Asial型口蹄疫病毒胶体金免疫层析检测方法的建立

为建立一种快速、简便、灵敏检测Asial型口蹄疫病毒的胶体金免疫层析方法(GICA).本研究采用柠檬酸三钠还原法制备胶体金颗粒,标记纯化的抗Asial型口蹄疫病毒的单克隆抗体,将该标记物与羊抗豚鼠IgG分别包被在硝酸纤维素膜(Nitrocellulose membrane)上,作为检测带和质控带.经条件优化,组装成检测Asial型口蹄疫的诊断试纸条.用该试纸条分别对A、O、c和Asial型口蹄疫病毒抗原以及猪水泡病病毒抗原等87份样品进行了检测,发现该试纸条不与口蹄疫病毒A、o、c型以及猪水泡病病毒抗原发生反应,特异性良好.用该试纸条对口蹄疫细胞毒(TCID50为6.25)的10倍系列稀释液进行了检测,最低可以检测到大约10-4.该试纸条与其他传统诊断方法的符合率为98.8%.初步实验确定该试纸条在4℃下可保存3个月、37℃和室温下大概可保存1周左右.该试纸条是一种快速、灵敏、特异的FMD抗原检测方法,对现场检测具有一定实用价值.     

鲤疱疹病毒Ⅱ型抗体胶体金检测试纸条的制备和分析

【背景】由鲤疱疹病毒Ⅱ型(cyprinid herpesvirus-2, CyHV-2)引起的疱疹病毒性造血坏死病在鲫和金鱼中的暴发给水产养殖业造成了巨大的经济损失。【目的】开发一种快速、现场检测鲫是否感染过CyHV-2和监测鲫CyHV-2IgM抗体水平的胶体金检测试纸条。【方法】将CyHV-2与胶体金结合作为金标抗原、Protein A作为检测线、兔源rORF66多克隆抗体进行划线作为质控线,分析胶体金试纸条最佳制备及组装条件,确定胶体金标记最适pH、金标抗原最适浓度,以及检测线(test line, T线)、质控线(control line, C线)最适划线浓度等。【结果】本研究制备的CyHV-2抗体胶体金试纸条可以使用全血测试,与常见的其他鱼类抗体血清无交叉反应,如草鱼呼肠孤病毒抗体阳性血清、鳜虹彩病毒抗体阳性血清等。试纸条最低限度可以检测到1:100稀释的阳性血清抗体,由试纸条检测线的深浅可以初步判断鱼体中抗体水平。试纸条通过对10条鲫鱼血清样品检测并和金鱼造血器官坏死病毒检测方法(GB/T 36194—2018)进行Kappa分析,Kappa值为0.80,表明二者有较高的符合...     

一种超高灵敏的埃博拉病毒胶体碳侧流免疫层析检测方法的建立

埃博拉出血热 (Ebola hemorrhagic fever, EHF) 由于其高感染性和高致死率特点,快速鉴别诊断并实施隔离是最有效的防止疫情扩散的措施。文中建立了一种可以快速、高灵敏筛查埃博拉病毒 (Ebola virus,EBOV)感染的现场检测技术,用碳纳米颗粒标记抗EBOV基质蛋白VP40兔多克隆抗体,组装成一种可在15 min内检测埃博拉病毒的胶体碳侧流免疫层析试纸条。将标记胶体碳颗粒的兔多抗喷涂于玻璃纤维素膜上制备碳标垫;以1 mg/mL的抗VP40单克隆抗体 (McAb,4B7F9) 和羊抗兔IgG,按照2 μL/cm的包被量印迹于硝酸纤维膜上,分别作为检测线与质控线,组装试纸条。该试纸条能够特异地检测EBOV重组VP40蛋白、EBOV病毒样颗粒(Virus-like particles,VLP) 和灭活EBOV,而与马尔堡病毒样颗粒 (MARV-VLP)、流感病毒A/PR/8 (IAV/PR/8)、黄热病毒 (YFV-17D)、登革热病毒2型 (DEN2) 无交叉反应,显示良好的特异性,对1 500份阴性血清进行检测,假阳性率为1.3‰,仅为WHO授权ReEBOV?胶体金试纸的1/100;该胶体碳试纸条检测灭活EBOV的最低检出限为100 ng/mL (相当于106 copies/mL),远优于ReEBOV?胶体金试纸条检出限 (10 μg/mL,相当于108 copies /mL)。热稳定性评价显示试纸条可在室温稳定保存1年以上。文中建立的EBOV胶体碳免疫层析试纸条能够快速、超高灵敏、特异地检测EBOV,为现场快速筛查EBOV感染提供一种新方法。     

