中国流行株HIV-1Gag与IFN-α2b重组质粒的构建与实验免疫研究

目的探讨中国流行株 ＨＩＶ－ １Ｇａｇ与 ＩＦＮ－ α２ｂ共表达重组核酸疫苗质粒的免疫效果。方法以 核酸疫苗质粒ｐＩＲＥＳ１ｎｅｏ为表达载体，构建重组核酸疫苗质粒ｐＩＲＥＳ１－Ｇａｇ、ｐＩＲＥＳ１－Ｇａｇ－ＩＦＮ，通过间接免疫荧光 试验、ＤｏｔＥＬＩＳＡ检测Ｃａｇ／ｈＩＬ－２／ｈＩＬ－６基因的表达产物。另将此重组核酸疫苗质粒免疫ＢＡＬＢ／ｃ小鼠，进行淋巴细 胞转化试验、ＣＤ４＋、ＣＤ８＋Ｔ淋巴细胞数量测定、细胞毒性Ｔ淋巴细胞（ＣＴＬ）特异性杀伤作用检测及血清抗体检测。 结果构建的重组质粒转染ＢＨＫ细胞后可表达目的基因，免疫小鼠后可有效地刺激淋巴细胞增殖，诱导特异性 ＣＴＬ反应，当和 ＩＦＮ－α２ｂ共表达时免疫效果更加显著。结论与 Ｇａｇ蛋白共表达的 ＩＦＮ－ａ２ｂ能够进一步提高细胞 免疫与体液免疫水平，构建的重组质粒为ＨＩＶ－１ＤＮＡ疫苗的研究奠定了一定实验基础。

HIV-1gag/IFNα-2b表达产物免疫小鼠的实验研究

为了将艾滋病病毒核心蛋白(gag)与干扰素(IFNα-2b)融合基因表达的融合蛋白作为免疫原免疫小鼠,观察小鼠的体液免疫和细胞免疫应答。将IFNα-2b基因片段插入到gag基因的nt531位点,经脂质体转染与血凝素阴性蚀斑筛选出重组痘苗病毒。经SDS-PAGE和Westexn blot鉴定表达产物。用重组病毒vJ38gag/IFNα-2b免疫小鼠,用ELISA方法检测血清IgG抗体含量,用流式细胞仪测定小鼠脾CD4^+、CD8^+T淋巴细胞计数。结果表明,血清IgG抗体含量逐渐增高,实验组与对照组比较差异有显著意义(P<0.05)。CD4^+、T淋巴细胞计数与对照组比较差异有显著意义(P<0.05)。结论:重组痘苗病毒vJ38gag/IFNct-2b能增强小鼠的体液免疫和诱导细胞免疫。

HIV-Specific IL-2^+ and/or IFN-γ^+ CD8^+ T Cell Reponses during Chronic HIV-1 Infection in Former Blood Donors

Objective Conflicting data have been generated from previous studies to determine which kind of relationship exists between HIV-1 specific CD8 Tcell responses and HIV-1 viral load or CD4 count over the course of infection.In this study,153 HIV-1 infected LTNPs were enrolled to investigate the role of HIV-1 specific CD8 T-cell responses in chronic HIV-1 infection among HIV-1 infected former blood donors.Methods The patients were stratified into three groups according to CD4 count：CD4≥500 cells/μL;350 cells/μL≤CD4〈500 cells/μL;CD4〈350 cells/μL.PBMCs were isolated from the patients＇ anticoagulated blood samples.IL-2 and IFN-γ secretions of CD 8 T cells against 17 HIV-1 consensus B full peptide pools were analyzed by using ICS assay.Results An overall inverse correlation were observed between CD4 count and plasma viral load.Although no significant difference was observed during the comparisons of frequency/breadth of HIV-1 specific CD8 T cell responses,CD4 count stratification analysis showed that different correlation pattern existed in three strata：as for patients whose CD4 counts were less than 350 cells/μL,no significant correlations were identified between frequency/breadth of HIV-1 specific CD8 T cell responses and CD4 count/viral load;as for patients whose CD4 counts ranged from 350 cells /μL to 500 cells/μL,significant correlation was only observed between the response breadth of IL-2＋IFN-γ＋ CD8 T cells and CD4 count;however,as for patients whose CD4 counts were more than 500 cells/μL,direct correlations were identified between IL-2＋IFN-γ＋/IL-2＋/IFN-γ＋ CD8 T cells and viral load or CD4 count.Conclusions Universal consistent inverse correlation was only indentified between CD4 count and viral load.The relationship between HIV-1 specific CD8 T cell responses and CD4 count/viral load varied in different CD4 strata,which showed that better preserved CD4 T cells were correlated with better CD8 T cell functions.

