Metastatic human hepatocellular carcinoma models in nude mice and cell line with metastatic potential

Metastatic human HCC model is needed for the studies on mechanism and intervention of metastatic recurrence. By using orthotopic implantation of histologically intact tissues of 30 surgical specimens, a patient-like metastatic model of human HCC in nude mice (LCI-D20) and a low metastatic model of human HCC in nude mice (LCI-D35) have been established. All mice with transplanted LCI-D20 tumors exhibited extremely high metastatic ability including spontaneous metastasis to liver, lungs, lymph nodes and peritoneal seeding. Remarkable difference was also found in expression of some of the invasiveness related genes and growth factors between the LCI-D20 and LCI-D35 tumors. PAI-1 increased gradually following tumor progression in LCI-D20 model, and correlated with tumor size and AFP level. Phasic expression of tissue intercellular adhesion molecule-1 in this model was also observed. Using corneal micropocket model, it was demonstrated that the vascular response induced by LCI-D20 tumor was stronger than that induced by LCI-D35 tumor. Similar report on metastatic human HCC model in nude mice and human HCC cell line with metastatic potential was rarely found in the literature. This LCI-D20 model has been widely used for the studies on intervention of metastasis, including anti-angiogenesis,antisense approach, metalloproteinase inhibitor, differentiation inducer, etc. It is concluded that the establishment of metastatic human HCC model in nude mice and human HCC cell line with metastatic potential will provide important models for the in vitro and in vitro study of HCC invasiveness, angiogenesis as well as intervention of HCC recurrence.

Possible mechanisms associated with immune escape and apoptosis on anti-hepatocellular carcinoma effect of Mu Ji Fang granules

BACKGROUND Hepatocellular carcinoma(HCC)is one of the most common digestive system cancers with high mortality rates worldwide.The main ingredients in Mu Ji Fang Granules(MJF)are alkaloids,flavonoids,and polysaccharides.MJF has been used in the clinical treatment of hepatitis,cirrhosis and HCC for more than 30 years.Few previous studies have focused on the mechanism of MJF on tumor immunology in the treatment of HCC.AIM To explore the mechanism of action of MJF on tumor immunology in the treatment of HCC.METHODS The absorbable ingredients of MJF were identified using Molecule Network related to High Performance Liquid Chromatography-Electron Spray Ionization-Time of Flight-Mass Spectrometry,and hub potential anti-HCC targets were screened using network pharmacology and pathway enrichment analysis.Forty male mice were randomly divided into the Blank,Model,and MJF groups(1.8,5.4,and 10.8 g/kg/d)following 7 d of oral administration.Average body weight gain,spleen and thymus indices were calculated,tumor tissues were stained with hematoxylin and eosin,and Interferon gamma(IFN-γ),Tumor necrosis factorα(TNF-α),Interleukin-2,aspartate aminotransferase,alanine aminotransferase,alpha-fetoprotein(AFP),Fas,and FasL were measured by Enzyme-linked Immunosorbent Assay.Relevant mRNA expression of Bax and Bcl2 was evaluated by Real Time Quantitative PCR(RTqPCR)and protein expression of Transforming growth factorβ1(TGF-β1)and Mothers against decapentaplegic homolog(SMAD)4 was assessed by Western blotting.The HepG2 cell line was treated with 10 mg/mL,20 mg/mL,30 mg/mL,40 mg/mL of MJF,and another 3 groups were treated with TGF-β1 inhibitor(LY364947)and different doses of MJF.Relevant mRNA expression of TNF-α,IFN-γ,Bax and Bcl2 was evaluated by RT-qPCR and protein expression of TGF-β1,SMAD2,p-SMAD2,SMAD4,and SMAD7 was assessed by Western blotting.RESULTS It was shown that MJF improved body weight gain and tumor inhibition rate in H22 tumorbearing mice,protected immune organs and liver function,reduced the HCC indicator AFP,affected immunity and apoptosis,and up-regulated the TGF-β1/SMAD signaling pathway,by increasing the relative expression of TGF-β1,SMAD2,p-SMAD2 and SMAD4 and decreasing SMAD7,reducing immune factors TNF-αand IFN-γ,decreasing apoptosis cytokines Fas,FasL and Bcl2/Bax,and inhibiting the effect of LY364947 in HepG2 cells.CONCLUSION MJF inhibits HCC by activating the TGF-β1/SMAD signaling pathway,and affecting immune and apoptotic cytokines,which may be due to MJF adjusting immune escape and apoptosis.

