甘薯潜隐病毒单克隆抗体的制备及初步鉴定

以原核表达的甘薯潜隐病毒(SPLV)的外壳蛋白(CP)为抗原免疫小鼠,经过细胞融合和亚克隆,筛选出2株稳定分泌抗SPLV CP的单克隆抗体杂交瘤细胞株(5B11-2和5G8-2),并分别制备了单克隆抗体腹水。间接ELISA结果表明,用SPLV CP包被酶联板,5B11-2和5G8-2单克隆抗体的效价均为1∶512 000;用感染SPLV的甘薯叶片汁液包被酶联板,2株单克隆抗体的效价均为1∶6 400。抗体类型及亚类鉴定结果表明,2株单克隆抗体均为IgG1、κ轻链。Western blot分析表明,2株单抗均能与SPLV CP和感染SPLV的甘薯叶片汁液有特异性反应。利用单克隆抗体建立的间接抗原包被ELISA(ACP-ELISA)检测SPLV方法,病叶1∶3 840倍稀释仍能检测到病毒。血清学和RT-PCR检测结果表明,制备的单克隆抗体可用于田间甘薯样品的检测。     

李痘病毒单克隆抗体及TAS-ELISA试剂盒的研制

将纯化的李痘病毒(Plum pox virus,PPV)制剂免疫BALB/c小鼠,用SP2/0骨髓瘤细胞与经李痘病毒免疫的BALB/c小鼠的脾细胞融合,有限稀释法克隆和间接ELISA法筛选出2株稳定分泌李痘病毒单克隆抗体的杂交瘤细胞株3F1,7A8。用间接ELISA方法对所获得的2个杂交瘤细胞株进行亚型鉴定分别为IgG1、IgG3。间接ELISA方法测定腹水效价分别为3F1:1.0×106,7A8:1.0×105。以多克隆抗体为包被抗体、单克隆抗体为检测抗体的TAS-ELISA试剂盒与李痘病毒的D株系、M株系的病毒分离物均有反应,与同属的马铃薯A病毒、莴苣花叶病毒、西瓜花叶病毒2号、马铃薯Y病毒坏死株系不发生交叉反应。     

单抗I-ELISA和TAS-ELISA检测百合无症病毒的研究

 以抗百合无症病毒(Lily symptom less virus,LSV)的单克隆抗体为核心,建立了间接ELISA (I-ELISA)和三抗体夹心ELISA (TAS-ELISA)的检测方法。I-ELISA检测体系中,病叶汁液和单克隆抗体腹水的工作浓度分别为1:20和1:6 000,对病叶汁液的检测灵敏度达到了1:2 560,可检测到提纯病毒绝对量为1.35 ng。TAS-ELISA检测体系中捕获抗体和单克隆抗体腹水的工作浓度分别为1:200和1:6 000,检测病叶汁液的灵敏度达到了1:5 120,对于提纯病毒可检测到0.68 ng。使用美国Agdia公司双抗体夹心ELISA (DAS-ELISA)检测试剂盒对病叶汁液的检测灵敏度为1:2 560,提纯病毒检出量1.35 ng。用3种ELISA方法检测了采自浙江省丽水市的46个田间样品,I-ELISA、TAS-ELISA和DAS-ELISA测出的阳性样品数分别为19、21和18个,阳性率为41%、46%和39%。灵敏度检测和田间样品检测结果显示,TAS-ELISA的灵敏度高于DAS-ELISA和I-ELISA。相同样品I-ELISA所测出的OD₄₀₅值和P/N值普遍高于DAS-ELISA,表明LSV单抗比多抗具有更强的特异性和更高的灵敏度。     

水稻条纹病毒单克隆抗体的制备及检测应用

 用水稻条纹病毒(RSV)免疫的BALB/c小鼠脾细胞与SP2/0鼠骨髓瘤细胞融合,经筛选克隆,获得4株能稳定传代且分泌抗RSV单克隆抗体的杂交瘤细胞。各株单抗腹水的ELISA效价均在1:80000~1:5120000之间。Westernblot分析表明,4株单抗均与RSV的35kDa的外壳蛋白亚基有特异反应。建立了间接ELISA测定RSV的方法,4株单抗检测病汁液的稀释度能达到2560倍以上,与其它病毒无交叉反应。对江苏省部分县市的大田灰飞虱带毒率进行检测,结果显示灰飞虱的带毒率为12.5%~41.5%     

