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1.
Serological and molecular evidence for the complexity of the leafroll disease of grapevine 总被引:1,自引:0,他引:1
Samples of leafroll-infected grapevines from various countries, as well as local sources, were tested by ELISA with antisera against two closteroviruses (GVA and NY-1) and a potyvirus (GPV) thought to be associated with leafroll. Many of the samples reacted positively with more than one antiserum, and often with all three. Positive reactions with GPV antiserum were corroborated by molecular dot-blot hybridization. One of the closteroviruses, grapevine virus A (GVA) was originally isolated from a grapevine affected by stem-pitting; furthermore, a grapevine with stem-pitting reacted positively with all three antisera, and with a potyvirus probe by dot-blot hybridization. All the leafroll-diseased vines reacted, at least in some tests, with one or more of the antisera. Hence, in spite of the complexity of this syndrome, healthy and diseased grapevines could be distinguished. 相似文献
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A. Rowhani Steve Daubert K. Arnold M. Al Rwahnih V. Klaassen D. Golino J. K. Uyemoto 《European journal of plant pathology / European Foundation for Plant Pathology》2018,151(4):919-925
An interactive relationship between vitiviruses and grapevine leafroll viruses was characterized in grapevine. Grapevine viruses A and B (GVA and GVB) were found more frequently in the presence of co-infecting Grapevine leafroll associated viruses (GLRaV-1, ?2 or ?3) than in their absence. The titers of the vitiviruses in co-infection with leafroll viruses were found to be higher than were their titers in the absence of leafroll virus infection. The occurrence of vitivirus-associated stem-pitting symptoms was correlated with leafroll virus co-infection. Specific pairing associations on the species level were found between different viti- and leafroll virus species: GVB was associated preferentially with GLRaV-2; GVA was associated preferentially with GLRaV-1 and GLRaV-3. In contrast to the increase in vitivirus titer seen with leafroll virus co-infection, the incidence and titer of grapevine leafroll virus appeared to be unaltered by vitivirus co-infection. The potential for a synergistic enhancement of grapevine disease in co-infected vines is discussed. 相似文献
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Large Scale Evaluation of Primers for Diagnosis of Rupestris Stem Pitting Associated Virus-1 总被引:2,自引:0,他引:2
G. Nolasco A. Mansinho M. Teixeira Santos C. Soares Z. Sequeira C. Sequeira P.K. Correia O.A. Sequeira 《European journal of plant pathology / European Foundation for Plant Pathology》2000,106(4):311-318
The unavailability of adequate immunological reagents has prevented the use of ELISA for the diagnosis of rupestris stem pitting disorder of grapevines. In this work, the performance of five primer pairs for broad-scale detection of rupestris stem pitting associated virus-1 by RT-PCR using ds-RNA templates was compared and contrasted with biological indexing. The virus was widespread among the budwood of 35 Portuguese grapevine varieties assayed, with a prevalence of 85%. The biological assay proved to be unreliable as an index of infection due to the high number of false negatives. Five sets of primers were assayed and compared by means of their relative sensitivity and negative predictive value. The primer pair specific for the coat protein gene was excluded because of the difficulty in identifying the specific amplified product. From the other four primer pairs, those specific for the helicase domain of the putative polymerase gene had the highest sensitivity and negative predictive value. However, a high confidence in the assay, as desirable for a certification scheme, could not be obtained by the sole use of this primer pair. An additional pair should be used in a separate or in a multiplex RT-PCR reaction. 相似文献
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X. Y. Wang C. W. Zhang W. T. Huang J. Yue J. J. Dou L. Y. Wang Q. Wang Y. Q. Cheng 《Plant pathology》2020,69(1):149-158
