博尔纳病病毒实时荧光定量PCR诊断试剂盒的评价与应用

目的 评价博尔纳病病毒(Borna disease virus,BDV)实时荧光定量PCR(FQ RT-PCR)试剂盒的各项指标,并了解其实际应用效果.方法 使用BDV OL持续感染细胞株、非BDV病毒序列转染的OL细胞、正常的OL细胞,对BDV RT-PCR试剂盒的敏感性、特异性、重复性和稳定性进行评估,同时检测部分临床病人和动物外周血液RNA.结果 试剂盒可以检测出的病毒RNA最低浓度为10~2,相当于1.5个病毒拷贝数.特异性好,无非特异检出.不同批次的试剂盒的检测结果变异系数接近1.加速破坏的试剂盒和正常试剂盒检测结果之间变异系数在2以内.对临床病人检测阳性率为3.6%,对动物检测阳性率为4.4%.结论 试剂盒敏感性、特异性、重复性和稳定性均佳,是BDV基础研究、流行病学调查、临床检测的良好工具.     

博尔纳病病毒持续感染细胞系中病毒RNA的原位PCR检测

目的建立检测博尔纳病病毒(BDV)RNA的原位PCR方法。方法首先设计BDV特异性引物以及检测BDV-RNA的原位PCR扩增系统．然后对BDV持续感染细胞(BDV／OL)和正常细胞(OL细胞)爬片进行原位PCR扩增,进而分别用DNA酶或RNA酶消化处理BDV／OL细胞爬片后,再进行原位PCR扩增。结果经原位PCR扩增后．约60％～70％的BDV持续感染细胞核中出现了阳性反应信号,但正常细胞无信号出现,并且病毒感染细胞中的阳性信号在RNA酶消化作用下消失,但不受DNA酶作用的影响。结论该研究建立的PCR检测方法具有BDV和RNA特异性,可以应用于检测相关动物或神经精神疾病患者的脑组织中BDV-RNA,为进一步证明BDV的致病性奠定基础。     

检测博尔纳病病毒RNA的RACE技术的建立

目的建立检测博尔纳病病毒(BDV)RNA的3′RACE(rapid amplification of cDNA ends)方法。方法根据已知的BDV p40基因序列设计上游引物sp1;提取BDV(H1766株)持续感染OL细胞的总RNA,用引物sp1和oligo dT进行3′RACE扩增,将PCR产物克隆到pGEM-T载体并转化到大肠埃希菌中,制备阳性菌落的目的质粒,进行序列测定和同源性比对;同时对检测BDV RNA的3′RACE方法的特异性和敏感性进行分析。结果建立了检测BDV RNA的3′RACE技术;所获得的BDV p40基因的3′末端扩增产物的核苷酸序列与已知BDV(H1766株)p40基因的核苷酸序列同源性为100%;本方法对BDV RNA(mRNA)具有特异性,但对BDV p40基因重组质粒无扩增结果;并且可以检测到0.04 ng以上含量的BDV感染细胞的总RNA。结论检测BDV RNA的3′RACE技术可以排除实验室污染造成的BDV基因扩增的假阳性,并可用于进一步分析BDV基因序列的特点以及评价BDV相关基因的表达情况。     

Real-time TaqMan RT-PCR快速检测犬瘟热病毒方法的研究

按照犬瘟热(CDV)N基因序列,设计合成了特异性引物和探针,经各反应条件的优化,建立了Real-time荧光定量RT-PCR技术,对细胞培养物、肝脏、肺脏、脑、脾脏、淋巴结以及鼻腔拭子等组织病料中的CDV进行了特异性检测和敏感性试验。同时,利用建立的Real-time荧光定量RT-PCR方法与常规RT-PCR以及韩国BIOINDIST生产的BIT RAPID CDV检测试剂盒对57份临床样品进行了检测。结果:用20pmol/mL的引物浓度各1uL和20pmol/mL的探针浓度0．3uL,获得的荧光信号最强,曲线平滑。敏感性高,可检测到1．24×10—3ng/uL的病毒RNA;特异性强,与NDV、AIV、NiPV等RNA病毒不发生交叉反应。试验重复性的变异系数(CV)分别为2．3%、2．5%和4．2%;与常规RT-PCR和BIOINDIST生产的BIT RAPID CDV检测试剂盒相比较,该方法具有快速、特异、敏感、可定量,并可同时检测大量样品等优点。     

