various sample types- cell culture, tissue samples and extracted RNA (10 pg) and measured on traditional qPCR and high-throughput qPCR platforms. The workflow is comprised of four steps – cell lysis, reverse transcription, pre-amplification and qPCR. Key features of this protocol are; processing low input samples directly to reverse transcription without RNA extraction which minimizes sample loss, pre-amplification enables amplification of cDNA from single cells to detectable levels for qPCR and measuring up to 400 genes from a single cell sample/10 pg of RNA (starting material). Robust, reproducible and versatile this protocol can be adapted to several upstream and downstream techniques.

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Single-Cell Gene Expression Analysis Identifies Chronic Alcohol-Mediated Shift in Hepatocyte Molecular States After Partial Hepatectomy

Cited by 13 publications

References 56 publications

Cellular plasticity balances the metabolic and proliferation dynamics of a regenerating liver

Cellular plasticity balances the metabolic and proliferation dynamics of a regenerating liver

Epithelial splicing regulatory protein 2–mediated alternative splicing reprograms hepatocytes in severe alcoholic hepatitis

Single cell high-throughput qRT-PCR protocol

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