The study of anti-hepatitis drug dimethyl dicarboxylate biphenyl on invasion of human hepatocellular carcinoma MHCC97-H cells and its active mechanisms

Objective： To assess the anti-invasive effect of DDB and its possible active mechanism in human hepatocellular carcinoma MHCC97-H with high metastasis potential. Methods： MTT assay was used to evaluate the cytotoxicity of DDB to MHCC97-H cells and the anti-adhesion of DDB on MHCC97-H cells to laminin （LN） and fibronectin （FN）. The anti-invasive effect of DDB was detected by the transwell chamber experiment. VEGF, nm23-H1 and uPAR mRNA transcriptions were determined by RT-PCR assay. The secretion and expression of a-fetal protein （AFP） were analyzed by ELISA and flow cytometry, respectively. Results： DDB at non-cytotoxic concentrations （10, 50 and 100 μmol/L） obviously inhibited the adhesion of MHCC97-H on LN and FN. In the transwell chamber experiment, the inhibition rates of the invasion of DDB 50 and 100 μmol/L on MHCC97-H cells were 25.8% and 32.3%, respectively. By RT-PCR assay, DDB 50 and 100 μmol/L decreased VEGF, nm23-H1 and uPAR mRNA expressions in MHCC97-H cells. The ELISA assay showed that 50, 100 and 200 μmol/L DDB decreased the AFP secretion of MHCC97-H cells, the inhibitory rates were 16.5%, 17.5% and 48.5%, respectively. DDB also decreased the expression of AFP in MHCC97-H cells by flow cytometry assay. Conclusion： DDB, an anti-hepatitis drug, at non-cytotoxic concentrations showed significant anti-invasion effect in human hepatocellular carcinoma MHCC97-H cells, and the inhibition of VEGF, nm23-H1 and uPAR expression should contribute to the anti-invasion property of DDB.

Anti-angiogenesis effect of melittin on Mock/MHCC97-H cells by the regulation of cathepsin S in vivo

Objective： To study the anti-angiogenesis effect of melittin on human hepatoma Mock/MHCC97-H cells by regulatingthe expression of cathepsin S （CatS） in vivo. Methods： Models of in situ transplantation tumor of Mock/MHCC97-Hcells and silencing cathepsin shRNA-CatS/ MHCC97-H cells in nude mice were established. The model mice wererandomly divided into four groups. In the A1 group, the mice were inoculated with shRNA-CatS/MHCC97-H cells andtreated with melittin. In the A2 group, the mice were inoculated with shRNA-CatS/MHCC97-H cells and treated withsaline. In the B1 group, the mice were inoculated with Mock/MHCC97-H cells and treated with melittin. In the B2 group,the mice were inoculated with Mock/MHCC97-H cells and treated with saline. The A1 and B1 group were injected withmelittin （80 mg/kg） intraperitoneally every day. The A2 and B2 group were injected with 0.2 mL normal salineintraperitoneally every day. After administration for 25 days, the animals were sacrificed. The tumor size and weight innude mice in each group were recorded. The expression of CD34 protein in the xenograft tumor tissues was detected byimmunohistochemistry. The expression of Cat S, VEGF-A, p-VEGFR2, Ras, Raf, p-Raf, MEK1, p-MEK1, ERK1/2 andp-ERK1/2 proteins were detected by western blot. Results： The B1 group had significantly smaller tumor volumes andlower tumor weights than the B2 group （both P 〈 0.001）. There was no significant difference between the A1 group andA2 group in tumor volumes and weights. The number of CD34-positive microvessels in the B2 group was significantlyhigher than that in the A2 group （P 〈 0.001）. The number of CD34-positive microvessels in the B1 group wassignificantly lesser than that in the A1 group （P 〈 0.001）. Most strikingly, in the model featuring inoculation ofMock/MHCC97-H cells, CatS, VEGF-A, p-VEGFR2, Ras, Raf, p-Raf, MEK1, p-MEK1, ERK1/2 and p-ERK1/2expression were inhibited when treated with melittin. However, in the model featuring the inoculation ofshRNA-CatS/MHCC97-H cells, no such effects were observed with similar treatments. Conclusion： Melittin can inhibitthe growth of tumors and angiogenesis by blocking the CatS-VEGf-A signaling pathway.

舒芬太尼调控miR-1抑制肝癌细胞MHCC97-H增殖、侵袭和迁移的机制研究

目的探讨舒芬太尼调控微小RNA-1(miR-1)表达对人肝癌MHCC97-H细胞增殖、侵袭和迁移的影响及其机制。方法本研究起止时间为2018年3月至2019年9月,采用细胞计数试剂盒(CCK-8)实验检测不同浓度的舒芬太尼对人肝癌MHCC97-H细胞活力的影响,q RT-PCR检测舒芬太尼对MHCC97-H细胞中miR-1表达的影响;通过脂质体转染法将miR-1抑制剂(inhibitor)及阴性对照转染至MHCC97-H细胞,实验分为Control组、舒芬太尼(Sufentanil)组、转染对照(Sufentanil+NC)组和转染(Sufentanil+miR-1)组。细胞计数试剂盒(CCK-8)实验检测各组MHCC97-H细胞增殖能力,Transwell实验检测各组MHCC97-H细胞侵袭能力,划痕实验检测各组MHCC97-H细胞迁移能力,蛋白质印迹法(Western blotting)检测各组MHCC97-H细胞中基质金属蛋白酶-2(MMP-2)和基质金属蛋白酶-9(MMP-9)蛋白表达情况。结果不同浓度的舒芬太尼对肝癌MHCC97-H细胞活力具有不同程度的抑制作用;与Control组比,Sufentanil组MHCC97-H细胞中miR-1的表达[(1.00±0.09)比(2.25±0.24)]明显升高(P<0.05),细胞增殖[(0.54±0.05)比(0.34±0.03)]、侵袭[(106.24±8.25)个比(51.34±5.02)个]和迁移能力[(37.36±4.01)%比(16.34±1.72)%]降低(P<0.05),MMP-2[(0.33±0.04)比(0.15±0.02)]和MMP-9[(0.24±0.02)比(0.11±0.01)]的表达下调(P<0.05);与Sufentanil+NC组比,Sufentanil+miR-1组MHCC97-H细胞中miR-1的表达[(2.20±0.21)比(1.42±0.15)]明显降低(P<0.05),细胞增殖[(0.32±0.03)比(0.46±0.04)]、侵袭[(52.36±5.14)个比(91.16±6.06)个]和迁移能力[(17.11±1.71)%比(29.85±3.10)%]升高(P<0.05),MMP-2[(0.15±0.02)比(0.27±0.02)]和MMP-9[(0.13±0.01)比(0.19±0.02)]的表达上调(P<0.05)。结论舒芬太尼可通过调控miR-1的表达抑制人肝癌MHCC97-H细胞的增殖、侵袭和迁移,其机制可能与调控MMP-2和MMP-9表达有关。