Efforts to control viral diseases of grapevine include the production of certified material and development of virus-resistant transgenic grapevines. However, effective antiviral agents, once the viruses have infected the plants, are still lacking. This study shows that a crude garlic extract has significant antiviral activity against grapevine viruses. Replication of grapevine leafroll-associated virus 2 (GLRaV-2) was obviously inhibited in grapevine cv. Cabernet Sauvignon calli treated with diluted (1:100) garlic extract. The relative RNA levels of GLRaV-2 and grapevine fleck virus (GFkV) in cv. Summer Black grapevine in in vitro-grown plantlets 10 days after treatment with diluted (1:100) garlic extract were about 22% and 20%, respectively, of that in controls. The viral RNA accumulation of GLRaV-2, GFkV, grapevine virus A (GVA), grapevine fanleaf virus (GFLV) and grapevine rupestris stem pitting-associated virus (GRSPaV) in field-grown grapevine cv. Centennial Seedless plants sprayed with diluted (1:100) garlic extract were about 31–40%, 26–38%, 18–31%, 17–42% and 15–18%, respectively, of that in controls. Moreover, the garlic extract treatment led to a significant decrease in viral RNA accumulation of GLRaV-3, GLRaV-2, GVA, GFkV, GFLV, GRSPaV and grapevine Pinot Gris virus in pot-grown grapevine cv. Shine Muscat plants, and viral disease symptoms in these plants were obviously attenuated. In addition, this extract significantly induced expression of pathogenesis-related protein genes and stimulated activity of antioxidant enzymes in grapevines. Taken together, these results indicate that the crude garlic extract acts as a significant inhibitor against a broad range of grapevine viruses. 相似文献
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Grapevines were surveyed for the presence of virus and virus-like diseases in the Albanian viticultural districts of Shkoder, Lesh, Kruje, Durres, Tirana, Elbasan, Lushnje and Vlora. Symptoms of grapevine degeneration, leafroll and rugose wood were observed in all areas surveyed, whereas fleck was found in volunteer plants of Vitis rupestris at Elbasan, and enation disease in a few vines near Durres. Viruses identified were grapevine fanleaf nepovirus, grapevine fleck virus, grapevine virus A, and grapevine leafroll-associated closteroviruses I and III. ELISA tests showed that 83.5% of 530 Vitis vinifera vines and 46% of 24 American rootstocks individually checked were infected by one or more viruses. The presence of Xiphinema index , the major vector of grapevine fanleaf nepovirus, was recorded from vineyards affected by yellow mosaic. 相似文献
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Stanković Ivana Zečević Katarina Delibašić Goran Jović Jelena Toševski Ivo Krstić Branka 《植物病害和植物保护杂志》2023,130(1):181-188
Journal of Plant Diseases and Protection - Grapevine rupestris stem pitting-associated virus (GRSPaV), a member of the genus Foveavirus, is a commonly detected grapevine virus around the world.... 相似文献
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‘阳光玫瑰’是我国从日本引进的葡萄优良品种。为了明确我国‘阳光玫瑰’葡萄病毒病的病原,本研究采用小RNA测序技术对2株显症和无症状的‘阳光玫瑰’葡萄样品进行病毒鉴定结果显示:显症样品中测定到8种病毒,其中包含葡萄蚕豆萎蔫病毒(Grapevine fabavirus, GFabV)和灰比诺葡萄病毒(Grapevine Pinot gris virus, GPGV);无症状样品中测定到3种葡萄病毒。对46个‘阳光玫瑰’样品进行14种葡萄病毒的RT-PCR检测,结果表明:‘阳光玫瑰’葡萄带毒率较高,病毒复合侵染情况普遍;显症样品中,GFabV检出率为88.2%,GPGV和葡萄浆果内坏死病毒(Grapevine berry inner necrosis virus,GINV)检出率为64.7%和29.4%,均明显高于无症状样品(13.8%和10.3%)。本研究旨在探明‘阳光玫瑰’葡萄携带病毒的种类和侵染状况,为其病毒病防控及病毒脱除奠定基础。 相似文献
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‘阳光玫瑰’是我国从日本引进的葡萄优良品种。为了明确我国‘阳光玫瑰’葡萄病毒病的病原,本研究采用小RNA测序技术对2株显症和无症状的‘阳光玫瑰’葡萄样品进行病毒鉴定结果显示:显症样品中测定到8种病毒,其中包含葡萄蚕豆萎蔫病毒(Grapevine fabavirus, GFabV)和灰比诺葡萄病毒(Grapevine Pinot gris virus, GPGV);无症状样品中测定到3种葡萄病毒。对46个‘阳光玫瑰’样品进行14种葡萄病毒的RT-PCR检测,结果表明:‘阳光玫瑰’葡萄带毒率较高,病毒复合侵染情况普遍;显症样品中,GFabV检出率为88.2%,GPGV和葡萄浆果内坏死病毒(Grapevine berry inner necrosis virus,GINV)检出率为64.7%和29.4%,均明显高于无症状样品(13.8%和10.3%)。本研究旨在探明‘阳光玫瑰’葡萄携带病毒的种类和侵染状况,为其病毒病防控及病毒脱除奠定基础。 相似文献
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Feiyun ZHANG Shigemitsu TORIYAMA Mami TAKAHASHI 《Journal of General Plant Pathology》2001,67(1):63-68
The genome of Ryegrass mottle virus (RGMoV) comprises 4210 nucleotides. The genomic RNA contains four open reading frames (ORFs). The largest ORF 2 encodes a
polyprotein of 947 amino acids (103.6 kDa), which codes for a serine protease and an RNA-dependent RNA polymerase. The viral
coat protein is encoded on ORF 4 present at the 3′-proximal region. Other ORFs 1 and 3 encode the predicted 14.6 kDa and 19.8
kDa proteins of unknown function. The consensus signal for frameshifting, heptanucleotide UUUAAAC and a stem-loop structure
just downstream is in front of the AUG codon of ORF 3. Analysis of the in vitro translation products of RGMoV RNA suggests that the 68 kDa protein may represent a fusion protein of ORF 2-ORF 3 produced
by frameshifting. The protease region of the polyprotein and coat protein have a low similarity with that of the sobemoviruses
(approximately 25% amino acid identity), while the RNA-dependent RNA polymerase region has particularly strong similarity
(54 to 60% of more than 350 amino acid residues). The sequence similarities of RGMoV to the sobemoviruses, together with the
characteristic genome organization indicate that RGMoV is a new species of the genus Sobemovirus.