沙冬青提取物(JA1)对小鼠肝癌H_(22)细胞体外增殖和皮下移植生长的抑制

采用噻唑蓝(MTT)还原法测定梯度浓度的沙冬青提取物(JA1)对体外培养小鼠肝癌细胞株H22增殖的影响;同时对皮下移植肿瘤H22小鼠灌服不同剂量的JA1以检测抑瘤率,进一步采用流式细胞术、光镜和透射电子显微镜技术,检测和观察JA1对小鼠移植性肿瘤H22的诱导凋亡作用。结果显示,JA1可显著抑制体外培养小鼠肝癌H22细胞的增殖,并且这种抑制存在浓度和时间关系。同时,JA1对小鼠皮下移植性肿瘤H22也有明显的抑制作用。流式细胞分析表明,JA1灌胃试验组瘤组织细胞DNA直方图上见有明显的凋亡峰;在光镜和电镜下,JA1灌胃试验组也见有明显的瘤细胞凋亡,表明JA1对体内、外H22细胞的增殖抑制是以诱导凋亡为基础的。

熊果酸对H22荷瘤小鼠抗肿瘤及免疫调节作用

目的探讨熊果酸(UA)对H22荷瘤小鼠抗肿瘤作用及免疫功能的影响。方法皮下移植建立H22荷瘤小鼠模型,腹腔注射不同剂量UA,检测抑瘤率和免疫器官指数,MTT法检测脾脏T、B淋巴细胞增殖能力,流式细胞术检测CD4+、CD8+T细胞亚群含量及比例,ELISA法检测血清细胞因子IL-2、IL-4和TNF-α的表达量。结果 UA对小鼠皮下移植性肿瘤H22有显著的抑制作用,可降低免疫器官中异常增大的脾指数,增强脾脏中T、B淋巴细胞增殖能力,提高淋巴细胞亚群CD4+T细胞表达及CD4+/CD8+T细胞亚群比例,促进血清IL-2、TNF-α表达,降低IL-4表达。结论 UA可抑制小鼠肝癌H22肿瘤生长,体内可以提高荷瘤小鼠的免疫能力,其抗肿瘤作用可能与机体的免疫调节作用相关。

Notch信号通路在小鼠肝癌细胞H22增殖凋亡中的作用及意义

目的观察Notch信号通路在小鼠肝癌细胞H22增殖和凋亡中的作用,并探讨其可能的机制。方法培养小鼠肝癌细胞株H22,将细胞随机分为A、B、C组,分别加入Notch信号激活剂rhNF-κB、抑制剂DAPT及PBS共培养48 h。用MTT法检测细胞吸光度值(A值)观察细胞增殖情况,流式细胞术检测细胞凋亡率,应用免疫组化法检测各相关处理过的细胞株,RT-PCR、Western blotting法分别检测H22细胞中的Notch1、Hes1、Bcl-2 mRNA及其蛋白。结果培养24、48、72、96 h后,A、B组与C组比较,细胞增殖差异明显(P均<0.05)。A、B、C组细胞凋亡率分别为25.52%±2.13%、0.91%±0.18%、8.91%±1.50%,A、B组与C组比较差异明显(P均<0.05)。与C组比较,A组细胞中Notch1、Hes1、Bcl-2 mRNA及其蛋白表达量均显著增加(P均<0.05),B组细胞中Notch1、Hes1、Bcl-2 mRNA及其蛋白表达量均显著降低(P均<0.05)。结论 Notch1信号通路在抑制小鼠肝癌细胞株H22增殖、促进其凋亡中发挥了重要的调控作用,其机制可能与调节靶基因Hesl、Bcl-2表达有关。

