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1.
Tri Asmira Damayanti Desmiarti Susilo Siti Nurlaelah Dewi Sartiami Tetsuro Okuno Kazuyuki Mise 《Journal of General Plant Pathology》2008,74(6):438-442
Severe mosaic with leaf malformation and green vein banding was observed on yam bean in West and Central Java, Indonesia.
Virions of the causal virus were flexuous filaments, about 700 nm in length, with a coat protein of 30 kDa. The virus was
transmitted by mechanical inoculation and by aphids in a nonpersistent manner. The nucleotide sequence of the coat protein
gene had the highest identity with that of Bean common mosaic virus (BCMV, genus Potyvirus) isolate VN/BB2-5. Based on demarcation criteria, including the genome sequence and host range, we tentatively designate
this isolate as BCMV-IYbn (Indonesian yam bean).
The nucleotide sequence reported is available in the DDBJ/EMBL/GenBank databases under accession number AB289438. 相似文献
2.
A. T. Ploeg D. J. F. Brown D. J. Robinson 《European journal of plant pathology / European Foundation for Plant Pathology》1992,98(5):291-300
Isolates of the PRN serotype of tobacco rattle virus (TRV) were transmitted with different efficiencies by the nematode vectorParatrichodorus pachydermus. Virus isolates which belonged to other serotypes were not acquired and/or transmitted by this vector, nor were PRN serotype isolates which had been obtained from naturally infected potato plants and maintained by mechanical transmission in the glasshouse for several years. PRN serotype TRV isolates from the Netherlands or from Scotland were equally well transmitted by initially virus-freeP. pachydermus populations from either country. Allowing a naturally viruliferous nematode population access for 3 weeks to uninfected or TRV-infected roots resulted in an increased proportion of the trichodorid population transmitting TRV. 相似文献
3.
为明确番茄黄化曲叶病毒北京分离物(Beijing isolate of tomato yellow leaf curl virus,TYLCV-BJ)致病性的强弱,以感染TYLCV-BJ的番茄叶片DNA为模板PCR扩增获得该分离物基因组全长序列,并构建该分离物的侵染性克隆,将其分别接种到番茄、烟草和拟南芥植株上,比较该分离物和TYLCV上海分离物2(TYLCV-Shanghai 2,TYLCV-SH2)致病性的差异。结果显示,该分离物基因组全长序列同TYLCV-SH2的相似度为99.03%,在番茄和烟草植株上TYLCV-BJ比TYLCV-SH2发病更早,症状更重,TYLCV DNA和外壳蛋白积累量更高。TYLCV-BJ可以通过农杆菌Agrobacterium tumefaciens注射法在拟南芥中复制和系统侵染,而TYLCV-SH2不能有效侵染拟南芥。表明TYLCV-BJ的致病性强于TYLCV-SH2,所建立的侵染性克隆有广泛的研究和应用价值。 相似文献
4.
Shin-ichi Fuji Nanae Mochizuki Masashi Fujinaga Makoto Ikeda Kouichi Shinoda Seiji Uematsu Hiromitsu Furuya Hideki Naito Fumiyoshi Fukumoto 《Journal of General Plant Pathology》2007,73(3):216-221
Alstroemeria plants were surveyed for viruses in Japan from 2002 to 2004. Seventy-two Alstroemeria plants were collected from Aichi, Nagano, and Hokkaido prefectures and 54.2% were infected with some species of virus. The
predominant virus was Alstroemeria mosaic virus, followed by Tomato spotted wilt virus, Youcai mosaic virus (YoMV), Cucumber mosaic virus (CMV), Alstroemeria virus X and Broad bean wilt virus-2 (BBWV-2). On the basis of nucleotide sequence of the coat protein genes, all four CMV isolates belong to subgroup IA. CMV
isolates induced mosaic and/or necrosis on Alstroemeria. YoMV and BBWV-2 were newly identified by traits such as host range, particle morphology, and nucleotide sequence as viruses
infecting Alstroemeria. A BBWV-2 isolate also induced mosaic symptoms on Alstroemeria seedlings. 相似文献
5.
