小麦黄色花叶病毒不同分离物外壳蛋白(CP)基因序列的比较分析

 核苷酸序列分析结果表明,小麦黄色花叶病毒(W YMV)不同分离物的外壳蛋白基因存在一定的差异。邓州分离物CP基因在其31~33nt处均缺失了3个核苷酸,其余分离物与潢川分离物及日本分离物长度一致,均为882nt。不同分离物CP基因核苷酸序列同源性为97.3%~98.9%,由此推导的氨基酸序列同源性为97.6%~99.3%,外壳蛋白N末端的110个氨基酸和C末端的55个氨基酸在各个分离物间是高度保守的。潢川分离物有5个氨基酸与其它5个分离物明显不同。WYMV不同分离物外壳蛋白序列分析结果进一步确认了WYMV与WSSMV为Bymovirus属的2种不同病毒。     

河南省地黄病毒病初步鉴定

 利用血清学、RT-PCR并结合核苷酸序列测定等方法,对河南省地黄病毒病进行了初步鉴定。结果表明,烟草花叶病毒(TMV)为侵染地黄的主要病毒;对TMV地黄分离物(TMV-RH) CP基因的序列分析结果表明,TMV-RH与TMV-U1株系CP基因的核苷酸同源性为86.5%,氨基酸同源性为94.3%;与已发表的TMV其它株系CP基因的核苷酸同源性在76.3%~88.5%之间,氨基酸同源性在79.3%~95.0%之间,同源性较低。根据不同株系CP的氨基酸序列进化树分析,推测该分离物可能为TMV的一个新株系。     

玉米弯孢霉叶斑病菌生物学特性的研究

 利用小麦黄花叶病毒(Wheat yellow mosaic virus,WYMV)和小麦梭条花叶病毒(wheat spindle streak mosaic virus,WSSMV)的特异性序列为引物,逆转录-PCR方法并配合免疫电镜观察,对采自我国四川陕西、河南、安徽、江苏5省9个县、市的27份感病田小麦样品进行检测。除2份样品未检测到病毒外,其余25份样品均为小麦黄花叶病毒所侵染,没有发现小麦梭条花叶病毒,由此表明在中国长江中、下游、淮河及渭河流域严重危害小麦的真菌传线状病毒应主要为小麦黄花叶病毒。     

小麦品种(系)对小麦黄花叶病毒抗性测定结果

 四川省天全县发生的小麦黄花叶病是由病毒侵染引起的土传病毒病,作者曾以土传小麦黄色花叶病(SBWYMV)的暂名报道了一些研究结果,现经进一步探明该病毒粒体为线条状,在自然条件下除侵染小麦属的一些品种外,还侵染大麦属和黑麦属的一些品种,这些更接近已报道的小麦黄花叶病毒(WYMV)的特性,故现采用小麦黄花叶病名。     

小麦黄花叶病毒罗田分离物细胞质内含体蛋自基因的序列分析

 利用RT-PCR,获得了小麦黄花叶病毒湖北罗田分离物细胞质内含体(CI)蛋白基因的cDNA克隆。序列分析结果表明,湖北罗田分离物CI基因由1977个核苷酸组成,编码一个由659个氨基酸组成的蛋白质。与已报道的河南潢川、四川雅安、江苏扬州及日本分离物序列比较,不同分离物之间核苷酸序列同源性在95.0%~97.5%之间,相应推导的氨基酸序列同源性在93.2%~97.1%之间。并对CI蛋白的功能进行了讨论。     

小麦黄花叶病毒罗田分离物细胞质内含体蛋自基因的序列分析

利用RT-PCR,获得了小麦黄花叶病毒湖北罗田分离物细胞质内含体(CI)蛋白基因的cDNA克隆。序列分析结果表明,湖北罗田分离物CI基因由1977个核苷酸组成,编码一个由659个氨基酸组成的蛋白质。与已报道的河南潢川、四川雅安、江苏扬州及日本分离物序列比较,不同分离物之间核苷酸序列同源性在95.0％～97.5％之间,相应推导的氨基酸序列同源性在93.2％～97.1％之间。并对CI蛋白的功能进行了讨论。     

