Identification of potential genes regulated by DNA methyltransferase 3B in a hepatocellular carcinoma cell line by RNA interference and microarray analysis.

Jun Xu, Hong Fan, Zhu-Jiang Zhao, Jian-Qiong Zhang, Wei Xie
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Abstract

Whether DNA methyltransferase 3B (DNMT3B) is deregulated in hepatocellular carcinoma cell lines is still unclear. The expression levels of DNMT3B protein in normal liver cell line, pericacinoma cell line and hepatocellular carcinoma cell lines were compared by both Western blotting and immunocytochemistry. Long-term downregulated DNMT3B in a hepatocellular carcinoma cell line SMMC-7721 was achieved using a RNAi recombinant plasmid. The suppression of DNMT3B induced by RNA interference was confirmed using semi-quantitative RT-PCR and Western blotting. High throughput cDNA microarray was used to analyze the expression profiling of downstream genes of DNMT3B displayed in the treated cell lines and control. In the result,DNMT3B in hepatocellular carcinoma cell lines was expressed at a significantly higher level compared to those in pericacinoma cell line and normal liver cell line. A specific DNMT3B siRNA stably expressed from a plasmid vector effectively suppressed the expression of DNMT3B in SMMC-7721 cell line. By microarray analysis,26 downregulated genes and 115 upregulated genes have been identified in the DNMT3B knockdown cell line,including some important developmental genes and tumor-related genes such as SNCG, NOTCH1, MBD3, WNT11, MAOA and FACL4. The discovery showed DNMT3B was over-expressed in most hepatocellular carcinoma cell lines examined and may be linked to the carcinogenesis of hepatocytes. An array of candidate genes that are involved in the action of DNMT3B have been identified,including those related to development.

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通过RNA干扰和芯片分析鉴定肝癌细胞系中受DNA甲基转移酶3B调控的潜在基因
DNA甲基转移酶3B(DNMT3B)在肝癌细胞系中的表达是否失调尚不清楚。本研究采用 Western 印迹法和免疫细胞化学法比较了 DNMT3B 蛋白在正常肝细胞系、包膜癌细胞系和肝癌细胞系中的表达水平。利用 RNAi 重组质粒实现了肝癌细胞株 SMMC-7721 中 DNMT3B 的长期下调。半定量 RT-PCR 和 Western 印迹法证实了 RNA 干扰对 DNMT3B 的抑制作用。利用高通量 cDNA 芯片分析了处理过的细胞系和对照组中 DNMT3B 下游基因的表达谱。结果发现,肝癌细胞株中 DNMT3B 的表达水平明显高于包膜癌细胞株和正常肝细胞株。由质粒载体稳定表达的特异性 DNMT3B siRNA 能有效抑制 DNMT3B 在 SMMC-7721 细胞系中的表达。通过芯片分析,DNMT3B敲除细胞系中发现了26个下调基因和115个上调基因,包括一些重要的发育基因和肿瘤相关基因,如SNCG、NOTCH1、MBD3、WNT11、MAOA和FACL4。研究发现,DNMT3B在大多数肝癌细胞系中过度表达,可能与肝细胞癌变有关。研究还发现了一系列参与 DNMT3B 作用的候选基因,包括与发育相关的基因。
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