葡萄A病毒(Grapevine virus A,GVA)为线性病毒科(Flexiviridae)葡萄病毒属(Vitivirus)的代表种,是葡萄皱木复合病(rugose wood complex disease)的重要病原之一,可引起葡萄嫁接成活率下降、春季萌芽延迟、生长减弱甚至衰退死亡等危害\[1,2\]。GVA为线状单链RNA病毒,基因组共编码5个开放阅读框(ORF1\|5),其中ORF4 编码外壳蛋白(coat protein, CP),是病毒粒子包裹和系统移动所必需的功能蛋白\[3,4\]。GVA自然寄主为葡萄,机械摩擦可侵染本氏烟等草本寄主\[2\],由于嫁接和无性繁殖材料调运等因素造成该病毒远距离传播,目前在世界多个国家和地区均有发生。 相似文献
6.
湖北省小麦黄花叶病病原的部分序列鉴定 总被引:1,自引:0,他引:1
从湖北省真菌传小麦黄花叶病病毒分离物中抽提病毒总RNA,应用逆转录-聚合酶链式反应(RT-PCR)方法,合成病毒外壳蛋白(CP)基因cDNA。对所获得的cDNA克隆进行序列测定及分析,结果表明,湖北省真菌传小麦黄花叶病病毒分离物与小麦梭条斑花叶病毒(WSSMV)、大麦黄花叶病毒(BaYMV)、大麦和性花叶病毒(BaMMV)等病毒CP基因相应序列的同源性均低于70%,而与报道的小麦黄花叶病毒(WYMV)分离物CP基因核苷酸及编码氨基酸序列同源性均超过97%。表明湖北省真菌传小麦黄花叶病病原应为小麦黄花叶病毒(WYMV)。 相似文献
7.
We determined the complete nucleotide sequence of RNA-1 and the 5-terminal region of RNA-2 from Broad bean wilt virus 1 (BBWV-1) isolate PV132. This report is the first analysis of the genome organization of BBWV-1. We also determined the complete nucleotide sequence of RNA-1 from Broad bean wilt virus 2 (BBWV-2) isolate IP and analyzed the genetic relations between BBWV-1 and BBWV-2. Similar to the BBWV-2 isolates, both RNAs of PV132 encoded a single large polyprotein, which was predicted to contain some functional proteins in a manner similar to those of comovirus. With respect to the deduced amino acid sequences of the mature proteins, PV132 and IP had only 20%–40% homology to comovirus. On the other hand, IP was 73%–98% homologous to BBWV-2 isolates, but PV132 was 39%–67% homologous to the isolates. Although the extent of the homologies differed, the homologies were limited between BBWV-1 and BBWV-2 not only for the coat protein but also for the other proteins. These results clearly support the placement of BBWV-1 and BBWV-2 in the genus Fabavirus as distinct species, proposed on the basis of double immunodiffusion tests.The nucleotide sequence data reported are available in the DDBJ/EMBL/GenBank databases under the accession numbers AB084450 (RNA-1 of isolate PV132), AB084451 (RNA-2 of isolate PV132), and AB023484 (RNA-1 of isolate IP) 相似文献
8.
A whitefly transmitted begomovirus was detected by PCR using begomovirus-specific primers from naturally infected Calendula officinalis plants showing yellow vein disease symptoms. An approximately 800 bp PCR amplicon was cloned and sequenced to identify the species of the virus isolate. Analysis of nucleotide sequence data resulted in its identification as the complete coat protein gene open reading frame (CP ORF) of 771 bp, which encoded 256 amino acid residues. The coat protein of the virus isolate shared maximum identities of 96–97% with four strains of Tobacco curly shoot virus (ToCSV) and an Ageratum enation virus (AgEV) during BLAST analysis of sequence data. Nucleotide- and amino acid-based phylogenetic analysis revealed the close relationship of the isolate with ToCSV strains, therefore it has been identified as an isolate of ToCSV and C. officinalis is considered to be a new host of ToCSV begomovirus. Association of a DNA-β molecule with the virus isolate was also detected by PCR and Southern hybridization tests using DNA-β specific primers and probe. 相似文献
9.