JA1对体外培养的Hep细胞和小鼠皮下移植性Hep细胞凋亡的影响

采用噻唑蓝(MTT)还原法、流式细胞术、光镜及透射电子显微镜技术等检测了梯度浓度的JA1(沙冬青提取物)对体外培养的小鼠肝癌细胞株Hep增殖的影响及诱导Hep细胞凋亡的作用;并检测了JA1对小鼠皮下移植性Hep细胞的生长抑制及诱导凋亡作用。结果显示,JA1可显著抑制小鼠Hep细胞的增殖,且这种抑制有浓度和时间依赖性。流式细胞仪分析显示,JA1处理后的Hep检测样本中有明显的DNA低含量颗粒("亚G1期"峰),细胞周期各时相分布发生了改变,细胞在G1期被阻滞。同时,JA1对小鼠皮下移植性Hep细胞也有明显的抑制作用。JA1灌胃试验组瘤组织细胞DNA直方图有明显的凋亡峰,细胞在G1期也被阻滞,光镜和电镜下可见大量凋亡肿瘤细胞。

来源于转移灶的人肝细胞癌细胞系HN-HC1的建立和特性

目的建立新的转移性人肝细胞癌细胞系并研究其生物学特性。方法从人肝细胞癌的腹腔转移灶取材,将标本分离成单细胞悬液,使用培养液进行原代和传代培养,取名为HN-HC1细胞,观察细胞的形态,绘制细胞生长曲线。于裸小鼠腹腔接种第18代HN-HC1细胞2×106个,观察癌细胞的生物学特性,检测AFP的表达。结果 HN-HC1细胞体外连续传代至第18代,形态上具有典型的恶性上皮细胞的特征,裸小鼠腹腔HN-HC1细胞成瘤率100%,移植瘤细胞中AFP呈强阳性表达。结论 HN-HC1细胞可能成为较稳定的来源于转移灶的人肝细胞癌细胞系,HN-HC1裸小鼠移植瘤是一种较理想的肝细胞癌动物模型,为肝细胞癌的研究提供了良好的动物实验平台。

Adeno-associated virus mediated endostatin gene therapy in combination with topoisomerase inhibitor effectively controls liver tumor in mouse model

AIM:rAAV mediated endostatin gene therapy has been examined as a new method for treating cancer.However, a sustained and high protein delivery is required to achieve the desired therapeutic effects.We evaluated the impact of topoisomerase inhibitors in rAAV delivered endostatin gene therapy in a liver tumor model. METHODS:rAAV containing endostatin expression cassettes were transduced into hepatoma cell lines.To test whether the topoisomerase inhibitor pretreatment increased the expression of endostatin,Western blotting and ELISA were performed.The biologic activity of endostatin was confirmed by endothelial cell proliferation and tube formation assays. The anti-tumor effects of the rAAV-endostatin vector combined with a topoisomerase inhibitor,etoposide,were evaluated in a mouse liver tumor model. RESULTS:Topoisomerase inhibitors,including camptothecin and etoposide,were found to increase the endostatin exPression level in vitro.The over-expressed endostatin, as a result of pretreatment with a topoisomerase inhibitor, was also biologically active.In animal experiments,the combined therapy of topoisomerase inhibitor,etoposide with the rAAV-endostatin vector had the best tumor- suppressive effect and tumor foci were barely observed in livers of the treated mice.Pretreatment with an etoposide increased the level of endostatin in the liver and serum of rAAV-endostatin treated mice.Finally,the mice treated With rAAV-endostatin in combination with etoposide showed the longest survival among the experimental models. CONCLUSION:rAAV delivered endostatin gene therapy in combination with a topoisomerase inhibitor pretreatment is an effective modality for anticancer gene therapy.

