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Gene expression profiles of hepatoma cell line BEL-7402.

机译:肝癌细胞系BEL-7402的基因表达谱。

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BACKGROUND/AIMS: To investigate the gene expression of cancer related genes in hepatoma cell line BEL-7402 through the usage of Atlas Human Cancer Array with 588 well-characterized human genes related with cancer biology. METHODOLOGY: Hybridization of cDNA membrane was performed with 32P-labeled cDNA probes synthesized from RNA isolated from Human hepatoma cell line BEL-7402 and non-cirrhotic normal liver which was liver transplantation donor. Bioinformatics was used to analyze the result. The reverse transcription polymerase chain reaction of 24 pairs of specimens and northern blot of 4 pairs of specimens were used to confirm the expression pattern of some genes identified by Atlas arrays hybridization. RESULTS: The differential expression cell cycle/growth regulator in hepatoma cell line BEL-7402 showed a stronger tendency toward cell proliferation with up-regulation of E2F-3 and TFDP-2. The anti-apoptotic factors such as Akt-1 were up-regulated. Whereas the promotive genes of apoptosis were down-regulated, such as BAK and caspase-3. Besides this, some genes were up-regulated, such as Integrin beta 8, DNA-PK, CSPCP, cyclin C etc. A number of genes were down-regulated, which included LAR, ABL2, SKY, TDGF1 etc. In general, expression of the cancer progression genes were up-regulated, while expression of anti-cancer progression genes were down-regulated. The results of reverse transcription polymerase chain reaction of 24 pairs of specimens and Northern Blot of 4 pairs of specimens were consistent with the expression pattern of some genes identified by Atals arrays hybridization. CONCLUSIONS: Investigation of gene expression profile of hepatoma cell line BEL-7402 should help to disclose the molecular mechanism of the onset, progression and prognosis of hepatocellular carcinoma. The quick and high-throughout method of profiling gene expression by cDNA array provides us with an overview of key factors that may be involved in hepatocellular carcinoma, and may find the clue to the study of hepatocellular carcinoma carcinogenesis and molecular targets of diagnosis and therapy.
机译:背景/目的:通过将Atlas人类癌症阵列与588个与癌症生物学相关的特征明确的人类基因一起使用,来研究肝癌细胞系BEL-7402中癌症相关基因的基因表达。方法:将32P标记的cDNA探针与cDNA膜杂交,该探针是从人肝癌细胞BEL-7402和非肝硬化正常肝脏(其是肝移植供体)分离的RNA中合成的。生物信息学被用来分析结果。用24对标本的逆转录聚合酶链反应和4对标本的northern印迹法证实了通过Atlas阵列杂交鉴定的一些基因的表达模式。结果:肝癌细胞BEL-7402中的差异表达细胞周期/生长调节剂随着E2F-3和TFDP-2的上调显示出更强的细胞增殖趋势。抗凋亡因子如Akt-1被上调。而凋亡的促进基因例如BAK和caspase-3被下调。除此之外,一些基因被上调,例如整合素β8,DNA-PK,CSPCP,细胞周期蛋白C等。许多基因被下调,包括LAR,ABL2,SKY,TDGF1等。癌进展基因的表达被上调,而抗癌进展基因的表达被下调。 24对标本的逆转录聚合酶链反应和4对标本的Northern Blot结果与通过Atals阵列杂交鉴定的某些基因的表达模式一致。结论:对肝癌细胞系BEL-7402基因表达谱的研究应有助于揭示肝细胞癌发病,进展和预后的分子机制。通过cDNA阵列分析基因表达的快速,高通量方法为我们提供了可能与肝细胞癌有关的关键因素的概述,并可能为研究肝细胞癌的发生,诊断和治疗的分子靶点提供线索。

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