用于识别不同细胞蛋白质组的噬菌体抗体芯片

将4个鼠源噬菌体抗体克隆和1个人源噬菌体抗体克隆偶联到羧基终止的硅片表面,制成分析型模型芯片.挑选健康人体淋巴细胞为正常细胞的代表, HeLa细胞为肿瘤细胞的代表,提取细胞的全部蛋白质并用荧光染料Cy3标记,与制成的分析芯片反应,得到了不同的结合图谱.实验结果表明,以噬菌体抗体为分子感受器的分析芯片可用于识别不同细胞的蛋白质组.     

利用pⅧ展示系统改进噬菌体抗体芯片

将展示单链抗体的重组噬菌体与羧基终止的硅片偶联, 制成噬菌体抗体芯片, 可用于检测多类蛋白质和蛋白质组. 通常抗体被展示于噬菌体外壳蛋白pⅢ上, 由此制备的芯片灵敏度和信噪比较低. 我们选用凝血酶特异的单链抗体为代表, 比较了pⅢ展示系统和pⅧ展示系统制成芯片的检测效果. 由于pⅧ展示系统的融合蛋白拷贝数多, 所受空间位阻小, 大幅度提高了噬菌体抗体芯片的灵敏度和信噪比, 有望用于制备新型蛋白质芯片.     

M13噬菌体在分析传感中的应用进展

为生物传感分析选择合适的目标识别分子是提高检测灵敏度和准确度的关键.为此,人们开发了一系列诸如小分子、抗体、多肽和适配体等亲和配体.基于噬菌体展示技术筛选出数千种特异性配体,可以噬菌体为组合元件构建生物传感探针.该方法具有优异的靶向能力,并具有较强的环境耐受性.常见的M13噬菌体表面由多达2700个拷贝的主要衣壳蛋白p...     

二乙氧基硫代磷酸酯类有机磷农药单链抗体的制备及广谱特异性

从分泌抗二乙氧基硫代磷酸酯类有机磷农药(DPPs)单克隆抗体(MAb)的杂交瘤细胞系(12C2)中提取了总RNA, 经RT-PCR反转录成cDNA, 设计带linker引物, 采用重叠延伸PCR制备单链抗体(scFv)基因, 将其克隆到噬菌体载体p3MH中, 构建成噬菌体单链抗体表达载体, 转化大肠杆菌表达出噬菌体表面展示scFv, 对经过Phage-ELISA鉴定的阳性克隆进行噬菌体外壳蛋白基因geneⅢ的去除, 用IPTG诱导其可溶性表达, 对表达产物进行SDS-PAGE, Western-Blot及ELISA鉴定, 并与亲本MAb进行性能对比. 结果表明, 可溶性表达的scFv分子量为27000; scFv与DPPs的交叉反应率比其亲本MAb提高了1.3~3.5倍, 表明其广谱特异性有所提高. 由于scFv与MAb相比具有诸多优点, 因此本研究为有机磷农药多残留检测方法的建立提供了一种更广谱、 更灵敏的新型识别分子.     

单链抗体PS-9的基因克隆、表达和免疫特性鉴定

成功地构建了鼠抗人胰腺癌单克隆抗体PS-9的单链抗体可变区基因(V_H-linker-V_L),并将该基因克隆到噬菌体表达载体pCANTAB5的外壳蛋白g3p基因中,使单链抗体以融合蛋白的形式表达在噬菌体的表面。免疫学鉴定结果表明,这种噬菌体抗体仍保留着亲代抗体的免疫特性,能与人粘液细胞癌LS-174-T细胞表面抗原特异结合。这项研究结果有助于鼠源性单克隆抗体的临床应用以及肿瘤导向诊断和治疗。     

