Bhattacharjya Sumana, Roy Kumar Singha, Ganguly Abira, Sarkar Shreya, Panda Chinmay K, Bhattacharyya Dibyendu, Bhattacharyya Nitai P, Roychoudhury Susanta
Cancer Biology and Inflammatory Disorder Division, Indian Institute of Chemical Biology, Council of Scientific and Industrial Research, 4, Raja S.C. Mullick Road, Kolkata, 700 032, India.
Tata Memorial Centre, ACTREC Sector 22, Navi Mumbai, Kharghar, 410210, India.
Mol Cancer. 2015 Feb 15;14:42. doi: 10.1186/s12943-015-0299-z.
Nucleoporins mediate nucleocytoplasmic exchange of macromolecules and several have been assigned active mitotic functions. Nucleoporins can participate in various mitotic functions like spindle assembly, kinetochore organisation and chromosome segregation- important for genome integrity. Pathways to genome integrity are frequently deregulated in cancer and many are regulated in part by microRNAs. Indeed, altered levels of numerous microRNAs have frequently been associated with tumorigenesis. Here, we unveil a microRNA-mediated regulation of the nucleoporin Nup214 and its downstream effect on genome integrity.
Databases/bioinformatic tools such as miRBase, Oncomine and RNAhybrid predicted Nup214 as a miR-133b target. To validate this, we used luciferase reporter assays, Real-Time PCR and immuno-blotting. Flow cytometry and immuno-blots of mitotic markers were used to analyse cell cycle pattern upon thymidine synchronization and miR-133b treatment. Mitotic indices and chromosomal abnormalities were assessed by immuno-fluorescence for FITC-tagged phospho-H3 as well as video-microscopy for GFP-tagged histone H4. Annexin V/propidium iodide staining, caspase3/PARP cleavage and colony formation assays were done to investigate cell death upon either miR-133b transfection or NUP214 knockdown by siRNA. UPCI:SCC084, HCT116, HeLa-H4-pEGFP and HEK293 (human oral squamous cell carcinoma, colorectal, cervical carcinomas and embryonic kidney cell lines, respectively) were used. miR-133b and NUP214 expressions were validated in cancer cell lines and tissues by Real-Time PCR.
Examination of head and neck tumour tissues and cancer cell lines revealed that Nup214 and miR-133b expressions are negatively correlated. In vitro, Nup214 was significantly downregulated by ectopic miR-133b. This downregulation elevated mitotic indices and delayed degradation of mitotic marker proteins cyclinB1 and cyclinA and dephosphorylation of H3. Moreover, this mitotic delay enhanced chromosomal abnormalities and apoptosis.
We have identified NUP214, a member of the massive nuclear pore complex, as a novel miR-133b target. Thus, we have shown a hitherto unknown microRNA regulation of mitosis mediated by a member of the nucleoporin family. Based on observations, we also raise some hypotheses regarding transport-dependent/independent functions of Nup214 in this study. Our results hence attempt to explain why miR-133b is generally downregulated in tumours and lay out the potential for Nup214 as a therapeutic target in the treatment of cancer.
核孔蛋白介导大分子的核质交换,其中一些已被赋予活跃的有丝分裂功能。核孔蛋白可参与多种有丝分裂功能,如纺锤体组装、动粒组织和染色体分离,这些对基因组完整性至关重要。通向基因组完整性的途径在癌症中经常失调,许多途径部分受微小RNA调控。事实上,许多微小RNA水平的改变经常与肿瘤发生相关。在此,我们揭示了微小RNA介导的核孔蛋白Nup214的调控及其对基因组完整性的下游影响。
利用miRBase、Oncomine和RNAhybrid等数据库/生物信息学工具预测Nup214为miR-133b的靶标。为验证这一点,我们使用了荧光素酶报告基因检测、实时定量聚合酶链反应和免疫印迹法。采用流式细胞术和有丝分裂标记物的免疫印迹法分析胸苷同步化和miR-133b处理后的细胞周期模式。通过免疫荧光检测FITC标记的磷酸化组蛋白H3以及通过视频显微镜检测GFP标记的组蛋白H4来评估有丝分裂指数和染色体异常。进行膜联蛋白V/碘化丙啶染色、半胱天冬酶3/聚(ADP-核糖)聚合酶切割和集落形成试验,以研究miR-133b转染或通过小干扰RNA敲低NUP214后的细胞死亡情况。分别使用UPCI:SCC084、HCT116、HeLa-H4-pEGFP和HEK293(分别为人口腔鳞状细胞癌、结直肠癌、宫颈癌和胚胎肾细胞系)。通过实时定量聚合酶链反应在癌细胞系和组织中验证miR-133b和NUP214的表达。
对头颈部肿瘤组织和癌细胞系的检测显示,Nup214和miR-133b的表达呈负相关。在体外,异位表达的miR-133b显著下调Nup214。这种下调提高了有丝分裂指数,延迟了有丝分裂标记蛋白细胞周期蛋白B1和细胞周期蛋白A的降解以及组蛋白H3的去磷酸化。此外,这种有丝分裂延迟增加了染色体异常和细胞凋亡。
我们已确定大型核孔复合体的成员NUP214是一种新的miR-133b靶标。因此,我们展示了核孔蛋白家族成员介导的一种迄今未知的微小RNA对有丝分裂的调控。基于观察结果,我们在本研究中还提出了一些关于Nup214的运输依赖性/非依赖性功能的假设。因此,我们的结果试图解释为什么miR-133b在肿瘤中通常下调,并阐明Nup214作为癌症治疗靶点的潜力。
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