PIWI相互作用RNA-13643通过促进PRMT1介导的GLI1甲基化作为一种新型致癌基因,从而促进甲状腺乳头状癌的发展。
PIWI interacting RNA-13643 contributes to papillary thyroid cancer development through acting as a novel oncogene by facilitating PRMT1 mediated GLI1 methylation.
作者信息
Zhang Zhongbo, Liu Ning
机构信息
Department of Pancreatic and Biliary Surgery, The First Affiliated Hospital of China Medical University, Shenyang 110001, China.
Department of Pancreatic and Biliary Surgery, The First Affiliated Hospital of China Medical University, Shenyang 110001, China.
出版信息
Biochim Biophys Acta Gen Subj. 2023 Nov;1867(11):130453. doi: 10.1016/j.bbagen.2023.130453. Epub 2023 Aug 30.
BACKGROUND
Recently, aberrant expression of PIWI-interacting RNAs (piRNAs) has been discovered in a variety of cancer cells. However, the roles of PIWI proteins and piRNAs in papillary thyroid carcinoma (PTC) are still elusive.
METHODS
RT-qPCR and Northern blotting were used to evaluate piR-13643 levels in PTC and para-carcinoma tissues, as well as in PTC cell lines. piR-13643 mimic and piR-13643 inhibitor were transfected into K-1 and B-CPAP cells. CCK-8, Transwell, annexin V-FITC/PI, flow cytometry and Western blot assays were performed to measure cell proliferation, invasion, apoptosis, cell cycle and E-cadherin and Vimentin proteins, respectively. Total RNA from B-CPAP cells was pulled down with PIWIL1, PIWIL2, or PIWIL3 specific antibodies or IgG as a control, respectively, followed by detection of piR-13643 expression with RT-qPCR. Immunoblotting of PRMT1 was detected in piR-13643 / PIWIL1 complex immune-precipitates by Co-IP assay. Subsequently, PRMT1 protein expression was detected by stably transfection of Flag tagged GLI1 (Flag-GLI1) into B-CPAP cells. Methylation assay with PRMT1 and wild-type or R597 lysine (R597K)-mutant GLI1. Then rescue experiments were applied to explore effects of piR-13643 and GLI1 on the malignant behavior of PTC cells. B-CPAP cells transfected with piR-13643 inhibitor were subcutaneously injected into nude mice to evaluate the effect of piR-13643 knockdown on the xenograft tumor growth of PTC.
RESULTS
piR-13643 was elevated in PTC patient specimens and cell lines. piR-13643 overexpression facilitated cell proliferation, invasion and Vimentin level, and restrained apoptosis and E-cadherin expression, whereas piR-13643 knockdown showed the opposite results. Mechanically, piR-13643 could bind to PIWIL1 to form the PIWIL1/piR-13643 complex, and PRMT1 enhanced GLI1 transcription by methylating GLI1 at R597. Further, PIWIL1/piR-13643 promoted PRMT1-mediated GLI1 methylation. GLI1 knockdown countered the effects of piR-13643 mimic on cell malignant behaviors. piR-13643 knockdown preeminently prevented the xenograft tumor growth of PTC in vivo.
CONCLUSIONS
This study confirmed that piR-13643 facilitates PTC malignant behaviors in vitro and in vivo by promoting PRMT1-mediated GLI1 methylation via forming a complex with PIWIL1, which may provide a novel insight for PTC treatment.
背景
最近,在多种癌细胞中发现了PIWI相互作用RNA(piRNA)的异常表达。然而,PIWI蛋白和piRNA在甲状腺乳头状癌(PTC)中的作用仍不清楚。
方法
采用RT-qPCR和Northern印迹法评估PTC组织、癌旁组织以及PTC细胞系中piR-13643的水平。将piR-13643模拟物和piR-13643抑制剂转染至K-1和B-CPAP细胞中。分别进行CCK-8、Transwell、膜联蛋白V-FITC/PI、流式细胞术和蛋白质印迹分析,以检测细胞增殖、侵袭、凋亡、细胞周期以及E-钙黏蛋白和波形蛋白的表达。分别用PIWIL1、PIWIL2或PIWIL3特异性抗体或IgG作为对照,从B-CPAP细胞中沉淀总RNA,随后用RT-qPCR检测piR-13643的表达。通过免疫共沉淀法检测piR-13643 / PIWIL1复合物免疫沉淀物中PRMT1的免疫印迹。随后,通过将Flag标记的GLI1(Flag-GLI1)稳定转染至B-CPAP细胞中,检测PRMT1蛋白表达。采用PRMT1与野生型或R597赖氨酸(R597K)突变型GLI1进行甲基化检测。然后进行拯救实验,以探究piR-13643和GLI1对PTC细胞恶性行为的影响。将转染了piR-13643抑制剂的B-CPAP细胞皮下注射到裸鼠体内,以评估piR-13643敲低对PTC异种移植瘤生长的影响。
结果
piR-信号通路643在PTC患者标本和细胞系中升高。piR-13643过表达促进细胞增殖、侵袭和波形蛋白水平,抑制凋亡和E-钙黏蛋白表达,而piR-13643敲低则显示出相反的结果。机制上,piR-13643可与PIWIL1结合形成PIWIL1/piR-13643复合物,PRMT1通过在R597处甲基化GLI1增强GLI1转录。此外,PIWIL1/piR-13643促进PRMT1介导的GLI1甲基化。GLI1敲低抵消了piR-13643模拟物对细胞恶性行为的影响。piR-13643敲低显著抑制了PTC在体内的异种移植瘤生长。
结论
本研究证实,piR-13643通过与PIWIL1形成复合物促进PRMT1介导的GLI1甲基化,从而在体外和体内促进PTC的恶性行为,这可能为PTC治疗提供新的思路。
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