双层类脂膜非标记乙型肝炎表面抗原免疫传感器

采用固体铂盘电极支撑的双层类脂膜（Pt-BLM）技术崮定乙肝表面抗体（HBsAb）,研制成Pt-B12M-HBsAb电位型非标记免疫传感器,用于检测人血清中乙肝表抗原（HBsAg）。对影响构筑BLM的各种凶素进行了研究,用循环伏安法对Pt-BLM进行了表征。传感器对HBsAg呈Nernstu向应,其线性范围为2～320μg／L,线性回归方程为△V=-1．09＋32．41gρ（HBsAg）,线性相关系数r=0．9998。该传感器响应迅速,灵敏度高,稳定性及选择性好,于4℃干态保存4周,其响应信号基本不变。将其用于临床血清检验,结果满意。     

溶胶-凝胶-HBsAb膜免疫传感器的研制与应用

采用溶胶-凝胶(Sol-gel)技术,成功地将乙肝表面抗体(HBsAb)包埋于Sol-gel中,再滴涂于铂盘电极表面,制成溶胶-凝胶-HBsAb膜非标记免疫传感器.根据抗原与抗体特异性结合形成的免疫复合物使敏感膜有效扩散截面积减小的特性,提出了利用铁氰化钾作为氧化还原探针间接检测乙肝表面抗原(HBsAg)的新方法.用循环伏安法(CV)对电极逐层修饰过程进行了表征,并探讨了对HBsAg定量检测的可行性及其响应机理.采用差示脉冲伏安法(DPV)检测人体血清中的HBsAg.线性范围5～320μg/L,线性相关系数r=0.997.该传感器响应迅速,灵敏度高,稳定性好.于4℃干态保存14d,其响应信号基本不变.将其用于108例临床血清检验,与酶联免疫吸附法(ELISA)的符合率为87.5％.     

基于双层纳米金修饰的高灵敏电位型乙肝表面抗原免疫传感器研究

基于电沉积和层层自组装技术，提出了一种新的生物分子固定化方法，研制成一种高灵敏电位型乙肝表面抗原免疫传感器。利用L-半胱胺酸（LCys）的双官能团结合双层纳米金，从而通过比表面积大，生物相容性好的纳米金胶吸附大量抗体，同时用聚乙烯醇缩丁醛（PVB）薄膜的笼效应把乙肝表面抗体（HBsAb）和纳米金固定在玻碳电极上，从而制得了高灵敏度、高稳定性的电位型免疫传感器。采用循环伏安法（CV）对电极的层层自组装过程进行了考察，并对该免疫传感器的性能进行了详细的研究。该免疫传感器线性范围是8．5～256．0ng／mL，线性相关系数为0．9978，灵敏度为89．0，检出限为3．1ng／mL。已用于病人的血清样品分析。     

等电位间隔-电位滴定法

对两点电位滴定法作出改进,提出了等电位间隔-电位滴定法。由数学推导证明,当P1的数值(P1为V1与Ve的比值以百分率表示;V1为在第1测量点所耗滴定剂的体积;Ve为滴定终点时所耗滴定剂的体积)达到95%,且在两点间的电位差值(ΔE)大于30mV时,滴定的相对误差(T)的计算值可达到小于0.1%。据此,在滴定过程中,记录两测量点之间的ΔE为30mV时的V及E值,当有两组数据的ΔE达到30mV并算得此时的T值≤0.1%时,即可停止滴定,并根据所给公式计算Ve及滴定结果。将此方法应用于包括中和反应、沉淀反应及氧化还原反应等多种滴定体系的电位滴定,所得结果与常规电位滴定法的测定结果一致。     

