Fibrinogen-like protein 2 fibroleukin expression and its correlation with disease progression in murine hepatitis virus type 3-induced fulminant hepatitis and in patients with severe viral hepatitis B

AIM： To evaluate the expression of fibrinogenlike protein 2 （fgl2） and its correlation with disease progression in both mice and patients with severe viral hepatitis. METHODS： Balb/cJ or A/J mice were infected intraperitoneally （ip） with 100 PFU of murine hepatitis virus type 3 （MHV-3）, liver and serum were harvested at 24, 48, and 72 h post infection for further use. Liver tissues were obtained from 23 patients with severe acute chronic （AOC） hepatitis B and 13 patients with mild chronic hepatitis B. Fourteen patients with mild chronic hepatitis B with cirrhosis and 4 liver donors served as normal controls. In addition, peripheral blood mononuciear cells （PBMC） were isolated from 30 patients （unpaired） with severe AOC hepatitis B and 10 healthy volunteers as controls. Procoagulant activity representing functional prothrombinase activity in PBMC and white blood cells was also assayed. A polyclonal antibody against fgl2 was used to detect the expression of both mouse and human fgl2 protein in liver samples as well as in PBMC by immunohistochemistry staining in a separate set of studies. Alanine aminotransferase （ALT） and total bilirubin （TBil） in serum were measured to assess the severity of liver injury.RESULTS： Histological changes were found in liver sections 12-24 h post MHV-3 infection in Balb/cJ mice. In association with changes in liver histology, marked elevations in serum ALT and TBil were observed. House fgl2 （mfgl2） protein was detected in the endothelium of intrahepatic veins and hepatic sinusoids within the liver 24 h after MHV-3 infection. Liver tissues from the patients with severe AOC hepatitis B had classical pathological features of acute necroinflammation. Human fgl2 （hfgl2） was detected in 21 of 23 patients （91.30%） with severe AOC hepatitis B, while only 1 of 13 patients （7.69%） with mild chronic hepatitis B and cirrhosis had hfgl2 mRNA or protein expression. Twenty-eight of thirty patients （93.33%） with severe AOC hepatitis B and 1 of 10 with mild chronic hepatitis B had detectable hfgl2 expression in PBMC. No hfgl2 expression was found either in the liver tissue or in the PBMC from normal donors. There was a positive correlation between hfgl2 expression and the severity of the liver disease as indicated by the levels of TBil. PCA significantly increased in PBMC in patients with severe AOC hepatitis B. CONCLUSION： The molecular and cellular results reported here in both mice and patients with severe viral hepatitis suggest that virus-induced hfgl2 prothrombinase/fibroleukin expression and the coagulation activity associated with the encoded fgl2 protein play a pivotal role in initiating severe hepatitis. The measurement of hfgl2/fibroleukin expression in PBMC may serve as a useful marker to monitor the severity of AOC hepatitis B and a target for therapeutic intervention.

Local Expression of Vaginal Th1 and Th2 Cytokines in Murine Vaginal Candidiasis under Different Immunity Conditions

To investigate the expression of vaginal Th1 and Th2 cytokines in rats with experimental vaginal candidiasis under different immune conditions, ICR murine vaginal candidiasis model was established and immno-suppressed murine models of vaginal cadidiasis were established in estrogen-treated mice. Non-estrogen-treated mice were used as controls. The mRNA level of Th1 （IL-2）/Th2 （IL-4, IL-10, TGF-β1） cytokines in murine vaginal tissues was determined by RT-PCR. The cykotine in local tissues was increased to different extent under normal immune condition. IL-2 mRNA was increased during early stage of infection, while IL-10 was increased transiently during late stage of infection. TGF-β1 production was found to be increased persistently. At same time, the expression of IL-2 mRNA was suppressed in immno-suppressed group, and the level of IL-4, IL-10, and TGF-β1 were higher than the normal immunity group to different degree during infection. The high level of IL-2 mRNA during early stage of infection was associated with clearance of mucosal Candidia albicans （C. albicans）, and its expression suppressed leading to decreased clearance of mucosal C. albican in immuno-suppression. The over-expression of IL-4 and IL-10 could significantly enhance the susceptibility to C. albicans infection in mice.

