PUBLICATION

Mercury-induced hepatotoxicity in zebrafish: in vivo mechanistic insights from transcriptome analysis, phenotype anchoring and targeted gene expression validation

Authors

Ung, C.Y., Lam, S.H., Hlaing, M.M., Winata, C.L., Korzh, S., Mathavan, S., and Gong, Z.

ID

ZDB-PUB-100408-6

Date

2010

Source

BMC Genomics 11: 212 (Journal)

Registered Authors

Gong, Zhiyuan, Korzh, Svitlana, Lam, Siew Hong, Mathavan, S., Winata, Cecilia Lanny

Keywords

none

Datasets

GEO:GSE18861

MeSH Terms

Animals
Apoptosis
Arsenic/toxicity
Cell Adhesion/drug effects
Cell Line
Gene Expression Profiling*
Hepatocytes/cytology
Hepatocytes/drug effects
Humans
Liver/cytology
Liver/drug effects*
Mercury/toxicity*
Oligonucleotide Array Sequence Analysis
Zebrafish/genetics*
Zebrafish/metabolism

(all 15)

PubMed

20353558 Full text @ BMC Genomics

CTD

20353558

Abstract

BACKGROUND: Mercury is a prominent environmental contaminant that causes detrimental effects to human health. Although the liver has been known to be a main target organ, there is limited information on in vivo molecular mechanism of mercury-induced toxicity in the liver. By using transcriptome analysis, phenotypic anchoring and validation of targeted gene expression in zebrafish, mercury-induced hepatotoxicity was investigated and a number of perturbed cellular processes were identified and compared with those captured in the in vitro human cell line studies. RESULTS: Hepato-transcriptome analysis of mercury-exposed zebrafish revealed that the earliest deregulated genes were associated with electron transport chain, mitochondrial fatty acid beta-oxidation, nuclear receptor signaling and apoptotic pathway, followed by complement system and proteasome pathway, and thereafter DNA damage, hypoxia, Wnt signaling, fatty acid synthesis, gluconeogenesis, cell cycle and motility. Comparative meta-analysis of microarray data between zebrafish liver and human HepG2 cells exposed to mercury identified some common toxicological effects of mercury-induced hepatotoxicity in both models. Histological analyses of liver from mercury-exposed fish revealed morphological changes of liver parenchyma, decreased nucleated cell count, increased lipid vesicles, glycogen and apoptotic bodies, thus providing phenotypic evidence for anchoring of the transcriptome analysis. Validation of targeted gene expression confirmed deregulated gene-pathways from enrichment analysis. Some of these genes responding to low concentrations of mercury may serve as toxicogenomic-based markers for detection and health risk assessment of environmental mercury contaminations. CONCLUSION: Mercury-induced hepatotoxicity was triggered by oxidative stresses, intrinsic apoptotic pathway, deregulation of nuclear receptor and kinase activities including Gsk3 that deregulates Wnt signaling pathway, gluconeogenesis, and adipogenesis, leading to mitochondrial dysfunction, endocrine disruption and metabolic disorders. This study provides important mechanistic insights into mercury-induced liver toxicity in a whole-animal physiology context, which will help in understanding the syndromes caused by mercury poisoning. The molecular conservation of mercury-induced hepatotoxicity between zebrafish and human cell line reveals the feasibility of using zebrafish to model molecular toxicity in human for toxicant risk assessments.

Genes / Markers

Marker	Marker Type	Name
agt	GENE	angiotensinogen
apom	GENE	apolipoprotein M
atp6v1e1b	GENE	ATPase H+ transporting V1 subunit E1b
cebpb	GENE	CCAAT enhancer binding protein beta
cebpd	GENE	CCAAT enhancer binding protein delta
cfb	GENE	complement factor B
cox7c	GENE	cytochrome c oxidase subunit 7C
dffa	GENE	DNA fragmentation factor, alpha polypeptide
fga	GENE	fibrinogen alpha chain
gsk3ab	GENE	glycogen synthase kinase 3 alpha b