HepG2.2.15-derived exosomes facilitate the activation and fibrosis of hepatic stellate cells

BACKGROUND The role of exosomes derived from HepG2.2.15 cells,which express hepatitis B virus(HBV)-related proteins,in triggering the activation of LX2 liver stellate cells and promoting liver fibrosis and cell proliferation remains elusive.The focus was on comprehending the relationship and influence of differentially expressed microRNAs(DE-miRNAs)within these exosomes.AIM To elucidate the effect of exosomes derived from HepG2.2.15 cells on the activation of hepatic stellate cell(HSC)LX2 and the progression of liver fibrosis.METHODS Exosomes from HepG2.2.15 cells,which express HBV-related proteins,were isolated from parental HepG2 and WRL68 cells.Western blotting was used to confirm the presence of the exosomal marker protein CD9.The activation of HSCs was assessed using oil red staining,whereas DiI staining facilitated the observation of exosomal uptake by LX2 cells.Additionally,we evaluated LX2 cell proliferation and fibrosis marker expression using 5-ethynyl-2′-deoxyuracil staining and western blotting,respectively.DE-miRNAs were analyzed using DESeq2.Gene Ontology(GO)and Kyoto Encyclopedia of Genes and Genomes(KEGG)pathways were used to annotate the target genes of DE-miRNAs.RESULTS Exosomes from HepG2.2.15 cells were found to induced activation and enhanced proliferation and fibrosis in LX2 cells.A total of 27 miRNAs were differentially expressed in exosomes from HepG2.2.15 cells.GO analysis indicated that these DE-miRNA target genes were associated with cell differentiation,intracellular signal transduction,negative regulation of apoptosis,extracellular exosomes,and RNA binding.KEGG pathway analysis highlighted ubiquitin-mediated proteolysis,the MAPK signaling pathway,viral carcinogenesis,and the toll-like receptor signaling pathway,among others,as enriched in these targets.CONCLUSION These findings suggest that exosomes from HepG2.2.15 cells play a substantial role in the activation,proliferation,and fibrosis of LX2 cells and that DE-miRNAs within these exosomes contribute to the underlying mechanisms.

Effect of IL-18 on peripheral blood mononuclear cells of chronic hepatitis B and hepatitis B virus DNA released by HepG2.2.15 cell lines

BACKGROUND: Interleukin-18 (IL-18), a pro-inflamma- tory cytokine that induces interferon-γ (IFN-γ) production in T cells and natural killer cells, plays a critical role in the T-lymphocyte helper type 1 ( Th1) response. This study was designed to explore the effect of IL-18 on peripheral blood mononuclear cells ( PBMCs) derived from chronic hepatitis B (CHB) and on hepatitis B virus (HBV) DNA released by HepG2.2.15 cell lines, which were transfected with hepatitis B virus gene in vitro. METHODS: PBMCs isolated from 25 healthy people and 25 patients with CHB were stimulated with HBcAg and IL-18 of various concentrations for 72 hours. The levels of IFN-γ in the supernatants of cultured PBMCs were determined by ELISA. After the stimulation of IL-18 of various concentra- tions, PBMCs derived from one patient were co-cultured for 96 hours with HepG2. 2. 15 cells which had been cul- tured for 24 hours, and then the supernatants were collected by centrifugation and used for HBV DNA quantitative as- say. RESULTS: When PBMCs were stimulated by HBcAg and IL-18 at various concentrations, the levels of IFN-γ in the supernatants of CHB groups were much higher than those in normal control groups, at 0.2 ng/ml: t =11.70, P< 0.01; at 1.0 ng/ml: t =16.19, P<0.01; and at5.0 ng/ml: t =20.12, P <0.01. In the CHB groups, the levels of IFN-γ in the supernatants of PBMCs stimulated by HBcAg alone were lower than both those stimulated by HBcAg and EL-18 at various concentrations and those stimulated by HBcAg and EL-18 (5.0 ng/ml) together with EL-12 (mild: t = 2.20, P<0.05; moderate; t=2.97, P<0.05; severe; t = 0.66, P >0.05). The content of HBV DNA in the superna- tant of co-cultivation of HepG2. 2. 15 cells and PBMCs without stimulated materials was higher than that stimula-ted by HBcAg and EL-18 at various concentrations of HBc- Ag and IL-18 together with IL-12/IFN-α1lb. CONCLUSION: DL-18 can induce IFN-γ secretion and pro- bably play a key role in the modulation of both innate and adaptive immunity. It has implications in improving im- munoregulatory effect and increasing the ability of immune cells to kill cells infected by virus.