小鼠肝癌细胞肺高转移株的建立及鉴定

目的:建立小鼠肝癌细胞肺高转移株,为研究转移相关分子机制提供合适的模型.方法:将H22肝癌腹水瘤细胞(简称M0)经尾静脉注入昆明小鼠,获取肺转移结节,再制备腹水瘤、尾静脉注射、形成肺转移瘤.重复操作获得第4代肺高转移株(简称M4),检测其小鼠肺转移能力和体外增殖能力、细胞分裂指数、染色体形态及细胞周期比例,并用RT-PCR方法测定RhoC基因mRNA的表达来进一步加以验证.结果:经尾静脉注射,M4较早出现肺转移,肺转移结节数多、体积大.M4与M0体外结果比较:倍增时间缩短了38.73%;细胞分裂指数是4.11%±0.11%,明显多于M0的4.70%±0.19%(P=0.014);S期比例是56.10±4.76%,明显高于M0的46.98±4.49%(P=0.022);二者染色体数目相同,但M4异型性明显;RhoC基因表达分别是1.011±0.163和0.486±0.045,M4的表达显著增高(P=0.0029).结论:建立了小鼠肝癌细胞肺高转移细胞株,其RhoC基因表达明显上调.

Bevacizumab抑制人肝癌细胞及其移植瘤的生长

目的探讨Bevacizumab对肝癌细胞株HepG2及荷肝癌裸鼠移植瘤生长的影响。方法不同浓度Bevacizumab处理HepG2细胞48 h后,MTT法检测Bevacizumab对细胞增殖的抑制作用,设不加药物的HepG2细胞为对照组。建立荷肝癌细胞株HepG2裸鼠皮下移植瘤模型,随机分为Bevacizumab组和空白对照组,观察用药前后肿瘤大小,计算抑瘤率;应用免疫组化计算肿瘤微血管密度。结果 Bevacizumab可抑制HepG2细胞增殖;与空白对照组比较,Bevacizumab可延缓移植瘤的生长,MVD值明显降低(P=0.000)。结论 Bevacizumab可直接抑制肝癌细胞株HepG2的增殖;Bevacizumab主要通过抑制新生血管的形成而抑制移植瘤的生长。

癌毒清对肝癌模型小鼠肿瘤组织病理及微血管密度的影响

目的:观察癌毒清对肝癌(hepatocellular carcinoma,HCC)模型小鼠肿瘤组织病理及微血管密度(microvessel density,MVD)的影响。方法:将50只小鼠腋下接种H22肝癌细胞株,建立肝癌异位移植瘤模型。将造模成功的小鼠随机分为模型组、癌毒清高剂量组、癌毒清中剂量组、癌毒清低剂量组及氟尿嘧啶组,每组各10只。癌毒清各剂量组给予不同剂量的癌毒清溶液灌胃,氟尿嘧啶组给予氟尿嘧啶腹腔注射,模型组给予等剂量蒸馏水灌胃。给药12 d后,脱颈处死,剥取瘤组织,称取瘤质量,计算抑瘤率和病理组织学检查,免疫组织化学法观察MVD。结果:与模型组比较,癌毒清高剂量组、癌毒清中剂量组、癌毒清低剂量组及氟尿嘧啶组瘤质量降低,以癌毒清高剂量组最为明显,差异具有统计学意义(P <0. 05)。癌毒清高剂量组、癌毒清中剂量组、癌毒清低剂量组抑瘤率分别为50. 91%、35. 25%、20. 10%,氟尿嘧啶组为43. 99%,与模型组比较,差异有统计学意义(P <0. 05)。与模型组比较,癌毒清高剂量组、癌毒清中剂量组、癌毒清低剂量组及氟尿嘧啶组MVD计数降低,以癌毒清高剂量组最为明显,差异具有统计学意义(P <0. 05)。结论:癌毒清的抗癌机制可能是通过降低肿瘤MVD,抑制肝癌微血管生成而实现的。