北美洲流行汉坦病毒多重荧光定量RT-PCR检测方法的建立

为了建立牛轭湖病毒(Bayou virus,BAYV)、纽约病毒(New York virus,NYV)、厄尼诺洛峡谷病毒(El Moro Canyon virus,ELMCV)以及岛景病毒(Isla Vista virus,ISLAV)四种病毒快速筛查、诊断的核酸检测技术,本研究选用上述四种病毒的N蛋白基因作为靶标区域设计四组特异性引物探针,建立四重实时荧光定量RT-PCR检测方法。用四种病毒体外转录RNA进行灵敏度和重复性验证,并使用其他病毒细胞培养物及体外转录RNA进行特异性验证。结果显示,四重实时荧光定量PCR扩增效率均可达到95%以上,四种病毒体外转录RNA灵敏度介于1～10拷贝/μL,与单重检测方法无明显差异,且与其他病毒无交叉反应。稳定性评价结果显示,批内、批间变异系数均在3%以内。本研究所建立的检测方法具有良好的敏感性、特异性和重复性,可用于相关样本的诊断与筛查。     

Real—time TaqMan RT—PCR快速检测犬瘟热病毒方法的研究

按照犬瘟热（CDV）N基因序列,设计合成了特异性引物和探针,经各反应条件的优化,建立了Real—time荧光定量RT—PCR技术,对细胞培养物、肝脏、肺脏、脑、脾脏、淋巴结以及鼻腔拭子等组织病料中的CDV进行了特异性检测和敏感性试验。同时,利用建立的Real—time荧光定量RT—PCR方法与常规RT—PCR以及韩国BIOINDIST生产的BITRAPIDCDV检测试剂盒对57份临床样品进行了检测。结果：用20pmol／mL的引物浓度各luL和20pmol／mL的探针浓度0.3uL,获得的荧光信号最强,曲线平滑。敏感性高,可检测到1.24×3ng／uL的病毒RNA;特异性强,与NDV、AIV、NiPV等RNA病毒不发生交叉反应。试验重复性的变异系数（CV）分别为2．3％、2．5％和4.2％;与常规RT—PCR和BIOINDIST生产的BITRAPIDCDV检测试剂盒相比较,该方法具有快速、特异、敏感、可定量,并可同时检测大量样品等优点。     

寨卡病毒、登革病毒、基孔肯雅病毒三重荧光定量RT-PCR检测方法的建立及评价

本研究旨在建立寨卡病毒(ZIKV virus,ZIKV)、登革病毒(Dengue virus,DENV)以及基孔肯雅病毒(Chikungunya virus,CHIKV)三种病毒快速筛查、诊断的核酸检测技术。选用ZIKV的NS1基因、DENV的NS5蛋白基因以及CHIKV的E1蛋白基因作为靶标区域设计三组特异性引物探针,建立三重实时荧光定量RT-PCR检测方法。用ZIKV、DENV、CHIKV病毒体外转录RNA和病毒细胞培养物对该方法的灵敏性、特异性、重复性等方面进行评价,最后临床样本以及模拟标本验证。结果显示:三重实时荧光定量RT-PCR检测方法扩增效率均可达到90%以上,三种病毒体外转录RNA最低检测限均低于15拷贝/PCR,病毒培养物最低检出限均低于10PFU/mL且与单重检测方法无明显差异。与其他病毒无交叉反应,变异系数均在2%以内。临床标本及模拟标本检出率均可达95%以上。本研究建立的检测寨卡病毒、登革病毒以及基孔肯雅病毒的三重实时荧光RT-PCR方法具有良好的敏感性、特异性和重复性,可用于寨卡病毒病等相关临床标本的检测。     

博尔纳病病毒接种Wistar 大鼠脑组织中病毒基因组的原位检测

本文旨在用原位杂交法探讨博尔纳病病毒( BDV) 接种Wistar 大鼠脑组织中BDV 基因组的分布情况。DIG RNA labeling kit 标记BDV p24 正链探针后, 用斑点实验检测该探针的标记效率, 斑点杂交法检测该探针的特异性。在其标记效率与特异性均达到实验要求后, 用该探针对颅内接种BDV( H1766 株) 的Wistar 大鼠脑组织中BDV 基因组进行原位杂交检测。结果发现, 接种3 周后, BDV 感染主要发生在皮质和海马, 仅少量发生在丘脑和下丘脑; 接种6 周后, 皮质和海马的BDV 感染仍然存在, 且丘脑和下丘脑的BDV 感染明显增强, 说明BDV 在大鼠脑组织中的分布范围随着感染时间的延长而逐步扩大。本文建立的原位杂交法可用于检测BDV 在Wistar 大鼠脑组织内的分布与迁移情况。     

