The Aurora kinases A and B control tumorigenesis by inhibiting apoptosis and promoting proliferation and metastasis, however, it remains unknown whether Aurora A and B overexpressed concomitantly and its clinical significance in hepatocellular carcinoma (HCC). Here, we obsearved Aurora A and B tended to overexpress parallelly on protein level (r = 0.8679, P < 0.0001) and their co-overexpression (Aurora AHBH), associated with the worst prognosis, was an independent predictor for the survival. Importantly, with the lower IC50 and stronger anti-tumor effect than selective inhibitors, SNS-314, the pan-inhibitor of Aurora kinases, which induced YAP (Yes-associated protein) reduction and resulted in P21 accumulation, significantly promoted the polyploidy (> 4N) formation and apoptosis in HCC. High YAP expression (YAPH) was associated with Aurora AHBH, and appeared to be an independent predictor for survival, but P21 not. Moreover, silencing YAP also induced P21 accumulation, and knockdown P21, which enhanced YAP accumulation and weakened the SNS-314-induced YAP reduction, impaired SNS-314-induced apoptosis. Therefore, P21 enhanced the apoptotic effect of SNS-314 in HCC. Taken together, our findings indicated Aurora kinases/YAP/P21 was an oncogenic signaling axis in HCC, and revealed targeting Aurora AHBH induced apoptosis by YAP suppression. Our results also provided a solid evidence for SNS-314 as a potential targeted therapy, and a proof-of-concept evidence for a possible combined therapy of SNS-314 plus Hippo pathway inhibitors on HCC.
Background:
MicroRNAs have recently been recognized to be engaged in the development of bone
diseases.
Objective:
This study was performed to elucidate the effects of miR-144-3p on proliferation and osteogenesis of
mesenchymal stem cells (MSCs) from the patients with steroid-associated osteonecrosis (ONFH) and its related
mechanism.
Method:
The expression level of miR-144-3p in the MSCs from the proximal femur of the patients was examined
by Real-time PCR. The cell proliferation ability was assayed by MTT. The differentiation ability of MSCs was
assayed by Alizarin Red S (ARS) staining. The interaction between miR-144-3p and frizzled4 (FZD4) was investigated
by Real-time PCR, western blot and luciferase reporter assay.
Results:
ONFH samples had the obviously high expression of miR-144-3p compared to the control. MiR-144-3p
had a negative effect on the proliferation and osteogenesis of MSCs. Via targeting FZD4, miR-144-3p decreased
β-catenin nuclear translocation, the transcription of RUNX2 and COL1A1. Over-expression of FZD4 partially
reversed miR-144-3p-induced decrease in the proliferation and osteogenesis of MSCs.
Conclusion:
MiR-144-3p might play an important role in the development of ONFH and might be used as a
novel class of therapeutic targets for this disease.
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