DNA vaccine encoding Der p2 allergen down-regulates STAT6 expression in mouse model of allergen-induced allergic airway inflammation

Background Activation of signal transducer and activator of transcription 6 （STAT6） plays a critical role in the late phase of Th2-dependent allergy induction. STAT6 is essential to Th2 cell differentiation, recruitment, and effector function. Our previous study confirmed that DNA vaccination inhibited STAT6 expression of spleen cells induced by allergen. In the present study, we determined whether DNA vaccine encoding Dermatophagoides pteronyssinus group 2 （Der p2 ） could down-regulate the expression and activation of STAT6 in lung tissue from asthmatic mice. Methods After DNA vaccine immunization, BALB/c mice were sensitized by intmperitoneal injection and challenged by intranasal instillation of rDer p2. The levels of the cytokines IL-4 and IL-13 in BAL fluid were measured by enzyme-linked immunosorbent assay. The lung tissue was assessed by immunohistochemical staining with anti-STAT6. The protein expression of STAT6 was determined by Western blot. The activation of STAT6 binding ability was analyzed with electrophoretic mobility shift assay. Results DNA vaccine encoding Der p2 allergen effectively decreased the levels of IL-4 and IL-13 in the asthmatic mice. Histological evidence and Western blot showed that the expression of STAT6 in the DNA treated mice was markedly attenuated. STAT6 binding to specific DNA motif in lung tissue from the gene vaccinated mice was inhibited. Condusion DNA vaccine encoding Der p2 prevents allergic pulmonary inflammation probably by inhibiting the STAT6 signaling pathway in mice with Der p2 allergen-induced allergic airway infammafion.

Co-administration of Interleukin-2 Enhances Cellular and Humoral Immune Responses to HIV Vaccine DNA Prime/MVA Boost Regime

Interleukine-2(IL-2) is a growth factor for antigen-stimulated T lymphocytes and is responsible for ~T-cell clonal expansion after antigen recognition. It has been demonstrated that DNA vaccine-elicited immune responses in mice could be augmented substantially by using either an IL-2 protein or a plasmid expressing ~IL-2. Twenty mice, divided into four experimental groups, were immunized with: (1) sham plasmid; ^(2) HIV-1 DNA vaccine alone; (3) HIV-1 DNA vaccine and IL-2 protein; or (4) HIV-1 DNA vaccine and IL-2 plasmid, separately. All the groups were immunized 3 times at a 2-week interval. Fourteen days after the last DNA vaccine injection, recombinant MVA was injected into all the mice except those in group 1. ELISA and ELISPOT were employed to investigate the effect of IL-2 on DNA vaccine immune responses. The obtained results strongly indicate that the efficacy of HIV vaccine can be enhanced by co-administration of a plasmid encoding IL-2.

HER2-Specific Vaccines for HER2-Positive Breast Cancer Immunotherapy

Anti-human epidermal growth factor receptor-2 (HER2) immunization can be elicited by vaccination with DNA encoding the extra- or intra-cellular domain (ECD or ICD) of HER2, naked or encap-sulated in viral vectors. HER2-peptides derived from ECD or ICD of HER2, and HER2-pulsed dendritic cells (DCs) or engineered DCs expressing HER2, respectively. We performed a computer- based literature search which includes but is not limited to the following keywords: breast cancer, immunotherapy, HER2-peptide vaccine, HER2-DNA vaccine, HER-DC vaccine, HER2 vaccine, and HER2/neu, in PubMed, Medline, EMBO and Google Scholar;data from recently reported clinical trials were also included. Drawing upon this synthesis of literature, this work summarizes the de-velopment and current trend in experimental and clinical investigations in HER2-positive breast cancer using HER2-specific vaccine and immunotherapy, focusing especially on: (i) DNA-;(ii) peptide-;and (iii) DC-based vaccines. It addresses interventions that have been applied to overcome immunotolerance thereby to improve treatment outcomes. These include blocking the inhibitory cytotoxic T lymphocyte-associated protein-4 (CTLA-4), which is expressed at high levels by regulatory T (Treg) cells, or complete Treg depletion to improve T-cell activation. Moreover, modulatory interventions can provide further improvement in the efficacy of HER2-specific vaccine. The interventions include the use of immunogenic adjuvants such as cytokines interleukin-12 (IL-12), tumor necrosis factor (TNF)-α and granulocyte-macrophage colony-stimulating factor (GM-CSF), the use of Toll-like receptor (TLR) ligands and tetanus toxin’s universal epitopes such as the CD4+ help T (Th)-epitope P30, and the use of either chimeric or heterogenous xenogeneic HER2. Combining active HER2-vaccination with adoptive trastuzumab antibody immunotherapy is likely to increase the effectiveness of each approach alone. The development of effective HER2-vaccines for breast cancer remains a critical challenge. Though these novel interventions seem promising, further investigation is still needed since the results are preliminary. Furthermore, the review discusses the challenges and future perspectives in HER2-vaccine research and development.