番茄溃疡病菌单克隆抗体的制备与鉴定

为制备并鉴定番茄溃疡病菌(Clavibacter michiganensis subsp.michiganensis,Cmm)的单克隆抗体(McAbs),用全菌皮下免疫BALB/C小鼠,采用B细胞杂交瘤技术,经免疫、融合、间接ELISA筛选和克隆等,获得稳定分泌抗体的阳性杂交瘤细胞株,得到了抗番茄溃疡病菌的单克隆抗体。经免疫后获得3株单抗分别为1A4、1C3和1B7,经亚类鉴定分别是IgM、IgG1、IgG1;纯化腹水间接ELISA效价分别为1:3.2×106、1:8.1×105、1:3.2×106;与其他同属不同亚种无交叉反应。结果表明:3株单克隆抗体均具有较高特异性和敏感性,可作为番茄溃疡病菌的检测抗体,其中,1A4的效果最好。番茄溃疡病菌单克隆抗体的获得为进一步研发番茄溃疡病检测试剂盒奠定了基础。     

南方水稻黑条矮缩病毒和水稻黑条矮缩病毒的单抗制备及其检测应用

 用与牛血清白蛋白偶联的南方水稻黑条矮缩病毒（Southern rice black-streaked dwarf virus,SRBSDV）衣壳蛋白的C端12个氨基酸多肽为抗原免疫BALB/c小鼠,经细胞融合、筛选、克隆,获得2株能稳定传代并分泌抗SRBSDV和水稻黑条矮缩病毒（Rice black-streaked dwarf virus,RBSDV）单克隆抗体（MAb）的杂交瘤细胞株3F1、5G1。3F1、5G1单克隆抗体腹水间接ELISA效价达10^-6,抗体类型及亚类均为IgG1, kappa链。 Western blot分析表明,2株单克隆抗体均与SRBSDV和RBSDV的外壳蛋白亚基有特异反应。利用单克隆抗体3F1建立的dot-ELISA检测方法能准确、特异、灵敏地检测田间稻飞虱及水稻样品中的SRBSDV和RBSDV。SRBSDV和RBSDV单克隆抗体的制备及检测方法的建立为水稻黑条矮缩病的诊断、预测预报及科学防控提供了技术支撑。     

分泌抗玉米细菌性枯萎菌单克隆抗体细胞瘤株的建立及抗体测定

 用玉米细菌性枯萎菌(745)免疫BALB/C小鼠得到的脾细胞与骨髓瘤细胞SP2/0-Ag14融合,获得G₅、C₂和D₁3株稳定分泌抗745菌的单克隆抗体的细胞瘤株。用ELISA间接法测定抗体滴度为1:25600。其中G₅和D₁能与所有供试的9个745菌株系有不同程度的反应,而C₂只与7个745菌株反应。3个单克隆抗体均不与供试的同属其它菌反应。     

南芥菜花叶病毒单克隆抗体的研制及检测应用

将纯化的南芥菜花叶病毒(Arabis mosaic virus,ArMV)制剂免疫Balb/c小鼠,末次免疫后第3天取其脾细胞与SP2/0细胞融合,采用选择性培养基、有限稀释法克隆和间接ELISA方法进行筛选,成功获得了2株稳定分泌ArMV单克隆抗体的杂交瘤细胞株并分别命名为3F7,4G10。用间接ELISA方法对所获得的2个杂交瘤细胞株进行亚型鉴定分别为IgA(3F7)、IgG1(4G10)。间接ELISA效价测定结果:3F7为1:106,4G10为1:108。以单克隆抗体为包被抗体、多克隆抗体为检测抗体的TAS-ELISA检测试剂盒能检测感染ArMV的昆诺藜病汁液的灵敏度为1:1600。     

番茄环斑病毒单克隆抗体的制备及检测

将纯化的番茄环斑病毒(Tomato ringspot virus,ToRSV)制剂免疫BALB/c小鼠,末次免疫后第3天取其脾细胞与SP2/0细胞融合,采用选择性培养基、有限稀释法克隆和间接ELISA方法进行筛选,成功获得了2株分泌ToRSV单克隆抗体的杂交瘤细胞株并分别命名为1H8、1D4.用间接ELISA方法对所获得的2个杂交瘤细胞株进行亚型鉴定均为IgG1亚类.间接ELISA效价测定结果1H8为1:105,1D4为1:106.TAS-ELISA实验结果表明此2株杂交瘤细胞所分泌的单克隆抗体均能与本研究室保存的从德国引进的番茄环斑病毒分离物、从美国ATCC引进的番茄环斑病毒分离物PV-100、PV-174、PV-239发生特异性反应,而不与同属其它3种病毒:烟草环斑病毒(Tobacco ringspot virus,TRSV)、南芥菜花叶病毒(Arabis mosaic virus,ArMV)、马铃薯黑环斑病毒(Potato black ringspot virus,PBRSV)发生反应.     

