A蛋白酶联法检测苹果褪绿叶斑病毒和茎沟病毒的研究

<正> 苹果褪绿叶斑病毒(CLSV)和茎沟病毒(SGV)是苹果的两种主要潜隐病毒,严重影响苹果的产量和质量。检测苹果潜隐病毒的传统方法是木本指示植物二重芽接鉴定法,但这种方法耗工费时。由于两种病毒不稳定和在苹果树中含量低,用经典的血清学方法不能直接检测苹果植株粗汁液中的病毒。近几年国外采用酶联免疫吸附法(EL     

检测砂梨潜隐病毒的IC-RT-PCR和TC-RT-PCR的研究

以砂梨为试材,在生物学和血清学检测的基础上,采用免疫捕作RT-PCR穴IC-RT-PCR雪和试管捕作RT-PCR穴TC-RT-PCR雪技术,对苹果褪绿叶斑病毒(Applechloroticleafspotvirus,ACLSV)和苹果茎沟病毒(Applestemgroovingvirus,ASGV)进行了检测分析。结果表明,TC/IC-RT-PCR均能有效检测梨粗提液中的ACLSV和ASGV,分别获得了大小约358bp和499bp的目标扩增片段;但IC-RT-PCR检测ACLSV的效果受到病毒分离株间血清学关系影响。与传统的RT-PCR相比,IC/TC-RT-PCR不仅灵敏度更高,而且不需提取总RNA,可以简化操作程序和减少苯酚、氯仿类有机试剂对人体的伤害和对环境的污染,适合于大量梨样品的病毒快速灵敏检测。     

梨和苹果腐烂病菌不同培养表型菌株的致病性分析

The pathogenicity of three strains (F-SD-8, F-BJ-2c-2 and F-HN-2a-1) of Valsa mali var. pyri causing pear canker and one strain (F-SX-A6) of V. mali var. mali causing apple canker in China were comparatively tested by wound inoculation on in vitro twigs of pear, apple and some other woody plants, and in vivo twigs of pear. Significant pathogenicity differentiation was detected in V. mali var. pyri. Generally strains F-SD-8 and F-BJ-2c-2 were highly pathogenic on pear although their culturing characteristics differed greatly. The strain F-SX-A6 was more aggressive on apple than on pear, and the strain F-HN-2a-1 showed significant lower pathogenicity on ten pear cultivars and other seven species of woody plants. Our results confirmed that two variants of V. mali had host preference and were also aggressive to crabapple, apricot, and peach besides apple and pear. Meanwhile, strains F-SD-8 and F-BJ-2c-2 could induce the formation of pycnidia on in vivo twigs of pear, which was not observed on in vivo twigs inoculated with F-HN-2a-1 and F-SX-A6.     

来源于新疆的3 个苹果褪绿叶斑病毒分离物的分子变异研究

Apple chlorotic leaf spot virus (ACLSV) isolates from Korla pear (KI-2), New pear no. 7 (XI-1) and Red Fuji apple (API-4) were collected from XinJiang and characterized by analyzing sequences of their near genomic 3忆-terminal. The RT-PCR products were cloned, and analyzed by single-strand conforma-tion polymorphism (SSCP). Eight out of 39 collected positive clones showing different SSCP patterns were sequenced. The results showed that the amplified products had sizes ranging 676 - 703 bp, including partial coat protein (CP) gene (506 bp, accounts for 87% of the complete cp gene) and 3忆-terminal non-coding re-gion (3忆NCR) sequences. The cp gene sequences from isolate KI-2 showed a high intra-isolate divergence,with 84. 8% - 85. 4% identities at the nucleotide (nt) level, and the intra-isolate identities were 99. 8 % and 92.5% - 99. 8 % for isolate XI-1 and API-4, respectively. Phylogenetic analysis on the nt sequences of cpgene showed that the analyzed ACLSV variants from three isolates fell into two different clusters. A variant KI-2-6 from KI-2 was clustered into a group with an apple isolate aclsv-c from China and a plum isolated from France, and all other variants fell into a large cluster. The 3忆NCR sequences of these variants were identical ranging 80. 6% - 100 % .     

