[No authors listed]
Osteoarthritis (OA) is a common musculoskeletal disease and is related to the function of chondrocytes. The aim of the present study was to investigate the effects of miRâ302dâ3p on chondrocytes. (qPCR) was conducted to detect mRNA expression, while western blotting was performed to investigate protein expression in these cells. RNAs mimics, inhibitors and small interfering (si)RNAs were respectively transfected into chondrocytes (CHONâ001 cell line), after which, a Cell Counting Kitâ8 assay was performed to detect chondrocyte viability. Giemsa staining of the cells was also conducted to analyze the colony formation ability of the cells. Additionally, cell apoptosis was evaluated with an apoptosis detection kit using flow cytometry. A scratchâwound assay was conducted to investigate cell migration. Bioinformatics analysis using TargetScan 7.2 revealed the potential the target gene of microRNA (miR)â302dâ3p; a dual luciferase reporter assay determined the target gene. Suppression of miRâ302dâ3p increased the viability of cells, cell colony number and migration; CHONâ001 cell apoptosis was also inhibited. miRâ302dâ3p mimics decreased the luciferase activity of reporter plasmids containing the wild-type 3'âuntranslated region of Uncâ51âlike kinase 1 (ULK1). siULK1 decreased CHONâ001 cell viability and migration. Furthermore, siULK1 promoted the expression of phosphorylated IκÎα and p65, while miRâ302dâ3p inhibitor suppressed the expression of phosphorylated IκÎα and p65. Inhibition of miRâ302dâ3p could promote the proliferation and migration, and inhibit the apoptosis of chondrocytes, potentially by upregulating ULK1; thus, inflammation may be suppressed. The findings of the present study suggest miRâ302dâ3p and ULK1 as potential therapeutic targets for the prevention and treatment of OA.
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