Maternal Murine Cytomegalovirus Infection during Pregnancy Up-regulates the Gene Expression of Toll-like Receptor 2 and 4 in Placenta

Increasing evidence has revealed that maternal cytomegalovirus （CMV） infection may be associated with neurodevelopmental disorders in offspring. Potential relevance between the placental inflammation and CMV-related autism has been reported by clinical observation. Meanwhile, abnormal expression of Toll-like receptor 2 （TLR2） and TLR4 in placenta of patients with chorioamnionitis was observed in multiple studies. IL-6 and IL- 10 are two important maternal inflammatory mediators involved in neurodevelopmental disorders. To investigate whether murine CMV （MCMV） infection causes alterations in placental IL-6/10 and TLR2/4 levels, we analyzed the dynamic changes in gene expression of TLR2/4 and IL-6/10 in placentas following acute MCMV infection. Mouse model of acute MCMV infection during pregnancy was created, and pre-pregnant MCMV infected, lipopolysaccharide （LPS）-treated and uninfected mice were used as controls. At E13.5, E 14.5 and E 18.5, placentas and fetal brains were harvested and mRNA expression levels of placental TLR2/4 and IL-6/10 were analyzed. The results showed that after acute MCMV infection, the expression levels of placental TLR2/4 and IL-6 were elevated at E13.5, accompanied by obvious placental inflammation and reduction of placenta and fetal brain weights. However, LPS 50 ktg/kg could decrease the IL-6 expression at E13.5 and E14.5. This suggests that acute MCMV infection during pregnancy could up-regulate the gene expression of TLR2/4 in placental trophoblasts and activate them to produce more pro- inflammatory cytokine IL-6. High dose of LPS stimulation （50 gg/kg） during pregnancy can lead to down-regulation of IL-6 levels in the late stage. Imbalance of IL-6 expression in placenta might be associated with the neurodevelopmental disorders in progeny.

Local Th1/Th2 Cytokine Expression in Experimental Murine Vaginal Candidiasis

In order to investigate the expression of Th1 and Th2 cytokines in the vaginal candidiasis caused by Candida, the fungal vaginitis model was established in female ICR mice by intravaginal inoculation of suspension of C. albicans after the animals were pretreated with estradiol. Reverse transcriptase-polymerase chain reaction （RT-PCR） was used to detect the expression of IL-2, IL-4, IL-10 and TGF-β1 in the vagina in the mice of different groups at different time points after the beginning of the experiment. The average expression level of IL-2 mRNA in group D （estrogen-treated mice） was significantly higher than that in groups H （estrogen-untreated mice） and I （control group） on the day 2. The average expression level of IL-4 mRNA in group D was significantly higher than that in groups I and H on the day 5. The average expression level of IL-10 mRNA in group D was significantly higher than that in groups H and I from day 7 to 11. The average expression level of TGF-β1 mRNA in group D was significantly higher than that in groups H and I at all time points. It was concludes that the high-level expression of IL-2 mRNA during early infection was associated with clearance of mucosal C. albicans, and the high-level expression of IL-10 mRNA during late stage of the infection was related to susceptibility to infection. TGF-β1 may play a predominant role when the virtual absence of changes in other Th-type cytokines during infection.

LPS-induced activation of phospholipase A_2 phospholipase C and protein kinase C of murine macrophage-like cell lines (J774 and P388Dl)~1

A murine maorophage-like cell line, J774, acquri ed, in response to LPS, an ability to kill tumor necrosis factor (TNF)-insensitive target P815 mastocytoma cells, whereas another cell line, P388D1, did not. LPS-triggered signaling mechanisms between the two cell lines were compared with an aim to inquire about the possible nature of the above-mentioned difference. The results showed that two cell lines respond to LPS-treatment by parallel activation of both phospholipases C and A2 (PLC and PLA2) to approximately the same extent. The maximum response of both enzymes of J774 cells was noted within 10 min of the treatment, whereas that of P388D1 cells required more than 20 min. The other properties of LPS-responsive enzymes studied were similar between two cell lines, includingAotivation of PLC and PLA2 and PKC in macrophages by LPSGa2+ augmentation of enzyme activation, participation of guanine nuoleotide binding (G) proteins in the initial activation processes, and inhibition of enzyme activation by the prior treatment of cells with cholera or pertussis toxins etc. Moreover, LPS-triggered activation of PLC and PLA2 was found to be followed by the increase of PKC activities in both cell lines. In spite of these similarities, J774 cells possessed both basic and acidic forms of PKC activities, while P 388D1 cells owned only PKC of basic form. Nevertheless, the question why J774 cells, but not P388D1 cells, can acquire the tumorioidal activity, aganist P815 cells following LPS-treatment remains to be answered.