Received 28 June 2000/ Accepted in revised form 14 November 2000 相似文献
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Grapevine leafroll‐associated virus 3 (GLRaV‐3) is associated with grapevine leafroll disease, one of the most economically important viral diseases of grapevines. This disease impacts on both vine health and grape quality; reduction in yield, brix and wine colour are among its detrimental effects. Many methods, including serological and molecular procedures, have been developed for the detection of GLRaV‐3; however, there is no PCR‐based assay available to quantify virus populations within plant tissues. A real‐time RT‐PCR assay with TaqMan probe was developed for specific and reliable quantitative detection of GLRaV‐3 in infected tissues. The designed primers and probes target the conserved sequence in the RNA‐dependent RNA polymerase (RdRp) domain of the viral genome to prevent amplification of most subgenomic and defective RNAs. This protocol was used to examine the seasonal dynamics and translocation of GLRaV‐3 in field‐grown grapevines. The results showed that the virus spread quickly from trunks to new growing shoots and leaves early in the growing season, and most samples still harboured detectable virus during late summer and autumn. The seasonal progress of one GLRaV‐3 isolate was compared in four grapevine cultivars (Chardonnay, Cabernet Sauvignon, Italia and Thompson Seedless). Within cultivars there was little variability in the distribution and translocation of GLRaV‐3, except for in Thompson Seedless. This quantitative detection assay will be a valuable tool for GLRaV‐3 diagnosis, disease monitoring and population ecology studies. 相似文献
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Rupestris Stem Pitting Associated Virus-1 is Consistently Detected in Grapevines that are Infected with Rupestris Stem Pitting 总被引:1,自引:0,他引:1
Baozhong Meng Ray Johnson Silvano Peressini Philip L. Forsline Dennis Gonsalves 《European journal of plant pathology / European Foundation for Plant Pathology》1999,105(2):191-199
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我国部分地区沙地葡萄茎痘相关病毒分离物外壳蛋白序列变异分析 总被引:2,自引:2,他引:0
为明确我国葡萄中沙地葡萄茎痘相关病毒(GRSPaV)的感染情况及病毒外壳蛋白(coat protein,CP)基因的变异特点,从而为其致病性、病害的防治以及抗病毒基因工程等研究提供依据,本研究对采自我国16个省市自治区的65个葡萄品种305株葡萄样品中的GRSPaV进行RT-PCR检测,根据地区与品种差异选取了24个阳性样品进行cp基因克隆与测序分析,并对不同RNA提取方法进行了比较。结果显示,114株样品被GRSPaV侵染,平均带毒株率为37.4%;分离物间及同一分离物不同克隆间的序列差异较大,从24个分离物克隆获得的37条cp基因序列与来源于不同国家的12个GRSPaV分离物的核苷酸序列同源性为80.5%~99.7%,氨基酸序列同源性为88.8%~100%;各个分离物的遗传距离无明显地域差异;SiO2吸附法比SDS法和CTAB法更适宜葡萄样品RNA的提取。 相似文献
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为研究新疆葡萄中沙地葡萄茎痘伴随病毒(Grapevine rupestris stem pitting associated virus,GRSPa V)、葡萄斑点病毒(Grapevine fleck virus,GFk V)及葡萄病毒A(Grapevine virus A,GVA)的发生情况和新疆分离株系统进化关系,分别克隆3种病毒新疆分离株部分基因区域,应用RT-PCR对新疆64份葡萄样品中上述3种病毒进行检测,并进行系统进化分析。结果显示,GRSPa V、GFk V和GVA的检出率分别为31.3%、62.5%和25.0%。新疆GRSPa V分离株(KJ801847)与美国GRSPa V分离株(AY368590)同源性达96.59%;新疆GFk V分离株(KJ801846)与日本GFk V分离株(AB222861)及中国辽宁GFk V分离株(JF927942)的同源性分别为91.70%和91.03%;新疆GVA分离株(KJ801845)与波兰GVA分离株(JN860997)同源性为93.88%,与中国四川GVA分离株(HQ671655)及辽宁GVA分离株(FJ445220)的同源性分别为92.92%和89.53%。表明3种葡萄病毒在新疆发生比较普遍,且新疆分离株与国内其它地方的分离株存在较大差异。 相似文献
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To evaluate wood colonization and interactions with Vitis spp. of Phaeomoniella chlamydospora, a fungal agent involved in Esca disease, isolate CBS 229.95 was transformed using a pCT74 construct which contained the genetic markers for synthetic green fluorescent protein (sGFP) and hygromycin B phosphotransferase. Nine stable P. chlamydospora fungal transformants (Pch-sGFP lines) were obtained using polyethylene-glycol-mediated transformation of protoplasts. These were characterized for sgfp and hygromycin B phosphotransferase (hph) genome insertions and for sGFP fluorescence emission, using quantitative polymerase chain reaction and fluorimetric systems, respectively. No correlation was