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Experimental Studies on PNP Suicide Gene Therapy of Hepatoma

机译:肝癌PNP自杀基因治疗的实验研究。

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To investigate the killing effect of PNP/MeP-dR suicide gene system on hepatoma cells, pcDNA3.0/PNP, an eukaryotic expression vector harboring E. coli PNP gene, was transfected into human hepatoma HepG2 cells by liposome-mediated method. A HepG2 cell line with stable PNP gene expression, HepG2/PNP, was established with presence of G418 selection. The cell growth curves were determined with trypan blue staining. The sensitivity of HepG2/PNP to MeP-dR and bystander effects were assayed by MTT and FCM methods. The enzymatic activity of the product of PNP gene was determined by HPLC method. The cytotoxic effects of MeP-dR on HepG2/PNP cells were obvious (IC_(50) =4. 5 μmol/L) and all HepG2/PNP cells were killed 4 days after the treatment with 100 μmol/L MeP-dR. In mixed cultures containing increasing percentages of HepG2/PNP cells, total population killing was demonstrated when HepG2/PNP cells accounted for as few as 5 % of all HepG2 cells 8 days after the treatment with 100 μmol MeP-dR. High-pressure liquid chromatography (HPLC) demonstrated that the PNP enzyme could convert MeP-dR into 6-MP. PNP/MeP-dR suicide gene system had an advantage over traditional suicide gene systems for hepatoma gene therapy. Our e results suggest that high-level bystander effects of this system result in significant anti-tumor responses to hepatoma gene therapy, especially in vivo.
机译:为了研究PNP / MeP-dR自杀基因系统对肝癌细胞的杀伤作用,通过脂质体介导的方法将携带大肠杆菌PNP基因的真核表达载体pcDNA3.0 / PNP转染到人肝癌细胞HepG2中。在存在G418选择的情况下,建立了具有稳定PNP基因表达的HepG2细胞系HepG2 / PNP。用锥虫蓝染色确定细胞生长曲线。通过MTT和FCM方法检测HepG2 / PNP对MeP-dR的敏感性和旁观者效应。通过HPLC法测定PNP基因产物的酶活性。 MeP-dR对HepG2 / PNP细胞具有明显的细胞毒性作用(IC_(50)= 4。5μmol/ L),用100μmol/ L MeP-dR处理4天后,所有HepG2 / PNP细胞均被杀死。在用100μmolMeP-dR处理8天后,当HepG2 / PNP细胞只占所有HepG2细胞的5%时,证明了总的群体杀死率在HepG2 / PNP细胞百分比增加的混合培养物中。高压液相色谱法(HPLC)证明PNP酶可以将MeP-dR转化为6-MP。在肝癌基因治疗中,PNP / MeP-dR自杀基因系统具有优于传统自杀基因系统的优势。我们的研究结果表明,该系统的高水平旁观者效应导致对肝癌基因治疗(尤其是体内)的显着抗肿瘤反应。

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