首页> 外文会议>The 2nd International Conference on Bioinformatics and Biomedical Engineering(iCBBE 2008)(第二届生物信息与生物医学工程国际会议)论文集 >Expression analysis of signal transducer and activator of transcription 2 (stat2) gene in esophageal, gastric and lung cancer tissues
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Expression analysis of signal transducer and activator of transcription 2 (stat2) gene in esophageal, gastric and lung cancer tissues

机译:信号转导子和转录激活因子2(stat2)基因在食管,胃和肺癌组织中的表达分析

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To further investigate the molecular mechanism of esophageal carcinogenesis, screen out and validate the genes expressed differently in esophageal cancer. mRNA differential display (DD-PCR) was employed to search differently expressed fragments, some of which were cloned and sequenced. By homology analysis in GenBank, corresponding homologous genes of those fragments were found. The corresponding genes of those differently expressed fragments were validated by Real-time quantitative PCR. By DD-PCR, one EST was identified to be Homo sapiens signal transducer and activator of transcription 2 (stat2) gene. The mRNA analysis result by real-time quantitative PCR showed that the expression level of stat2 gene in esophageal cancer (n=16, p<0.05), gastric cancer (n=12, p<0.05) and lung cancer tissues (n=16, p<0.05) were significantly higher than that in normal tissues. The ORF of stat2 gene was 2556 base pair long and encodes 852 amino acids. The molecular weight was about 97.9KD. The over-expression of stat2 gene in esophageal cancer, gastric cancer and lung cancer may indicate an important role in these carcinogenesis.
机译:为了进一步研究食管癌变的分子机制,筛选并验证在食管癌中表达不同的基因。 mRNA差异显示(DD-PCR)用于搜索不同表达的片段,其中一些片段已克隆并测序。通过GenBank中的同源性分析,发现了那些片段的相应同源基因。通过实时定量PCR验证那些不同表达的片段的相应基因。通过DD-PCR,一个EST被鉴定为智人信号转导子和转录激活子2(stat2)基因。实时定量PCR的mRNA分析结果表明,stat2基因在食管癌(n = 16,p <0.05),胃癌(n = 12,p <0.05)和肺癌组织(n = 16)中的表达水平,p <0.05)显着高于正常组织。 stat2基因的ORF长2556个碱基对,编码852个氨基酸。分子量约为97.9KD。 stat2基因在食管癌,胃癌和肺癌中的过度表达可能表明在这些致癌作用中的重要作用。

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