Tsutomu Matsumoto Hideki Yamamoto Shin-ichi Fuji Masayasu Inoue 《Journal of General Plant Pathology》2007,73(3):222-224
A novel potyvirus, tentatively named Ornithogalum virus 2 (OV-2) because only its nucleotide sequence of the coat protein gene has been revealed, was isolated for the first
time from Ornithogalum thyrsoides. OV-2 had a flexuous particle (700–740 nm in length) and was sap and aphid transmissible. The virus had a narrow host range;
of 36 test plants in 12 families, only O. thyrsoides and O. dubium were infected. Because the virus caused characteristic stripe mosaic on O. thyrsoides, we propose Ornithogalum stripe mosaic virus (OrSMV), instead of OV-2 for the proper name of the virus.
The nucleotide sequence data reported is available in the DDBJ/EMBL/GenBank databases under accession number AB271783. 相似文献
10.
On plants at 59 sugarcane plantations in Central and East Java, Indonesia, we found virus-like symptoms such as streak mosaic.
The virus was transmitted mechanically and was sett-borne. The nucleotide sequence of the coat protein gene had the highest
identity with that of Sugarcane streak mosaic virus (SCSMV) isolate Pakistani. We tentatively designate this isolate as SCSMV-Idn (Indonesia). 相似文献
11.
Ramesh R. Chavan Michael N. Pearson Dan Cohen 《European journal of plant pathology / European Foundation for Plant Pathology》2009,124(2):247-259
Actinidia chinensis and A. deliciosa plants from China, showing a range of symptoms, including vein clearing, interveinal mottling, mosaics and chlorotic ring
spots, were found to contain ~300 nm rod-shaped virus particles. The virus was mechanically transmitted to several herbaceous
indicators causing systemic infections in Nicotiana benthamiana, N. clevelandii, and N. occidentalis, and local lesions in Chenopodium quinoa. Systemically- infected leaves reacted with a Tobacco mosaic virus polyclonal antibody in indirect ELISA. PCR using generic and specific Tobamovirus primers produced a 1,526 bp sequence spanning the coat protein (CP), movement protein (MP), and partial RNA replicase genes
which showed a maximum nucleotide identity (88%) with Turnip vein clearing virus and Penstemon ringspot virus. However, when the CP sequence alone was considered the highest CP sequence identity (96% nt and 98% aa) was to Ribgrass mosaic virus strain Kons 1105. The morphological, transmission, serological and molecular properties indicate that the virus is a member
of subgroup 3 of the genus Tobamovirus. 相似文献
12.
S. Kreiah M. L. Edwards W. S. Hawes A. T. Jones D. J. F. Brown W. J. McGavin J. I. Cooper 《European journal of plant pathology / European Foundation for Plant Pathology》1996,102(3):297-303
The coding sequences in RNA2 for the coat proteins (CP) of strawberry latent ringspot virus (SLRSV) were modified and amplified using polymerase chain amplification reactions (PCR) to facilitate their expression inAgrobacterium tumefaciens-transformedNicotiana tabacum Xanthi-nc. The coding sequences for the smaller capsid protein (S, 29kDa) and that for the theoretical precursor of L and S (P, 73kDa) had ATG initiation codon sequences added at the 5-proximal Ser/Gly (S/G) cleavage site in the unmodified sequence. The sequence coding for the larger of the two proteins of mature SLRSV capsids (L, 44kDa) had an ATG codon added at its 5 S/G site and a TAG stop codon sequence added at the 3-proximal S/G site. The P, L and S proteins were expressedin planta to a maximum concentration of 0.01 % of total extractable proteins but did not assemble into virus-like particles. When challenged by mechanical inoculation with virus particles or viral RNA, and compared with control plants, tobacco plants (primary transgenic clones or S1 and S2, kanamycin-resistant seedlings) expressing the virus capsid subunits separately, or their precursor, decreased the accumulation of SLRSV particles in inoculated leaves and fewer plants became invaded systemically. In experiments in which the roots of seedlings were exposed to SLRSV-carrying vector nematodes (Xiphinema diversicaudatum), SLRSV was detected in the roots of non-transformed control tobacco plants (6/20) and in transgenic tobacco expressing the L protein (7/40), but not in any of 25 tobacco plants expressing the S protein or in 35 expressing the P protein. This is the second example of CP-mediated resistance to virus inoculation by nematode vectors. 相似文献
13.