中国流行株HIV-1gag和hIL-2/hIL-6核酸疫苗构建与实验免疫研究

目的探讨中国流行株 HIV- 1gag与 h IL - 2 /h IL - 6共表达重组核酸疫苗质粒的免疫效果。方法以核酸疫苗质粒 p IRES1neo为表达载体 ,构建重组核酸疫苗质粒 p IRES1- gag、p IRES1- gag- h IL- 2、p IRES1- gag- h IL- 6 ,通过间接免疫荧光试验、Dot- EL ISA检测 gag/h IL - 2 /h IL - 6基因的表达产物。另将此重组核酸疫苗质粒免疫 Balb/c小鼠 ,进行淋巴细胞转化试验、CD4+ 、CD8+ T淋巴细胞数量测定、细胞毒性 T淋巴细胞 (CTL )特异性杀伤作用检测及血清抗体检测 ,结果构建的重组质粒转染 BHK细胞后可表达目的基因 ,免疫小鼠后可有效地刺激淋巴细胞增殖、诱导特异性 CTL 反应 ,当和 h IL- 2 /h IL- 6共表达时免疫效果更加显著。讨论与 Gag蛋白共表达的 h IL- 2 /h IL- 6能够进一步增强免疫鼠的细胞免疫与体液免疫水平 ,构建的重组质粒为 HIV-

IL-2、IFN-α和IFN-γ上调肾透明细胞癌786-0细胞B7-H1的表达

目的:研究IL-2、IFN-α和IFN-γ对人肾透明细胞癌786-0细胞上B7-H1表达的影响。方法:IL-2、IFN-α和IFN-γ刺激786-0细胞,RT-PCR检测刺激后786-0细胞B7-H1mRNA的表达,免疫细胞化学、免疫荧光染色和流式细胞术检测刺激后786-0细胞中B7-H1蛋白的表达。结果:RT-PCR检测结果显示,IL-2、IFN-α和IFN-γ组786-0细胞的B7-H1mRNA表达量明显高于未经刺激的786-0细胞(0.75±0.06、0.68±0.05、0.95±0.08vs0.30±0.03,P(0.05或P<0.01);免疫细胞化学和免疫荧光检测结果显示,B7-H1蛋白主要表达在786-0细胞的细胞膜上,IL-2、IFN-α和IFN-γ刺激后B7-H1表达明显上调;流式细胞术检测结果显示,IL-2、IFN-α和IFN-γ组786-0细胞的B7-H1分子表达阳性率明显高于未经刺激的786-0细胞[(65.70±3.26)%、(56.52±1.75)%、(84.05±3.52)%vs(20.49±1.03)%,P<0.01]。结论:IL-2、IFN-α和IFN-γ均上调786-0细胞B7-H1mRNA和蛋白的表达,其中IFN-γ上调程度最高,IFN-α上调程度最低。