应用斑点酶联免疫吸附试验对实验性临床病料的初步检测

先用实验室保存的口蹄疫病毒A和O两个血清型标准毒株分别制备出单克隆抗体(McAb)和多克隆抗体(PcAb),然后取经人工感染O型猪产生的水泡液或1:10稀释的水泡皮研磨浸出液,滴一滴(约2～4μl)至硝酸纤维素膜。硝酸和醋酸混合膜和醋酸纤维素膜的印圈中央,自然干燥,加封闭液作用30分钟,常规洗条;分组分别滴加ⅥcAb和PcAb,洗涤;加辣根过氧化物酶标记兔抗BALB/C鼠免疫球蛋白结合     

以猪IgG重链恒定区为抗原载体的抗口蹄疫病毒DNA疫苗的研制

口蹄疫(Foot-and-Mouth Disease, FMD)是当今世界上最为严重的家畜传染病之一,主要危害猪、牛、羊等偶蹄动物.FMD的致病原为FMD病毒(FMDV),属小RNA病毒科口蹄疫病毒属,有A、O、C、SATⅠ、SATⅡ、SATⅢ及AsiaⅠ共7个血清型.FMDV结构较简单,完整的病毒颗粒由4种结构蛋白VP1、VP2、VP3及VP4各60个拷贝构成的衣壳包裹一条单股正链RNA组成,其中VP1是主要的抗原蛋白[1].     

口蹄疫病毒Asia1/YNBS/58株全基因组序列分析

口蹄疫是由口蹄疫病毒(Foot-and-mouth dis-ease virus,FMDV)感染引起的偶蹄动物(猪、牛、羊、骆驼等)共患的一种急性、烈性、接触性传染病。FMDV是小核糖核酸病毒科(Picornaviridae)口蹄疫病毒属(Aphthovirus)的成员,有7个血清型,分别为O、A、C、Asia1、SAT1、SAT2、SAT3,完整     

双重荧光RPA扩增方法快速鉴别两种血清型水泡性口炎病毒

本研究利用重组酶聚合酶扩增(RPA)技术,根据水泡性口炎病毒印第安纳型(VSV-IND)和新泽西型(VSVNJ)相对保守的L基因为靶序列设计并筛选出两套特异性的引物和探针,建立了快速鉴别检测水泡性口炎病毒两种血清型的双重荧光RT-RPA方法。试验结果表明,该方法特异性强,与猪水泡病病毒(SVDV)、口蹄疫病毒(FMDV)、蓝舌病病毒(BTV)、猪繁殖与呼吸综合征病毒(PRRSV)、牛病毒性腹泻病毒(BVDV)、猪瘟病毒(CSFV)等灭活抗原核酸无交叉反应;灵敏度高,最低可检测核酸浓度为12.7fg/μL;简便快速,反应时间短(15min),且重复性好。利用所建立方法对124份临床样品进行检测,结果与双重荧光RT-PCR一致。本文为VSV-IND和VSV-NJ的快速鉴别检测提供一种新方法,尤其适合现场检疫或基层实验室的快速检测。     