大豆花叶病毒单克隆抗体(SMV-McAb)的研究

 用大豆花叶病毒免疫的BALB/c小鼠脾细胞与Sq2/0鼠骨髓瘤细胞融合,获得3株分泌抗大豆花叶病毒单克隆抗体的杂交瘤细胞株,S-1、S-2和S-3。它们的鼠腹水滴度高达1:10⁷,能被大豆花叶病毒兔抗血清所阻断。单克隆抗体与其它三种植物病毒不起反应,对大豆花叶病毒的不同株系有特异性差异。     

Comparison and differentiation of Wheat Yellow Mosaic Virus(WYMV), Wheat Spindle Streak Mosaic Virus (WSSMV) and Barley Yellow Mosaic Virus (BaYMV) isolates using WYMV monoclonal antibodies

Twelve monoclonal antibodies (MAbs) were obtained by immunizing mice with a French isolate (F1) of wheat yellow mosaic virus (WYMV). Three of these (3D12, 2C1, 6C3) belong to the IgM class and the nine others to the IgG class (3D8, 3H1, 2B8, 1F2, 3C10, 4F12, 3H9, 1G5, 54). In antigen-coated plate (ACP) ELISA and indirect double antibody sandwich (IDAS) ELISA, all MAbs recognize the WYMV (F1) both in the form of purified particles and in wheat leaf extract. The analysis of numerous French isolates of WYMV shows a variable reactivity with MAbs 3D8, 3H1, 2B8, 3C10, 3H9 and 1G5 in IDAS — and ACP-ELISA. The Japanese isolate of WYMV and United States isolates of wheat spindle streak mosaic virus (WSSMV) were detected in IDAS- and ACP-ELISA by ten of the MAbs tested showing that the wheat bymoviruses originating from the three locations share a high epitopic homology. French isolates of barley yellow mosaic virus (BaYMV; pathotypes 1 and 2) were only detected in ACP-ELISA with MAbs 6C3, 3D8, 3H1 and 2B8 whereas the two Japanese strains (I-1, II-1) of MaYMV were recognized with these and also with that of 3C10. In IDAS-ELISA, the two Japanese strains were clearly detected by MAbs, 6C3, 3D8, 3H1, 1F2, 3C10 and 1G5 and the British and Belgian (pathotype 2) isolates only by that of 6C3. Only the Japanese strain of BaYMV, 1-1 could be detected with MAb 3H9 in this ELISA system.     

基于单克隆抗体的南方菜豆花叶病毒血清学检测技术

为建立南方菜豆花叶病毒(southern bean mosaic virus,SBMV)的快速、简便、高通量检测技术,加强该病毒的口岸检验检疫,以提纯的SBMV粒子为免疫原免疫BALB/C小鼠,利用杂交瘤技术获得3株杂交瘤细胞株19C3、19H9和20G4,其分泌的SBMV腹水单抗效价均达到10-7,且3个单抗与感染SBMV大豆叶片组织粗提液有强烈的特异性免疫反应,而不与感染南方豇豆花叶病毒(southern cowpea mosaic virus,SCPMV)的豇豆、健康的大豆、毛豆、豌豆、蚕豆和菜豆叶片组织粗提液发生免疫反应。以制备的单抗为核心,建立了检测植物中SBMV的ACP-ELISA和dotELISA两种血清学方法。3个单抗中19H9单抗的检测灵敏度最高,以其建立的ACP-ELISA和dot-ELISA方法检测大豆病叶粗提液的灵敏度分别达到1∶163 840和1∶10 240稀释浓度。利用建立的dot-ELISA方法可从上海口岸截获的大豆种子中检测出SBMV,且该检测结果得到RT-PCR方法验证。表明制备的SBMV单抗及建立的SBMV血清学检测技术可有效用于我国SBMV的口岸检验检疫。     