Nico M. Horn Nasir Saleh Yuliantoro Baliadi 《European journal of plant pathology / European Foundation for Plant Pathology》1991,97(2):125-127
Using ELISA to determine whether cowpea mild mottle virus (CMMV) was present in soybean and groundnut seeds, the virus was not detected in 4144 seeds harvested from seven CMMV-infected soybean genotypes and in 214 seeds collected from CMMV-infected groundnut plants (cv. Gajah). These results, together with those of other researchers, suggest that, under the conditions tested, CMMV is not transmitted by seed. This in contrast to what is generally accepted and published in reviews. 相似文献
14.
采用RT-PCR方法克隆了黄瓜绿斑驳花叶病毒辽宁分离物(Cucumber green mottle mosaic virus Liaoning isolate, CGMMV-LN)的cp基因并连接到原核表达载体pGEX-4T-3和pET-22b (+)上, 将获得的重组子pGEX-4T-3-CGMMV CP和pET-22b (+)-CGMMV CP转化大肠杆菌BL21后用IPTG进行诱导表达。SDS-PAGE和W estern blot分析表明, cp基因在大肠杆菌中获得了高效表达, 融合蛋白分子量分别为43.8 kDa和17.3 kDa。将17.3 kDa融合蛋白纯化后免疫家兔, 制备了CGMMV特异性抗血清, 抗原包被间接ELISA法(ACP-ELISA)测定抗血清的效价为1/20 000。 相似文献
15.
An isolate of ryegrass mosaic virus (RMV-SA) was found in Italian ryegrass plants in two areas in South Africa. Preliminary characterization indicated that the virus exhibited the same symptoms and host range as RMV strains previously found in Canada and the UK. The virus was transmitted by the eriophyid mite Abacarus hystrix. Particle structure and size were comparable to the USA and UK strains. The coat protein and RNA were found to be slightly larger than previously reported, being 32kDa and 2·8 × 106 , respectively. The virus exhibited serological cross-reactivity with antisera to RMV-Wales and RMV-Canada but was not serologically related to other Rymovirus members. 相似文献
16.
Kaoru Hanada Fumiyoshi Fukumoto Manabu Kusunoki Mitsuro Kameya-Iwaki Yuko Tanaka Toru Iwanami 《Journal of General Plant Pathology》2006,72(6):383-386
An undescribed spherical virus ca. 30 nm in diameter was isolated from gladiolus (Gladiolus spp.) plants in Japan. The virus had a moderate host range within eight families. Purified virus preparations contained two
large RNA components and one coat protein with mobility similar to Cycas necrotic stunt virus (CNSV) from cycas (Cycas revolute). The virus was serologically closely related to CNSV. Its nucleotide sequence of the coat protein gene had 89% common identity
with that of CNSV. These results indicated that the virus isolated from gladiolus is a new strain of CNSV.
The nucleotide sequence data reported are available in the DDBJ/EMBL/Gen Bank databases under the accession number AB237656. 相似文献
17.
18.