Asia I口蹄疫vp2蛋白单克隆抗体的制备及单抗竞争ELISA方法的建立

制备Asia I口蹄疫病毒vp2单克隆抗体(mAb)并建立了单抗竞争ELISA方法。用纯化的Asia I型口蹄疫病毒vp2重组蛋白免疫BALB/c小鼠, 将免疫小鼠的脾细胞与骨髓瘤SP2/0细胞融合, 采用间接ELISA和有限稀释法筛选杂交瘤细胞。分别用ELISA、Western blotting检测mAb腹水的效价及其特异性。筛选到杂交瘤细胞2株, 腹水效价均在100×29以上; 以纯化后的Asia I型口蹄疫病毒vp2重组蛋白作为抗原, 利用Asia I型口蹄疫病毒vp2单抗酶标物建立了竞争ELISA方法用来检测Asia I型口蹄疫抗体。临床应用表明, 该方法与UBI公司的口蹄疫全病毒抗体检测试剂盒总符合率达89.0%, 和荷兰赛迪公司的口蹄疫病毒LPB-ELISA抗体检测试剂盒总符合率达86.5%。     

猪O型口蹄疫病毒抗体化学发光酶联免疫检测方法的建立

表达并纯化猪O型口蹄疫病毒(FMDV)VP1重组蛋白作为检测抗原,建立了一种快速检测猪O型口蹄疫病毒抗体的化学发光酶联免疫(CLEIA)检测方法。建立的VP1-CLEIA方法特异性为100%,板内变异系数在1.10%–6.70%之间,板间变异系数在0.66%–4.80%之间,具有较好的特异性和重复性,且灵敏度高于ELISA方法。通过对山东、辽宁、河北地区采集的250份临床血清的检测表明,该方法与间接ELISA试剂盒的符合率为93.50%,与液相阻断ELISA试剂盒的符合率为94.00%,表明本次建立的VP1-CLEIA检测方法可以用于猪O型FMDV感染或疫苗免疫后抗体水平检测。     

胶体金免疫层析试纸条技术在病毒检测领域的应用研究现状北大核心CSCD

胶体金免疫层析试纸条技术是一种快速、灵敏和精准的固相标记检测技术,胶体金免疫层析试纸条具有价格低廉、操作简便、检测快捷和特异性强的优点,具有在短时间内灵敏、准确地定性检测出相关病毒的潜在能力,有效解决传统检测方法在医学、兽医、动植物病毒检测和农药残留检测等领域存在检测时间长、设备不便和专业性强的弊端。目前在检测领域,该技术在检测细菌性疾病、病毒性疾病和预防传染性疾病大面积扩散等方面都有应用,因此,该技术在检验方面具有巨大的发展空间。文中主要对胶体金免疫层析技术进行综述,并对该技术在生物病毒检测方面进行总结和展望。     

A screening lateral flow immunochromatographic assay for on-site detection of okadaic acid in shellfish products

A lateral flow immunochromatographic (LFIC) test strip based on a colloidal gold-monoclonal antibody (McAb) conjugate was developed for on-site rapid detection of okadaic acid (OA) in shellfish. It applies a competitive format using an immobilized toxin conjugate and free toxin present in samples. The McAb against OA was conjugated with 20-nm colloidal gold as detector reagent. The toxin in the sample competed with the immobilized toxin to bind to the gold conjugated with McAb. The colloidal gold/McAb/toxin mobile complex was not captured by OA-bovine serum albumin (BSA) on the test line, but it was captured by goat anti-mouse immunoglobulin G (IgG) on the control line. The color density of the test line correlated with the concentration of toxin in the range of 10-50 ng ml(-1). The qualitative detection limit of 150 μg kg(-1) sample was close to the European Union (EU) regulatory limit (160 μg kg(-1)). Therefore, these strips were able to directly and qualitatively estimate the consuming safety of shellfish. They require no equipment because of available visual results, and they screened numerous samples within 10 min. The results were further confirmed by high-performance liquid chromatography tandem mass spectrometry (HPLC-MS/MS). As a food safety screening tool, the test strips are convenient and useful to rapidly on-site test the presence of OA in shellfish products.     