一种侵染滇重楼的Potexvirus病毒分离物分子鉴定及其3′末端序列分析

从云南武定的滇重楼上得到一个病毒分离物Paris-YN,病毒粒体为弯曲线状。利用RT-PCR扩增获得一条1074bp的片段,序列比较分析发现其与马铃薯X病毒属(Potexvirus)病毒3′末端的结构最为相似,且与属内的白三叶草花叶病毒等20个不同分离物3′末端有36.7%～58.9%的同源性;该病毒cp基因长639个核苷酸,编码212个氨基酸(22.8kDa),与20个Potexvirus病毒分离物的CP氨基酸序列比较发现,Paris-YN与白三叶草花叶病毒的CP氨基酸同源性最高(60.1%)。证据表明,该分离物可能为Potexvirus的新成员,暂命名为重楼X病毒(Paris polyphylla virus X)。     

一种侵染滇重楼的Potexvirus病毒分离物分子鉴定及其3'末端序列分析

 从云南武定的滇重楼上得到一个病毒分离物Paris-YN,病毒粒体为弯曲线状。利用RT-PCR扩增获得一条1074bp的片段,序列比较分析发现其与马铃薯X病毒属(Potexvirus)病毒3'末端的结构最为相似,且与属内的白三叶草花叶病毒等20个不同分离物3'末端有36.7%~58.9%的同源性;该病毒cp基因长639个核苷酸,编码212个氨基酸(22.8kDa),与20个Potexvirus病毒分离物的CP氨基酸序列比较发现,Paris-YN与白三叶草花叶病毒的CP氨基酸同源性最高(60.1%)。证据表明,该分离物可能为Potexvirus的新成员,暂命名为重楼X病毒(Paris polyphylla virus X)。     

黄瓜绿斑驳花叶病毒山西西瓜分离物外壳蛋白基因序列分析

通过病毒dsRNA分离技术、非序列依赖性PCR扩增(sequence-independent amplification,SIA)技术和RTPCR等手段对采自山西太谷的西瓜病样进行了检测与鉴定,确定其为黄瓜绿斑驳花叶病毒(Cucumber green mottle mosaic virus,CGMMV)所侵染。为明确CGMMV西瓜分离物(CGMMV-SXTG)的分类地位,本研究进一步克隆了CGMMV-SXTG的外壳蛋白基因(coat protein,CP)全序列并进行序列分析,系统进化树分析显示该分离物与亚洲分离物亲缘关系较近,而与欧洲分离物亲缘关系较远,表明该病毒的不同分离物在分组上可能与地域有一定的关系;接着对不同分离物的CP基因核苷酸序列和氨基酸序列进行同源性比对分析,结果表明该分离物与中国山东分离物(TANG)同源性最高,分别达到99.8%和99.6%。     

小麦对黄花叶病的抗性鉴定及典型品种的遗传分析

 本研究针对来自江苏、河南、四川、湖北、日本和美国的37个小麦品种,在进行小麦抗黄花叶病的抗病性鉴定、调查的基础上,结合分子生物学检测(RT-PCR和ELISA),证实小麦品种扬辐9311对小麦黄花叶病毒(WYMV)表现免疫。将该品种与表现高感的小麦品种进行杂交和回交,通过对其后代抗感分离的调查与分析,确定了小麦品种扬辐9311对黄花叶病的抗性受一对显性基因控制,并为寻找小麦抗黄花叶病基因的分子标记提供理论依据和实验材料。同时,本文对小麦抗黄花叶病表现的影响因素及宁麦9号的抗病性进行了分析和讨论。     

Serological relationships between five fungally transmitted cereal viruses and other elongated viruses

F(ab')₂ and protein A ELISA tests were used to investigate the serological affinities of five fungally transmitted cereal viruses: barley yellow mosaic (BaYMV), barley mild mosaic (BaMMV), oat mosaic (OMV), wheat yellow mosaic (WYMV) and oat golden stripe (OGSV). Within this group only BaYMV and WYMV were related. Chinese and UK isolates of BaYMV appeared to be similar. In tests using antisera to 29 other elongated viruses, BaYMV was related to one isolate of bean yellow mosaic poty virus (BYMV-G) and OGSV had affinities with BYMV-G, potato virus M, red clover vein mosaic (both carlaviruses) and perhaps Hordeum mosaic virus. The results were confirmed in immunoelectron microscopic tests. No affinities were found for BaMMV, OMV or WYMV.     