氧氟沙星噬菌体库的构建、筛选及抗体结构模拟

应用噬菌体展示和重组抗体技术制备抗氧氟沙星单链抗体(scFv)库,筛选获得氧氟沙星特异性噬菌体scFv以及同源模拟其三维结构。将从氧氟沙星杂交瘤细胞提取的总RNA,用RT-PCR反转录合成cDNA,以针对鼠源重链可变区(VH)及轻链可变区(VL)基因的兼并引物,扩增获得VH和VL可变区基因,通过SOE-PCR法将VH基因和VL基因通过柔性多肽Linker(Gly4Ser)3拼接成全长scFv基因片段,将双酶切后的scFv基因片段插入T7噬菌体,经体外包装后转化宿主菌BLT5403,成功构建库容量为3×105pfu/mL的抗体库,经4轮吸附-洗脱-扩增的富集,采用直接竞争ELISA筛选到4个特异性噬菌体scFv,运用Expasy软件模拟特异性scFv的三维结构。为进一步大量表达氧氟沙星单链抗体奠定了基础。     

基于核酸分子杂交的免疫芯片抗体固定新方法

基于核酸分子杂交原理构建了一种新型抗体固定方法.先将抗体与寡核苷酸单链交联,再将两者的复合物与固相载体表面上的互补寡核苷酸链结合,从而将抗体固定到载体的表面.在磁珠表面对该固定方法进行实验,证明了方法的可行性.以本方法构建了针对转基因Bt Cry1Ac蛋白的免疫芯片,用Cy3标记二抗对其探针固定效果进行分析,并且在芯片上对Bt Cry1 Ac蛋白进行梯度浓度检测试验.结果表明,以本方法构建的抗体芯片,探针分布具有良好的特异性;探针层分布均匀,非特异吸附小;检测灵敏度达到0.01 ～ 0.05 μg/L;此外,通过杂交核酸双链的解离成功实现了芯片的再生,有助于解决传统抗体固定方法中芯片不可再生的问题.     

γ-羟基膦酸酯诱导梭曼水解单链抗体酶

新型半抗原３－羟基－１－对硝基苯基甲磷酸单频哪基酸酯（Ｐ_６），与血蓝蛋白结合后（Ｐ_６－ＬＰＨ）免疫小鼠，从小鼠脾细胞出发构建单链抗体ｃＤＮＡ文库和噬菌体表面呈现文库．用固相化抗原 Ｐ_６－ＢＳＡ对噬菌体抗体库进行了 ４轮淘选，从中筛选到１１株对梭曼水解有催化作用的单链抗体.对其中一株（ＥＰ_６）进行可溶性抗体的制备，经凝胶过滤和离子交换层析纯化后，ＳＤＳ－ＰＡＧＥ为 ３１ｋｕ的单一条带．酶动力学常数测定其对梭曼水解的催化常数为ｋ_（ｃａｔ）＝１９８ｍｉｎ~(－１)，Ｋ_ｃａｔ／Ｋ_ｕｎｃａｔ＝１２２ ４１９．单链抗体酶ＥＰ６_０．１６ｍｇ·ｍＬ~(－１)与梭曼 ０． １３２ ｍｍｏｌ· Ｌ~（－１）在 ２０℃共温１ｈ后给小鼠背部皮下注射相当于１． １个致死剂量的梭曼， １９只小鼠全部存活，而对照组 １４只小鼠 ３０ ｍｉｎ内全部死亡．小鼠体内抗毒实验显示惊厥潜伏期及死亡时间延长．     

在丝状噬菌体主要外壳蛋白上展示外源多肽的载体

利用基因工程手段,构建了两个用于在丝状噬蓖体主要外壳蛋白表面展示外源多肽的载体,这类载体可以使编码外源多肽的ＤＮＡ片段定向克隆到外壳蛋白的Ｎ末端ＤＮＡ序列中或附近,被修饰的外壳蛋白将分布于野生型丝状噬菌体外壳蛋白单位中间。     