Expression of Prothrombinase/fibroleukin Gene fg12 in Lung Impairment in a Murine Severe Acute Respiratory Syndrome Model

To evaluate the role of murine fibrinogen like protein 2 (mfgl2) /fibroleukin in lung impairment in Severe acute respiratory syndrome (SARS), a murine SARS model induced by Murine hepatitis virus strain 3 (MHV-3) through trachea was established. Impressively, all the animals developed interstitial pneumonia with extensive hyaline membranes formation within alveoli, and presence of micro-vascular thrombosis in the pulmonary vessels. MHV-3 nucleocapsid gene transcripts were identified in multiple organs including lungs, spleen etc. As a representative proinflammatory gene, mfgl2 prothrombinase expression was evident in terminal and respiratory bronchioles, alveolar epithelia and infiltrated cells in the lungs associated with fibrin deposition and micro-vascular thrombosis. In summary, the established murine SARS model could mimic the pathologic characteristics of lungs in patients with SARS. Besides the physical damages due to virus replication in organs, the up-regulation of novel gene mfgl2 in lungs may play a vital role in the development of SARS associated lung damage.

Intravitreal injection of resveratrol inhibits laser-induced murine choroidal neovascularization

AIM:To determine the effects of intravitreal resveratrol(RSV)on murine laser-induced choroidal neovascularization(CNV).METHODS:The toxicity of RSV to choroidal endothelial cell(CEC)was measured using thiazolyl blue tetrazolium bromide(M一)assay.Effects of RSV on choroidal endothelial cell(CEC)migration were evaluated with a modified Boyden chamber assay,while tube formation was evaluated in a 2-D gel assay.CNV was induced by laser photocoagulation in mice.The effects of intravitreal injection of RSV on CNV development were evaluated by fluorescein angiography(FA),confocal analysis of isolectin B4 labeled choroidal flat mounts,and histologic examination of CNV membranes.Immunostaining was used to analyze the expression and phosphorylation of vascular endothelial growth factor receptor 2(VEGFR2).RESULTS:No significant cell toxicity was observed in CEC if the concentration of RSV was less than 200 pmol/L(P>0.05).RSV inhibited vascular endothelial growth factor(VEGF)-induced CEC migration(P<0.05)and tube formation(P<0.05)invitro.Furthermore,intravitrealinjectionof RSV significantly inhibited laser induced CNV formation in mice.The FA leakage,CNV volume and CNV area analysis revealed that there were 41%,45%,and 58%reduction in RSV-treated eyes(1.691±0.1032,178163±78623μm^3 and 6508±619.0μm^2,respectively)compared with those in control(2.724±0.08447,379676±98382μm3and16576±2646μm^2,respectively;P<0.05).Phospho-VEGFR2expression was much weaker in the sections of CNV lesions in RSV injected mice compared with that in control(P<0.05).CONCLUSION:Intravitreal injection of RSV exerts an inhibitory effect on CNV,which may through suppressing endothelial cell migration,tube formation and VEGFR2 phosphorylation.

