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Expression of Dnmt1 demethylase MeCP2 and methylation of tumor-related genes in human gastric cancer

机译:人胃癌中Dnmt1脱甲基酶MeCP2的表达及肿瘤相关基因的甲基化

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摘要

AIM: To explore the effect of DNA methyltransferase, demethylase and methyl-CpG binding protein MeCP2 on the expressions and methylation of hMSH2 and proto-oncogene in human gastric cancer.METHODS: Paired samples of primary gastric cancer and corresponding para-cancerous, non-cancerous gastric mucosae were obtained from surgically resected specimens of 28 patients. Transcription levels of Dnmt1, mbd2, MeCP2, p16INK4A, hMSH2 and c-myc were detected by using real-time PCR or RT-PCR. Promoter methylation of p16INK4A, c-myc and hMSH2 genes was assayed by methylation-specific PCR (MSP) and sequencing (mapping). Their relationships were analyzed by Fisher’s exact test using the software SPSS.RESULTS: The average mRNA level of Dnmt1 gene from cancerous tissue was higher and that of mbd2 gene from cancerous tissue was lower than that from non-cancerous tissue, respectively. mbd2 was lower in cancerous tissue than in non-cancerous tissue in 14 (50.0%) of patients but higher in 3 cases (10.7%) of non-cancerous gastric tissue (P < 0.001). c-myc expression was up-regulated in cancer tissues (P < 0.05). The up-regulation of mbd2 was found in all patients with hypomethylated c-myc. The transcriptional levels of p16INK4A and MeCP2 genes did not display any difference between gastric cancerous and matched non-cancerous tissues. There were down-regulation and hypermethylation of hMSH2 in cancer tissues, and the hypermethylation of hMSH2 coexisted with down-regulated transcription. However, the transcription level of the above genes was not associated with biological behaviours of gastric cancers.CONCLUSION: The up-regulation of proto-oncogene may be the consequence of epigenetic control of gene expression by demethylase, and mbd2 is involved in the regulation of hMSH2 expression in human gastric cancer.
机译:目的:探讨DNA甲基转移酶,脱甲基酶和甲基CpG结合蛋白MeCP2对人胃癌中hMSH2和原癌基因的表达和甲基化的影响。从28例患者的手术切除标本中获得了癌性胃粘膜。通过实时PCR或RT-PCR检测Dnmt1,mbd2,MeCP2,p16 INK4A ,hMSH2和c-myc的转录水平。 p16 INK4A ,c-myc和hMSH2基因的启动子甲基化通过甲基化特异性PCR(MSP)和测序(作图)进行检测。结果:与非癌组织相比,癌组织中Dnmt1基因的平均mRNA水平较高,而癌组织中mbd2基因的平均mRNA水平则低于非癌组织。癌组织中的mbd2低于非癌组织中的mbd2(14.5%),但3例癌组织中的mbd2(10.7%)更高(P <0.001)。癌组织中c-myc表达上调(P <0.05)。在所有甲基化程度较低的c-myc患者中发现mbd2上调。 p16 INK4A 和MeCP2基因的转录水平在胃癌组织和匹配的非癌组织之间无差异。在癌组织中存在hMSH2的下调和甲基化,并且hMSH2的高甲基化与转录下调共存。结论:上述基因的转录水平与胃癌的生物学行为无关。结论:原癌基因的上调可能是脱甲基酶对基因表达进行表观遗传控制的结果,而mbd2参与了胃癌的调控。 hMSH2在人胃癌中的表达。

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