基于噬菌体展示抗体的电化学发光免疫传感器检测相思子毒素研究

以多克隆抗体包被磁性微球制备捕获探针,以表面负载大量三联吡啶钌标记物的噬菌体展示抗体为发光探针有效放大信号,成功建立了相思子毒素电化学发光免疫传感检测方法。利用本方法检测相思子毒素,浓度在0.005～100μg/L范围内与电化学发光强度呈良好的对数线性关系,拟合方程为lgY=0.701lgX+1.767(R=0.9964,N=7,p<0.0001),检测限达0.005μg/L(S/N=3)。与采用单克隆抗体制备标记探针相比,检测灵敏度提高20倍,可用于相思子毒素的痕量检测。     

3-Isopropyloxy-6-morpholino-2-phenylphenalen-1-one as Lipophilic Fluorescent Probe for Lymphocyte Investigations

Fluorescent properties of two naphthalimides and a phenalenone derivative in organic solvents and when they bind to human peripheral blood lymphocytes were investigated. Different spectral characteristics were observed using lymphocytes of healthy donors and patients with nonmalignant (chronic myeloid leukemia) and malignant (B-cell lymphoid leukemia) diseases. It was found that spectral properties of the used fluorophores in cell suspension qualitatively characterize its structural and functional alterations during pathological phenomena. The intensity of fluorescence increased in samples from patients with B-cell lymphoid leukemia, and the fluorescence maximum shifted to the long-wavelength region by 20 nm compared with normal lymphocytes. It is concluded that 3-isopropyloxy-6-morpholino-2-phenylphenalen-1-one as most promising probe may be applied to the study of malignant diseases.     

Autoantibodies to nuclear antigens: correlation between cytotoxicity and DNA-hydrolyzing activity

The cytotoxicity of DNA-specific autoantibodies from sera of patients with systemic lupus erythematosis (SLE) and with lymphoproliferative diseases, and from blood of healthy donors was examined on tumor-cell lines L929 and HL-60. DNA-binding IgG fractions from SLE and chronic lymphocytic leukemia (CLL) sera were cytotoxic at concentrations of up to 10(-10) M. No detectable changes in cell viability were observed after incubation with antibodies devoid of DNA-binding activity and DNA-specific antibodies isolated from blood of healthy donors and patients with T-cell lymphoma, B-cell lymphosarcoma, and acute B-cell leukemia. There was good correlation between the cytotoxic activity and DNA-hydrolyzing activity of anti-DNA antibodies. The cytotoxic effect of DNA-binding antibodies presumably was complement-independent, because it was attributed only to the Fab fragment. The cytotoxic effect was completely inhibited by preincubation with double-stranded DNA (dsDNA). Both the cytotoxic effect and the DNA-hydrolyzing activity of anti-DNA antibodies were significantly increased in the antibody fraction that displayed cross-reactivity with nuclear matrix proteins. Possible mechanisms for the formation and pathogenicity of cytotoxic anti-DNA antibodies are discussed in this article.     

红细胞标记抗体的化学发光免疫分析

用红细胞代替辣根过氧化物酶作为双抗体夹心免疫分析中第二抗体的标记物, 建立了一种红细胞标记抗体的免疫化学发光测定乙型肝炎病毒表面抗原的新方法. 在免疫反应完成后, 结合了抗原-抗体免疫复合物的致敏红细胞在低渗溶液中溶血, 释放出血红蛋白. 基于血红蛋白对鲁米诺-H2O2体系化学发光具有催化作用的原理, 采用化学发光法测定血红蛋白含量. 测得的血红蛋白发光强度与待测抗原浓度呈线性关系. 采用这种方法可检测出0.5 ng/mL的乙型肝炎病毒表面抗原. 将该方法与酶联免疫吸附分析(ELISA)结合起来对乙型肝炎患者血清乙肝病毒表面抗原(HBsAg)进行检测, 两者符合率均为97%, 表明本法具有良好的灵敏度和特异性, 可用于临床标本测试.     