MDM2的异常表达对胃癌细胞增殖、侵袭、迁移以及对CD4^(+)T和CD8^(+)T细胞免疫浸润的影响

目的 探讨鼠双微体同源基因2(murine double minute 2,MDM2)在胃癌中的表达,以及MDM2的表达对胃癌细胞增殖、侵袭、迁移以及CD4^(+)T和CD8^(+)T细胞免疫浸润的影响。方法 从基因表达综合(Gene Expression Omnibus,GEO)数据库中提取胃癌芯片数据集GSE62254,统计分析MDM2在胃癌中的表达情况。通过基因表达谱交互分析(Gene Expression Profiling Interactive Analysis,GEPIA)数据库分析MDM2表达对胃癌患者预后的影响。基于单样本基因集富集分析(single-sample gene-set enrichment analysis,ssGSEA)探讨GSE62254中23种免疫细胞的浸润情况。免疫组织化学法检测临床样本组织中MDM2和CD4^(+)T和CD8^(+)T细胞的表达。细胞实验,分为sh组(shRNA-MDM2下调MDM2表达)和sh-NC组(shRNA-MDM2-NC无下调MDM2表达的作用),si组(siRNA-MDM2降低MDM2表达)和si-NC组(siRNA-MDM2-NC无降低MDM2表达的作用),pc组(pcDNA3.1-MDM2过表达MDM2)和pc-NC组(pcDNA3.1-MDM2-NC无过表达MDM2的作用),mimic组(MDM2 mimic上调MDM2表达)和mimic-NC组(MDM2-NC无上调MDM2表达的作用)。动物实验,分为si组(下调MDM2表达)、si-NC组(无下调MDM2表达),mimic组(升高MDM2表达)、mimic-NC组(无升高MDM2表达),每组各5只小鼠。5-乙炔基-2′-脱氧尿苷(5-ethynyl-2′-deoxyuridine,EdU)以及Transwell小室检测各组细胞的增殖、迁移与侵袭性能。动物实验检测各组细胞的体内生长与转移能力;Western blot检测细胞和小鼠瘤体组织中MDM2、增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)、E-钙黏着蛋白(E-cadherin)和波形蛋白(Vimentin)的表达;同时细胞计数试剂盒(cell counting kit 8,CCK-8)检测小鼠脾组织单细胞悬液中CD8^(+)T细胞的体外杀伤肿瘤细胞的能力。结果 与癌旁正常组织相比,MDM2在胃癌组织的表达明显升高(P<0.05);与MDM2高表达患者相比,MDM2低表达患者的总生存期生存曲线明显升高(P<0.05);与MDM2高表达组相比,MDM2低表达组中CD4^(+)T、CD8^(+)T细胞的浸润明显升高(P<0.05);临床样本的免疫组织化学和相关性分析结果显示,MDM2的表达与CD4^(+)T、CD8^(+)T细胞的浸润水平呈负相关关系。细胞实验结果显示,与si-NC组相比,si组PAMC-82细胞中EDU阳性细胞比例、细胞侵袭和迁移数量以及细胞中MDM2、PCNA以及Vimentin的表达明显下降,E-cadherin的表达明显升高(P均<0.05);与mimic-NC组相比,mimic组PAMC-82细胞中EDU阳性细胞比例、细胞侵袭和迁移数量以及细胞中MDM2、PCNA以及Vimentin的表达明显升高,E-cadherin表达明显下降(P均<0.05)。动物实验结果显示,与si-NC组相比,si组小鼠瘤体组织的质量、病灶转移比例、瘤体组织中MDM2、PCNA和Vimentin的表达明显下降,瘤体组织中E-cadherin表达、CD4^(+)T免疫组织化学评分、CD8^(+)T免疫组织化学评分明显升高(P均<0.05);与mimic-NC组相比,mimic组小鼠瘤体组织的质量、病灶转移比例、瘤体组织中MDM2、PCNA和Vimentin的表达明显升高,瘤体组织中E-cadherin表达、CD4^(+)T免疫组织化学评分、CD8^(+)T免疫组织化学评分明显下降(P均<0.05)。小鼠脾组织中CD8^(+)T细胞对各组PAMC-82细胞的体外杀伤实验结果显示,si组细胞的存活率明显下降(P<0.05);与mimic-NC组相比,mimic组细胞的存活率明显升高(P<0.05);酶联免疫吸附试验(enzyme-linked immunosorbent assay,ELISA)结果显示,与si-NC组相比,si组细胞上清液中γ干扰素(interferon gamma,IFN-γ)及肿瘤坏死因子α(tumor necrosis factor alpha,TNF-α)的含量明显升高(P均<0.05),与mimic-NC组细胞相比,mimic组细胞中IFN-γ及TNF-α的含量明显下降(P均<0.05)。结论 在胃癌中,MDM2的表达升高,高表达的MDM2能明显促进细胞的增殖、迁移和侵袭,增强肿瘤细胞抵抗CD4^(+)T、CD8^(+)T细胞的杀伤能力,促进胃癌进展。