基于包被包膜糖蛋白抗体纳米金磁性微粒的无试剂安培免疫传感器

在玻碳电极(GCE)表面固定对H2O2有催化还原活性的富马酸二甲酯联吡啶铜(GCE|CuL);再在GCE|CuL表面修饰一层金磁微粒-壳聚糖复合膜(nano Au/Fe3O4/Chit), 进而固定艾滋病毒(HIV)诊断标志物--包膜糖蛋白(gp160)抗体(anti gp160), 由此构建了一类快速检测 gp160的无试剂安培免疫传感器.当该传感器在含gp160溶液中37 ℃下温育30 min后, 传感器表面生成的免疫复合物随gp160浓度的增大而增加, 导致CuL 对H2O2 电催化还原效果降低, 催化电流呈现下降趋势.在PBS溶液(pH 7.0)和-300 mV下, 催化电流的降低值ΔIo与gp160浓度在1～400 μg/L 呈线性关系; 检出限为0.5 μg/L(3σ).研制的免疫传感器检测gp160时, 一步免疫反应即可得结果, 较相同条件下包被gp160抗体的纳米金单分子层修饰电极灵敏度更高, 检测范围更宽, 有望用于艾滋病人血清标志物gp160快速筛测.     

表面等离子体子共振生物传感器用于乙肝表面抗原的测定

运用自行研制的表面等离子体子共振（SPR）生物传感器，采用自组装成膜技 术并以戊二醛作偶联剂，在传感片表面修饰HBsAg单克隆抗体，将其用于乙肝表面 抗原（HBsAg)的检测。实验结果表明SPR生物传感器对HBsAg的检出限为0.06ng/mL 。与传统的酶联免疫吸附试验（ELISA）相比，SPR生物传感器的检出灵敏度明显高 于ELISA法。用该SPR生物传感器对HBsAg质控血清与纯化的HBsAg溶液进行比较检测 ，结果表明该SPR生物传感器对HBsAg具有好的特异选择性。     

纳米金修饰玻碳电极固载抗体电位型白喉类毒素免疫传感器的研究

将巯基乙胺 (AET)固载到玻碳电极 (GCE)表面 ,进而化学吸附纳米金 (NG) ,并通过半胱氨酸 (Cys)用戊二醛 (GA)作交联剂将白喉抗体 (anti Diph)固定在玻碳电极上 ,从而制得高灵敏电位型白喉类毒素 (Diph)免疫传感器 .通过循环伏安法考察了电极表面的电化学特性 ,并对该免疫传感器的性能进行了详细的研究 .该传感器对白喉类毒素检测的线性范围是 2 4～ 60 0ng·mL-1,斜率为 3 8.9mV/decade ,线性相关系数为 0 .9979,检出限为 5 .2ng·mL-1,并将其用于生物制品中白喉类毒素的检测 ,其结果令人满意     

高灵敏电位型免疫传感器对乙型肝炎表面抗原的诊断技术研究

以乙型肝炎表面抗原和乙型肝炎表面抗体为模型免疫蛋白，对传染病的诊断技术进行了研究. 利用吸附在铂电极表面Nafion膜中负电性的磺酸基与乙型肝炎表面抗体(HBsAb)分子中的氨基阳离子之间的静电作用实现抗体的结合，同时通过纳米金(Au)增加抗体的固定量，以及聚乙烯醇缩丁醛(PVB)薄膜的笼效应把乙型肝炎表面抗体和纳米金固定在铂电极上，从而制得高灵敏、高稳定电位型免疫传感器(PVB/Au/HBsAb/Nafion/Pt). 通过循环伏安法和交流阻抗技术考察了电极表面的电化学特性，并对该免疫传感器的性能进行了详细的研究. 该免疫传感器具有制备简单、灵敏度高、线性范围宽、响应时间快(<3 min)、稳定性好、寿命长(>4个月)、选择性高等特点，将其用于病人的血清样品分析，其结果令人满意.     