烟草环斑病毒的定量检测技术研究

目的:建立特异、灵敏、快速的TaqMam实时荧光定量PCR方法,用于烟草环斑病毒(TRSV)的定量检测。方法:用纳米磁珠法提取病毒RNA,构建包含烟草环斑病毒全CP序列的质粒标准品。根据CP保守序列设计特异性的引物和TaqMam荧光探针,构建标准曲线,建立TRSV的实时荧光绝对定量PCR方法,并对该方法的特异性、灵敏度和重复性进行评估。结果:建立的方法特异性好,与南芥菜花叶病毒、马铃薯X病毒和马铃薯Y病毒均无交叉反应;至少能检测到767个病毒拷贝,灵敏度比普通PCR高100倍;同一样品试验内及试验间重复性实验的变异系数均小于3%,重复性好;检测结果准确可靠,构建的标准曲线有较好的线性关系(R2=0.997)。结论:建立的TRSV TaqMan实时荧光定量PCR检测方法可满足口岸高通量、快速、准确的检验检疫要求。     

大鼠疑似泰勒氏病毒荧光定量检测方法的建立

目的建立一种能在临床上快速、准确地检测大鼠疑似泰勒氏病毒(Theiler’s-like virus of rats,TLV)的方法,采用TaqMan探针荧光定量聚合酶链式反应(qPCR)技术,特异性针对TLV病毒核酸进行检测。方法通过基因合成序列作为质粒标准品的模板,同时选择特异性的序列在3622~3729 nt处,设计一对引物和TaqMan性探针,优化反应体系及条件,进行qPCR扩增,从而建立TLV TaqMan探针qPCR方法,并对其灵敏度、稳定性和特异性进行评价。结果建立的TLV qPCR检测方法,标准曲线线性关系良好,R~2值可达到0.99,灵敏性最低能够检测到10个拷贝数/μL,对比普通PCR方法,高出其100倍;对其他常见大鼠病毒均无非特异反应;重复性良好,批内和批间变异系数均小于1%。结论利用TaqMan探针建立快速检测TLV的荧光定量PCR方法,该方法具有操作简便、灵敏度高、特异性好等特点。     

五种国产与进口小鼠病毒ELISA抗体检测试剂盒的比较研究

目的评价国产小鼠病毒抗体ELISA检测试剂盒。方法选择国产与进口小鼠淋巴细胞脉络丛脑膜炎病毒（LCMV）、肝炎病毒（MHV）、仙台病毒（SV）、腺病毒（MAV）、细小病毒（MPV）ELISA抗体检测试剂盒,进行敏感性、特异性、精密性、稳定性、可信度试验比较。结果国产与进口试剂盒：同种试剂盒之间灵敏度相差最低为2倍,差异显著（P〈0.05）,最高为16倍,差异极显著（P〈0.01）;特异性试验显示每种试剂盒,与其他4种病毒均无交叉反应;精密性试验显示5种试剂盒批内平均变异系数均小于10%;稳定性试验显示5种试剂盒相对偏差均小于25%;分别选择已知36份小鼠血清进行检测,国产和进口LCMV、MHV、SV、MPV符合率均为100%;国产MAV符合率为86.1%,进口MAV符合率均为100%,二者之间差异极显著（P〈0.01）。结论除国产MAV试剂盒敏感性、可信度低于进口外,国产LCMV、MHV、SV、MPV试剂盒与进口同种试剂盒相比,在敏感性、特异性、精密性、稳定性和可信度方面均良好。     

用ELISA法检测2.5S鼠神经生长因子

鼠颌下腺提纯的２５ＳＮＧＦ免疫家兔,获得兔抗ＮＧＦ抗体,研制出鼠２５ＳＮＧＦＥＬＩＳＡ检测试剂盒,该试剂盒灵敏度小于１ｎｇ／ｍｌ,在６７０～０８４ｎｇ／ｍｌ范围内,线性良好,ｒ＝０９９。与大鼠、小鼠及人血浆无非特异反应,在大鼠血浆中,ＮＧＦ样品回收率在９１％～１０７％之间,变异系数小于１０％（ｎ＝４）。结果表明：本试剂盒操作简便,灵敏度高,特异性强,适合药代动力学研究及生产过程中的ＮＧＦ检测。     