鼠β-防御素2(mBD2)真核表达质粒的构建及稳定表达株的鉴定

目的:对小鼠β防御素-2(mBD2)基因进行克隆,构建其真核表达载体,筛选出稳定表达细胞株,并研究mBD2的生物学特性及其抗肿瘤机制。方法:通过向BALB/c小鼠腹腔注射内毒素(LPS),建立小鼠急性时相反应,取其肺组织提取总RNA,采用RT-PCR方法扩增小鼠mBD2基因,经EcoRⅠ和XhoⅠ双酶切后插入相同酶切的pcDNA3.1(+)真核表达载体,对其进行酶切和测序鉴定。将构建好的真核表达质粒pcDNA3.1(+)/mBD2转染SiHa细胞,采用G418进行稳定表达株的筛选,用免疫荧光染色和RT-PCR鉴定细胞内mBD2蛋白表达情况。结果:提取小鼠肺组织总RNA,采用RT-PCR方法扩增了250bp左右的产物,通过EcoRⅠ和XhoⅠ双酶切,构建了真核表达质粒pcDNA3.1(+)/mBD2。SiHa被该质粒转染后,在100mg/LG418浓度下筛选20d,得到了稳定表达mBD2的细胞株,用免疫荧光染色显示mBD2蛋白在胞质中有大量表达,RT-PCR反应扩增到了mBD2的mRNA。结论:成功地构建了pcDNA3.1(+)/mBD2真核表达质粒,mBD2蛋白在SiHa细胞中能稳定表达,这些结果为进一步深入研究mBD2的生物学特性及其抗肿瘤的作用奠定了基础。

壳聚糖纳米颗粒包裹对鼠白细胞介素2基因表达和调节小鼠免疫效应的影响

本实验制备壳聚糖纳米颗粒 (CNP) ,包裹小鼠白细胞介素 2基因 (mIL 2 )真核表达质粒 (VRMIL 2 ) ,肌注接种 2 1d昆明小鼠 ,观察mIL 2基因体内表达及其对免疫应答和免疫保护的影响。实验结果发现 :CNP包裹VRMIL 2注射小鼠血液中IgG、IgM和IgA不同程度地增多 ,均显著高于CNP包裹空白质粒组 (P <0 .0 5 ) ;其血清中IL 2、IL 4和IL 6的含量明显升高 ,与对照组差异显著 (P <0 .0 5 ) ;外周血液的白细胞和淋巴细胞数量也较对照组显著增加。免疫后 35d以大肠杆菌口服攻毒实验小鼠 ,检测发现 :CNP包裹VRMIL 2组小鼠的上述免疫指标除中性粒细胞外均显著多于对照小鼠 ,VRMIL 2接种小鼠均健康存活 ,而对照小鼠均发病 ;尽管CNP包裹VRMIL 2接种小鼠的体液和细胞免疫指标与未包裹VRMIL 2免疫鼠差异不显著 (P >0 .0 5 ) ,但剂量仅为后者的 1/ 5。这些结果表明 :壳聚糖纳米颗粒包裹VRMIL 2可显著提高外源IL 2基因体内表达水平 ,明显增强体液和细胞免疫水平的效应 ,增强对大肠杆菌的抗病力 ,提示壳聚糖纳米颗粒包裹IL 2基因可明显增强动物的体液和细胞免疫 ,可作为有效的抗感染免疫调节剂。

鼠双微粒体2蛋白、P53在口腔白斑和鳞癌中的表达及其相关性的研究

目的研究鼠双微粒体2(MDM2)和P53在口腔白斑及鳞癌中的表达及其相关性。方法采用免疫组织化学SP方法对15例正常口腔黏膜组织、24例口腔白斑(OLK)组织及41例口腔鳞癌组织中的MDM2蛋白和P53蛋白进行检测。结果正常黏膜中未见MDM2和P53阳性表达,口腔白斑和口腔鳞癌组织中MDM2阳性率分别为58.3%和75.6%,P53的阳性率分别为37.5%和68.3%,与正常组相比均具有显著性差异(P<0.05)。口腔白斑和口腔鳞癌组相比,MDM2阳性率没有显著性差异(P>0.05),P53阳性率具有显著性差异(P<0.05)。两种指标进一步的相关性分析显示,MDM2与P53蛋白在口腔白斑组(P=0.018)及口腔鳞癌组(P=0.000)中均呈现正相关的关系。结论 MDM2在口腔白斑和口腔鳞癌中的高表达提示该基因在口腔鳞癌的发生发展中起显著作用,其与P53表达的相关性表明这二者可能在口腔鳞癌的形成过程中起协同作用。

