原生质体再生对糙皮侧耳Pleurotus ostreatus病毒脱除的效果

以糙皮侧耳Pleurotus ostreatus菌株新831和豫6为材料,从这两个菌株的菌丝体中提取了糙皮侧耳病毒基因组,共有3个dsRNA片段,大小分别为8.2kb、2.6kb和1.1kb。采用菌丝尖端分离脱毒、原基组织分离脱毒和原生质体再生脱毒技术对糙皮侧耳菌丝体进行脱毒处理,利用dsRNA技术对脱毒效果进行检测。结果显示,原基组织分离脱毒后3个条带依然存在;菌丝尖端分离脱毒后,8.2kb和1.1kb 2个条带完全脱除,2.6kb的条带亮度有所减弱;原生质体再生脱毒后3个条带完全脱除;对3种脱毒技术得到的菌株进行生理生化指标测定,结果显示,原生质体再生脱毒菌株的菌丝生长速度、生物量、呼吸强度、纤维素酶活等均明显优于出发菌株、原基组织分离脱毒和菌丝尖端分离脱毒菌株;栽培结果表明,原生质体再生脱毒菌株前两茬菇的生物学效率达到96.4%－99.1%,比出发菌株提高19.9%－25.4%,并且菌盖宽度和长度有所增加,表明原生质体再生技术可以有效脱除糙皮侧耳菌株病毒,提高糙皮侧耳栽培产量。     

广东烟草花叶病毒株系研究

烟草花叶病毒（TMV）引起的烟草花叶病在广东不同的烟草主产区存在着症状的差异。从广东梅州和南雄烟区采集的138个TMV标样中,选取6个不同症状的分离物作为研究对象,发现它们在不同种属寄主和不同烟草品种上表现明显的TMV普通株特征症状,虽然在某些寄主上其症状也有一些差异,但未能反映株系间的差异。这6个分离物具有几乎相同的病毒粒体形态、电泳迁移率、钝化温度以及紫外吸收特征。经琼脂双扩散法和间接ELISA法的血清学反应,表明它们具较强的血清学关系。因而它们有很强的同源性。经病毒粒体外壳蛋白的氨基酸分析,在氨基酸总数上,分离物GD1和GD3各有156个氨基酸．GD2和GD4各有159个,GD5和GD6分别有158和157个氨基酸。上述分析试验结果初步表明,在广东不同烟草主产区引起的症状有所差异的6个分离物均属IMV普通株。     

我国水稻条纹病毒RNA3片段序列分析—纤细病毒属重配的又一证据

测定了来源于我国水稻条纹叶枯病常年流行区的辽宁盘锦 (PJ)、云南昆明 (KM)、云南宜良 (YL)及病害暴发区的江苏洪泽 (HZ)的水稻条纹病毒 (RSV) 4个分离物RNA3全长序列 ,其长度分别为 2 480bp、2 5 0 9bp、2 489bp和 2 497bp。与已报道的RSV云南Y、日本T和M分离物RNA3序列进行比较的结果表明 ,这 7个分离物可分为两组 ,其中 ,KM、YL分离物为一组 ,PJ、HZ、Y、T和M分离物为另一组。组与组之间 ,RNA3的毒义链 (vRNA3)及RNA3的毒义互补链 (vcRNA3)上的ORF的核苷酸同源性分别为 97%～ 98%和 93%～ 94% ,但在氨基酸水平上则没有明显差异。结合上述RSV分离物RNA4的核苷酸全序列比较结果 ,推测认为RSV自然种群中存在两个与地理因素相关的不同类型的亚群 ,Y分离物不同片段具有不同来源可能是由重配引起的。     

侵染西番莲属(Passiflora)植物的五个黄瓜花叶病毒分离物的特性比较

从紫果西番莲(Passiflora edulis)、杂交种西番莲(P. edulis X P.edulis var. flavicarpa)、黄果西番莲(P.edulis var. flavicarpa)、转心莲(P.caerulea)及龙珠果(P.foetida)分离到的5个黄瓜花叶病毒(CMV)分离物(PE、PE2、PEf、PC、PF)所作的生物学性质、理化特性和血清学关系的比较研究结果表明,5个分离物在寄主反应及血清学性质上存在不同,而在病毒粒体形态、体外抗性、蚜虫传毒和病毒外壳蛋白分子量方面无明显差异.根据5个分离物的寄主反应和血清学关系,可将其区分为CMV的两个亚组,其中PE、PE2、PC和PF属CMV亚组I,PEf属CMV亚组II.     