Thy-1通过调控Notch1通路促进肝癌细胞EMT进程

目的:探索细胞表面抗原Thy-1通过调控Notch1通路促进肝癌HepG2和MHCC-97细胞上皮间质转化(EMT)。方法:选用具有高转移特性的MHCC-97细胞和低转移特性的HepG2细胞作为研究对象,WB检测细胞内Thy-1、Notch1蛋白表达水平。用重组慢病毒转染MHCC-97和HepG2细胞,构建高表达与低表达Thy-1蛋白的细胞,再分别用Notch1激动剂rhNF-κB(1gsu/ml)和Notch1抑制剂MW167(100μmol/L)处理细胞24 h。Transwell实验检测Thy-1表达变化、rhNF-κB和MW167处理对细胞侵袭能力的影响,qPCR检测对Notch1 mRNA表达的影响,WB实验检测细胞内EMT相关蛋白表达的影响。结果:MHCC-97细胞中Thy-1、Notch1蛋白表达量均高于HepG2细胞(P<0.05)。成功构建Thy-1过表达的HepG2细胞和Thy-1低表达的MHCC-97细胞。与亲本HepG2细胞相比,Thy-1过表达HepG2细胞侵袭能力显著增强[(475.78±80.37)vs(183.23±55.34)个,P<0.05)]、波形蛋白表达显著升高(P<0.05)、上皮钙黏素蛋白表达显著降低(P<0.05)、Notch1 mRNA表达水平显著升高(P<0.05);与亲本MHCC-97细胞相比,Thy-1沉默的MHCC-97细胞侵袭能力显著降低[(237.44±62.18)vs(543.56±77.94)个,P<0.05)]、波形蛋白表达显著降低(P<0.05)、上皮钙黏素蛋白表达显著升高(P<0.05)、Notch1 mRNA表达水平显著降低(P<0.05)。而Notch1激活剂或抑制剂处理上述肝癌细胞可逆转由于Thy-1沉默或过表达所造成的改变。结论:Thy-1可通过调控Notch1表达影响肝癌HepG2和MHCC-97细胞的EMT。

臭牡丹含药血清通过PI3K/Akt信号通路对肝癌细胞的影响

目的:从磷脂酰肌醇3-激酶(PI3K)/丝氨酸苏氨酸蛋白激酶(Akt)信号通路角度探讨臭牡丹含药血清对肝癌MHCC97-H细胞的影响及可能的机制。方法:臭牡丹15%含药血清作用于MHCC97-H细胞,细胞增殖/毒性法(CCK-8)观察臭牡丹含药血清对细胞增殖的影响,以筛选最佳作用时间和浓度;Annexin V-FITC/碘化丙啶(PI)双染法检测细胞凋亡;蛋白免疫印迹法(Western blot)检测臭牡丹含药血清作用于细胞72 h后对PI3K/Akt信号通路中关键蛋白中第10号染色体缺失的磷酸酶及张力蛋白同源的基因(PTEN),磷酸化Akt(p-Akt)和磷脂酰肌醇3-激酶(PI3K)蛋白表达的影响;实时荧光定量聚合酶链式反应(Real-time PCR)检测臭牡丹含药血清作用于细胞72 h后对核转录因子-κB(NF-κB)和肿瘤坏死因子-α(TNF-α)mRNA表达的影响。结果:CCK-8结果显示,与空白组比较,臭牡丹含药血清对肿瘤细胞的增殖抑制作用呈剂量和时间依赖性。其中高剂量组抑制作用最为明显,在24,48,72 h的最大抑制率分别达到28%,32%,43%;流式细胞术结果显示,与空白组比较,随着臭牡丹含药血清浓度的增加,细胞的生长均受不同程度抑制,细胞的凋亡比例亦相应增加,72 h干预组抑制作用显著(P <0. 01),臭牡丹含药血清组各时间段最大凋亡率达19. 48%,19. 72%(P <0. 05);Western blot结果显示,与空白组比较,臭牡丹含药血清干预下各组PTEN表达量均升高(P <0. 05),PI3K,p-Akt蛋白表达均减少(P <0. 05);Real-time PCR结果显示,与空白组比较,臭牡丹含药血清可以下调NF-κB mRNA表达,上调TNF-αmRNA的表达(P <0. 05)。结论:臭牡丹含药血清可以有效抑制MHCC97-H肝癌细胞增殖并促进其凋亡,可能与PI3K/Akt信号通路并影响其关键因子有关。