IL-2和IL-12联合基因治疗小鼠肝癌的实验研究

目的 探讨瘤内注射共表达mIL 12和hIL 2质粒DNA抗小鼠肝癌皮下移植瘤的作用。方法 构建pDC5 11hIL2 mIL12、pDC5 11mIL 12、pDC5 11hIL 2真核表达质粒载体 ;ELISA方法检测各组质粒在真核细胞的表达 ;小鼠肝癌H2 2皮下移植瘤瘤内注射各组质粒DNA后 ,检测不同时间血清中细胞因子浓度 ;观察各组小鼠存活时间 ,肿瘤大小变化 ;并检测各组小鼠脾脏细胞毒T淋巴细胞 (cytotoxicTlymphocyte ,CTL)活性。对各治疗组在质粒DNA注射后一月进行瘤体组织学观察。结果 酶切鉴定各组质粒载体 ,均示构建成功 ,并能在真核细胞内高效表达相应细胞因子。瘤内注射各组质粒载体后 ,pDChIL2 mIL12组在不同时间表达的hIL2和mIL12分别与pDC5 11hIL2组 (F =71 11,P <0 0 1)、pDC5 11mIL12组 (F =3 0 70 ,P <0 0 5 )比较有显著性差异。mIL 12基因和hIL 2基因联合治疗组 ,肿瘤生长明显受抑制 ,疗效显著优于各单独治疗组和对照组 (P <0 0 5 ) ,并且小鼠脾细胞CTL杀伤活性增强。双基因联合治疗组 ,病灶内肿瘤细胞坏死明显 ,炎性细胞广泛浸润。结论 IL 12、IL 2基因治疗可抑制小鼠肝癌H2 2皮下移植瘤的生长 ,提高机体的抗肿瘤免疫应答 ,两者联合运用可产生协同效应。

大蒜素调节Bcl-2/Bax促进宫颈癌U14细胞凋亡的研究

目的探讨大蒜素对小鼠宫颈癌U14细胞凋亡的影响及作用机制。方法体外培养U14细胞,将细胞分为对照组(不加大蒜素处理组)和大蒜素组(质量浓度分别为5、10和20mg.L-1)。采用四甲基偶氮噻唑蓝法测定大蒜素作用24、48、72h时对U14细胞的增殖抑制率;膜联蛋白A5-绿色荧光素/碘化丙啶双染法流式细胞术检测U14细胞的凋亡率;逆转录聚合酶链反应和免疫印迹法分别检测U14细胞Bcl-2和Bax mRNA和蛋白的表达水平。结果 5、10和20mg.L-1大蒜素组对U14细胞增殖的抑制率:24h时分别为(6.6±1.41)%、(23.5±2.79)%和(58.9±1.65)%,48h时分别为(25.5±2.89)%、(47.9±8.78)%和(69.5±3.72)%,72h时分别为(58.9±1.66)%、(78.9±1.19)%和(92.6±7.33)%,均显著高于对照组(P<0.05),且细胞增殖抑制率呈浓度和时间依赖性。5、10和20mg.L-1大蒜素组作用24h后,细胞凋亡率分别为(9.22±0.55)%、(22.34±1.53)%和(35.73±1.98)%,与对照组的(3.23±0.35)%比较差异有统计学意义(P<0.05),且呈浓度依赖性。与对照组比较:10、20mg.L-1组Bcl-2mRNA和蛋白表达均下调(P<0.05),而10、20mg.L-1组Bax mRNA和蛋白表达均上调(P<0.05)。结论大蒜素可能通过上调Bax表达,下调Bcl-2的表达诱导U14细胞凋亡。

MDM2在消化系肿瘤中作用的研究进展

MDM2为小鼠双微体基因,是近几年发现的一种癌基因,对细胞生长有调节作用.其生物学作用是增强细胞的生存活力,使细胞生存期延长,促进细胞增生及肿瘤的生长.近年来,许多研究显示MDM2参与了许多肿瘤的发生发展,且该基因与恶性肿瘤的浸润、转移和不良预后有关,尤其与食管癌、胃癌、结肠癌和肝癌等消化系肿瘤关系密切.因此,研究MDM2与消化系肿瘤的关系在肿瘤防治中具有重要的意义.本文结合国内外文献就MDM2在消化系肿瘤发生发展及其转移过程的研究进展作一综述.

