Your search keyword '"Trees virology"' showing total 11 results

1. A rapid silica spin column-based method of RNA extraction from fruit trees for RT-PCR detection of viruses.

Author

Yang F, Wang G, Xu W, and Hong N

Subjects

Silicon Dioxide, Centrifugation methods, Chromatography methods, Plant Diseases virology, RNA, Viral isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods, Trees virology, Virology methods

Abstract

Efficient recovery of high quality RNA is very important for successful RT-PCR detection of plant RNA viruses. High levels of polyphenols and polysaccharides in plant tissues can irreversibly bind to and/or co-precipitate with RNA, which influences RNA isolation. In this study, a silica spin column-based RNA isolation method was developed by using commercially available silica columns combined with the application of a tissue lysis solution, and binding and washing buffers with high concentration guanidinium thiocyanate (GuSCN, 50% w/v), which helps remove plant proteins, polysaccharides and polyphenolic compounds. The method was successfully used to extract high quality RNA from citrus (Citrus aurantifolia), grapevine (Vitis vinifera), peach (Prunus persica), pear (Pyrus spp.), taro (Colocosia esculenta) and tobacco (Nicotiana benthamiana) samples. The method was comparable to conventional CTAB method in RNA isolation efficiency, but it was more sample-adaptable and cost-effective than commercial kits. High quality RNA isolated using silica spin column-based method was successfully used for the RT-PCR and/or multiplex RT-PCR amplification of woody fruit tree viruses and a viroid. The study provided a useful tool for the detection and characterization of plant viruses., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

2. Development of multiplex polymerase chain reaction assay for simultaneous detection of clostero-, badna- and mandari-viruses along with huanglongbing bacterium in citrus trees.

Author

Meena RP and Baranwal VK

Subjects

Closterovirus isolation & purification, DNA Primers, Flexiviridae isolation & purification, India, Plant Diseases microbiology, Plant Diseases prevention & control, Plant Diseases virology, Plant Viruses genetics, Rhizobiaceae isolation & purification, Sensitivity and Specificity, Trees virology, Citrus microbiology, Citrus virology, Closterovirus genetics, Flexiviridae genetics, Multiplex Polymerase Chain Reaction methods, Rhizobiaceae genetics

Abstract

Citrus trees harbor a large number of viral and bacterial pathogens. Citrus yellow vein clearing virus (CYVCV), Indian citrus ringspot virus (ICRSV), Citrus yellow mosaic virus (CYMV), Citrus tristeza virus (CTV) and a bacterium, Candidatus Liberibacter asiaticus (CLa) associated with huanglongbing (HLB) disease, the most prevalent pathogens in citrus orchards of different regions in India and are responsible for debilitating citriculture. For detection of these viral and bacterial pathogens a quick, sensitive and cost effective detection method is required. With this objective a multiplex polymerase chain reaction (mPCR) assay was developed for simultaneous detection of four viruses and a bacterium in citrus. Several sets of primers were designed for each virus based on the retrieved reference sequences from the GenBank. A primer pair published previously was used for greening bacterium. Each pair of primers was evaluated for their sensitivity and differentiation by simplex and mPCR. The constant amplified products were identified on the basis of molecular size in mPCR and were compared with standard PCR. The amplicons were cloned and results were confirmed with sequencing analysis. The mPCR assay was validated using naturally infected field samples for one or more citrus viruses and the huanglongbing bacterium. The mPCR assay developed here will aid in the production of virus free planting materials and rapid indexing for certification of citrus budwood programme., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

3. One-step multiplex quantitative RT-PCR for the simultaneous detection of viroids and phytoplasmas of pome fruit trees.

Author

Malandraki I, Varveri C, Olmos A, and Vassilakos N

Subjects

Phytoplasma genetics, Plant Diseases microbiology, Plant Diseases virology, Sensitivity and Specificity, Time Factors, Trees microbiology, Trees virology, Viroids genetics, Multiplex Polymerase Chain Reaction methods, Phytoplasma isolation & purification, Real-Time Polymerase Chain Reaction methods, Rosaceae microbiology, Rosaceae virology, Viroids isolation & purification

Abstract

A one-step multiplex real-time quantitative reverse transcription polymerase chain reaction (RT-qPCR) based on TaqMan chemistry was developed for the simultaneous detection of Pear blister canker viroid and Apple scar skin viroid along with universal detection of phytoplasmas, in pome trees. Total nucleic acids (TNAs) extraction was performed according to a modified CTAB protocol. Primers and TaqMan MGB probes for specific detection of the two viroids were designed in this study, whereas for phytoplasma detection published universal primers and probe were used, with the difference that the later was modified to carry a MGB quencher. The pathogens were detected simultaneously in 10-fold serial dilutions of TNAs from infected plant material into TNAs of healthy plant up to dilutions 10(-5) for viroids and 10(-4) for phytoplasmas. The multiplex real-time assay was at least 10 times more sensitive than conventional protocols for viroid and phytoplasma detection. Simultaneous detection of the three targets was achieved in composite samples at least up to a ratio of 1:100 triple-infected to healthy tissue, demonstrating that the developed assay has the potential to be used for rapid and massive screening of viroids and phytoplasmas of pome fruit trees in the frame of certification schemes and surveys., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2015

4. The effectiveness of somatic embryogenesis in eliminating the cocoa swollen shoot virus from infected cocoa trees.

Author

Quainoo AK, Wetten AC, and Allainguillaume J

Subjects

Cacao embryology, Electrophoresis, Capillary methods, Plant Shoots virology, Polymerase Chain Reaction methods, Seeds growth & development, Trees virology, Badnavirus isolation & purification, Cacao virology, Plant Diseases virology, Seeds virology