siRNA沉默Livin基因表达在抑制裸鼠肝癌生长中的作用研究

目的目的应用RNA干扰技术抑制人肝癌细胞株MHCC97H中凋亡抑制因子Livin的表达,研究Livin基因在抑制裸鼠肝癌细胞移植瘤生长中的作用。方法设计针对Livin基因目标序列的siRNA,将其经脂质体Lipofectamine^(TM)2000转染至肝癌细胞株MHCC97H细胞,采用RT-PCR、Westernblot方法检测转染后的MHCC97H细胞中Livin基因的mRNA和蛋白质表达。通过建立裸鼠的荧光素酶(Luciferase)标记的MHCC97H肝癌细胞移植瘤模型,监测肿瘤体积、重量,通过活体成像技术观察siRNA注射治疗移植瘤的效果。结果在Livin-siRNA转染后的MHCC97H细胞中,Livin基因的mRNA和蛋白质表达显著下降(P<0.05),siRNA注射治疗移植瘤后,肿瘤重量、体积及荧光素酶信号均显著性下降(P<0.05)。结论通过RNA干扰技术阻断MHCC97H细胞中Livin的表达,可抑制裸鼠肝癌移植瘤的生长,提示Livin基因在肝癌的发生、发展过程中起重要作用。

索拉非尼与重组腺病毒H101对肝癌细胞株HepG2的作用及机制研究

目的:研究索拉非尼与重组腺病毒H101对肝癌细胞株HepG2的作用并分析其具体机制。方法:选择索拉非尼、重组腺病毒H101分别组成重组腺病毒H101组、索拉非尼组、两药联合组以及空白对照组,并分别作用于购自中国科学院上海细胞生物研究所细胞库的肝癌细胞株HepG2。采用流式细胞技术检测HepG2细胞的凋亡情况;采用Western blot法检测细胞外信号调节激酶1/2(ERK1/2)、磷酸化ERK1/2(p-ERK1/2)以及髓样细胞白血病-1(Mcl-1)蛋白相对表达量;采用酶联免疫吸附法检测不同组别细胞培养上清液中的血管内皮生长因子(VEGF)水平。结果:重组腺病毒H101组、索拉非尼组、两药联合组的G0-G1期与G2-M期细胞均明显低于空白对照组,S期细胞均明显高于空白对照组,且两药联合组较重组腺病毒H101组与索拉非尼组更明显,差异均有统计学意义(均P<0.05);重组腺病毒H101组、索拉非尼组、两药联合组的HepG2细胞凋亡率明显高于空白对照组,而两药联合组又明显高于重组腺病毒H101组与索拉非尼组,差异均有统计学意义(均P<0.05)。重组腺病毒H101组、索拉非尼组、两药联合组的p-ERK1/2、Mcl-1蛋白相对表达量和VEGF表达均明显低于空白对照组,而两药联合组又明显低于重组腺病毒H101组与索拉非尼组,差异均有统计学意义(均P<0.05)。结论:索拉非尼、重组腺病毒H101均可抑制肝癌细胞株HepG2的增殖,并诱导其凋亡,控制VEGF表达,联合应用具有更明显的效果,其主要机制可能与二者协同作用有效抑制p-ERK1/2、Mcl-1蛋白表达有关。

