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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 >Apoptosis-inducing effect of Caspase-3 over-expressed on gastric cancer cell line SGC7901
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Apoptosis-inducing effect of Caspase-3 over-expressed on gastric cancer cell line SGC7901

机译:过表达Caspase-3对胃癌细胞SGC7901的凋亡诱导作用

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To investigate the apoptosis-inducing effect of Caspases-3 expressed by constructed eukaryotic vector on gastric cancer cell line SGC7901.PCR was employed to amplify the sequences of both small and large subunits of Caspases-3. Its products were separately cloned into the Sma I site of pBluescript KS+ to generate both plasmids pBS/SS and pBS/LS. The small subunit fragment was excised from plasmid pBS/SS with BamH I and then inserted into the BamH I site of plasmid pBS/LS preceding that of the large subunit to yield plasmid pBS/Rev-Caspase-3. Rev-Caspase-3 cDNA was excised with Kpn I+Xba I and then subcloned into plasmid pcDNA3.1 (+) to construct Rev-Caspase-3 eukaryotic expression vector pcDNA/Rev-Caspase-3, which was used to transiently transfect SGC7901 cell line. Cell count, MTT assay and electron microscopy were used to confirm the antiproliferation and apoptosis-inducing effect of Rev-Caspase-3 expression on gastric cancer cells.Plasmid pBS/Rev-Caspase-3 and eukaryotic expression vector pcDNA/Rev-Caspase-3 were successfully constructed. SGC7901 cells were transiently transfected by either pcDNA/Rev-Caspase-3 or pcDNA3.1 (+) for 24, 48, 72, and 96 h respectively. Cell growth was measured by cell count and MTT assay. In cell count assay, the cell numbers were 1.8×106, 1.55×106, 2.0×106, and 3.1×106 in the experimental group and 2.5×106, 3.1×106, 4.0×106, and 5.7×106 in the control group at 24, 48, 72 and 96 h respectively. The growth of SGC7901 cells was suppressed by Rev-Caspase-3 in a time-dependent manner (P<0.05). The results of MTT assay were similar to that of cell count (P<0.05). The characteristics of apoptosis such as chromatin condensation, crescent formation and margination were seen and more obvious with time in the given-experimental period in the experimental group, but not easily observed in the control group.The expression of Rev-Caspase-3 by the apoptosis of gastric cancer cell line SGC7901, which may exhibit a potential way in gastric cancer gene therapy.
机译:为了研究构建的真核载体表达的Caspases-3对胃癌细胞SGC7901的凋亡诱导作用。采用PCR技术扩增Caspases-3的大小亚基。将其产物分别克隆到pBluescript KS +的Sma I位点,以生成质粒pBS / SS和pBS / LS。用BamHI将小亚基片段从质粒pBS / SS中切除,然后插入大亚基之前的质粒pBS / LS的BamHI位点,得到质粒pBS / Rev-Caspase-3。用Kpn I + Xba I切除Rev-Caspase-3 cDNA,然后亚克隆到质粒pcDNA3.1(+)中,构建Rev-Caspase-3真核表达载体pcDNA / Rev-Caspase-3,将其瞬时转染SGC7901。细胞系。用细胞计数,MTT法和电镜观察Rev-Caspase-3表达对胃癌细胞的抑制增殖和诱导凋亡作用。质粒pBS / Rev-Caspase-3和真核表达载体pcDNA / Rev-Caspase-3被成功建造。 SGC7901细胞分别被pcDNA / Rev-Caspase-3或pcDNA3.1(+)瞬时转染24、48、72和96 h。通过细胞计数和MTT测定法测量细胞生长。在细胞计数测定中,实验组的细胞数为1.8×106、1.55×106、2.0×106和3.1×106,对照组的细胞数为2.5×106、3.1×106、4.0×106和5.7×106分别在24、48、72和96小时。 Rev-Caspase-3抑制SGC7901细胞的生长呈时间依赖性(P <0.05)。 MTT法检测结果与细胞计数相似(P <0.05)。实验组在给定的实验期内可见染色质凝集,新月形形成和边缘化等凋亡特征,并随时间变化更明显,而对照组则不容易观察到。Rev-Caspase-3的表达胃癌细胞SGC7901的凋亡,可能在胃癌基因治疗中具有潜在的作用。

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