鲤鱼(Cyprinus carpio)血清生长激素变化的酶联免疫吸附测定

本研究的目标是纯化鲤鱼(Cyprinus carpio)生长激素,用于制备抗鲤鱼生长激素的单克隆抗体,建立鲤鱼生长激素的酶联免疫吸附测定(enzyme-linked immunosorbent assays,ELISA)技术,并用所建立的技术检测不同环境下养殖的鲤鱼的血清生长激素水平的变化.利用柱纯化技术纯化酵母表达草鱼(Ctenopharyngodon idella)生长激素,免疫新西兰白兔(Oryctolagus cuniculus),获得抗草鱼生长激素多克隆抗体.摘取鲤鱼垂体,从中提取生长激素,经层

圆形碘孢虫单链抗体库的筛选与阳性克隆特征分析

噬菌体抗体库已成为单克隆抗体生成的重要技术之一。本文通过用圆形碘孢虫相关抗原对已构建的鼠源免疫噬菌体展示单链组合抗体文库进行生物淘选,并对几株相对亲和力较高的阳性单克隆序列特征、相对亲和力及热稳定性等进行了分析。ELISA、间接免疫荧光及免疫印迹等进行特征鉴定。结果表明,噬菌体抗体库技术对于分离抗圆形碘孢虫不同表位抗原是可行的,将为粘体动物的抗原物质及分布、寄生虫-宿主相互关系等研究提供丰富的抗体来源。

抗对虾白斑综合症病毒的单链抗体A1的表达和生物化学特性

用噬菌体展示技术制备了抗对虾白斑综合症病毒(WSSV)的单链抗体A1。该抗体在30℃培养条件下诱导表达20h后,其蛋白表达量可达总菌体蛋白的3.67%。用亲和层析柱和SephadexG-100层析柱可将单链抗体A1纯化为一条单电泳条带,其分子量约为31.5kD。用等电聚焦电泳测定,其等电点为pH5.8。ELISA测定表明冻干的单链抗体A1在室温储藏4年后与WSSV结合仍具有较高的活力。

抗对虾白斑综合症病毒单链抗体P1D3基因在毕赤酵母中的分泌表达

为了将可中和对虾白斑综合症病毒(WSSV)的单链抗体P1D3在酵母中实现表达,以原核表达载体M13噬菌粒为模板,设计带有SnaBⅠ和EcoRⅠ酶切位点的特异性引物,通过PCR方法扩增P1D3基因。经过酶切、连接反应将该基因连入大肠杆菌-酵母穿梭质粒pPIC9K上。重组质粒pPIC9K-scFvP1D3经BglⅡ线性化后,用电转化的方法转入毕赤酵母(Pichiapastoris)GS115中。通过PCR和DNA测序,挑选和鉴定阳性克隆。经甲醇诱导,P1D3在酵母中获得分泌表达。ELISA实验结果表明,酵母表

微囊藻毒素在沉水植物苦草中的积累

研究了微囊藻毒素RR在大型沉水植物苦草根、叶组织中的积累作用 ,通过ELISA方法检测发现 ,苦草可以吸收MC RR ,其吸收具有时间和剂量效应 ,根的吸收作用强于叶。第 7d叶对MC RR的吸收已经达到平衡 ,而根对MC RR的吸收在处理第 16d时还在上升。苦草根和叶对MC RR的最大吸收量分别可达到 14 83± 0 12 μg/g FW和0 32± 0 0 2 6 μg/g FW。在 0 0 0 0 1mg/L的低浓度下 ,苦草根和叶对MC RR的吸收量分别为 0 5 9± 0 0 83pg/g

抗对虾白斑综合症病毒单链抗体A1基因在酵母中表达及其与抗原结合活性

通过PCR从噬菌粒载体上扩增一种抗对虾白斑综合症病毒 (WSSV)的单链抗体A1(ScFvA1)基因 ,并构建于大肠杆菌 酵母穿梭质粒载体pPIC9K上。经PCR ,酶切 ,测序鉴定重组克隆 ,发现重组成功。将重组质粒pPIC9K ScF vA1转化毕赤酵母 (Pichiapastoris)GS115中 ,利用甲醇诱导 ,将单链抗体A1在酵母中进行了初步表达。经SDS PAGE电泳 ,发现其大小约为 32KD ,通过ELISA实验 ,证明表达上清液中的单链抗体具有很高的WSSV结合活性。