Autoantibodies to nuclear antigens

Thecytotoxicity of DNA-specific autoantibodies from sera of patients with systemic lupus erythematosis (SLE) and with lymphoproliferative diseases, and from blood of healthy donors was examined on tumor-cell lines L929 and HL-60. DNA-binding IgG fractions from SLE and chronic lymphocytic leukemia (CLL) sera were cytotoxic at concentrations of up to 10⁻¹⁰ M. No detectable changes in cell viability were observed after incubation with antibodies devoid of DNA-binding activity and DNA-specific antibodies isolated from blood of healthy donors and patients with T-cell lymphoma, B-cell lymphosarcoma, and acute B-cell leukemia. There was good correlation between the cytotoxic activity and DNA-hydrolyzing activity of anti-DNA antibodies. The cytotoxic effect of DNA-binding antibodies presumably was complement-independent, because it was attributed only to the Fab fragment. The cytotoxic effect was completely inhibited by preincubation with double-stranded DNA (dsDNA). Both the cytotoxic effect and the DNA-hydrolyzing activity of anti-DNA antibodies were significantly increased in the antibody fraction that displayed cross-reactivity with nuclear matrix proteins. Possible mechanisms for the formation and pathogenicity of cytotoxic anti-DNA antibodies are discussed in this article.     

Considerations on antibody-phage display methodology

For almost 15 years phage display is being used for the selection of specific antigen-binders from artificial libraries of single chain antibodies. Filamentous phages have been developed in a way to express foreign proteins on the surface and at the same time carrying the genetic information of the surface expressed molecule within the phage capsid. This property guarantees the coupling of phenotype and genotype during phage amplification and affinity selection. The possibility to generate large antibody libraries and the simplified antibody-backbone of a single chain antibody has made antibody-phage display to a powerful tool for the development of new therapeutics against various human diseases. In this review we discuss the general principles and latest developments and applications in antibody phage display technology.     

用多克隆抗体构建的夹心免疫传感器检测心肌肌钙蛋白I

用表面等离子体子共振生物传感器构建对心肌肌钙蛋白I特异性的免疫传感器检测心肌肌钙蛋白I,并建立两种检测方法:直接法的最低检测限为2.5μg/L,基于传感膜上的夹心免疫法的灵敏度为0.5μg/L,检测范围为0.5～20μg/L,批内及批间精密度分别为3.5%～4.9%,6.1%～7.4%;用夹心法及国外试剂盒对40名健康献血者和20例急性心肌梗死患者血清心肌肌钙蛋白I水平进行检测,两者符合率为95%.     

Relationship between the aggregation of nanoparticles bearing zinc ions and cytotoxicity and morphology of blood cells

The effect of nanoparticles bearing magnetic and nonmagnetic zinc nuclei on lymphocytes from healthy donors and leukemic cells of patients (15–20 years old) with acute B-lymphoblastic leukemia (B-ALL) and acute myeloid leukemia (AML) was considered. The studies by confocal and fluorescence microscopy showed an apoptotic effect of nanoparticles bearing zinc ions. An increase in the aggregation of the nanoparticles and cell self-aggregation, resulting in a decrease in cytotoxicity, were observed in the case of the magnetic isotope. In spite of this, cell apoptosis under the action of even aggregated nanoparticles bearing magnetic ⁶⁷Zn was significantly higher than the apoptosis with lymphocytes of healthy donors and with nanoparticles bearing zinc of the total isotope composition.     

Surface plasmon resonance-enabled mass spectrometry arrays

Biosensors that utilize surface plasmon resonance (SPR) as a method of detection of protein interactions can be used for selective separation of proteins prior to MS analysis. The combination of SPR and MS results in a unique multiplexed detection technology capable of both quantitative and qualitative protein analysis. To further the development of a high-throughput SPR-MS approach, the possibility of arraying binding ligands on SPR chips for affinity capture of proteins and their MS analysis was explored. Antibodies to beta-2-microglobulin, cystatin C, transferrin, and insulin-like growth factors I and II were arrayed on a large number of SPR chips. Human plasma samples were injected over the antibody array chips in an SPR Biosensor, after which on-chip MS analysis was performed to detect the bound proteins. Signals from the targeted proteins were observed for each antibody-derivatized chip, indicating successful antibody immobilization and protein capture. The SPR-MS arrays are robust, highly reproducible, and are capable of high-throughput analysis.