信号肽与猪链球菌GDH融合的DNA疫苗构建及体液免疫研究

目的设计、构建猪链球菌GDH真核表达载体并研究DNA疫苗免疫小鼠的体液免疫。方法在猪链球菌保护性抗原GDH基因5′末端引入人IL-2信号肽序列,通过PCR进行拼接,得到的融合DNA片段经过酶切克隆入质粒pcDNA3.0,构建核酸疫苗重组质粒pcDNA3.0-gdh。通过肌肉注射途径将重组质粒pcDNA3.0-gdh免疫小鼠,经ELASA实验和Western blot进行检验。结果构建的表达载体在小鼠体内表达出正确的目的蛋白,能诱导体液免疫。结论构建的DNA疫苗能够引起体液免疫,为研究猪链球菌核酸疫苗提供分子工具。

重组人白介素2卡介苗的构建及表达

采用聚合酶链反应及基因工程技术，克隆卡介苗（ＢＣＧ）的主要分泌抗原Ａｇ８５Ｂ基因的５’端第９４～２１１的核苷酸的信号肽序列和构建重组人ＩＬ－２穿梭表达质粒，并用酶联免疫吸附法（ＥＬＩＳＡ）鉴定外源基因在ＢＣＧ中的表达。结果表明，构建的ＢＣＧ重组体能表达和分泌人ＩＬ－２。此将试用于临床治疗膀胱癌病人。

基因修饰对鸡新城疫病毒F48E9株HN基因DNA疫苗表达效力的影响

DNA疫苗的免疫效果与抗原基因的表达量和免疫原性有直接关系,为了提高目的基因的表达量,本研究对NDV F_(48)E_9株的HN基因进行了修饰,对修饰前后HN基因表达水平进行了比较。利用分子生物学软件将NDV F_(48)E_9株的HN基因的密码子全部替换为鸡体内偏嗜性密码子,同时在HN基因的5′端加上同样已替换密码子的禽流感病毒HA蛋白信号肽序列以期望提高目的蛋白在细胞中的表达。修饰后HN基因命名为SoptiHN,剔除信号肽的HN基因命名为optiHN。将SoptiHN、optiHN和F_(48)E_9株的HN基因分别克隆到真核表达载体pVAX1和含有多个鸡体内最适免疫刺激序列CpG-ODN的载体pVAX1-CpG中,将他们分别命名为pV-SoptiHN、pVC-SoptiHN、pV-optiHN、pVC-optiHN和pV-HN、pVC-HN,用这些质粒转染293T细胞,48小时后间接免疫荧光和Western blotting检测细胞中瞬时表达的HN蛋白。结果显示,与未经修饰的HN基因相比,修饰后的HN基因体外瞬时表达水平明显提高,并且密码子优化与添加信号肽序列这两种途径都可以提高HN基因的体外表达量.