observed between sgfp copy number genome insertion and sGFP fluorescence expression. Cuttings of Vitis vinifera 'Montepulciano', 'Verdicchio', 'Sangiovese', 'Biancame', and 'Cabernet Sauvignon'; and the grapevine rootstocks 'Kober 5BB', 'SO4', '420A', '1103P', and V. rupestris were inoculated by immersion in a conidial suspension of the selected fungal Pch-sGFP71 line and incubated at 4 ± 1 and 25 ± 1°C. Wood colonization was estimated through epifluorescence microscopy and was affected by incubation temperature. After 6 months at 4 ± 1°C, the fungal growth was completely inhibited. At 25 ± 1°C, the highest extent of wood colonization was recorded in Montepulciano and Verdicchio, with the lowest in the rootstocks SO4 and V. rupestris. The expression of the Pch-sGFP71 transformed line was localized in the xylem area, primarily around the vessels. The use of sGFP-transformed P. chlamydospora helped to clarify different aspects associated with the location of this pathogen in grapevine tissue, before disease symptom expression. 相似文献
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Ilhem Selmi Davide Pacifico Arezki Lehad Egidio Stigliano Dalila Crucitti Francesco Carimi Naima Mahfoudhi 《Plant pathology》2020,69(6):1051-1059
Grapevine rupestris stem pitting-associated virus (GRSPaV) is one of the most widespread grapevine viruses and is transmitted mainly by grafting. GRSPaV presence was tested in 487 samples representative of the Tunisian grapevine germplasm (including autochthonous, table, wine, wild grape, and rootstock varieties) from different Tunisian regions. GRSPaV infection was detected in 51.3% of samples from different Tunisian regions, among which the table grapevine cultivars were the most commonly infected (68.7%). Genetic variability of GRSPaV isolates from wild and cultivated grapevines was assessed by sequencing the partial capsid protein (CP) gene of 19 Tunisian isolates and 1 Italian GRSPaV isolate from Sicily, and the partial RNA-dependent RNA polymerase (RdRp) gene of 13 Tunisian GRSPaV isolates. According to phylogenetic analysis of CP nucleotide sequences obtained in this study and sequences retrieved from GenBank, Tunisian isolates fell into four phylogenetic groups already described (I, II, III, and IV) and two new phylogenetic groups (VI and VIII). Phylogenetic analysis of the partial RdRp gene revealed that Tunisian isolates of GRSPaV are distributed into four phylogroups. This study highlights the importance of regular monitoring of GRSPaV infections in Tunisia, with special regard to those grapevine accessions employed in conservation and selection programmes. In particular, the presence of new GRSPaV genetic variants and infection of wild grapevines must be taken into account in order to choose a correct control strategy. 相似文献
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Pasquale Saldarelli Adib Rowhani Geoffrey Routh Angelantonio Minafra Michele Digiaro 《European journal of plant pathology / European Foundation for Plant Pathology》1998,104(9):945-950
RT-PCR with degenerate primers was used for the screening of the genome of some members of the Closterovirus, Vitivirus and Trichovirus genera. Two sets of primers, targeted to conserved sequences of the heat shock protein 70 homologue of closteroviruses or to the RNA dependent RNA polymerase genes of tricho- and vitiviruses, amplified the expected fragments from total RNA extracts or double-stranded RNAs of infected plants. Amplified cDNAs were cloned, sequenced and phylogenetically analyzed. Results support the allocation of grapevine viruses A, B, D and heracleum latent virus (HLV) in the genus Vitivirus, whereas, the detection of a HSP70 homologue in grapevine leafroll-associated viruses agrees with their assignment in the genus Closterovirus. The use of degenerate primers for the identification of grapevine viruses belonging to Vitivirus and Closterovirus genera is envisaged. 相似文献