丙型肝炎病毒抗体化学发光免疫检测方法的建立及其临床应用简

目的：建立丙型肝炎病毒（rmv）抗体化学发光免疫检测方法,并分析其临床应用价值。方法：应用基因工程重组的HCV抗原包被微孔板,以辣根过氧化物酶标记的羊抗人IgG为二抗,并结合鲁米诺化学发光底物系统,建立HCV抗体化学发光免疫检测方法;应用HCV抗体诊断试剂国家参考品分析所建立方法的特异性、灵敏度、稳定性和精密性,并-9北京万泰公司的ELISA试剂盒同时检测临床血清样本350份,比较检测结果。结果：检测结果符合国家参考品质量标准。批内变异系数5．1％。6．6％,批间变异系数9-5％;试剂盒置37℃考核3d,其稳定性良好;与万泰公司的ELISA检测结果对照,阳性符合率分别为99．0％,阴性符合率分别为100％,总符合率为99．4％;Kappa值为0．986,一致性强度最强。结论：建立了特异、敏感和稳定的HCV抗体化学发光免疫检测方法,适用于HCV感染的批量筛查,具有较大的临床应用价值。     

Comparison of three ELISA kits for the differentiation of foot-and-mouth disease virus-infected from vaccinated animals

A study was performed to validate 3 FMDV 3ABC-I-ELISA kits developed in China for the differentiation of FMDV infected and vaccinated animals. Sets of sera from naive and vaccinated cattle as well as from cattle that had been infected were tested for antibodies against nonstructural proteins (NSPs) of FMDV by commercial diagnosis kits, Ceditest® FMDV-NS (Ceditest® kit), UBI® FMDV NONSTRUCTURAL PROTEIN ELISA DIRECTION INSERT (UBI® kit) and a FMDV 3ABC-I-ELISA kit developed at the Lanzhou Veterinary Research Institute. The test parameters (sensitivity and specificity) of the three kits were determined, and the result obtained from FMD 3ABC-I-ELISA kit was compared with that obtained from two foreign kits. The results indicated that the coincidence rate between the FMDV 3ABC-I-ELISA and Ceditest® kits was 98.05%, and the coincidence rate between the FMDV 3ABC-I-ELISA and UBI® kits was 94.4%; the sensitivity of both Ceditest® and FMDV 3ABC-I-ELISA kit was 100%. However, the sensitivity of the UBI® kit was only 81.8%. With sera from naive or vaccinated non-infected animals, the specificity of all tests exceeded 90%.     

基于环介导恒温扩增技术的大肠杆菌O157:H7快速检测试剂盒的评价

【目的】评价基于环介导恒温扩增技术(LAMP)的大肠杆菌O157:H7(Escherichia coli O157:H7)快速检测试剂盒的实效性。【方法】测定快速检测试剂盒的特异性、灵敏度、重复性、保质期以及运输稳定性,并与传统方法对比检测实际样品。【结果】大肠杆菌O157:H7标准菌株样品均检测为阳性,非大肠杆菌O157:H7标准菌株样品均检测为阴性,未发现有交叉反应;试剂盒最低检验限为29 CFU;该试剂盒的特异性、灵敏度及准确度与传统方法相比具有较高的一致性;试剂盒对高菌量目标菌和阴性菌样品的检测重复率均为100%,对低菌量目标菌样品的批间检测重复率为94%。试剂盒可在4°C保存9个月以上,并且可进行变温储存72 h以上。【结论】该试剂盒特异性好,灵敏度高,重复性好,储存方便,检测结果稳定、可靠,适用于对食品中大肠杆菌O157:H7的检测需求。     

Comparison of Three ELISA Kits for the Differentiation of Foot-and-mouth Disease Virus-infected from Vaccinated Animals

A study was performed to validate 3 FMDV 3ABC-I-ELISA kits developed in China for the differentiation of FMDV infected and vaccinated animals.Sets of sera from naive and vaccinated cattle as well as from cattle that had been infected were tested for antibodies against nonstructural proteins (NSPs) of FMDV by commercial diagnosis kits,Ceditest(R)FMDV-NS (Ceditest(R) kit),UBI(R) FMDV NONSTRUCTURAL PROTEIN ELISA DIRECTION INSERT (UBI(R) kit) and a FMDV 3ABC-I-ELISA kitdeveloped at the Lanzhou Veterinary Research Institute.The test parameters (sensitivity and specificity) of the three kits were determined,and the result obtained from FMD 3ABC-I-ELISA kit was compared with that obtained from two foreign kits.The results indicated that the coincidence rate between the FMDV 3ABC-I-ELISA and Ceditest(R) kits was 98.05%,and the coincidence rate between the FMDV 3ABC-I-ELISA and UBI(R) kits was 94.4%; the sensitivity of both Ceditest(R) and FMDV 3ABC-I-ELISA kit was 100%.However,the sensitivity of the UBI(R) kit was only 81.8%.With sera from naive or vaccinated non-infected animals,the specificity of all tests exceeded 90%.     