Cytogenetical survey of black rats,Rattus rattus,in southwest and Central Asia,with special regard to the evolutional relationship between three geographical types

A chromosome survey of the black rat, Rattus rattus, was made from animals collected at different localities in Southwest and Central Asia. Asian type black rats (2 n=42) were distributed in northern India, northern Pakistan, while the Oceanian type rats (2 n=38) were found in southern India, southern Pakistan and Central Asia. A border line of distribution of rats with Asian and Oceanian types can be drawn dividing India and Pakistan into northern and southern parts. A hybrid type between Asian and Oceanian types was found in Karachi, Pakistan. Rats with 40 chromosomes, probably a transient type from Asian to Oceanian type, were found in Sri Lanka (Ceylon). It is suggested that these three geographic variants have developed via sequential events of Robertsonian fusion of acrocentric chromosomes in Asian type black rats. This fusion probably took place somewhere in southern India. The Oceanian type black rats that thus developed in southern India migrated widely to the rest of the world through Central Asia and Europe accompanying the movement of mankind.     

微生物探金野外工作箱的研究

介绍了新研制的微生物探金野外工作箱 ,它使用方便、准确、快速、灵敏、重复性能好 ,且能定性和定量检测土壤样品中的金。检测土壤样品 116份 ,结果有 10 6份为阳性 ,9份为阴性 ,其中有一个样品为灰色区 ,与化学分析方法检测对比完全吻合。     

新型冠状病毒胶体金抗原快速检测试剂的研制及性能评价*

目的:建立新型冠状病毒(severe acute respiratory syndrome coronavirus 2,SARS-CoV-2)胶体金抗原快速检测试剂的制备方法,并对检测试剂的性能指标进行评价。方法:采用柠檬酸三钠还原法制备胶体金溶液,用鼠抗核衣壳蛋白(nucleocapsid protein, NP)单克隆抗体及二硝基苯酚-牛血清白蛋白(DNP-BSA)作为标记抗体,硝酸纤维素膜上分别包被鼠抗核衣壳蛋白单克隆抗体和兔抗DNP多抗作为检测线和质控线制备免疫胶体金试纸条;对试剂最低检出限、交叉反应性、加速稳定性及临床诊断特异性和灵敏度进行性能评价。结果:检测热灭活培养物的最低检出限为2.0×10² TCID₅₀/mL;测试16种常见呼吸道病原体高浓度样本均无交叉反应;试剂盒50℃加速破坏8周稳定。临床及健康人群鼻咽拭子样本测试,诊断灵敏度为96.67%(29/30),特异性为99.23%(129/130),总符合率为98.75%(158/160);一致性检验Kappa值为0.959 0,P<0.05。结论:SARS-CoV-2胶体金抗原快速检测试剂检测灵敏度和特异性高,检测速度快,操作便携,无需设备,肉眼观察,可作为现有核酸检测法的补充手段,用于新型冠状病毒的早期筛查。     

Preclinical Detection of Porcine Circovirus Type 2 Infection Using an Ultrasensitive Nanoparticle DNA Probe-Based PCR Assay

Porcine circovirus type 2 (PCV2) has emerged as one of the most important pathogens affecting swine production globally. Preclinical identification of PCV2 is very important for effective prophylaxis of PCV2-associated diseases. In this study, we developed an ultrasensitive nanoparticle DNA probe-based PCR assay (UNDP-PCR) for PCV2 detection. Magnetic microparticles coated with PCV2 specific DNA probes were used to enrich PCV2 DNA from samples, then gold nanoparticles coated with PCV2 specific oligonucleotides were added to form a sandwich nucleic acid-complex. After the complex was formed, the oligonucleotides were released and characterized by PCR. This assay exhibited about 500-fold more sensitive than conventional PCR, with a detection limit of 2 copies of purified PCV2 genomic DNA and 10 viral copies of PCV2 in serum. The assay has a wide detection range for all of PCV2 genotypes with reliable reproducibility. No cross-reactivity was observed from the samples of other related viruses including porcine circovirus type 1, porcine parvovirus, porcine pseudorabies virus, porcine reproductive and respiratory syndrome virus and classical swine fever virus. The positive detection rate of PCV2 specific UNDP-PCR in 40 preclinical field samples was 27.5%, which appeared greater than that by conventional and real-time PCR and appeared application potency in evaluation of the viral loads levels of preclinical infection samples. The UNDP-PCR assay reported here can reliably rule out false negative results from antibody-based assays, provide a nucleic acid extraction free, specific, ultrasensitive, economic and rapid diagnosis method for preclinical PCV2 infection in field, which may help prevent large-scale outbreaks.     