Efficacies of β-L-D4A against Hepatitis B virus in 2.2.15 cells

AIM:To investigate the antiviral effect of beta-L-enantiomer of 2',3'-didehydro-2',3'-dideoxyadenosine (β-L-D4A) on 2.2.15 cells transfected with the hepatitis B virus (HBV) genome. METHODS:Lamivudine (3TC) as a positive control. Then, HBV DNA in treated 2.2.15 cells and the Hepatitis B surface antigen (HBsAg) in the culture supernatants were detected to determine the inhibitory effect of β-L-D4A. At the same time, 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) was used to detect the survival ratio of 2.2.15 cells. RESULTS:β-L-D4A has a dose-dependent inhibitory effect on HBV DNA replication;this effect was apparent when the concentration was above 1 mol/L. When β-L-D4A was at the highest concentration, 100 mol/L, the HBsAg inhibition ratio was above 50%. The Therapeutic index (TI) of β-L-D4A was above 2.1. CONCLUSION:β-L-D4A has a dose-dependent inhibitory effect on the replication of HBV DNA and the secretion of HBsAg at low toxicity.

Interleukin-10 Is Expressed in HepG2.2.15 Cells and Regulated by STAT1 Pathway

This study investigated the expression profiles of IL-10 gene in three human hepatoma cell lines including Huh7, HepG2, and HepG2 transfected with a plasmid containing hepatitis B virus （HBV） named HepG2.2.15. RT-PCR analysis demonstrated that IL-10 message RNA was absent in HepG2 and Huh7 cells, whereas it was present in HepG2.2.15 cells, which was consistent with ELISA result. Furthermore, except for lamivudine other antiviral treatments did not significantly decrease the HBV DNA level in HepG2.2.15 cells, while they had different effects on the expression of IL-10 protein, although stimulation by LPS had no significant effect. In addition, except for poly（I：C）, the other treatments decreased the expression of IL-10 protein to different degrees, but had no sig-nificant effects on the expression of NF-κB and MyD88. Meanwhile, all treatments we used had effect on the expression of STAT1. In conclusion, IL-10 was expressed in HepG2.2.15 cells and STAT1 pathway might be involved in the regulation of IL-10 expression in HepG2.2.15 cells, but it was not the sole pathway, the exact mechanism warrants further study.

胎盘免疫调节因子对HepG 2.2.15细胞毒性及HBV DNA分泌作用的影响

目的观察胎盘免疫调节因子（PF）在体外的抗乙肝病毒（HBV）作用及安全性。方法将质量浓度分别为0．032—20．000mg／ml的PF作用于体外培养的人肝癌细胞系HepG 2．2．15细胞，通过MTT比色法观察细胞增殖抑制率及半数毒性质量浓度（TC50），以荧光定量PCR法检测HBV DNA水平（以拉米夫定为阳性对照组）。结果PF处理后细胞增殖抑制率为0．75％～58．21％且呈浓度依赖性，作用72h后TC50为13．61mg／ml；PF作用72h和144h后，细胞上清液中HBV DNA拷贝量显著降低，与阳性对照组水平相似。结论PF在体外有显著抗HBV作用，且细胞毒性较小。

荔枝核提取物对HepG2.2.15细胞系HBsAg与HBeAg表达的影响

目的 :研究荔枝核对乙型肝炎病毒的抑制作用及其有效部位。方法 :应用HepG 2 .2 .15细胞系培养系统检测荔枝核提取物A、B、C、D、E、F对HBsAg与HbeAg表达的影响。 结果 :荔枝核提取物A、B、C、D、E、F (2 0 0 ,10 0mg·L-1)对HBsAg和HbeAg表达均有抑制作用 ,其中E成分作用最强 ,在 2 0 0mg·L-1的浓度下 ,于实验第 3天对HBsAg的抑制率为 5 0 % ,对HBeAg的抑制率为 2 0 % ,于实验第 9天对HBsAg的抑制率为90 .9% ,对HBeAg的抑制率为84 .3% (与对照组比较P <0 .0 1)。结论 :荔枝核提取物体外有较强的抗乙肝病毒作用。