TNFα、IL-6、IL-4、IL-2对IFNγ抗弓形虫感染作用的影响

目的探讨 TNFα、IL- 6、IL- 4、IL- 2对 IFNγ诱导的小鼠腹腔巨噬细胞 ( mouse peritoneal maerophage,MPM)抗弓形虫 ( toxoplasm a gondii,TG)效应的机制。方法应用 3H- U标记的 TG在 MPM内的增殖实验及 1 2 5 I- Ud R标记的细胞毒实验 ,结果和结论 1高浓度 TNFα只能诱导 MPM轻微的抗 TG效应 ,而与亚剌激量 IFNγ结合几乎可以完全抑制 TG增殖 ;抗TNFα在 IFNγ诱导 MPM的最初阶段 ,可消除 IFNγ诱导的 ΜΡΜ 的抗 ΤG效应 ,与 ΙFNγ诱导 ΜΡΜ 产生内源性 ΤΝ Fα的作用相同。2 IL- 6可促进 TG在 MPM内的增殖 ,并能逆转 IFNγ诱导的 MPM抗 TG效应。3IL- 4在体外可部分抑制 TG在MPM内的增殖 ,其作用机制与 TNFα无关 ,但与 IFNγ有相加作用。4体外应用 IL- 2对 MPM抗 TG作用无影响 ;体内应用IL- 2明显延长急性 TG感染小鼠的生存时间 ( P<0 .0 5 ) ,治疗组小鼠脾细胞杀伤肿瘤细胞及 TG感染自身细胞的能力 ,均明显高于对照组 ( P<0 .0 0 1) ;而正常小鼠 NK细胞及 L AK细胞杀伤自身感染 TG靶细胞能力 ,显著低于杀伤肿瘤细胞的能力 ( P<0 .0 0 1) ;经 IL- 2诱导的 L AK细胞杀伤自身感染 TG靶细胞的能力 ,明显高于 NK细胞 ( P<0 .0 0 1) ,并与 L AK细胞杀伤肿瘤靶细胞的能力无明显差别 ( P>0 .0 5 )

新生血管抑制分子IP-10/Crg-2的cDNA克隆及序列鉴定

目的： 拟获得编码ＩＰ１０ （ＩＦＮγｉｎｄｕｃｉｂｌｅ ｐｒｏｔｅｉｎ１０） 和Ｃｒｇ２ （ｃｙｔｏｋｉｎｅ ｒｅｓｐｏｎｓｉｖｅ ｇｅｎｅ２） 的ｃＤＮＡ 序列。方法： 针对ＩＰ１０ 和Ｃｒｇ２ 的ｃＤＮＡ序列设计相应引物， 通过反转录ＰＣＲ技术， 分别从用ＩＦＮγ及ＴＮＦα处理的人成纤维细胞及Ｂａｌｂ／ｃ 小鼠肝脏中， 扩增出编码ＩＰ１０ 和Ｃｒｇ２ 的全基因序列， 并将其克隆入载体ｐＵＣ１９及ｐＧＥＭ３Ｚｆ （＋ ） 中， 通过酶切及序列测定鉴定重组载体。结果： 经序列测定证实， 重组载体含有正确地分别编码ＩＰ１０ 及Ｃｒｇ２ 的ｃＤＮＡ序列。结论： 获得的阳性克隆分别含有３０６ｂｐ 和３１４ｂｐ 的重组片段， 为进一步对其生物学活性和配体进行研究奠定了基础。