HIV-1中国流行株gag与hIL-2在重组痘苗病毒中的共表达及其与核酸疫苗的实验免疫研究

目的：将HIV-1中国流行株B亚型gag基因、gag和hIL-2基因在天坛株痘苗病毒中进行共表达，以期获得重组痘苗病毒，观察细胞因子的佐剂作用，与核酸疫苗混合免疫，评价免疫效果，为新型艾滋病疫苗研制开发打下基础。方法：将HIV-1中国流行株 gag基因、gag和hIL-2基因片段插入到 pJ38载体启动子下游，经同源重组和血凝素阴性空斑筛选重组痘苗病毒，SDS-PAGE、Western blot检测目的蛋白。以重组病毒和核酸疫苗免疫Balb/c小鼠，进行淋巴细胞转化实验、CTL、CD4+、CD8+ T细胞数目以及血清抗体的细胞免疫和体液免疫指标检测。结果：获得了重组痘苗病毒 vJ38gag和 vJ38gag-IL-2。与 vJ38-gag相比，vJ38gag-IL-2，具有更好的免疫原性，重组痘苗病毒免疫3次的效果好于重组病毒免疫2次，以2rVV-DNA混合免疫效果最好。结论：重组痘苗病毒vJ38gag和vJ38gag-IL-2能够表达外源蛋白并诱导机体产生细胞免疫和体液免疫。细胞因子IL-2发挥了免疫佐剂的作用。

HIV-1中国流行株gag-hIL-2重组痘苗病毒与pIRES-gag-hIL-2核酸疫苗联合免疫的实验研究

目的 将HIV 1中国流行株B亚型gag和hIL 2基因在天坛株痘苗病毒中进行共表达 ,与核酸疫苗联合免疫 ,评价免疫效果 ,为新型艾滋病疫苗开发研制奠定基础。方法 将HIV 1中国流行株gag hIL 2基因片段插入到痘苗病毒载体pJ38启动子下游 ,经同源重组和血凝素阴性空斑筛选重组痘苗病毒 ,SDS PAGE、Westernblot检测目的蛋白。以重组病毒和核酸疫苗免疫BALB c小鼠 ,进行淋巴细胞转化实验及血清抗体的细胞免疫和体液免疫指标检测。结果 获得了重组痘苗病毒vJ38gag IL 2 ,具有更好的免疫原性 ,3rVV效果好于 2rVV ,以 2rVV DNA混合免疫效果最好。结论 重组痘苗病毒vJ38gag IL

Differential Expressions of Selected Activating and Inhibitory Receptors on K562-Stimulated Natural Killer (NK) Cells in HIV-1 and HIV-2 Infections

Context: The functional activity of NK cells depends on the balance between the engagement of activating and inhibitory receptors on the cell surface with their ligands, which enables them to kill infected cells. Objectives: The aim of this study was to evaluate and compare expressions of selected activating and inhibitory receptors on stimulated NK cells in HIV-1 and HIV-2 infections. Methods: PBMCs were analysed for activating (NKp30, NKp44, NKp46) and inhibitory (CD158a, CD158b, p70) receptor expressions in 30 HIV-1, 30 HIV-2 and 30 HIV uninfected healthy control (HC) subjects by flow cytometry after stimulating with K562 cells. Results: There was an expression of other receptors following an already in vitro engagement of NK cells with K562 cells. Higher expression of the activating receptors, NKp44 (p = 0.029) and NKp46 (p = 0.032) on NK cells from HIV-2 compared to HIV-1 infected individuals but similar NKp30 expression (p = 0.980). The levels of expression of inhibitory receptor CD158a were similar between HIV-1 and HIV-2 infected subjects (p = 0.309) but there was significant up-regulation of inhibitory receptors p70 (p = 0.010) and CD158b (p = 0.05) in HIV-1 compared to HIV-2 subjects. Conclusion: Despite the in vitro engagement of NK cells with stimulating K562 cells, our data showed differential expressions of other selected activating and inhibitory receptors in HIV-1 and HIV-2 infected subjects.