青钱柳提取物对HepG2 2.2.15细胞HBsAg和HBeAg表达的影响

目的研究青钱柳提取物体外抗乙肝病毒作用。方法青钱柳用75%乙醇提取后按溶剂极性萃取,获得的三氯甲烷部位经柱层析得到Fr.2组分。体外培养HepG2 2.2.15细胞,MTT法检测青钱柳提取物Fr.2组分对HepG22.2.15细胞的细胞毒作用,用ELISA法检测HepG2 2.2.15细胞培养液中HBsAg和HBeAg的表达。结果青钱柳提取物Fr.2组分对HepG2 2.2.15细胞无明显的细胞毒作用。与对照组比较,Fr.2组分对HBsAg和HBeAg的表达均有显著性抑制作用(P<0.01或0.05)。结论青钱柳提取物体外具有较强的抗乙肝病毒作用。

HH胶囊抗乙肝病毒的体外(2.2.15细胞)实验研究

目的研究HH胶囊体外抗2.2.15细胞乙肝病毒作用。方法 HepG2.2.15是最常用的乙肝病毒感染的体外实验模型,用不同浓度的HH胶囊干预2.2.15细胞,用CCK-8检测药物细胞毒性,酶联免疫法检测乙肝病毒表面抗原(HB-sAg)和乙肝病毒e抗原(HBeAg),荧光定量聚合酶链反应法检测乙肝病毒脱氧核糖核酸(HBV DNA)。结果 HH胶囊可以不同程度降低细胞外HBsAg、HBeAg、HBV DNA及细胞内HBV DNA,此作用具有时间和药物浓度依赖性。结论 HH胶囊具有良好的抗HBV作用。

核酶对2.2.15细胞中HBeAg表达抑制作用的初步观察

目的：观察针对ＨＢＶ Ｃ 区双位点核酶对２ ．２ ．１５ 细胞中ＨＢｅＡｇ 表达的抑制作用。方法：利用亚克隆技术，从质粒ｐ ＧＥＭ － Ｒｚ１２３ 切下ＥｃｏＲ Ｉ－ Ｂａｍ Ｈ Ｉ 片段克隆于真核表达质粒ｐＢＢＳ２１２ 中，将该质粒转染２ ．２ ．１５ 细胞，用ＥＬＩＳＡ 及免疫组化方法观察该核酶对ＨＢｅＡｇ 合成的抑制作用。结果：细胞中表达出针对ＨＢＶ Ｃ 区核酶，该核酶对ＨＢｅＡｇ 的抑制率达４８ ．６ ％ 。结论：该双位点核酶可能通过针对ＨＢＶ Ｃ 区基因的剪切作用，阻断Ｃ

阿的福韦在鸭乙型肝炎模型及2.2.15细胞中抗乙型肝炎病毒的药效研究

目的 :观察阿的福韦体内抗鸭乙型肝炎病毒 (DHBV)的作用及体外抗乙型肝炎病毒 (HBV)效果。方法 :采用鸭乙型肝炎动物模型 ,用阿的福韦口服治疗 10天 ,检测用药前后血清中的DHBVDNA、DHBsAg ,并取肝脏样本提取总DNA ,作SouthernBlot分析。此外 ,以 2 .2 .15细胞为靶细胞 ,给药后通过检测细胞培养液中HBsAg、HBeAg和HBVDNA观察阿的福韦抗HBV效果。结果 :阿的福韦各剂量组用药后均能使血清中的DHBVDNA显著降低或极显著降低 (P <0 .0 5或P <0 .0 1) ,但停药后有DHBVDNA回升现象 ;用药前后DHBsAg无明显改变。肝组织SouthernBlot分析亦显示用药后肝脏中DHBVDNA有明显降低 ,停药后DHBVDNA反跳明显。大剂量阿的福韦加入细胞培养 12天 ,对HBsAg抑制率为 17.0 1% ,对HBeAg抑制率为 2 6 .80 % ,对HBVDNA抑制率为 2 6 .92 %。结论 :阿的福韦在鸭体内有抗鸭乙型肝炎病毒的作用 ,但停药后DHBVDNA有“反跳”现象 ;

