实时荧光定量RT-PCR技术检测siRNA对HBV复制的干扰效果

目的运用实时荧光定量RT-PCR的方法,检测小RNA分子(small interfering RNAs,siRNA)对乙型肝炎病毒(hepatitis B virus,HBV)复制的抑制作用。方法在HepG2.2.15细胞内导入筛选的三条特异抗HBV的siRNA分子,用实时荧光定量RT-PCR的方法,检测干扰后HBV的mRNA表达水平。结果导入特异siRNA分子的细胞中HBV的mRNA表达量明显降低。结论实时荧光定量RT-PCR技术能准确可靠的检测mRNA的表达水平,对siRNA分子干扰效果的评价有很好的应用价值。

Effects of grafting cell penetrate peptide and RGD on endocytosis and biological effects of Mg-CaPNPs-CKIP-1 siRNA carrier system in vitro

Calcium phosphate nanoparticles(CaPNPs)have good biocompatibility as gene carriers;however,CaPNPs typically exhibit a low transfection efficiency.Cell penetrate peptide(TAT)can increase the uptake of nanoparticles but is limited by its non-specificity.Grafting adhesion peptide adhesion peptide on carriers can enhance their targeting.The Plekho1 gene encodes casein kinase-2 interacting protein-1(CKIP-1),which can negatively regulate osteogenic differentiation.Based on the above,we produced a Mg-CaPNPs-RGD-TAT-CKIP-1 siRNA carrier system via hydrothermal synthesis,silanization and adsorption.The effects of this carrier system on cell endocytosis and biological effects were evaluated by cell culture in vitro.The results demonstrate that CaPNPs with 7%Mg(60 nm particle size,short rod shape and good dispersion)were suitable for use as gene carriers.The carrier system boosted the endocytosis of MG63 cells and was helpful for promoting the differentiation of osteoblasts,and the dual-ligand system possessed a synergistic effect.The findings of this study show the tremendous potential of the Mg-CaPNPs-RGD-TAT-CKIP-1 siRNA carrier system for efficient delivery into cells and osteogenesis inducement.

抑制TUBA1C的过表达在卵巢癌细胞株CAOV3、SKOV3细胞增殖侵袭中的作用机制探讨

目的探讨抑制α-微管蛋白特异性1C链(TUBA1C)过表达对卵巢癌细胞株CAOV3、SKOV3细胞增殖、侵袭的影响,初步阐明TUBA1C在上皮性卵巢癌中的作用机制。方法通过脂质体介导抑制TUBA1C基因的过表达质粒转染CAOV3、SKOV3细胞,CAOV3分为3组:CAOV3实验组、CAOV3空载体转染组和CAOV3空白对照组;SKOV3分为3组:SKOV3实验组、SKOV3空载体转染组和SKOV3空白对照组。采用RT-PCR法检测TUBA1C表达;CCK-8法及Transwell小室体外侵袭实验评价TUBA1C基因抑制后对卵巢癌细胞增殖、侵袭的影响。结果靶向TUBA1C基因的siRNA明显、特异性地抑制TUBA1C mRNA的表达水平;培养72h CAOV3实验组细胞增殖能力较空载体转染组和空白对照组明显降低,差异有统计学意义(P<0.05);侵袭实验结果提示SKOV3实验组穿膜细胞数量为(0.95±0.12)个/视野,较空载体转染组降低,差异有统计学意义(P<0.01),CAOV3实验组穿膜细胞数量为(1.13±0.14)个/视野,较空白对照组降低.但差异无统计学意义(P>0.05)。结论抑制TUBA1C基因过表达可抑制CAOV3、SKOV3细胞的增殖、侵袭能力,有望成为卵巢癌治疗的新靶点。

7-difluoromethoxyl-5,4'-di-n-octylgenistein inhibits growth of gastric cancer cells through downregulating forkhead box M1

AIM: To investigate whether the 7-difluoromethoxyl-5, 4'-di-n-octylgenistein (DFOG), a novel synthetic genistein analogue, affects the growth of gastric cancer cells and its mechanisms. METHODS: A series of genistein analogues were prepared by difluoromethylation and alkylation, and human gastric cancer cell lines AGS and SGC-7901 cultured in vitro were treated with various concentrations of genistein and genistein analogues. The cell viability was measured by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay. The cells were incubated by DFOG at different concentrations. The growth inhibitory effects were evaluated using MTT and clonogenic assay. The distribution of the phase in cell cycle was analyzed using flow cytometric analysis with propidium iodide staining. The expression of the transcription factor forkhead box M1 (FOXM1) was analyzed by reverse transcription-polymerase chain reaction and Western blotting. The expression levelsof CDK1, Cdc25B, cyclin B and p27KIP1 protein were detected using Western blotting. RESULTS: Nine of the genistein analogues had more effective antitumor activity than genistein. Among the tested analogues, DFOG possessed the strongest activity against AGS and SGC-7901 cells in vitro. DFOG significantly inhibited the cell viability and colony formation of AGS and SGC-7901 cells. Moreover, DFOG efficaciously arrested the cell cycle in G2/M phase. DFOG decreased the expression of FOXM1 and its downstream genes, such as CDK1, Cdc25B, cyclin B, and increased p27KIP1 at protein levels. Knockdown of FOXM1 by small interfering RNA before DFOG treatment resulted in enhanced cell growth inhibition in AGS cells. Up-regulation of FOXM1 by cDNA transfection attenuated DFOG-induced cell growth inhibition in AGS cells. CONCLUSION: DFOG inhibits the growth of human gastric cancer cells by down-regulating the FOXM1 expression.

COX-2 silencing inhibits cell proliferation in A549 cell

Objective: The aim of this study was to explore the effects on malignant proliferation of A549 cell by silencing cy-clooxygenase (COX)-2. Methods: In the present study, we constructed three siRNA vectors producing small interference RNA. The siRNA vectors and the vacant vectors were transfected into A549 cell with lipofectamine respectively and the transfected cell strains were constructed. The change of COX-2 expression levels was examined by Western blot and RT-PCR. The effects on the proliferation of lung cancer cells were studied by cell growth curve, clonogenic assay and xenograft assays. Results: The siRNA expression vectors produced marked effects in A549 cell but the inhibited effects were different. The effect of psi-10 was best and the mRNA and protein levels of COX-2 reduced 61.2% and 56.2% respectively in A549-si10 cell in contrast to the control. The growth of A549 cell slowed and the colony formation rate reduced after silencing COX-2. In xenograft assays, the growth speeds of tumor became slow and the numbers of tumor reduced after silencing COX-2. Conclusion: The si10 target of COX-2 has the best silencing effect in A549 cell and the best inhibition effect on malignant proliferation of A549 cell in vivo and in vitro.