马铃薯Y病毒pl基因的克隆与序列分析

利用依据马铃薯Y病毒(PVY)pl基因序列设计合成的一对引物YP1,YP2,以带毒烟草总RNA为模板,通过RT-PCR方法扩增得到了0.83kb的目的条带,测序结果表明为PVY pl基因。通过对PVY P1蛋白氨基酸序列分析发现PVY不同分离物间P1蛋白氨基酸序列存在明显差异,氨基酸序列同源性在64％～94％间。依据P1蛋白氨基酸序列建立了PVY系统关系树并对PVY进行了类型分析。     

互补DNA杂交分析和血清学方法对香石竹环斑病毒分离物的研究

在联帮德国奥卡河中分离到一种病毒分离物(W),通过鉴别寄主反应的测定,病毒粒子的电子显微镜观察,cDNA斑点杂交和血清学的研究,鉴定出这一病毒分离物为香石竹环斑病毒。其外壳蛋白亚基的分子量为3.8×10~4。cDNA吸印转移杂交分析表明,香石竹环斑病毒的两个RNA组份(RNA~1、RNA_2)之间没有核苷酸序列同源性。RNA_1和RNA_2分别由3.7和1.5仟碱基组成。     

马铃薯Y病毒p1基因的克隆与序列分析

利用依据马铃薯Y病毒(PVY)pl基因序列设计合成的一对引物YPI,YP2,以带毒烟草总RNA为模板,通过RT-PCR方法扩增得到了0.83kb的目的条带,测序结果表明为PVY pl基因.通过对PVY P1蛋白氨基酸序列分析发现PVY不同分离物间P1蛋白氨基酸序列存在明显差异,氨基酸序列同源性在64%-94%间.依据Pl蛋白氨基酸序列建立了PVY系统关系树并对PVY进行了类型分析.     

水稻条纹病毒RNA4基因间隔区序列分析——混合侵染及基因组变异证据

克隆和测定了我国水稻条纹病毒（RSV）22个分离物 RNA4基因间隔区（Intergenic region,IR）序列,序列比较结果表明,我国RSV RNA4 IR在长度上存在634bp、654bp及732bp 3种不同的类型,其中3种不同类型的序列在云南省均有存在,而在其它省份仅存在654bp 类型的序列,云南省还存在不同片段类型序列在同一分离物中混合侵染的现象。序列内部具有两个重要的结构特征,一是具有插入序列;二是有两处反向重复序列,可形成两个明显的发夹结构,其中一个序列比较保守,形成的发夹结构稳定;但另一个发夹结构由于碱基变异导致其稳定性在各个分离物中差异较大。本论文还讨论了插入片段特性、不稳定的发夹结构的形成最低自由能及病毒致病性分化的关系。     

水稻条纹病毒中国分离物和日本分离物RNA2节段序列比较

测定了来源于我国水稻条纹叶枯病常年流行区的云南楚雄(CX)及病害暴发区的江苏洪泽(HZ)的水稻条纹病毒(RSV)2个分离物RNA2全长序列,其长度分别为3506bp和3514 bp.与已报道的日本T和O分离物RNA2序列进行比较的结果表明,这4个分离物可分为两组,其中,HZ、T和O分离物为一组,组内分离物之间,RNA2的毒义链(vRNA2)及RNA2的毒义互补链(vcRNA2)上的ORF的核苷酸一致性分别为97.2%～98.0%和96.8%～97.1%,5′端和3′端非编码区的序列则完全一致.但HZ分离物与T分离物的亲缘关系更为密切,其基因间隔区(IR)与T和O分离物的等长.另一组为我国CX分离物,组与组之间,vRNA2及vcRNA2上的ORF的核苷酸一致性分别为95.0%～95.7%和93.9%～94.4%.CX分离物的IR与HZ分离物相比缺失了一段8 nt的片段.5′端非编码区的序列完全一致,但3′末端非编码区有一个碱基的差异.这些结果表明,RSV在自然界的分子变异与其地理分布具有密切的关系.此外,非编码区序列的高度保守性暗示着它们在病毒基因转录和复制的调控方面具有重要的功能.本文还讨论了RSV的分子流行病学.     