铁氰化钆修饰电极的制备及表征

应用电化学循环扫描法于玻碳电极表面沉积并形成铁氰化钆修饰电极(GdHCF/GC),扫描电镜(SEM)显示,有两种大小和外形明显不同的颗粒状GdHCF附着在电极表面.红外光谱表明,GdCHF的C≡N弯曲振动吸收峰出现在2062.5 cm-1处.循环伏安法测试表明,在0.2 mol/L NaC l溶液中,GdHCF/GC电极出现两对氧化还原峰,扫速为20 mV/s时,其氧化还原峰的式量电位分别为E0’(I)=192.5 mV和E0’(II)=338.5 mV.研究了不同支持电解质对GdHCF/GC电极电化学性能的影响,GdHCF对Na+离子有优先选择性.     

多巴胺修饰自组装金电极作为生物传感器测定核酸

采用衍生化接枝法制备了多巴胺(DA)-半胱氨(Cys)自组装修饰金电极(DA-Cys-SAM),研究了其电化学性质。在pH 7.5的Tris-HCl底液中,采用循环伏安法测定其Epa=218 mV,Epc=120 mV,ΔE=98 mV,ipa/ipc≈1,电极反应准可逆。采用示差脉冲法(DPV)研究发现DA氧化峰电流随DNA质量浓度提高而显著变大且峰电位不变,峰电流的增加值与DNA质量浓度在1×10-7~1.2×10-5g/mL范围内成正比,检出限达5×10-8g/mL,相对标准偏差为3.2%(n=8,5×10-7g/mL DNA)。该电极对DNA测定具有特异性,对实际样品进行了测定。     

非竞争性毛细管电泳免疫分析乙肝表面抗原

用硫脲标记乙肝抗体(抗-HBs),基于抗原．抗体高选择性识别,建立了非竞争性毛细管电泳免疫分析乙肝表面抗原的新方法。研究了混合温育时间、缓冲溶液酸度和浓度、进样时间的影响。在5mmol／L Tris-20mmol／L H3BO3-3mmol／L EDTA(pH7．0)的运行缓冲溶液中,游离的标记抗体和抗原抗体复合物在15min内完全分离。HBsAg在4．0—50mg／L范围内与复合物的峰面积呈良好的线性关系;相对标准偏差小于6％;检出限为3．0mg／L。该方法用于乙肝病人血清和正常人血清中HBsAg的测定,结果令人满意。     

In vivo hepatitis B virus-neutralizing activity of an anti-HBsAg humanized antibody in chimpanzees

Previously, we constructed a humanized antibody (HuS10) that binds to the common a antigenic determinant on the S protein of HBV. In this study, we evaluated its HBV-neutralizing activity in chimpanzees. A study chimpanzee was intravenously administered with a single dose of HuS10, followed by intravenous challenge with the adr subtype of HBV, while a control chimpanzee was only challenged with the virus. The result showed that the control chimpanzee was infected by the virus, and thus serum HBV surface antigen (HBsAg) became positive from the 14(th) to 20(th) week and actively acquired serum anti-HBc and anti-HBs antibodies appeared from the 19(th) and 23(rd) week, respectively. However, in the case of the study chimpanzee, serum HBsAg became positive from the 34(th) to 37(th) week, while actively acquired serum anti-HBc and anti-HBs antibodies appeared from the 37(th) and 40(th) week, respectively, indicating that HuS10 neutralized the virus in vivo and thus delayed the HBV infection. This novel humanized antibody will be useful in the immunoprophylaxis of HBV infection.     

红细胞标记抗体的电化学免疫分析

研究了红细胞标记抗体的电化学免疫分析法。用乙型肝炎单克隆抗体致敏的红细胞作双抗陕 心免疫分析的酶标二抗替代物。在免疫反应完成后，结合抗原－抗体免疫复合物上的敏化红细胞在低渗溶液中溶血，释放出血红蛋白。     

自组装抗-HBs膜免疫电极的研制和应用

乙型肝炎表面抗原;自组装单分子层;硫脲;自组装抗-HBs膜免疫电极的研制和应用     

200例乙型肝炎病毒感染者对乙肝预防认知情况调查

为了解乙型肝炎病毒（HBV）新感染人群对乙肝预防的认知情况,对2000年7月－12月在本院就诊的200例HBV感染者做了调查,发现未注射疫苗的人群,94．5％是因对乙肝预防认知程度差所致,其中地区、职业、文化程度的差异是影响认知程度的重要因素。因此,加大对预防工作的投入,加强宣传教育,特别是在我省专州地县、偏远山区,是控制HBV感染的首要途径。     