2.2.15细胞生长规律的探讨及在药物筛选中应用

目的 探讨 2 .2 .15细胞生长及其分泌HBsAg和HBeAg的规律以及在药物筛选中的应用。方法 利用HBV的体外细胞培养系统 (2 .2 .15细胞系 )建立抗HBV药物筛选的实验技术常规 ,对 2 .2 .15细胞及其分泌HBsAg和HBeAg的特性进行初步观察 ,并在此基础上对几种药物体外抗HBV活性进行研究。结果 选择每孔接种 0 .1mL浓度为 3× 10 8L-1的 2 .2 .15细胞培养至 8～ 12d为细胞指数生长期 ,滴板后第 1天上清中HBsAg和HBeAg均阳性 ,第 12天达高峰且含量最高。药物阿特福韦二吡呋酯、鞣花鞣质、无环鸟苷、α -干扰素对细胞的半数毒性浓度分别为 0 .6 7M ,0 .4 9g/L ,0 .75g/L ,>10× 10 8IU/L ,对病毒HBsAg和HBeAg的治疗指数 (TI)分别为 2 79,4 .4 7;2 7.2 2 ,5 .4 4 ;1,1;1,1。结论 2 .2 .15细胞抗HBV药物筛选以 3× 10 8L-1/孔培养至 12d作为常规方法较为合适。阿特福韦二吡呋酯、鞣花鞣质均有显著体外抗病毒作用 ,可以作为阳性药物对照。

愈肝胶囊对2.2.15细胞分泌HBsAg、HBeAg的抑制作用

目的 :观察愈肝胶囊对HBV转染细胞表达功能的影响。方法 :本研究以乙型肝炎病毒 (HBV )基因转染的人肝癌细胞系 2 2 15细胞作为筛选抗HBV药物的细胞模型 ,观察愈肝胶囊对 2 2 15细胞分泌HBsAg、HBeAg的影响 ;并以四甲基氮唑蓝 (MTT )比色法检测药物对细胞的毒性。结果 :愈肝胶囊对 2 2 15细胞分泌HBsAg和HBeAg有显著抑制作用 ,半数中毒剂量 (TC5 0 )为 1 79mg/ml,对 2 2 15细胞分泌HBsAg和HBeAg抑制率分别为70 81% ,83 96% ;半数有效剂量 (IC5 0 )HBsAg为 0 86,HBeAg为 0 13。治疗指数 (TI)分别为HBsAg 2 0 8,HBeAg 13 76。 结论 :愈肝胶囊在体外有一定的抗HBV作用。

芪黄冲剂体外(2.2.15细胞)抗病毒的药效学研究

目的 通过体外抗病毒实验研究芪黄冲剂在无明显细胞毒性浓度下对2 .2 .15细胞分泌HBsAg、HBeAg颗粒的影响,以验证芪黄冲剂对病毒复制的影响。方法 用MTT法测定芪黄冲剂在不同浓度下的细胞毒性,ELISA法检测芪黄冲剂及其拆方在不同浓度下在9～12d及第13天对共同培养的2 .2 .15细胞分泌HBsAg、HBeAg颗粒的影响。结果 芪黄冲剂1～4号在各浓度下均无明显细胞毒性,芪黄冲剂对2 .2 .15细胞分泌HBsAg、HBeAg颗粒有明显的抑制作用。结论 芪黄冲剂和其拆方组份(1～4组份)对HBV -DNA转染肿瘤细胞株(2 .2 .15细胞)无明显和直接的细胞毒性作用。芪黄冲剂可抑制2 .2 .15细胞分泌HBsAg、HBeAg ,具有良好的抗乙型肝炎病毒的作用。