Sensitivity and specificity of Czechoslovak ELISA HBsAg Sevac tests: comparison with other third-generation tests and counter-immunoelectrophoresis

Two variants of sandwich-type ELISA (Enzyme Linked Immunosorbent Assay) kits for HBsAg detection (Sevatest ELISA HBsAg Macro I and Sevatest ELISA HBsAg Micro I) in human sera and plasmas were developed. As the solid phase, the ELISA Macro kit and ELISA Micro kit make use of polystyrene microtubes, and polystyrene microtitration plates, respectively, of Czechoslovak production (Koh-i-noor, Dalecín). Capture anti HBs antibody for adsorption to solid phase and rabbit anti HBs antibody for labelling with horse-radish peroxidase were prepared for both tests. The sensitivity of both ELISA kits for HBsAg, equal to approx. 2 ng/ml, was determined by titrating six selected HBsAg-positive sera and the WHO Agk 76 panel of HBsAg-positive sera and the results were compared with those obtained by ELISA, RIA (Radioimmunoassay) and RPHA (Reverse passive hemagglutination) kits of different producers and by counter-immunoelectrophoresis (CIEP). The sensitivity of the new ELISA kits was comparable to that of other producers' ELISA kits, higher than that of RPHA kits and only a little lower than that of RIA kits. A set of sera of patients hospitalised with different diagnoses was tested for HBsAg. The detection rate by ELISA Macro kit 2.8 and 1.5 times higher than by CIEP and RPHA (Raphadex B), respectively, and 1.1 time lower than by RIA (Austria II).     

Usefulness of immunoenzyme diagnostic kits and latex tests for isolation of rotaviruses

The aim of this study was to compare characteristic parameters of 4 diagnostic kits available in Poland-immunoenzymatic Rotazyme II and Enzygnost kits and latex kits Rotalex and Slidex. Studies were performed on 67 samples of feces of children treated because of diarrhea. The sensitivity, specificity, frequency of positive tests, false positives and false negatives and the accuracy of the tests under evaluation were determined. The results obtained were further verified using a reference test electrophoresis of RNA of rotavirus. The highest sensitivity was found for Enzygnost, Rotazyme II and Rotalex, 97%, 92% and 90%, respectively, and the lowest for Slidex- 79%, while the specificity was higher for latex kits than for immunoenzymatic kits. The accuracy of the results was highest for Rotalex kit (92%), next for Enzygnost kit (88%), Rotazyme (87%), and Slidex (84%). The significant correlation between OD value readings in spectrophotometer in Rotazyme II kit and the results of visual reading in latex test was found. All tested kits were found to be useful for diagnostic purposes. Rotalex kit due to the high accuracy of the results obtained, methodological simplicity, short time of testing and relatively low price could be a based test in hospital laboratories.     

Pathogenesis of Borna Disease Virus: Granulocyte Fractions of Psychiatric Patients Harbor Infectious Virus in the Absence of Antiviral Antibodies

Borna disease virus (BDV) causes acute and persistent infections in various vertebrates. During recent years, BDV-specific serum antibodies, BDV antigen, and BDV-specific nucleic acid were found in humans suffering from psychiatric disorders. Furthermore, viral antigen was detected in human autopsy brain tissue by immunohistochemical staining. Whether BDV infection can be associated with psychiatric disorders is still a matter of debate; no direct evidence has ever been presented. In the present study we report on (i) the detection of BDV-specific nucleic acid in human granulocyte cell fraction from three different psychiatric patients and (ii) the isolation of infectious BDV from these cells obtained from a patient with multiple psychiatric disorders. In leukocyte preparations other than granulocytes, either no BDV RNA was detected or positive PCR results were obtained only if there was at least 20% contamination with granulocytes. Parts of the antigenome of the isolated virus were sequenced, demonstrating the close relationship to the prototype BDV strains (He/80 and strain V) as well as to other human virus sequences. Our data provide strong evidence that cells in the granulocyte fraction represent the major if not the sole cell type harboring BDV-specific nucleic acid in human blood and contain infectious virus. In contrast to most other reports of putative human isolates, where sequences are virtually identical to those of the established laboratory strains, this isolate shows divergence in the region previously defined as variable in BDV from naturally infected animals.