中国汉族人HIV-1辅助受体等相关基因CCR5、CCR2b、CXCR4和SDF1编码区SNP位点调查

目的调查中国汉族人群中HIV-1感染相关基因CCR5、CCR2b、CXCR4及SDF1编码区的基因多态性特点,为我国的艾滋病防治提供基础数据。方法 CCR5用2对引物进行PCR扩增,用PCR产物做模板直接测序。CCR2b编码区经PCR扩增后,用测序引物逐段分别测序。CXCR4(cDNA编号AF147204)编码区用2对引物进行PCR扩增,然后测序。SDF1编码区用4对引物进行PCR扩增,然后分别测序。样本总数为45例,测序结果用DNAstar综合分析,寻找和鉴定SNP位点。结果 CCR5基因编码区共发现6个SNP位点,4个引起氨基酸改变,1个单碱基缺失,引起移码突变和翻译提前终止。184A→G、503G→T、668G→A、999G→T等位基因频率分别为1.1％、21.1％、8.9％和10.0％。CCR2b编码区共发现8个SNP位点,6个错义突变,即43位G→C、190位G→A、260位C→A、302位C→A、315位G→C、433位G→A,突变频率分别为:30.0％、27.8％、32.2％、5.6％、10.0％和3.3％。CXCR4编码区共发现7个SNP位点,3个错义突变即38位C→T、90位A→T、712位A→C,1个终止突变:106位G→T,基因突变频率分别为:4.4％、4.4％、10.0％和3.3％。在SDF1编码区发现1个错义SNP位点:192位G→T,突变频率为8.9％;1例单碱基缺失:100位T缺失(100△T),引起34位氨基酸移码突变。结论中国汉族人HIV-1相关基因编码区有自己的多态性特点。4个HIV-1相关基因编码区共找到22个SNP位点,17个为首次报道;2个单碱基缺失均导致移码突变和翻译提前终止,1个已经报道。它们对HIV-1感染和艾滋病病程的影响值得进一步研究。

Gag/IFNα-2b融合基因在痘苗病毒中共表达研究

目的 本实验将编码AIDS病毒 (HIV -1)核心蛋白gag与编码干扰素 (IFNα -2b)基因插入以痘苗病毒复制非必需区血凝素 (HA)基因为侧翼 ,牛痘病毒包涵体 (ATI)启动子和串联的p7 5突变型早期启动子为基本构件的痘苗病毒表达载体 (pJ3 8) ,经与野生型痘苗病毒在细胞内同源重组 ,获得具有生物活性的重组痘苗病毒vJ3 8gag/IFNα -2b。方法 经免疫荧光、Dot -ELISA、SDS -PAGE、Western -blot等方法检测表达产物 ,分析免疫小鼠后血清抗体IgGOD4 90 值与T淋巴细胞的变化。结果 vJ3 8gag/IFNα -2b能表达Gag/IFNα -2b融合蛋白 ,分子量约 60kDa。免疫小鼠实验表明血清抗体IgGOD4 90 值、CD+ 4、CD+ 8T淋巴细胞计数的组间比较 (P <0 0 0 1) ,含IFNα -2b与单纯vJ3 8gag组相比 (P >0 0 5) ,但呈渐进性增高的趋势。 结论 重组痘苗病毒表达的gag/IFNα

HIV-2 Gag蛋白的表达研究

HIV-2是引起艾滋病的主要病原之一,与HIV-1相比,其致病性弱,感染的潜伏期长,有的甚至不发展成艾滋病。但HIV-2的易感宿主较HIV-1广,除人和猩猩之外,HIV-2还能感染猴等灵长类动物,这将为艾滋病疫苗和实验动物模型的研究提供有利条件。 我们应用原核高效表达载体pBV220在大肠杆菌中分别表达了HIV-2gag全部和部分蛋白(去掉与pol重叠序列)。在此基础上我们又将gag全部和部分序列置于痘苗病毒P7.