脱氧核酶及锁核酸核酶对2.2.15细胞中HBsAg和HBeAg表达的抑制作用

目的:观察针对HBV前C/C区的脱氧核酶(DNAzyme)及锁核酸核酶(LNAzyme)对2.2.15细胞中HBsAg、HBeAg表达的抑制作用。方法:设计合成针对HBV前C/C区2031位点的10-23DNAzyme、点硫代修饰的10-23DNAzyme及LNAzyme。本实验设对照组和10-23DNAzyme组、点硫代修饰的10-23DNAzyme组、LNAzyme实验组。对照组包括空白对照组、单纯脂质体对照组、单纯10-23DNAzyme对照组、无关10-23DNAzyme对照组。观察在0.16、0.64、1.28、1.60及1.92μmol.L-1浓度下及12、24、36、48、60、72、84及96 h时间段对2.2.15细胞的HBsAg、HBeAg表达的抑制效应。结果:10-23DNAzyme及LNAzyme作用于2.2.15细胞后,可明显抑制HBsAg、HBeAg的表达,且抑制率LNAzyme明显高于点硫代修饰的10-23DNAzyme,而后者又明显高于未进行任何修饰的10-23DNAzyme组。LNAzyme及点硫代修饰的10-23DNAzyme对HBsAg的最高抑制率分别是(91.6±8.4)%和(78.4±2.0)%,对HBeAg的最高抑制率分别是(90.1±5.2)%和(76.4±4.8)%;在给药后12 h就表现出抑制效应,48 h达高峰,LNAzymes、点硫代修饰的10-23DNAzyme有效抑制时间分别是为84及72 h。其对2.2.15细胞未见明显的细胞毒性作用。结论:10-23DNAzyme及LNAzyme对2.2.15细胞具有明显的高效阻断HBV的HBsAg、HBeAg表达的作用,且LNAzyme优于DNAzyme,是一类特异的高效的抗HBV治疗剂。

苯丙氨酸二肽类化合物073对2.2.15细胞分泌HBsAg和HBeAg的影响

目的观察苯丙氨酸二肽类化合物073对2.2.15细胞分泌HBsAg、HBeAg的影响。方法以2.2.15细胞为研究对象,通过细胞毒性实验确定苯丙氨酸二肽类化合物073对细胞的最大无毒浓度(TC0),在最大无毒浓度以下将药物用培养液对倍稀释成50、25、12.5μg.mL-1加入2.2.15细胞进行培养,每4d换同浓度药物培养液;分别收集第4、8天以及停药后4天的培养液上清,酶联免疫法(ELISA)测定HBsAg、HBeAg含量。结果苯丙氨酸二肽类化合物073最大无毒浓度为50μg.mL-1,在最大无毒浓度时对HBsAg有明显的抑制作用,第8天时的抑制率为59.3%,半数抑制浓度(IC50)为22.9μg.mL-1,治疗指数(TI)为3.1;但对HBeAg无明显抑制作用,第8天时的抑制率仅为25.5%。结论苯丙氨酸二肽类化合物073对2.2.15细胞HBsAg有显著的抑制作用。

2.2.15细胞上清HBVDNA定量检测方法的比较

目的拟筛选和比较2.2.15细胞上清中HBVDNA定量检测的方法。方法分别采用3种方法抽提HBVDNA,抽提物分别采用Taqman荧光定量、SYBR荧光定量PCR技术检测其滴度。结果直接应用上清分别采取热变性,碱裂解法抽提HBVDNA均为阴性,而应用PEG沉淀后检测结果证实细胞上清中有高拷贝的分泌性HBVDNA,Taqman荧光定量方法的敏感性高于SYBR实时定量PCR,在高拷贝时,两种方法的检测结果一致。结论PEG沉淀法是2.2.15细胞上清HBVDNA提取的有效方法,Taqman荧光定量方法敏感性高,是HBVDNA定量检查的首选方法。SYBR法简便,经济,也可用于上清HBVDNA的检测。

