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The whole transcriptome analysis and the circRNA-lncRNA network construction in arsenic trioxide-treated mice myocardium - 03/06/22

Doi : 10.1016/j.biopha.2022.113183 
Yanan Jiang a, b, c, 1 , Xiuyun Shen a, 1 , Chaorun Dong a , Fengnan Zhi a , Yang Gao d , Chunpeng Shi a , Yuqiu Chao a , Jincheng Xu a , Desi Shang e , Juan Xu c , Baofeng Yang a, b, , Xia Li c, , Yunlong Bai a, b,
a Department of Pharmacology (State-Province Key Laboratories of Biomedicine, Pharmaceutics of China, Key Laboratory of Cardiovascular Research, Ministry of Education), College of Pharmacy, Harbin Medical University, Harbin, China 
b Translational Medicine Research and Cooperation Center of Northern China, Heilongjiang Academy of Medical Sciences, Harbin, China 
c College of Bioinformatics Science and Technology, Harbin Medical University, Harbin, China 
d Department of Gastroenterology and Hepatology, The Second Affiliated Hospital of Harbin Medical University, Harbin, China 
e The First Affiliated Hospital, Hengyang Medical School, University of South China, Hengyang, Hunan, China 

Corresponding authors at: Department of Pharmacology (State-Province Key Laboratories of Biomedicine, Pharmaceutics of China, Key Laboratory of Cardiovascular Research, Ministry of Education), College of Pharmacy, Harbin Medical University, Harbin, ChinaDepartment of Pharmacology (State-Province Key Laboratories of Biomedicine, Pharmaceutics of China, Key Laboratory of Cardiovascular Research, Ministry of Education), College of Pharmacy, Harbin Medical UniversityHarbinChina⁎⁎Corresponding author.

Abstract

Background/Aims

Arsenic trioxide (ATO) is an effective anti-cancer drug. Nonetheless, it possesses cardiotoxic effects which limit its clinical application. The present study aims to elucidate the molecular basis of ATO-induced cardiotoxicity through using whole transcriptome analysis.

Methods

The whole transcriptome in ATO-treated mice myocardium was analyzed using RNA sequencing technique. These results were confirmed by real-time PCR. The lncRNA-mRNA and circRNA-mRNA co-expression networks were constructed. Finally, a circRNA-lncRNA co-regulated competing endogenous RNA (ceRNA) network was constructed. GO and KEGG pathway analyses were performed. The expression levels of Txnip and Spp1 in ATO-treated neonatal mouse cardiomyocytes were validated by real-time PCR.

Results

A total of 113 mRNAs, 159 lncRNAs, 35 miRNAs, and 94 circRNAs were differentially expressed in ATO-treated mice myocardium. A lncRNA-circRNA co-regulation network was constructed. Function annotation revealed that aberrantly expressed genes may be enriched in the ‘Wnt signaling pathway’, ‘Hippo signaling pathway’, ‘Notch signaling pathway’, etc. Finally, the expression levels of Txnip and Spp1 were validated in ATO-treated cardiomyocytes, which was in accordance with the RNA-sequencing results.

Conclusion

ATO altered coding and noncoding RNA profiles in myocardium of mice. The ATO-related lncRNA-circRNA co-regulation network was constructed. Genes in the co-regulation network are likely to play important roles in the cardiotoxicity of ATO. This study provides new insights into the prevention and treatment of ATO-induced cardiotoxicity.

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Graphical Abstract




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Highlights

ATO altered coding and noncoding RNA profiles in myocardium of mice.
The ATO-related lncRNA-circRNA co-regulation network was constructed.
Genes in the co-regulation network are likely to play important roles in the cardiotoxicity of ATO.

El texto completo de este artículo está disponible en PDF.

Abbreviations : APL, ATO, ceRNA, CircRNA, EMT, LncRNA, LQTS, miRNA, PCC, TLR9

Keywords : Arsenic trioxide, Cardiotoxicity, RNA sequencing, Noncoding RNA


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