C. Soria M. L. Gomez-Guillamon J. E. Duffus 《European journal of plant pathology / European Foundation for Plant Pathology》1991,97(5):289-296
The agent causing a yellowing disease of melon (Cucumis melo), which results in severe losses in crops under plastic on the coastal plains of southeast Spain, was shown to be transmitted in a semipersistent manner by the greenhouse whitefly (Trialeurodes vaporariorum Westwood). The agent was transmitted by grafting, but not by mechanical inoculation or through seeds. The agent was acquired in the minimum period tested (2 h) and could infect plants in an infection feeding interval of 6 h.
Capsella bursa-pastoris, Cucumis melo, C. sativus, Cucurbita moschata, Cichorium endivia, Lactuca sativa andTaraxacum officinale were found susceptible.Results suggest that the yellowing disease affecting melon crops in the southeast of Spain is due to a pathogen similar to beet pseudo yellows virus, but this has to be confirmed by serology. 相似文献
19.
A domain of the readthrough protein of barley yellow dwarf virus (NY-RPV isolate) is essential for aphid transmission 总被引:1,自引:0,他引:1
P. F. McGrath R. M. Lister B. G. Hunter 《European journal of plant pathology / European Foundation for Plant Pathology》1996,102(7):671-679
Luteoviruses are obligately transmitted by aphids and contain two capsid proteins, the coat protein (CP) coded for by open reading frame (ORF) 3, and the readthrough protein (RTP), produced by readthrough of the amber termination codon of ORF 3 into the contiguous ORF 5. Previous studies have suggested that it is the RTP that determines transmissibility and vector specificity. To investigate which capsid protein or protein part contains determinants for the transmission of the NY-RPV isolate of barley yellow dwarf virus (BYDV) by its vectorRhopalosiphum padi, we produced three fusion proteins by expressing NY-RPV cDNA inE. coli. These respectively represented the CP alone (P3), a region of the RTP immediately following the amber termination codon (P5a), and the remainder of the RTP (P5b). Polyclonal antisera raised against the P3, P5a and P5b proteins each gave distinctive reactions against purified NY-RPV on Western blots. Also, in ELISA tests, antisera raised against all three fusion proteins detected purified intact virions. When mixed with purified virions and fed toR. padi through Parafilm membranes, immunoglobulins (Igs) from antisera raised against P3 and P5b had no effect on transmission, whereas Ig from antiserum against P5a interfered with transmission. P5a antiserum Ig had no effect on the transmission of the P-PAV isolate of BYDV byR. padi. The results demonstrate that while neither the CP itself nor the terminal region of the RTP are key determinants for transmission, a specific domain in the central part of the RTP is an important determinant in the transmission of NY-RPV byR. padi, though apparently not of P-PAV. 相似文献
20.
对曹琦和濮祖芹早期分离到的烟草坏死病毒大豆分离物的生物学、血清学和外壳蛋白的序列进行了进一步研究。该分离物能侵染8科29种植物, 除系统侵染大豆和本生烟外, 其余寄主均为局部侵染。电镜下病毒粒子呈球状, 直径约28nm。基因组为单组分RNA, 大小约为3.7 kb, 具有2条亚基因组, 分别约为1.6 kb和1.3 kb。外壳蛋白亚基的分子量约为30 kDa。血清学试验表明, 该分离物与TNV柳树分离物的抗血清呈特异反应, 与同属坏死病毒属(Necrovirus)的烟草坏死病毒D(TNV-D)和甜菜黑色焦枯病毒(BBSV)无血清学关系。利用简并引物通过RT-PCR克隆了该分离物的外壳蛋白基因。序列分析表明, 该分离物与烟草坏死病毒A(TNV-A)、TNV-D和TNV-DH的外壳蛋白分别具有88.77%、45.13%和45.49%的氨基酸序列一致性。因此, 该大豆分离物属于TNV-A的一个新株系, 命名为TNV-AC。 相似文献