Development of primers to characterize the mitochondrial control region of the snow leopard (Uncia uncia)

The snow leopard (Uncia uncia) is a rare carnivore living above the snow line in central Asia. Using universal primers for the mitochondrial genome control region hypervariable region 1 (HVR1), we isolated a 411‐bp fragment of HVR1 and then designed specific primers near each end of this sequence in the conserved regions. These primers were shown to yield good polymerase chain reaction products and to be species specific. Of the 12 snow leopards studied, there were 11 segregating sites and six haplotypes. An identification case of snow leopard carcass (confiscated by the police) proved the primers to be a useful tool for forensic diagnosis in field and population genetics studies.     

锦鸡儿属植物分布研究

依据每个种的地理分布范围,确定了出六种分布类型,并编制了属的分布密度图。结合各类发布特点及其形态特征,认为东亚西南部为其起源中心,而中亚来其变异分化中心。起源第三纪中期的原始类群Ser.Caragana,在寒旱主要压力下分化适应,形成现代化布格局。     

Radiosensitization of DNA by gold nanoparticles irradiated with high-energy electrons

Zheng, Y., Hunting, D. J., Ayotte, P. and Sanche, L. Radiosensitization of DNA by Gold Nanoparticles Irradiated with High-Energy Electrons. Radiat. Res. 168, 19-27 (2008). Thin films of pGEM-3Zf(-) plasmid DNA were bombarded by 60 keV electrons with and without gold nanoparticles. DNA single- and double-strand breaks (SSBs and DSBs) were measured by agarose gel electrophoresis. From transmission electron micrographs, the gold nanoparticles were found to be closely linked to DNA scaffolds, probably as a result of electrostatic binding. The probabilities for formation of SSBs and DSBs from exposure of 1:1 and 2:1 gold nanoparticle:plasmid mixtures to fast electrons increase by a factor of about 2.5 compared to neat DNA samples. For monolayer DNA adsorbed on a thick gold substrate, the damage increases by an order of magnitude. The results suggest that the enhancement of radiosensitivity is due to the production of additional low-energy secondary electrons caused by the increased absorption of ionizing radiation energy by the metal, in the form of gold nanoparticles or of a thick gold substrate. Since short-range low-energy secondary electrons are produced in large amounts by any type of ionizing radiation, and since on average only one gold nanoparticle per DNA molecule is needed to increase damage considerably, targeting the DNA of cancer cells with gold nanoparticles may offer a novel approach that is generally applicable to radiotherapy treatments.     

A simple and rapid immunochromatographic test strip for detection of white spot syndrome virus (WSSV) of shrimp

A simple strip-test kit for white spot syndrome virus (WSSV) detection was developed using monoclonal antibody W29 (against the VP28 structural protein) conjugated with colloidal gold as the detector antibody. A rabbit anti-recombinant VP28F118 (rVP28) protein antibody in combination with a W28 monoclonal antibody was used as the capture complex at the test line (T), and goat anti-mouse IgG antibody (GAM) was used as the capture antibody at the control line (C). For evidence, the ready-to-use strip was kept in a plastic case and stored in a desiccated plastic bag. A sample volume of 100 microl gill homogenate in application buffer was applied to the sample chamber at one end of the strip and allowed to flow by chromatography through the nitrocellulose membrane to the other end. In test samples containing WSSV, the virus bound to the monoclonal antibody conjugated with colloidal gold and the resulting complex was captured by the antibodies at T to give a reddish-purple band. Any unbound monoclonal antibody conjugated with colloidal gold moved across T to be captured by the GAM and formed a band at C. In samples without WSSV or with WSSV below the limit of detection of the kit, only the band at C was seen. This method was 4 times less sensitive than dot blotting, and about 2 000 000 times less sensitive than 1-step PCR. Nonetheless, it could be used to screen individual shrimp or pooled shrimp samples to confirm high levels of WSSV infection or WSSV disease outbreaks. The beneficial features of this kit are that simple, convenient and quick results can be obtained without the requirement of sophisticated tools or special skills.