我国大蒜潜隐病毒的基因组结构及3′端序列的变异

从我国6个省市12个大蒜样品上共检出10个不同的香石竹潜隐病毒属(Carlavirus)分离物, 测定了浙江分离物ZJ1的基因组全序列和其他9个分离物的基因组3′端序列. ZJ1分离物RNA基因组全长8363个核苷酸, 3′端具polyA尾, 含6个可读 框(ORF), 分别编码复制酶, TGB1, TGB2, TGB3, CP和NABP, 基因组结构和其他Carlavirus属成员相似. 序列分析表明, 10个分离物均为大蒜潜隐病毒(GarLV), 不同分离物TGB2, TGB3和NABP的差异大于CP的差异, 且这些分离物和葱潜隐病毒(ShLV)也具有很高的同源性. 系统进化树分析表明, 大蒜来源的GarLV分离物可以分成4个类群, 我国分离物分别属于4个不同类群.     

Reappearance of Cucumber mosaic virus Isolates Belonging to Subgroup IB in Tomato Plants in North-eastern Spain

A disease characterized by symptomless leaves and fruit decolouration, loss of consistency and mild deformation on ripening was detected in tomato fields in north‐eastern Spain during 2003 and 2004. DAS‐ELISA analysis revealed the presence of the Cucumber mosaic virus (CMV) in all diseased plants. CMV isolates were characterized by polyacrylamide gel electrophoresis (PAGE) analysis of double‐stranded RNAs (dsRNAs) and nucleotide sequence analysis, and compared with some CMV isolates belonging to different subgroups used as controls. A total of 12 isolates obtained from the infected tomato plants selected for this study gave the same electrophoresis pattern for the three genomic dsRNAs, which was different to the patterns showed by the CMV isolates collected in the same region a few years ago. The identity of the complete nucleotide sequence of one of these CMV isolates and the partial sequence of other five isolates compared to the Tfn strain from Italy and the BAR92/1 isolate from tomato collected in Barcelona in 1992 was higher than 99%, both belonging to subgroup IB of CMV. The CMV isolates of this subgroup found in eastern Spain in previous studies were not detected after 1996. The nucleotide sequences of two isolates that were chosen as representatives of the CMV isolates more frequently detected in previous years revealed that they belonged to the CMV subgroups IA. The origin and the possible causes of reappearance of CMV IB isolates in north‐eastern Spain are discussed.     

Identification and sequencing of a novel insertion sequence, IS1471, in Burkholderia cepacia strain 2a

Abstract Eighty-one isolates of Rhizoctonia solani AG4 were obtained from soil samples with diverse geographic origins in Korea. Forty-five out of 81 isolates (56%) contained at least one dsRNA molecule with their sizes ranging from 2.3 to > 23.1 kb. Nine different sizes of dsRNA molecules were found and extensive variation in banding patterns was observed among isolates. By comparing the sizes and combinations of dsRNAs, 21 distinct banding patterns were observed. Cytoplasmic fractions from 3 isolates showed the same dsRNA band patterns as those from the total cell extracts. The dsRNAs were stable through 10 successive hyphal tip cultures and serial transfers onto the potato dextrose agar supplemented with cycloheximide or emetine. The presence or absence of dsRNAs was not apparently correlated with disease severity, phenol oxidase activity, and geographic origin.     

