[No authors listed]
Burkitt lymphoma (BL) has a high mortality rate and its treatment is currently limited to chemotherapy combined with immunotherapy. The long nonâcoding RNA antisense nonâcoding RNA in the INK4 locus (ANRIL) has been identified as an oncogene that can regulate cell proliferation and apoptosis in multiple types of cancer. However, the function of ANRIL in BL remains unknown. The present study aimed to determine the effect of ANRIL on cell proliferation and apoptosis in BL. Reverse transcriptionâquantitative PCR was used to analyze the expression levels of ANRIL in BL cells. The effect of ANRIL knockdown on BL cells was determined using Cell Counting Kitâ8, flow cytometric, western blotting, immunofluorescence staining and Hoechst staining assays. The results revealed that ANRIL silencing inhibited the proliferation and promoted the apoptosis of BL cells. In addition, the expression levels of cyclin D1, E2F transcription factor 1 and Bclâ2 were downregulated, while the expression levels of cyclinâdependent kinase inhibitor 1A, Bclâ2âassociated X protein, cleavedâcaspaseâ9/proâcaspaseâ9 and cleavedâcaspaseâ3/proâcaspaseâ3 were upregulated. Furthermore, the knockdown of ANRIL activated the TGFâβ1 signaling pathway, as evidenced by the upregulated expression levels of TGFâβ1, phosphorylated (p)âSMAD2/3/SMAD2/3, pâSMAD1/SMAD1 and sphingosineâ1âphosphate receptor 2. Moreover, the protective effect of ANRIL silencing in BL could be inhibited by the TGFâβ receptor type I/II dual inhibitor, LY2109761. In conclusion, the findings of the present study suggested that the knockdown of ANRIL may inhibit cell proliferation and promote cell apoptosis in BL by regulating the TGFâβ1 signaling pathway, which may provide a novel target for the treatment of BL.
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