人IL-2信号肽基因增强柯萨奇病毒B3型VP1 DNA疫苗诱导的中和抗体应答

目的 将人白细胞介素 2 (hIL 2 )信号肽基因与柯萨奇病毒B组 3型 (CVB3)的VP1基因融合 ,构建分泌型VP1真核表达质粒pcDNA3/sVP1;免疫小鼠后 ,通过测定血清特异性中和抗体效价及对致死量CVB3攻击的保护作用 ,评价疫苗的免疫效果。方法 采用重叠区基因扩增法 ,将hIL 2信号肽基因连同其下游 11个氨基酸残基的基因与CVB3VP1基因拼接 ,获得分泌型VP1(sVP1)的基因 ;将sVP1基因克隆至真核表达载体pcDNA3,构建分泌型VP1真核表达质粒pcDNA3/sVP1;肌注免疫小鼠 ,测定血清中CVB3特异性中和抗体的效价 ;第 3次免疫后 2周 ,腹腔内注射 10 0 0TCID50 的CVB3,观察小鼠生存情况。结果 成功构建了分泌型VP1真核表达质粒pcDNA3/sVP1,插入的sVP1基因中含有hIL 2信号肽及其下游 11个氨基酸残基的基因以及VP1基因 ;pcDNA3/sVP1可比对照质粒pcDNA3/VP1诱导小鼠产生更高水平的中和抗体。结论 hIL 2信号肽基因增强了柯萨奇病毒B3型VP1DNA疫苗诱导的中和抗体应答 。

信号肽和辅助性T细胞表位以及GST表位增强猪带绦虫保护性抗原诱导免疫应答的初步研究

目的 研究信号肽和辅助性T细胞表位以及GST表位增强猪带绦虫保护性抗原诱导的免疫应答。方法 在猪绦虫融合抗原 pCC2 7(本室从六钩蚴cDNA表达文库筛选的三个保护性抗原经拼接所得 )基因片段 5′末端引入人IL - 2信号肽、一个通用型辅助性T淋巴细胞表位 ,谷胱甘肽还原酶的T和B淋巴细胞表位 (TGG) ,经pGEX4T - 2表达鉴定 ,序列分析后构建成DNA疫苗 ,通过肌肉注射途径将这种DNA疫苗免疫小鼠。结果 这种含辅助表位的DNA疫苗诱导的免疫应答效果明显超过对照组 ,对绦虫卵攻击的保护率为 90 %。结论 构建了含绦虫融合抗原 pCC2 7及TGG的核酸疫苗 ,动物试验结果表明 ,TGG表位既可提高IgG、IgG1、IgG2a的水平 ,又进一步增强Th1和Th2细胞间的平衡关系。免疫小鼠对绦虫卵的攻击具有很好的保护作用。

日本乙型脑炎病毒PrMΔE与tPA信号肽融合基因DNA疫苗的研究

采用RT-PCR和重叠PCR方法分别扩增出日本乙型脑炎病毒PrMΔE基因和tPA信号肽序列,并将其插入载体pVAX1,将纯化后的重组质粒转染COS-7细胞,用间接免疫荧光法检测质粒在细胞中的瞬时表达情况,并用制备的质粒免疫昆明小鼠,检测其特异性血清IgG抗体水平、促脾淋巴细胞增长率及攻毒保护率。结果显示,真核表达质粒pVAX-tPA-PrMΔE构建成功;间接免疫荧光试验显示,该质粒在COS-7细胞中的表达产物可与鼠抗日本乙型脑炎病毒单克隆抗体发生特异性反应,tPA信号肽序列能明显增强PrMΔE基因DNA疫苗的免疫原性,显著提高小鼠的体液免疫和细胞免疫水平,能强有力地抵抗强毒株CZ-1的攻击。结果表明,成功构建了日本乙型脑炎病毒PrMΔE基因与tPA信号肽序列融合基因DNA疫苗(pVAX-tPA-PrMΔE),为日本乙型脑炎病毒基因工程疫苗的进一步研究及应用奠定了基础。