抗小鼠TLR-2胞外段B细胞识别表位抗体抑制肉瘤生长的初步研究

目的观察抗小鼠TLR-2胞外段B细胞识别表位抗体对小鼠肉瘤S180生长的影响。方法在对小鼠Toll样受体2(mTLR-2)B细胞优势表位预测的基础上,合成B细胞识别表位20mer短肽,将其与载体蛋白偶联,制备免疫原。所得兔抗mTLR-2胞外段B细胞识别表位多克隆抗体TSP-1纯化后,采用Westernblotting、免疫组织化学和流式细胞仪进行初步鉴定。小鼠肉瘤株S180细胞注射小鼠左后肢,其中实验组混合100μg纯化抗体TSP-1,无关免疫球蛋白对照组混合100μg正常兔IgG,空白对照组仅接种S180。小鼠经麻醉分别于10、14、18d处死,称量瘤质量并计算抑瘤率。结果Westernblotting显示在相对分子质量约95000处可见清晰的反应条带;免疫组织化学和流式细胞术检测显示抗体可与表达天然mTLR-2的J774A.1细胞反应;实验组小鼠肉瘤生长明显受到抑制,其瘤质量在10、14、18d与对照组相比差异显著(P<0.05);抑瘤率分别为77%、51%和53%。结论局部应用抗mTLR-2胞外段B细胞识别表位抗体可抑制小鼠肉瘤S180生长,且表现在肿瘤生长的早期。

卵巢上皮性癌组织中MDM2蛋白的表达及其临床意义

目的:探讨人的小鼠双微粒体(MDM2)蛋白在正常卵巢组织、卵巢良性上皮性肿瘤组织及卵巢上皮性癌组织中的表达,阐明其表达与卵巢上皮性癌临床病理特征的关系。方法:选取手术切除的组织标本,其中正常卵巢组织20例、卵巢良性上皮性肿瘤组织20例和卵巢上皮性癌组织58例,应用免疫组织化学法检测MDM2蛋白的表达情况。结果:MDM2蛋白在卵巢上皮性癌组织中的表达水平明显高于正常卵巢组织和卵巢良性上皮性肿瘤组织(P<0.05),MDM2蛋白在卵巢上皮性癌组织中的阳性表达率随手术病理分期的升高而增高,但在不同分化程度和组织学类型中的表达差异无统计学意义(P>0.05)。结论:MDM2蛋白的高表达可能促进卵巢癌的发生发展,其在卵巢上皮性癌组织中的高表达可能预示着该肿瘤侵袭性高、预后差、易复发。

人着色性干皮病基因D对HepG2细胞Mdm2和Mdm4表达的影响

目的:探讨人剪切修复基因着色性干皮病基因D(xeroderma pigmentosum D,XPD)对肝癌细胞鼠双微体2(murine double minute 2,Mdm2)和鼠双微体4(murine double minute 4,Mdm4)表达的影响。方法:用脂质体转染法将重组质粒pEGFP-N2/XPD和空载质粒pEGFP-N2转染进入人肝癌细胞株HepG2,实验分为3组:(1)空白对照组;(2)pEGFP-N2组;(3)pEGFP-N2/XPD组。用MTT法观察细胞的增殖活力;用流式细胞术检测细胞周期和凋亡率;用RT-PCR和Western blotting检测XPD、Mdm2、Mdm4和P53表达量的变化。结果:MTT结果显示,重组质粒pEGFP-N2/XPD的转染抑制了肝癌细胞的增殖活力;流式细胞术结果显示,重组质粒pEGFP-N2/XPD的转染引起了G1期细胞增加,S期减少,凋亡率增加。RT-PCR和Western blotting检测发现,重组质粒pEGFP-N2/XPD的转染使得XPD表达增高,同时使得Mdm2和Mdm4表达降低,P53表达增高。结论:XPD能下调肝癌细胞中Mdm2和Mdm4的表达,上调P53表达,并能抑制肝癌细胞增殖及诱导其凋亡。

小鼠TLR-2N末端基因的克隆表达和抗体制备

目的克隆mTLR-2基因氨基端序列,并表达和纯化N端融合蛋白,制备抗mTLR-2N末端的多克隆抗体。方法采用PCR技术扩增编码mTLR-2N端1～153氨基酸的基因,并将其克隆到pET32A载体中,测序验证;用大肠杆菌表达融合蛋白,并以Probond树脂柱纯化;免疫家兔制备多克隆抗体,采用免疫组化、流式细胞术及间接ELISA检测抗体特异性及效价。结果成功构建了融合表达载体pET-N,表达和纯化了相应的融合蛋白,所制备多克隆抗体可与pGEX-N表达的融合蛋白反应,并可结合表达TLR-2的RAW264.7及转染mTLR-2全长基因的CHO细胞。结论获得了mTLR-2N末端重组融合蛋白及其可与天然mTLR-2结合的多克隆抗体。