
hsa‐miR‐106b‐5p participates in the development of chronic thromboembolic pulmonary hypertension via targeting matrix metalloproteinase 2
Author(s) -
Miao Ran,
Dong Xingbei,
Gong Juanni,
Wang Ying,
Guo Xiaojuan,
Li Yidan,
Liu Min,
Wan Jun,
Li Jifeng,
Yang Suqiao,
Wang Wang,
Kuang Tuguang,
Zhong Jiuchang,
Zhai Zhenguo,
Yang Yuanhua
Publication year - 2020
Publication title -
pulmonary circulation
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.791
H-Index - 40
ISSN - 2045-8940
DOI - 10.1177/2045894020928300
Subject(s) - microrna , downregulation and upregulation , chronic thromboembolic pulmonary hypertension , matrix metalloproteinase , pathogenesis , mmp2 , medicine , gene , transcription factor , bioinformatics , pulmonary hypertension , biology , immunology , genetics
Background Chronic thromboembolic pulmonary hypertension (CTEPH) is characterized by elevated pressure in pulmonary arteries. This study was performed to explore the critical miRNAs and genes affecting the pathogenesis of CTEPH. Methods GSE56914 dataset (10 CTEPH whole blood samples and 10 control samples) was downloaded from the Gene Expression Omnibus database. Using limma package, the differentially expressed miRNAs (DE‐miRNAs) were acquired. After miRNA‐target pairs were obtained using miRWalk2.0 tool, a miRNA‐target regulatory network was built by Cytoscape software. Using DAVID tool, significantly enriched pathways involving the target genes were identified. Moreover, the protein–protein interaction network and transcription factor‐target regulatory network were built by the Cytoscape software. Additionally, quantitative real‐time PCR (qRT‐PCR) experiments and luciferase assay were conducted to validate miRNA/gene expression and miRNA–target regulatory relationship, respectively. Results There were 25 DE‐miRNAs (8 up‐regulated and 17 down‐regulated) between CTEPH and control groups. The target genes of has‐let‐7b‐3p, has‐miR‐17‐5p, has‐miR‐3202, has‐miR‐106b‐5p, and has‐miR‐665 were enriched in multiple pathways such as “Insulin secretion”. qRT‐PCR analysis confirmed upregulation of hsa‐miR‐3202, hsa‐miR‐665, and matrix metalloproteinase 2 ( MMP2 ) as well as downregulation of hsa‐let‐7b‐3p, hsa‐miR‐17‐5p, and hsa‐miR‐106b‐5p. Luciferase assay indicated that MMP2 was negatively mediated by hsa‐miR‐106b‐5p. Conclusions These miRNAs and genes were associated with the pathogenesis of CTEPH. Besides, hsa‐miR‐106b‐5p was involved in the development of CTEPH via targeting MMP2 .