Analysis of double-stranded RNA and virus-like particles in trichothecene-producing strains of<Emphasis Type="Italic">Fusarium graminearum</Emphasis>

Double-stranded RNAs (dsRNAs) have been found in two isolates of the plant pathogenic fungus Fusarium graminearum which produce trichothecene mycotoxins. The isolates 8.2 and 19.2 had dsRNAs in the size of about 2.0 kb and 6.0 kb, respectively, which were associated with capsid proteins and persisted within the cytoplasm of the infected host cells as encapsidated virus-like particles (VLPs). The dsRNAs contained in the VLP pellets were the same size as the dsRNA isolated in total nucleic acid preparations. In the VLP pellets the isolate 19.2 had a second dsRNA with the size of about 1.6 kb. After mycovirus purification one icosahedral particle of about 28 nm in diameter from the isolate 8.2 and two icosahedral particles of about 28 nm and 38 to 40 nm in diameter from the isolate 19.2 could be identified with electron microscopy. SDS-PAGE analysis of the VLPs from the isolate 8.2 revealed one major protein component of approximately 65 kDa, while the isolate 19.2 had two major protein bands at about 94 kDa and 105 kDa. Both isolates were studied for potential trichothecene production. Tox5 PCR showed a 658 bp fragment in each isolate. In addition, both strains were able to produce the trichothecenes deoxynivalenol (DON), the derivatives acetyl-DON (3-A-DON, 15-A-DON) and nivalenol (NIV) in vitro.     

Viruslike particles in tentoxin-producing strains of Alternaria alternata.

Double-stranded (ds) RNAs associated with viruslike particles have been found in six isolates of Alternaria alternata which produce tentoxin. Isolates had from one to three dsRNAs ranging in size from 1.0 to 5.1 kilobase pairs. In two isolates the dsRNAs were associated with 30-nm particles. No dsRNA was detected in any of six other tentoxin-producing isolates or nine isolates which did not produce tentoxin.     

豇豆单孢锈菌中病毒样颗粒中双链RNA的存在

从北京西郊清华园附近田间豇豆上采集的豇豆单孢锈菌(Uormyces vignal Barcl)夏孢子。萌发后提取双链RNA,电泳分析可测出300—8000碱基对的三组双链RNA。从萌发的孢子中通过差迷离心提取病毒样颗粒,可获得二种类型的病毒样颗粒,一种直径为35—40nm的等轴颗粒。另一种为长短不等的棒状颗粒,用提纯物提取核酸电泳分析与直接从孢子中提取的双链RNA有相同的核酸带,从而证明这些双链RNA存在于病毒样颗粒中。     

Diversity of viruses in Cryphonectria parasitica and C. nitschkei in Japan and China, and partial characterization of a new chrysovirus species

We surveyed native populations of the chestnut blight fungus, Cryphonectria parasitica, in Japan and China, and C. nitschkei, a sympatric species on chestnut trees in Japan, to learn more about the diversity of hypoviruses and other double-stranded (ds) RNA viruses. In a sample of 472 isolates of C. parasitica and 45 isolates of C. nitschkei from six prefectures in Japan, we found 27 containing one or more dsRNAs. Twelve isolates of C. parasitica and two isolates of C. nitschkei were infected with Cryphonectria hypovirus 1 (CHV-1); four of these 12 C. parasitica isolates also contained other dsRNAs that did not hybridize to CHV-1. In China, only one of 85 C. parasitica isolates was CHV-1-infected; no dsRNAs were detected in the other isolates from China. No other known hypoviruses were found in this study. However, we found two previously undescribed dsRNAs in Japan approximately 9 kb in size that did not hybridize to each other or to any known dsRNAs from C. parasitica. We also found three additional groups of dsRNAs, one of which represents the genome of a new member of the virus family Chrysoviridae and was found only in C. nitschkei; the other two dsRNAs were found previously in isolates of C. parasitica from Japan or China. The most significant result of this survey is the discovery of novel dsRNAs that can be characterized in future research.     