草鱼生长激素在毕赤酵母中的高效分泌表达

为大量获得具有生物学活性的草鱼生长激素 ,对草鱼生长激素cDNA在毕赤酵母中的表达进行了研究。将草鱼生长激素cDNA克隆入毕赤酵母表达载体pGAPZ α B ,构建表达载体pGAPZ α B GH。在三磷酸甘油醛脱氢酶 (GAP)启动子的调控作用下 ,一个类似于天然生长激素大小、分子量约 2 2kD的蛋白获得表达 ,其表达量约 5 0mg L。Western杂交表明 :表达的蛋白与兔抗草鱼生长激素的多克隆抗体特异结合 ,证实该表达蛋白为草鱼生长激素 ;受体夹心式ELISA检测表明 :表达的草鱼生长激素具生

一种筛选对虾白斑综合症病毒中和抗体的新方法

用对虾淋巴组织的原代培养细胞与对虾白斑综合症病毒进行相互作用,洗去不能结合的病毒,然后用甲醛固定,再用ELISA法检测所吸附的病毒。当病毒与抗血清保温后,抑制病毒与细胞的吸附能力的抗血清中应含有中和抗体。此方法可以在缺少细胞系的情况下,简便地筛选到中和抗体。

HLA-DQB1*0301与胃腺癌及幽门螺杆菌感染的关系

为探讨HLA DQB1等位基因与胃腺癌临床特征及其幽门螺杆菌 (Hp)感染的关联性 ,运用序列特异性引物聚合酶链反应技术 ,检测无亲缘关系湖北汉族健康人 136例、胃癌组 6 3例患者的HLA DQB1基因。内镜活检、Giemsa染色和 (或 )外周血ELISA检查胃粘膜Hp感染情况。SAS软件统计处理。结果表明HLA DQB1 0 30 1与湖北汉族人胃腺癌呈正关联。携带与非携带该等位基因患者 ,其临床特征包括患者平均患病年龄、性别比、肿瘤原发部位、肿瘤TNM分期、肿瘤细胞分化程度 ,以及Hp感染率等情

人类白细胞抗原-DRB1与胃腺癌及其临床特征和幽门螺杆菌感染的相关性

目的　探讨人类白细胞抗原 (HLA) DRB1等位基因与胃腺癌及其临床特征和幽门螺杆菌(Hp)感染的关联性。方法　运用序列特异性引物聚合酶链反应和等位基因序列分析技术 ,检测无亲缘关系湖北省汉族健康人 136例、胃癌组 6 3例的HLA DRB1基因。内镜活检、Giemsa染色和 (或 )外周血ELISA检查胃黏膜Hp感染情况。SAS软件数据处理。 结果　HLA DRB10 90 1、12等位基因均与湖北省汉族人胃腺癌呈正相关 ;HLA DRB115等位基因则呈负相关。携带及非携带上述各等位基因患者 ,分

圆形碘泡虫免疫原性的研究

间接红细胞血凝试验结果表明，自然感染圆形碘泡虫的鲫鱼血清中存在循环抗体，并且感染强度与抗体水平不相关。以圆形碘泡虫孢子的可溶性蛋白为抗原，制备多抗。ELISA和IFAT试验表明，不同发育时期的圆形碘泡虫存在共同抗原，并且粘孢子虫具有属特异性抗原。圆形碘泡虫的抗原成分主要集中在虫体后部的一特异位点及四周的虫壁上，两个极囊无抗原成分；而其营养体的抗原成分存在于整个虫体。关桥碘泡虫与兔抗圆形碘泡虫抗体的结合部位主要在其前方的壳壁上和孢质中，极丝也有微弱的反应，其营养体中的抗原成分也存在于整个虫体。

用酶联免疫吸附试验快速检测虹鳟的传染性胰脏坏死病病毒

<正> 我国于1987年从进口的虹鳟中分离了传染性胰脏坏死病病毒(Infectious pancreatic necrosis virus简称IPNV),并进行了血清学鉴定。由于病鱼没有特有的临床症状,所以迅速查找鱼体内特异性的病毒是十分必要的。本文报道了用酶联免疫吸附试验(ELISA)鉴定细胞培养中分离出的IPN病毒及从鱼组织中直接检测IPN

Detection of microcystins in environmental samples using surface plasmon resonance biosensor