Production of monoclonal antibodies to potato virus YNTN strain and their use for strain differentiation

Four mouse monoclonal antibodies (MAbs) against potato virus Y (PVY) were produced. MAb 4C1 reacted with four isolates of PVY^NTN and only very weakly with one isolate of the necrotic strain of PVY (PVY^N). It did not react with other isolates of the ordinary strain of PVY tested. MAb 2C9 reacted with all isolates tested and can be used to produce a specific diagnostic kit for routine PVY detection. Other MAbs had different specificities and reacted with isolates of various strains of PVY. MAbs did not react with seven other members of the Potyvirus group including potato virus A. A MAb-based ELISA, using MAb 4C1, was devised and shown to detect PVY^NTN specifically.     

Examination of the relationships between vegetative compatibility groups and races in Fusarium oxysporum f.sp. dianthi

The feasibility of identifying races of Fusarium oxysporum f.sp. dianthi by tests for vegetative compatibility type was investigated. Nitrate non-utilizing nitl and NitM mutants were generated from 51 isolates of F. oxysporum f.sp. dianthi , 18 isolates of f. oxysporum from Dianthus spp. not belonging to f.sp. dianthi and, for comparison, 11 isolates of F. proliferatum from Dianthus spp. Vegetative compatibility groups (VCGs) among the isolates were identified by pairing all nitl with all NitM mutants.
Vegetative compatibility was found between isolates of F. oxysporum f.sp. dianthi races 1 and 8 (VCG 0022), races 2, 5 and 6 (VCG 0021) and race 4 (VCG 0020), and wilt-causing isolates previously classified as F. redolens from D. caryophyllus (VCG 0023) and D. barbatus (VCG 0024), Three self-compatible wilt-causing isolates were vegetatively incompatible with all other isolates (VCGs 0025,0026 and 0027), Two VCGs were found among isolates of F. oxysporum from D. caryophyllus not belonging to f.sp. dianthi ; six non-pathogenic isolates were self-compatible but vegetatively incompatible with all other isolates. The foot-rot-associated isolates of F. proliferatum from D. caryophyllus constituted a separate VCG.
Virulence analyses revealed at least four new races among VCGs 0023 to 0027, New Isolates could be categorized as races as a result of VCG analysis and VCG classification correctly indicated that the race identities previously ascribed to two old isolates had been incorrect. Vegetative compatibility tests offer the prospect for rapid identification of races, although inoculation tests continue to be necessary to differentiate races that belong to a single VCG.     

ELISA indexing of commercial carnations for carnation mottle virus using a urease-antibody conjugate

The high sensitivity of the urease form of enzyme-linked immunosorbent assay (ELISA) system allowed the use of pooled samples for the detection of carnation mottle virus (CarMV) with greater sensitivity than the phosphatase system. The urease-ELISA was used for a field assessment of the effectiveness of a Plant Improvement Programme (PIP) for carnations operated by the Victorian Department of Agriculture for the control of carnation mottle virus. On properties growing only PIP carnations, infection with CarMV averaged 0.95%. whereas cm properties growing carnations from ordinary commercial sources, all plants sampled contained the virus. The Plant Improvement Programme provided effective control of CarMV in Sim carnations.     

黄瓜绿斑驳花叶病毒单克隆抗体的研制

将纯化的黄瓜绿斑驳花叶病毒(Cucumber green mottle mosaic virus, CGMMV)制剂免疫BALB/c小鼠,最后一次免疫后第3天取其脾细胞与SP2/0细胞融合,经采用选择性培养基、有限稀释法克隆和间接ELISA方法进行筛选,成功获得了3株分泌CGMMV特异性单克隆抗体的杂交瘤细胞株并分别命名为3C9,3F7,2G10。用ELISA方法对所获得的3个杂交瘤细胞株进行亚型鉴定均为IgG2a,kappa链。 间接ELISA效价测定结果分别为3C9：1.024×107,3F7：2.56×106,2G10：1.28×106。此3株杂交瘤细胞所分泌的单克隆抗体均能与本研究室保存的其他3种不同的CGMMV分离物发生特异性反应,而不与其他3种同属成员病毒 烟草花叶病毒(Tobacco mosaic virus, TMV)、辣椒轻斑驳病毒(Pepper mild mottle virus, PMMoV)、齿瓣兰环斑病毒(Odontoglossum ringspot virus,ORSV) 发生反应。