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应用一种高度特异且可重复的cDNA代表性差异分析方法克隆人胃癌细胞中大蒜上调基因。

Applying a highly specific and reproducible cDNA RDA method to clone garlic up-regulated genes in human gastric cancer cells.

作者信息

Li Yong, Lu You-Yong

机构信息

Beijing Institute for Cancer Research, Beijing Laboratory of Molecular Oncology, School of Oncology, Peking University, 1 Da-Hong-Luo-Chang Street, Western District, Beijing 100034, China.

出版信息

World J Gastroenterol. 2002 Apr;8(2):213-6. doi: 10.3748/wjg.v8.i2.213.

Abstract

AIM

To develop and optimize cDNA representational difference analysis (cDNA RDA) method and to identify and clone garlic up-regulated genes in human gastric cancer (HGC) cells.

METHODS

We performed cDNA RDA method by using abundant double-stranded cDNA messages provided by two self-constructed cDNA libraries (Allitridi-treated and paternal HGC cell line BGC823 cells cDNA libraries respectively). Bam H I and Xho I restriction sites harbored in the library vector were used to select representations. Northern and Slot blots analyses were employed to identify the obtained difference products.

RESULTS

Fragments released from the cDNA library vector after restriction endonuclease digestion acted as good marker indicating the appropriate digestion degree for library DNA. Two novel expressed sequence tags (ESTs) and a recombinant gene were obtained. Slot blots result showed a 8-fold increase of glia-derived nexin/protease nexin 1 (GDN/PN1) gene expression level and 4-fold increase of hepatitis B virus x-interacting protein (XIP) mRNA level in BGC823 cells after Allitridi treatment for 72h.

CONCLUSION

Elevated levels of GDN/PN1 and XIP mRNAs induced by Allitridi provide valuable molecular evidence for elucidating the garlic's efficacies against neurodegenerative and inflammatory diseases. Isolation of a recombinant gene and two novel ESTs further show cDNA RDA based on cDNA libraries to be a powerful method with high specificity and reproducibility in cloning differentially expressed genes.

摘要

目的

开发并优化cDNA代表性差异分析(cDNA RDA)方法,以鉴定和克隆人胃癌(HGC)细胞中大蒜上调基因。

方法

我们利用两个自行构建的cDNA文库(分别为大蒜素处理的和父本HGC细胞系BGC823细胞的cDNA文库)提供的丰富双链cDNA信息进行cDNA RDA方法。文库载体中含有的Bam H I和Xho I限制性酶切位点用于选择代表性片段。采用Northern和斑点印迹分析来鉴定获得的差异产物。

结果

限制性内切酶消化后从cDNA文库载体释放的片段可作为良好标记,表明文库DNA的消化程度合适。获得了两个新的表达序列标签(EST)和一个重组基因。斑点印迹结果显示,大蒜素处理72小时后,BGC823细胞中神经胶质衍生的神经连接蛋白/蛋白酶神经连接蛋白1(GDN/PN1)基因表达水平增加8倍,乙型肝炎病毒x相互作用蛋白(XIP)mRNA水平增加4倍。

结论

大蒜素诱导的GDN/PN1和XIP mRNA水平升高为阐明大蒜对神经退行性疾病和炎症性疾病的疗效提供了有价值的分子证据。重组基因和两个新EST的分离进一步表明,基于cDNA文库的cDNA RDA是一种在克隆差异表达基因方面具有高特异性和可重复性的强大方法。

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