An indirect inhibitive surface plasmon resonance (SPR) immunoassay was developed for the microcystins (MCs) detection. The bioconjugate of MC-LR and bovine serum albumin (BSA) was immobilized on a CM5 sensor chip. A serial premixture of MC-LR standards (or samples) and monoclonal antibody (mAb) were injected over the functional sensor surface, and the subsequent specific immunoreaction was monitored on the BIAcore 3000 biosensor and generated a signal with an increasing intensity in response to the decreasing MCs concentration. The developed SPR immunoassay has a wide quantitative range in 1-100 mu g L-1. Although not as sensitive as conventional enzyme-linked immunosorbent assay (ELISA), the SPR biosensor offered unique advantages: (I) the sensor chip could be reusable without any significant loss in its binding activity after 50 assay-regeneration cycles, (2) one single assay could be accomplished in 50 min (including 30-min preincubation and 20-min BIAcore analysis), and (3) this method did not require multiple steps. The SPR biosensor was also used to detect MCs in environmental samples, and the results compared well with those obtained by ELISA. We conclude that the SPR biosensor offers outstanding advantages for the MCs detection and may be further developed as a field-portable sensor for real-time monitoring of MCs on site in the near future. (C) 2009 Published by Elsevier B.V.

Effects of adrenergic agents on the expression of zebrafish (Danio rerio) vitellogenin Ao1

Teleost vitellogenins (VTGs) are large multidomain apolipoproteins, traditionally considered to be estrogen-responsive precursors of the major egg yolk proteins, expressed and synthesized mainly in hepatic tissue. The inducibility of VTGs has made them one of the most frequently used in vivo and in vitro biomarkers of exposure to estrogen-active substances. A significant level of zebrafish vtgAo1, a major estrogen responsive form, has been unexpectedly found in heart tissue in our present studies. Our studies on zebrafish cardiomyopathy, caused by adrenergic agonist treatment, suggest a similar protective function of the cardiac expressed vtgAo1. We hypothesize that its function is to unload surplus intracellular lipids in cardiomyocytes for "reverse triglyceride transportation" similar to that found in lipid transport proteins in mammals. Our results also demonstrated that zebrafish vtgAo1 mRNA expression in heart can be suppressed by both (x-adrenergic agonist, phenylephrine (PE) and beta-adrenergic agonist, isoproterenol (ISO). Furthermore, the strong stimulation of zebrafish vtgAo1 expression in plasma induced by the beta-adrenergic antagonist, MOXIsylyl, was detected by Enzyme-Linked ImmunoSorbent Assay (ELISA). Such stimulation cannot be suppressed by taMOXIfen, an antagonist to estrogen receptors. Thus, Our present data indicate that the production of teleost VTG in vivo can be regulated not only by estrogenic agents, but by adrenergic signals as well. (c) 2009 Elsevier Inc. All rights reserved.

Detection of serum and mucosal antibody production and antibody secreting cells (ASCs) in large yellow croaker (Pseudosciaena crocea) following vaccination with Vibrio harveyi via different routes

The kinetics of mucosal and serum antibody response is well as antibody secreting cells (ASCs) production were studied in large yellow croaker following vaccination with inactivated Vibrio harveyi by different routes: oral administration. intraperitoneal (IP) injection and immersion. Indirect ELISA was used to measure the antibody level in serum and cutaneous mucus, and ELISPOT was used to monitor the ASCs derived from gill, blood and head kidney. The data demonstrated that IP injection resulted in the highest antibody levels in the systemic circulation, whereas immersion induced significant antibody levels in mucous. As for the ASCs response, IP injection induced high numbers of ASCs in the head kidney and blood; oral intubation only induced a slight ASCs response in the head kidney: immersion induced a much stronger ASCs response in the gill. These results indicate that mucosal antibodies following immersion immunization are independent of a systemic response and more sensitive, since it could be triggered earlier than serum antibodies. The mucosal antibodies following IP injection immunization may depend oil a systemic immune response. The protective effects of the three vaccination methods were compared by challenging with live V. harveyi. Survival of the three groups of vaccinated fish varied front 40 to 60%. while 100% mortality was found in control fish. Compared with IP and oral vaccination, immersion stimulated higher specific antibody titers in the mucosal system and achieved similar protection, so it is in effective and efficient method for immunizing a large number of fish against V harveyi (C) 2008 Elsevier B.V. All rights reserved.