原发性免疫性血小板减少症(ITP)患者CD5^+B细胞对CD4^+T细胞Th1/Th2型细胞因子分泌的影响

目的探讨原发性免疫性血小板减少症(immune thrombocytopenia,ITP)患者CD5+B细胞对CD4+T细胞分泌Th1/Th2型细胞因子的调节作用及其在大剂量地塞米松(high dose dexamethasone,HD-DXM)治疗后的变化。方法采集5例初发原发性ITP患者HD-DXM治疗前后外周静脉血各20 mL及5例健康对照者外周静脉血20 mL,Ficoll密度梯度离心法分离外周血单个核细胞(peripheral blood mononuclear cell,PBMC),进一步以免疫磁珠法分选CD5+B细胞、CD5-B细胞和CD4+T细胞。CD5+B细胞或CD5-B细胞与CD4+T细胞按1∶9、1∶5、1∶3、1∶1、3∶1的梯度比例混合培养72 h或144 h。ELISA方法检测细胞培养上清液中IFN-γ(代表Th1型细胞因子)和IL-4(代表Th2型细胞因子)水平。结果共培养72 h后,健康对照者CD5+B细胞与CD4+T细胞比例在1∶3时,细胞培养上清液IFN-γ浓度与T细胞单独培养时相比明显下降[(2 427.99±632.62)pg/mL vs.(1 109.25±338.10)pg/mL,P=0.001 2)];而ITP患者CD5+B细胞与CD4+T细胞比例在3∶1时才对IFN-γ的分泌有显著抑制[(3 060.02±493.98)pg/mL vs.(1 769.45±634.73)pg/mL,P=0.000 3]。共培养144 h后得到相似的结果。HD-DXM治疗有效的ITP患者CD5+B细胞与CD4+T细胞比例在1∶1时共培养72 h后,对IFN-γ的分泌有明显抑制[(3 600.02±838.00)pg/mL vs.(1 157.97±383.20)pg/mL,P<0.000 1]。健康对照者及ITP患者CD5+B细胞对CD4+T细胞分泌IL-4均无明显影响。结论原发性ITP患者CD5+B细胞抑制CD4+T细胞分泌Th1型细胞因子IFN-γ的能力明显受损,经HD-DXM治疗后CD5+B细胞抑制IFN-γ分泌的能力可部分恢复。

低分子柑桔果胶粉对哮喘小鼠Th1/Th2平衡及核因子NF-κB表达的影响

目的探讨核因子-κB(NF-κB)和Th1/Th2免疫失衡在哮喘小鼠模型中的作用及低分子柑桔果胶粉防治的机制。方法用卵清白蛋白(OVA)建立哮喘模型。BALB/c小鼠随机分为四组:正常对照组、哮喘组、低分子柑桔果胶治疗组、地塞米松治疗组,每组10只。留取支气管肺泡灌洗液(BALF)进行细胞总数计数和分类计数;应用ELISA法检测BALF中IL-4、IFN-γ浓度,采用免疫组化检测NF-κB的表达。结果低分子柑桔果胶粉治疗组血和BALF中IL-4的含量明显低于哮喘组(P<0.05);低分子柑桔果胶粉治疗组哮喘小鼠肺组织中NF-κB阳性细胞百分比显著低于哮喘组(P<0.05);哮喘小鼠肺组织中NF-κB表达与BLAF中的IL-4浓度成显著正相关(P<0.05),而与BLAF中的IFN-γ浓度成显著负相关(P<0.01)。结论低分子柑桔果胶粉能降低支气管哮喘小鼠血清及BALF中炎症因子IL-4的浓度,减轻支气管哮喘模型小鼠肺组织病理损害,可能的机制是调节Th1/Th2平衡及抑制NF-κB激活,减少气道上皮的NF-κB表达,从而阻止哮喘的发生发展。