纳米磁性微球免疫伏安法测定乙肝表面抗原

采用化学键合法将乙肝抗体固化在自行制备的纳米磁性高分子功能微球表面 ,利用免疫夹心反应原理 ,捕获溶液中的乙肝表面抗原和标记有辣根过氧化物酶的乙肝第二抗体 .在外加磁场的作用下 ,抗体抗原结合物从样品溶液中分离 ,在含有邻氨基苯酚和过氧化氢的底液中 ,生成具有电活性的化合物 3 氨基吩呃嗪 ,用示差脉冲伏安法进行测定 .响应电流与乙肝表面抗原浓度分别在 0 2～ 1 0和 1 0～ 5 0 0ng·mL-1成线性关系 ,检出限达 0 0 60ng·mL-1.采用本方法检测血清中乙肝表面抗原 ,灵敏度大大高于目前临床采用的酶联免疫吸附法 .     

Expression of Human Hepatitis B Virus Surface Antigen Gene in Transgenic Tobacco

Expression of Human hepatitis B virus surface antigen (HBsAg) gene in plant was reported for the first time. The recombinant plasmid pRoKⅡ-HBsAg was constructed by inserting HBsAg gene into the downstream of CaMV 35S promoter of binary vector pRoKⅡ and then introduced into Agrobacterium tumefaciens LBA4404. The kanamycin-resistant plants were obtained by Agrobacterium-mediated transformation system. It was shown that HBsAg gene was expressed in transgenic tobacco plants and their progenies by ELISA. The spherical particles of ψ 22 nm in the leaf extract of trangenic tobacco were observed by immunosorbent electron microscopy.     

AN HBV LARGE SURFACE ANTIGEN PROTEIN WHICH CAN BE SECRETED FROM MAMMALIAN CELLS

The N-terminal 54 base pairs (encoding amino acid residues 2—19) within the preS1 region of the human hepatitis B virus surface antigen gene were deleted by site-directed mutagenesis. Unlike the wild type large surface antigen protein; when this mutated gene was expressed in monkey kidney cell line COS-M6, the protein product (S301 protein) could be secreted from the cells. Moreover, the inhibition of the secretion of the major surface antigen protein by this altered large surface antigen protein was greatly reduced, suggesting that the deleted region contained a retention sequence which prevented the secretion of the large surface antigen. However, the coexpression of the major S protein was essential for the secretion of the S301 protein. When coexpressed, the secretion of these two proteins was synchronous. Like the wild type large surface antigen protein, the S301 protein could be translocated into ertdoplasmic reticulum and glycosylated after its synthesis in COS cells. The S301 protein was thermo     

The Properties of an HBV Surface Antigen Protein Carrying the Binding Site for the Receptor of Hepatocytes——Its Formation of Surface Antigen Particles and Secretion From Discrete Cell Lines

A human hepatitis B virus (HBV) gene, which encodes the major surface antigen protein(S protein) carrying the hepatocyte receptor-binding site, was constructed with site-directed mutagenesis and in vitro recombination. When expressed in monkey kidney cell line COS-M6, this gene product (S309 protein) formed surface antigen (HBsAg) particles and secreted from the cells. It was stable within the cells and in the culture medium and could be immunoprecipitated with antisera directed against plasma-derived HBsAg or synthetic preS1 polypeptide. Isopycnic CsCl gradient centrifugation showed that the density of S309 protein particles (1.25 g/ml) was slightly higher than that of S protein particles. The S309 protein was readily secretable from hepatoma cell lines, and the amount secreted was comparable to that of the S protein. By contrast, only about 10% of the S309 protein was secreted from COS-M6 cells, and its appearance in culture medium was delayed. The efficiency of the secretion of the S309 protein can b