CCR4对肝癌细胞索拉非尼放射敏感性及裸鼠成瘤的影响

目的探讨CC趋化因子受体4(CCR4)对肝癌细胞索拉非尼放射敏感性及裸鼠成瘤的影响。方法采用Westernblot检测CCR4在肝癌细胞系中的表达。利用慢病毒感染构建过表达及敲减CCR4的PLC/PRF/5和SMMC-7721稳转株,并采用Western blot进行验证。采用平板克隆形成实验检测CCR4对肝癌细胞放射敏感性的影响。通过裸鼠成瘤实验检测CCR4对肝癌细胞体内成瘤的影响。结果高转移肝癌细胞中CCR4呈高表达,低转移肝癌细胞中CCR4呈低表达。成功构建稳定过表达CCR4的PLC/PRF/5和敲减CCR4的SMMC-7721肝癌稳转株,过表达CCR4可逆转索拉非尼放疗对PLC/PEF/5的抑制作用,而敲减CCR4可增加SMMC-7721对索拉非尼放射敏感性。过表达CCR4可促进PLC/PEF/5裸鼠体内成瘤能力,而敲减CCK4可抑制SMMC-7721裸鼠体内成瘤能力,结论CCR4高表达能显著增强肝癌PLC/PEF/5细胞对索拉非尼放射抵抗及裸鼠体内成瘤能力,而敲减CCK4则可显著增加肝癌SMMC-7721细胞对索拉非尼放射敏感性并抑制其裸鼠体内成瘤能力。

夜香树甾体皂苷抗人肝癌裸鼠移植瘤的研究

目的:观察夜香树甾体皂苷(SSCN)对肝癌HepG2移植瘤的抑制作用,并探讨其抑瘤的可能机制。方法:从夜香树叶中提取并鉴定SSCN;建立BALB/c裸鼠HepG2肝癌模型,建模成功后将荷人肝癌裸鼠随机分为5组:生理盐水组(NS)、沙利度胺组(TLD 200 mg·kg-1),SSCN低,中,高组(4,6,8 mg·kg-1,ip,隔日1次,连续30 d),观察SSCN的肿瘤抑制作用。治疗期间测量皮下移植瘤的长径和短径;30 d后处死裸鼠,剖取肿瘤,行常规制片,HE染色,镜下观察肿瘤病变;免疫组化染色,观察并检测移植瘤中增殖细胞核抗原PCNA和Ki-67蛋白的表达。结果:TLD组裸鼠ip对肝癌HepG2 BALB/c裸鼠相对肿瘤增殖率为42.19%,SSCN 4,6,8 mg·kg-1的增殖率分别为48.26%,42.94%,41.57%,随着剂量的增高其相对肿瘤增殖率逐渐下降,SSCN抑制肿瘤生长的作用存在剂量依赖性。镜下观察,SSCN高剂量组见到大量坏死细胞外,部分肿瘤细胞体积较小,细胞核浓染。NS组荷瘤小鼠的肿瘤细胞中PCNA和Ki-67蛋白的表达率明显增高;而与NS组比较,TLD组和SSCN高剂量组PCNA和Ki-67蛋白的表达显著下降(P<0.05)。结论:夜香树甾体皂苷体内对BALB/c小鼠肝癌移植瘤有一定的抑制作用,其作用机制可能是通过下调PCNA和Ki-67基因蛋白的表达,从而抑制肿瘤细胞的增殖。

肝癌细胞系、肝癌组织及癌旁肝硬化组织中异常凝血酶原水平的研究

为阐明新的肿瘤标志——异常凝血酶原（ｄｅｓ－γ－Ｃａｒｂｏｘｙｐｒｏｔｈｒｏｍｂｉｎ，ＤＣＰ）在原发性肝癌（ＨＣＣ）中升高机制，本文检测了正常肝组织、肝癌组织和癌旁肝硬化组织中ＤＣＰ及总凝血酶原水平，同时测定了４株肝癌细胞系培养上清中ＤＣＰ含量。血浆ＤＣＰ升高与肝癌组织中ＤＣＰ水平相一致，癌组织中凝血酶原总量也明显增高，无论血浆中ＤＣＰ是否升高，癌旁肝硬化组织内ＤＣＰ水平均较正常组织高；４株肝癌细胞均产生ＤＣＰ，且ＤＣＰ产量随培养时间延长而增加。提示ＤＣＰ是肝癌细胞特异产物，肝癌组织中ＤＣＰ升高及凝血酶原总量的过度生成可能对肝癌血浆ＤＣＰ产生起重要作用，肝硬化组织中ＤＣＰ升高可能是一种癌前病变的标志。