干扰素α2b和λ1体外抗呼吸道合胞病毒活性研究

目的分析干扰素(interferon,IFN)α2b和λ1在Hep2细胞和人呼吸道上皮细胞(human airway epithelium,HAE)中抗呼吸道合胞病毒(respiratory syncytial virus,RSV)病毒活性。方法在Hep2细胞中,RSV(MOI=0.01)感染后,加入IFN-α2b或IFN-λ1,48 h后观察细胞病变(cytopathic effect,CPE)、RT-qPCR方法测定病毒载量、免疫荧光法检测RSV F蛋白及结晶紫法检测细胞存活率。在HAE细胞中,用IFN-α2b和IFN-λ1预处理24 h后,RSV(MOI=0.01)感染HAE,RT-qPCR方法测定第1~7天培养上清中的病毒载量,免疫荧光法检测RSV F蛋白及空斑法测定第7天培养上清中的病毒滴度。结果在Hep2细胞中,IFN-α2b和IFN-λ1处理组的CPE较病毒对照组均有所缓解,且均是高浓度组干扰素的CPE轻于低浓度组。不同浓度的IFN-α2b和IFN-λ1均可以显著降低RSV病毒载量(P<0.001),且高浓度组病毒载量明显低于低浓度组(P<0.001)。此外,IFN-α2b和IFN-λ1均能够降低RSV感染后F蛋白表达量,同时提高细胞存活率。在HAE细胞中,IFN-α2b和IFN-λ1均能抑制RSV病毒复制,降低病毒滴度(P<0.001)和降低RSV F蛋白表达量。结论IFN-α2b和IFN-λ1在传代细胞Hep2和HAE中对RSV均有较好抗病毒活性,为干扰素抗呼吸道病毒研究提供了数据参考。

Env/IFNα-2b融合基因在痘苗病毒中共表达研究

目的 本实验选择的真核表达载体 pJ16 ,是以痘苗病毒复制非必需区血凝素 (HA)基因为侧翼 ,以牛痘病毒包涵体 (ATI)启动子和串联的 p7 5突变型早期启动子为基本构件的痘苗病毒表达载体。插入编码AIDS病毒 (HIV -1)外膜蛋白env与编码干扰素IFNα - 2b基因。方法 经与野生型痘苗病毒在细胞内同源重组 ,挑选HA-斑。获得重组痘苗病毒vJ16env/IFNα - 2b。经免疫荧光、Dotblot、SDS -PAGE、Westernblot和免疫小鼠后血清抗体IgGOD值检测。结果 vJ16en/IFNα - 2b能表达Env -IFNα - 2b融合蛋白 ,分子量约 10 0kDa。免疫小鼠实验 ,血清抗体IgGOD值组间均数比较 (P <0 0 0 1) ,含IFNα- 2b与vJ6env组比较 (P >0 0 5 ) ,但有增高趋势。结论 重组病毒表达的Env -IFN融合蛋白具有良好的反应原性和免疫原性。

应用ELISPOT方法筛选确定HIV-1 B／C亚型疫苗六种抗原的H-2^d限制的T细胞表位

为了筛选和确定用于检测表达HIV-1 B'/C亚型病毒6种抗原(gp160、gag、polr、evt、at和nef)的艾滋病疫苗免疫小鼠后H-2d限制的特异性T细胞表位,本研究使用表达上述6种抗原的复制型DNA疫苗和非复制型重组痘苗病毒疫苗联合免疫BALB/c小鼠,通过矩阵设计将HIV-1 B(C)亚型6种相应抗原全序列肽库分别混合成肽池,使用肽池对免疫小鼠进行IFN-γELISPOT检测,根据检测结果确定肽库中特异反应的优势表位肽。结果显示:筛选到七条针对Gag的特异表位肽,其中有5条与文献报道相同,另2条为新表位肽;筛选到3条针对Pol蛋白特异表位肽,其中一条为新表位肽;筛选到2条针对gp160特异表位肽,其中一条为新表位肽;在Nef肽库中筛选到一条新的表位肽;从Tat肽库中筛选到3条表位肽,这三条肽在肽库中是连续的序列,都包含(或部分包含)网上公布的表位序列;在Rev肽库中没有筛选到能够产生阳性反应的特异性表位肽。本研究使用IFN-γELISPOT方法筛选和确定了可用于检测表达HIV-1 B'/C亚型病毒6种抗原(gp160、gag、pol、revt、at和nef)的艾滋病疫苗免疫小鼠后H-2d限制的特异性T细胞表位。

Interferon-β induced in female genital epithelium by HIV-1 glycoprotein 120 via Toll-like-receptor 2 pathway acts to protect the mucosal barrier

