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Isolation of a novel member of small G protein superfamily and its expression in colon cancer

机译:小G蛋白超家族成员的分离及其在结肠癌中的表达

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AIM: APMCF1 is a novel human gene whose transcripts are up-regulated in apoptotic MCF-7 cells. In order to learn more about this gene's function in other tumors, we cloned its full length cDNA and prepared its polyclonal antibody to investigate its expression in colon cancers with immunohistochemistry. METHODS: With the method of 5′ rapid amplification of cDNA end (RACE) and EST assembled in GenBank, we extended the length of APMCF1 at 5′ end. Then the sequence encoding the APMCF1 protein was amplified by RT-PCR from the total RNA of apoptotic MCF-7 cells and cloned into the prokaryotic expression vector pGEX-KG to construct recombinant expression vector pGEX-APMCF1. The GST-APMCF1 fusion protein was expressed in E. coli and used to immunize rabbits to get the rabbit anti-APMCF1 serum. The specificity of polyclonal anti-APMCF1 antibody was determined by Western blot. Then we investigated the expression of Apmcf1 in colon cancers and normal colonic mucosa with immunohistochemistry. RESULTS: A cDNA fragment with a length of 1 745 bp was obtained. APMCF1 was mapped to chromosome 3q22.2 and spanned at least 14.8 kb of genomic DNA with seven exons and six introns contained. Bioinformatic analysis showed the protein encoded by APMCF1 contained a small GTP-binding protein (G proteins) domain and was homologous to mouse signal recognition particle receptor β(SRβ). A coding region covering 816 bp was cloned and polyclonal anti-APMCF1 antibody was prepared successfully. The immunohistochemistry study showed that APMCF1 had a strong expression in colon cancer. CONCLUSION: APMCF1 may be the gene coding human signal recognition particle receptor p and belongs to the small-G protein superfamily. Its strong expression pattern in colon cancer suggests it may play a role in colon cancer development.
机译:目的:APMCF1是一种新型的人类基因,其转录本在凋亡的MCF-7细胞中上调。为了更多地了解该基因在其他肿瘤中的功能,我们克隆了其全长cDNA,并制备了其多克隆抗体,以通过免疫组织化学研究其在结肠癌中的表达。方法:采用GenBank中5'快速扩增cDNA末端(RACE)和EST的方法,我们延长了5'末端APMCF1的长度。然后,通过RT-PCR从凋亡MCF-7细胞的总RNA中扩增编码APMCF1蛋白的序列,并将其克隆到原核表达载体pGEX-KG中,构建重组表达载体pGEX-APMCF1。 GST-APMCF1融合蛋白在大肠杆菌中表达,用于免疫兔以获得兔抗APMCF1血清。通过Western印迹确定多克隆抗APMCF1抗体的特异性。然后我们通过免疫组织化学研究了Apmcf1在结肠癌和正常结肠黏膜中的表达。结果:获得1 745 bp的cDNA片段。 APMCF1被定位到3q22.2染色体,并跨越至少14.8 kb的基因组DNA,其中包含七个外显子和六个内含子。生物信息学分析表明,APMCF1编码的蛋白质包含一个小的GTP结合蛋白(G蛋白)结构域,与小鼠信号识别颗粒受体β(SRβ)同源。克隆了一个覆盖816 bp的编码区,成功制备了多克隆抗APMCF1抗体。免疫组织化学研究表明,APMCF1在结肠癌中有很强的表达。结论:APMCF1可能是编码人信号识别颗粒受体p的基因,属于小G蛋白超家族。它在结肠癌中的强表达模式表明它可能在结肠癌的发展中起作用。

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