Molecular comparisons amongst wheat bymovirus isolates from Asia, North America and Europe

To study the variation between wheat bymovirus isolates and to resolve uncertainties about the identity of the virus in some countries, leaves of infected plants were obtained from nine sites in China and from one each in Italy, Germany, USA and Canada. The German isolate was obtained from rye and the Canadian isolate was the type strain of wheat spindle streak mosaic virus (WSSMV). In RT-PCR, using primers designed from a partial sequence of a French isolate (tentatively described as WSSMV), genome fragments were obtained from the Italian and the French isolates but not from the Chinese ones. Conversely, products were consistently obtained from the Chinese isolates, but not from the Italian or French ones, when primers were designed from the sequence of a Japanese isolate of wheat yellow mosaic virus (WYMV). Nucleotide sequences were obtained from regions at or near the 3'-terminus of RNA1 of six Chinese isolates and the four from Europe and North America, usually including the coat protein. Nucleotide and amino acid sequence comparisons demonstrated that the European and North American isolates were extremely similar and were therefore WSSMV, while the Chinese isolates were close to the Japanese isolate and were thus WYMV.     

黄淮地区小麦品种对小麦黄花叶病毒抗性评价

小麦黄花叶病是由禾谷多黏菌传播的小麦黄花叶病毒引起的病害,近年在黄淮麦区呈蔓延加重趋势。为了给病害的防治和抗病育种工作提供依据,本研究利用分级评价方法对黄淮地区推广的小麦品种进行了田间抗病性鉴定。两年鉴定结果表明,在145个供试小麦品种中,‘濮优938’、‘新麦208’、‘豫麦416’、‘新原958’、‘豫麦70-36’、‘泛麦5号’等70个品种表现为免疫,占总数的48.28%;‘豫麦47’和‘邯6172’表现为抗病,占总数的1.38%;‘洪育2号’、‘花培2号’、‘偃展4110’、‘豫麦41’、‘郑麦9023’等48个品种表现为中抗,占总数的33.10%;‘兰天06129’、‘兰天0591’、‘徐麦9158’、‘徐麦0054’、‘徐麦1108’等25个品种表现为感病,占总数的17.24%。研究结果为指导小麦黄花叶病区合理选择小麦品种提供了科学依据。     

中国小麦黄花叶病毒(WYMV)分布的RT-PCR鉴定

 镰刀菌产生的单端孢霉烯毒素,包括DON、DAS和T-2毒素,是一类重要的植物病原真菌毒素。这类毒素不仅加强病菌的为害程度,而且人畜食用罹病谷物及其制成品易造成中毒。近年来,单端孢霉烯毒素的生物合成途径、关键酶及其基因克隆,毒素在致病过程中的作用,以及利用毒素作为选择压鉴定小麦抗病性和筛选抗病突变体均取得了明显进展。本文对此作一综述。     

Differences in cultivar response and complete sequence analysis of two isolates of wheat yellow mosaic bymovirus in China

Seeds of selected European and Japanese winter wheat cultivars were grown at two experimental sites in China, namely Yaan, Sichuan province (YA), and Yangzhou, Jiangsu province (YZ), where wheat yellow mosaic bymovirus (WYMV) was severe. There were some differential responses of the cultivars to the virus isolates present at the two sites. The complete nucleotide sequence of both RNAs of both virus isolates was determined. Their genome organization was identical to that reported for a Japanese isolate and the sizes were very similar. Nucleotide comparisons demonstrated that parts of the CI and NIa coding regions on RNA1 and the N-terminal part of the P2 coding region on RNA2 were particularly variable, while substantially conserved regions occurred in the 3' UTR of RNA2, the 7K, one part of the CI and parts of the NIb and coat protein. It seems unlikely that differences in the 7K and NIa-VPg proteins are responsible for virulence differences and the CI and NIb regions were considered the most promising for further study.