中国果树类病毒的发生及其研究进展(英文)

概述了在中国发生且己鉴定明确的5种果树类病毒,即苹果绣果类病毒(Apple scar skin viroid,ASSVd)、梨泡状溃疡类病毒(Pear blister canker viroid,PBCVd)、葡萄黄斑类病毒-1(Grapevine yellow speckle viroid-1,GYSVd-1)、柑橘裂皮类病毒(Citrus exocortis viroid,CEVd)和桃潜隐花叶类病毒(Peachlatent mosaic viroid,PLMVd)的研究进展,包括病害的首次发现、症状特征、发病规律、检测方法与防治对策以及这些类病毒的生物学与分子生物学特性。     

芋花叶病毒的RT-PCR检测及外壳蛋白基因序列分析

 采用RT-PCR技术对采自中国湖北、浙江和山东的91份芋[Colocasia esculenta（L.）Schott]样品的芋花叶病毒（Dasheen mosaic virus,DsMV）进行了检测,检出率为26.4%。对其中14个DsMV分离物的317 bp扩增产物（为外壳蛋白基因的一部分）序列分析的结果显示,各分离物内的核苷酸变异相对较低,而分离物间存在较大的分子变异,相似性为68.3% ~ 97.8%。对来自湖北和浙江的2个DsMV分离物DsMV-SCS和DsMV-JH的外壳蛋白基因（coat protein gene,cp）进行了测序,全长分别为951 bp和987 bp,二者cp核苷酸和氨基酸序列相似性分别为79.0%和82.3%,与已报道DsMV的cp核苷酸和氨基酸序列相似性分别为73.0% ~ 92.1%和74.8% ~ 98.2%,在构建的系统发育树上聚在两个不同的簇,各DsMV分离物的系统进化关系与其寄主和地理来源无显著相关性。     

梨离体植株中苹果茎沟病毒的脱除技术

为建立苹果茎沟病毒(ASGV,Apple stem grooving virus)的有效脱除方法,以3个梨品种的离体植株为材料,比较了4种脱毒方法对ASGV的效果.结果 显示,3个梨品种的离体植株在茎尖培养、茎尖病毒醚处理、茎尖变温热处理和茎尖病毒醚加变温热处理后,其平均脱毒率分别为50.0％、70.8％、69.6％和...     

柑橘裂皮类病毒广东分离物YC全长cDNA序列克隆及分析

柑橘裂皮类病毒(Citrus exocortis viroid, CEVd)是危害柑橘的重要病原之一,认清该类病毒的分子特性是进一步研究其致病机制的前提.本文利用RT-PCR技术对广东分离物YC的全长cDNA序列进行了扩增、克隆,获得了全长372bp的片段,对该片段进行测序及分析显示:CEVd广东分离物YC的分子结构域包括5个功能区即左手末端区(TL)、致病区(P)、中央保守区(C)、可变区(V)和右手末端区(TR).通过与GenBank已登陆序列的比对分析发现:与来自西班牙的分离物CEVd-f-1(登陆号:EF494677.1)的同源性高达98%;与湖北分离物CEVd-HB(登陆号:AY456136)的同源性仅为92.7%;与强度株系CEVd-A(登陆号:M30868)的同源性为96.8%,与弱毒株系CEVd-de26(登陆号:K00965)的92.4%.说明该广东分离物YC分子特性更接近强毒株系.这是国内首次对柑橘裂皮类病毒cDNA的分子特性进行报道.     

茶尺蠖核型多角体病毒多克隆抗体的制备及检测应用

以纯化的茶尺蠖核型多角体病毒(Ectropis obliqua nucleopolyhedrovirus,EcobNPV)作为抗原免疫大耳白兔,获得多克隆抗体,Indirect-ELISA效价为1∶51 200;工作浓度分别为EcobNPV 1∶1 600、兔抗血清1∶3 200。用所制备的多克隆抗体对提纯的多角体进行Western-blot分析表明制得的抗体对茶尺蠖核型多角体病毒有良好的特异性。应用于不同来源茶园昆虫多角体病毒分离株的检测,取得了理想的检测效果。     

不同来源苹果茎沟病毒分离物部分序列分子特性研究

[目的]明确为害新疆不同品种梨的苹果茎沟病毒(Apple Stem Grooving Virus,ASGV)侵染状况,并对获得的病毒基因序列进行分子鉴定.[方法]采用生物学和分子生物学方法对来源于新疆梨、砂梨及红梨上的ASGV进行检测,将获得基因序列进行比对分析.[结果]从10份新疆梨、2份砂梨及3份云南红梨样品上扩增到预期大小为500 by的ASGV扩增产物.对扩增产物进行克隆和测序,序列分析的结果显示,15个ASGV分离物的CP基因核昔酸及其编码的氨基酸序列相似性分别为88.2;-100;和95.6;-100;,CP基因核苷酸序列构建系统发育树显示,来源于库尔勒香梨分离物KII-3、KII-5、KII-7和新梨7号的分离物XII-5、XII -6,与早期已报道的库尔勒香梨分离物KRL-1及砂梨分离物P-6-1-17亲缘关系较近,聚集成簇.此外,库尔勒香梨的分离物KII-10、KII-14及新粱7号的分离物XII-10与云南红梨上2个分离物YN-2和YN-4聚集成簇,遗传距离较近.[结论]CP基因核昔酸序列系统发育树显示,来源于新获不同品种梨的8个ASGV 分离物及红梨上3个ASGV分离物位于两个不同的组群,存在复杂遗传变异现象.