水芹总酚酸对2.2.15细胞分泌HBsAg与HBeAg的抑制作用

目的观察水芹总酚酸对2.2.15细胞分泌HBsAg、HBeAg的抑制作用。方法以2.2.15细胞为研究对象,通过细胞毒性实验确定水芹总酚酸对细胞的最大无毒浓度(TC0),在最大无毒浓度以下将药物用培养液对倍稀释成500、250、125μg.mL-1加入2.2.15细胞进行培养,每4d换同浓度药物培养液;分别收集第4、8天以及停药后4d的培养液,酶联免疫法(ELISA)测定HBsAg、HBeAg含量。结果水芹总酚酸最大无毒浓度为500μg.mL-1,在最大无毒浓度时对HBsAg、HBeAg具有明显的抑制作用,第8天时的抑制率分别为59.33%和90%,半数抑制浓度(IC50)分别为484.17、379.89μg.mL-1,治疗指数(TI)分别为3.158、4.025,其中对HBeAg的抑制作用优于HBsAg。结论水芹总酚酸对2.2.15细胞分泌的HBsAg、HBeAg有显著的抑制作用。

甘草甜素对HepG2.2.15细胞株HBeAg水平及TLR4表达的影响

目的探讨甘草甜素(GL)对HepG2.2.15细胞上清HBeAg分泌,Toll样受体4(TLR4)信号分子的表达及对细胞增殖的影响。方法实时荧光定量PCR检测TLR4表达;直接免疫荧光流式细胞术(FCM)检测表达TLR4的阳性细胞率;ELASA检测HBV所分泌抗原;MTT检测细胞增殖活性,并与空白对照组比较。结果给药后HBVe抗原(HBeAg)的分泌结果显示,总体均数间差异显著(P<0.05),但甘草甜素各组与对照组比较差异无统计学意义;GL各组TLR4 mRNA及流式细胞TLR4的表达总体均数间均有显著差异(P<0.01),分别与对照组相比差异有显著性(P<0.01),100μg/mL组尤其明显;MTT实验显示,200μg/mL以下三个剂量组均可促进细胞增殖,50μg/mL组与对照组间差异显著(P<0.05);400μg/mL、800μg/mL两组均显著抑制细胞增殖(P<0.01);而MTT结果与HBeAg水平呈显著负相关(P<0.01),与TLR4表达无相关关系(P>0.05)。结论研究表明,甘草甜素对HepG2.2.15的e抗原分泌可能具有双向作用;细胞的存活率与e抗原呈负相关;TLR4在HepG2.2.15细胞株低表达,GL可上调TLR4表达,甘草甜素可影响先天免疫中的TLR4信号分子,有可能在体内通过免疫途径影响HBV复制和抗原分泌。

九头狮子草水浸膏对2.2.15细胞中对HBsAg、HBeAg的分泌和HBV DNA复制的抑制作用

目的:通过观察九头狮子草水浸膏对2.2.15细胞HBsAg、HBeAg的分泌及HBV DNA复制的影响,探讨其在体外的抗乙型肝炎病毒(HBV)作用。方法:将SD大鼠(n=10)随机分为九头狮子草水浸膏组和正常血清组,前者用九头狮子草水浸膏按2.7g.kg-1.d-1剂量灌胃,后者给予生理盐水10ml.kg-1.d-1灌胃,制备不同浓度含药血清及正常血清。2.2.15细胞培养上清液HBsAg、HBeAg测定采用免疫放射分析法,HBV DNA检测采用PCR杂交试验法,测定不同浓度含药血清抗HBV活性情况。结果:含药血清作用4天、8天时,各含药血清组抑制HBsAg、HBeAg分泌的作用优于空白血清细胞对照(指含正常血清)组(P<0.01、P<0.05)。作用4天时,不同浓度含药血清的抗HBV作用差异无显著性意义(P>0.05);作用8天时,不同浓度含药血清抑制HBeAg分泌的作用差异无显著性意义(P>0.05);10%、15%含药血清抑制HBsAg分泌的作用均优于5%含药血清(P<0.05),10%、15%含药血清相比较差异无显著性意义(P>0.05);作用8天时,各含药血清组HBV DNA低于细胞对照组和空白血清细胞对照(指含正常血清)组(P<0.01、P<0.05),5%、10%含药血清组与15%含药血清组相比较差异有显著性意义(P<0.05)。结论:九头狮子草水浸膏的含药血清在体外细胞培养中对2.2.15细胞分泌HBsAg、HBeAg及HBV DNA复制均有较好的抑制作用,10%含药血清的抑制作用优于5%、15%浓度。