Dynamics of double-stranded RNA segments in a Helicobasidium mompa clone from a tulip tree plantation

Eighty-three isolates of the violet root rot fungus, Helicobasidium mompa, were collected in a tulip tree plantation and analyzed for the dynamics of double-stranded (ds) RNA for five years. They were divided into eight mycelial compatibility groups (MCGs). Prevalent MCGs 60 and 68 included 61 and 11 isolates, respectively. Electrophoretic profiles of dsRNA in the first year collection of MCG 60 contained no or a single large dsRNA (more than 10 kb) with or without small dsRNAs (ca. 2.0-2.5 kb). Additional dsRNA fragments, i.e., a middle dsRNA (ca. 8.0 kb) or another type of small dsRNAs, became evident within MCG 60 isolates with time. Northern hybridization revealed the relatedness of all large and middle dsRNA fragments within MCG 60 but small fragments of dsRNA were variable. Large dsRNA fragment differed from that in other MCGs even in the same field. Correlation between specific dsRNA fragments and hypovirulence was not observed. Possible explanations for the accumulation of dsRNA fragments during the growth of disease patch by MCG 60 are discussed in terms of their internal changes such as evolution of novel dsRNA fragments from pre-existing viruses or fungal genomic DNA and horizontal transmissions.     

Incidence of dsRNA Mycoviruses in a Collection of Aspergillus fumigatus Isolates

A collection of clinical and environmental isolates of the opportunistic human pathogen, Aspergillus fumigatus, were screened for the presence of mycoviruses and 6.6?% of 366 isolates contained dsRNA segments ranging in size from ~1.0 to 4.0?kbp. The dsRNAs were categorised into three different groups comprising bipartite dsRNAs, quadripartite dsRNAs, representative isolates of which have both been sequenced, and an uncharacterised mycovirus, whose genome apparently consists of four dsRNAs 1-2.5?kbp in size. Here, we describe dsRNA incidence in the A. fumigatus isolates examined, their provenance and also note that on occasion individual isolates were infected with two groups of different dsRNAs.     

Analysis of cytomegalovirus genomes with restriction endonucleases Hin D III and EcoR-1.

Cleavage of genomes of eleven human, one simian, and one simian-related cytomegalovirus (CMV) isolate by the restriction endonucleases HinD III and EcoR-1 generated reproducible DNA fragments. The size range of CMV DNA fragments as estimated by contour length measurements in comparison with simian virus 40 form II DNA and by coelectrophoresis with EcoR-1 fragments of herpes simplex virus DNA varied between 15 X 10(6) and 0.5 X 10(6) daltons. Comparison of the cleavage products of each isolate in 1% agarose slab gels showed extensive comigration of fragments among the human CMV isolates. In the HinD III digests, three fragment bands comigrated among all human CMV isolates, and six fragments comigrated among most, but not all, human CMV isolates. In the EcoR-1 digests, nine fragment bands comigrated among all human CMV isolates, and five bands comigrated among most, but not all human isolates. Each isolate had a distinctive electrophoretic profile with either HinD III or EcoR-1 digests. No two isolates had identical HinD III or EcoR-1 patterns although some isolates did share more general pattern similarities than others. No clear-cut subgrouping of isolates based on cleavage pattern characteristics could be discerned. Comparison of HinD III and EcoR-1 patterns showed that human isolates differ greatly from nonhuman CMV isolates. HinD III and EcoR-1 digests of each isolate contained both major and minor molar classes of DNA fragments that ranged from about 1 and multiples of 1 M down to about 0.25 M; however, the summed molecular weights for major molar fragments resulting from HinD III or EcoR-1 digests of several isolates closely approximated the molecular weight of 10(8) of the intact genome.     

Double-stranded RNA and virus-like particles in the edible basidiomycete Flammulina velutipes (Enokitake)

One of the commercial strains of Flammulina velutipes was analyzed for the presence of double-stranded RNA (dsRNA) elements to examine the underlying mechanism of strain degeneration. As a result, two dsRNA elements sized 1.9 and 1.8 kb were detected in mycelium derived from spontaneously brown-colored fruit body. They were not detected in the normal strains or in fruiting-impaired degenerative isolates. The dsRNAs were not in the nuclear or mitochondrial fractions, but were located in the cytoplasmic fraction. The presence of virus-like particles of ca. 50 nm diameter associated with the dsRNAs was confirmed by electron microscopic observation.