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甲基化和转录因子YY1对非小细胞肺癌细胞中ID2表达的影响。

Effects of methylation and transcription factor YY1 on ID2 expression in non-small cell lung carcinoma cells.

作者信息

Tseng Yi-Hsin, Chou Wen-Ru, Liu Wei-Lun, Dung Zhong-Xuan, Lin Ching-Hao, Hsieh Chia-Hung, Wang Chi-Chung

机构信息

Graduate Institute of Biomedical and Pharmaceutical Science, Fu Jen Catholic University New Taipei, Taiwan.

Department of Internal Medicine, Fu Jen Catholic University Hospital, Fu Jen Catholic University New Taipei, Taiwan.

出版信息

Am J Cancer Res. 2024 May 15;14(5):2424-2438. doi: 10.62347/KXKL1421. eCollection 2024.

Abstract

The inhibitor of DNA-binding 2 (ID2) plays a major role in tumor dedifferentiation in non-small cell lung cancer (NSCLC). Studies have indicated an inverse correlation between ID2 expression and NSCLC cell invasiveness. However, the mechanisms through which ID2 activation is regulated are currently unclear. We overexpressed ID2 in H1299 cells and extensively characterized their cellular behaviors. By employing a serial deletion approach combined with a reporter assay, we pinpointed the basal promoter region of . We also examined the DNA methylation status of the promoter to elucidate the epigenetic mechanisms driving ID2 regulation. Our results revealed that ID2 overexpression effectively inhibited the migration, invasion, proliferation, and colony formation abilities of H1299 cells. The region from -243 to +202 played a major role in driving the transcriptional activity of . Sequence analysis results indicated that the transcription factor Yin Yang 1 (YY1) might be crucial in the regulation of ID2 expression. The ectopically expressed YY1 activated both the expression levels of ID2 and the transcriptional activity of the promoter, potentially contributing to its repressive activity on cancer cell growth. Furthermore, site-directed mutagenesis and chromatin immunoprecipitation assays revealed that YY1 may target the -120 and -76 sites of the promoter, thereby activating its transcriptional activity. The promoter regions were also fully methylated in CL1-5 cells, and the methylation level was correlated with the expression levels of the promoter. Moreover, the YY1-induced suppression of colony formation was counteracted by ID2 knockdown, which suggests that YY1 represses cell colony growth through the regulation of ID2. Our results indicate that YY1 plays a role in transactivating ID2 expression and might also contribute to the repression of colony growth through the regulation of ID2.

摘要

DNA结合抑制因子2(ID2)在非小细胞肺癌(NSCLC)的肿瘤去分化过程中起主要作用。研究表明ID2表达与NSCLC细胞侵袭性呈负相关。然而,目前尚不清楚ID2激活的调控机制。我们在H1299细胞中过表达ID2,并广泛表征了它们的细胞行为。通过采用串联缺失方法结合报告基因测定,我们确定了……的基础启动子区域。我们还检测了……启动子的DNA甲基化状态,以阐明驱动ID2调控的表观遗传机制。我们的结果表明,ID2过表达有效抑制了H1299细胞的迁移、侵袭、增殖和集落形成能力。-243至+202区域在驱动……的转录活性中起主要作用。序列分析结果表明,转录因子阴阳1(YY1)可能在ID2表达调控中起关键作用。异位表达的YY1激活了ID2的表达水平和……启动子的转录活性,可能有助于其对癌细胞生长的抑制活性。此外,定点诱变和染色质免疫沉淀试验表明,YY1可能靶向……启动子的-120和-76位点,从而激活其转录活性。在CL1-5细胞中,……启动子区域也完全甲基化,甲基化水平与……启动子的表达水平相关。此外,ID2敲低抵消了YY1诱导的集落形成抑制,这表明YY1通过调控ID2抑制细胞集落生长。我们的结果表明,YY1在反式激活ID2表达中起作用,也可能通过调控ID2对集落生长的抑制起作用。

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