More than 40%of HIV infections occur via female reproductive tract(FRT)through heterosexual transmission.Epithelial cells that line the female genital mucosa are the first line of defense against HIV-1 and other sexually transmitted pathogens.These sentient cells recognize and respond to external stimuli by induction of a range of carefully balanced innate immune responses.Previously,we have shown that in response to HIV-1 gp120,the genital epithelial cells(GECs)from upper reproductive tract induce an inflammatory response that may facilitate HIV-1 translocation and infection.In this study,we report that the endometrial and endocervical GECs simultaneously induce biologically active interferon-β(IFNβ)antiviral responses following exposure to HIV-1 that act to protect the epithelial tight junction barrier.The innate antiviral response was directly induced by HIV-1 envelope glycoprotein gp120 and addition of gp120 neutralizing antibody inhibited IFNβproduction.Interferon-βwas induced by gp120 in upper GECs through Toll-like receptor 2 signaling and required presence of heparan sulfate on epithelial cell surface.The induction of IFNβwas dependent upon activation of transcription factor IRF3(interferon regulatory factor 3).The IFNβwas biologically active,had a protective effect on epithelial tight junction barrier and was able to inhibit HIV-1 infection in TZM-bl indicator cells and HIV-1 replication in T cells.This is the first report that recognition of HIV-1 by upper GECs leads to induction of innate antiviral pathways.This could explain the overall low infectivity of HIV-1 in the FRT and could be exploited for HIV-1 prophylaxis.

HIV-1 Vpr protein activates the NF-κB pathway to promote G2/M cell cycle arrest

Viral protein R(Vpr) plays an important role in the replication and pathogenesis of Human immunodeficiency virus type 1(HIV-1). Some of the various functions attributed to Vpr, including the induction of G2/M cell cycle arrest, activating the NF-κB pathway, and promoting viral reverse transcription, might be interrelated. To test this hypothesis, a panel of Vpr mutants were investigated for their ability to induce G2/M arrest and to activate the NF-κB pathway. The results showed that the Vpr mutants that failed to activate NF-κB also lost the activity to induce G2/M arrest, which suggests that inducing G2/M arrest via Vpr depends at least partially on the activation of NF-κB. This latter possibility is supported by data showing that knocking down the key factors in the NF-κB pathway – p65, Rel B, IKKα, or IKKβ– partially rescued the G2/M arrest induced by Vpr.Our results suggest that the NF-κB pathway is probably involved in Vpr-induced G2/M cell cycle arrest.

The Immunity Induced by Recombinant Spike Proteins of SARS Coronavirus in Balb/c Mice

The immune effect of two recombinant protein fragments of spike protein in severe acute respiratory syndrome coronavirus (SARS CoV) was investigated in Balb/c mice. Two partial spike gene fragments S1 (322-1464 bp) and S2 (2170-2814 bp) of SARS coronavirus were amplified by RT-PCR, and cloned into pET-23a prokaryotic expression vector, then transformed into competent Escherichia E.coli BL21 (DE3)(pLysS) respectively. Recombinant proteins were expressed and puri- fied by Ni2+ immobilized metal ion affinity chromatography. The purified proteins mixed with com- plete Freund adjuvant were injected into Balb/c mice three times at a two-week interval. High titer antibody was detected in the serum of immunized Balb/c mice, and mice immunized with S1 protein produced high titer IgG1, IgG2a, IgG2b and IgG3, while those immunized with S2 protein produced high titer IgG1, IgG2a, but lower titer IgG2b and IgG3. Serum IFN-γ concentration was increased significantly but the concentrations of IL-2, IL-4 and IL-10 had no significant change. And a marked increase was observed in the number of spleen CD8+ T cells. The results showed that recombinant proteins of SARS coronavirus spike protein induced hormonal and cellular immune response in Balb/c mice.

中国人类免疫缺陷病毒-1B亚型Gag蛋白特异性T淋巴细胞的免疫应答

大量研究证明，细胞免疫特别是HIV特异性CTL在控制HIV感染中发挥关键作用。HIV-1特异性CTL应答不仅由HIV-1特异性抗原蛋白结构决定，同时也受到特异性人类白细胞抗原（HLA）I类抗原的限制。不同人群HLA—I类基因型分布频率不同，决定了不同人群HIV-1特异性CTL应答模式的不同。