Abstract

Investigations were undertaken on the use of somatic embryogenesis to generate cocoa swollen shoot virus (CSSV) disease free clonal propagules from infected trees. Polymerase chain reaction (PCR) capillary electrophoresis revealed the presence of CSSV in all the callus tissues induced from the CSSV-infected Amelonado cocoa trees (T1, T2 and T4). The virus was transmitted to primary somatic embryos induced from the infected callus tissues at the rate of 10 (19%), 18 (14%) and 16 (15%) for T1, T2 and T4, respectively. Virus free primary somatic embryos from the infected callus tissues converted into plantlets tested CSSV negative by PCR/capillary electrophoresis 2 years after weaning. Secondary somatic embryos induced from the CSSV-infected primary somatic embryos revealed the presence of viral fragments at the rate of 4 (4%) and 9 (9%) for T2 and T4, respectively. Real-time PCR revealed 23 of the 24 secondary somatic embryos contained no detectable virus. Based on these findings, it is proposed that progressive elimination of the CSSV in infected cocoa trees occurred from primary embryogenesis to secondary embryogenesis.

Published

2008

5. Application of a spotting sample preparation technique for the detection of pathogens in woody plants by RT-PCR and real-time PCR (TaqMan).

Author

Osman F and Rowhani A

Subjects

Edetic Acid pharmacology, Electrophoresis, Agar Gel, Evaluation Studies as Topic, Membranes, Artificial, Octoxynol pharmacology, Phytoplasma genetics, Phytoplasma isolation & purification, Phytoplasma virology, Plant Viruses genetics, Xylella genetics, Xylella isolation & purification, Xylella virology, Plant Viruses isolation & purification, Plant Viruses pathogenicity, Polymerase Chain Reaction methods, Reverse Transcriptase Polymerase Chain Reaction methods, Trees virology

Abstract

An extraction technique for reverse transcription-PCR (RT-PCR) detection of plant pathogens including viruses, bacteria and phytoplasma is described. The total nucleic acid of these plant pathogens was obtained by direct spotting of crude sap derived from infected leaf, petiole or cambial tissue onto two different types of membranes, positively charged Hybond N(+) Nylon and FTA membranes, and processed for use in PCR. Thirteen different plant viruses, Xylella fastidiosa (causal agent of Pierce's disease) and phytoplasmas were included in the experiment. A thermal treatment (95 degrees C for 10 min) of the Hybond N(+) Nylon discs in a buffered solution improved the detection, but for FTA membrane discs the thermal treatment was not required and the discs were directly placed in the PCR reaction cocktail. Specific amplification of genomic or ribosomal RNA fragments of these pathogens was obtained by one-step RT-PCR except for X. fastidiosa in which a fragment of the genomic DNA was used for amplification. The same sample preparation methods also worked well for real-time RT-PCR (TaqMan). The sample preparation techniques reported here could be used to store samples for future PCR test or for long distance shipment to a detection laboratory.

Published

2006

6. Single-step multiplex RT-PCR for simultaneous and colourimetric detection of six RNA viruses in olive trees.

Author

Bertolini E, Olmos A, Martínez MC, Gorris MT, and Cambra M

Subjects

Colorimetry methods, DNA Primers, Plant Diseases virology, Plant Viruses genetics, Plant Viruses isolation & purification, RNA Viruses genetics, Sensitivity and Specificity, Magnoliopsida virology, RNA Viruses isolation & purification, Reverse Transcriptase Polymerase Chain Reaction, Trees virology

Abstract

A single-step multiplex RT-PCR was developed for the simultaneous and colourimetric detection of six RNA viruses (Cucumber mosaic virus, Cherry leaf roll virus, strawberry latent ringspot virus, Arabis mosaic virus, Olive latent-1 virus and Olive latent-2 virus) which infect olive trees. Six compatible primer set for one-step RT-PCR amplification in a single closed-tube and 3' digoxigenin labelled probes were designed in optimal, specific and conserved regions. The method has been assessed with 195 Spanish field olive trees, suggesting that approximately 1.5% of the tested material was infected by Cucumber mosaic virus and 0.5% by Cherry leaf roll virus. This method saves time and reagent costs compared with monospecific RT-PCR which needs several reactions for the same number of tests. Using colourimetric detection, it is possible to analyse many samples, it increases sensitivity 10-fold, and whilst facilitating the interpretation of results, it avoids the use of gels and the toxic ethidium bromide. The method could be used routinely for sanitary and certification programmes.

Published

2001

7. Immunocapture reverse transcription-polymerase chain reaction combined with nested PCR greatly increases the detection of Prunus necrotic ring spot virus in the peach.

Author

Helguera PR, Taborda R, Docampo DM, and Ducasse DA

Subjects

Bromoviridae genetics, Enzyme-Linked Immunosorbent Assay methods, Fruit, Polymerase Chain Reaction methods, Reverse Transcriptase Polymerase Chain Reaction, Bromoviridae isolation & purification, Trees virology

Abstract

A detection system based on nested PCR after IC-RT-PCR (IC-RT-PCR-Nested PCR) was developed to improve indexing of Prunus necrotic ringspot virus in peach trees. Inhibitory effects and inconsistencies of the standard IC-RT-PCR were overcome by this approach. IC-RT-PCR-Nested PCR improved detection by three orders of magnitude compared with DAS-ELISA for the detection of PNRSV in leaves. Several different tissues were evaluated and equally consistent results were observed. The main advantages of the method are its consistency, high sensitivity and easy application in quarantine programs.

Published

2001

8. Comparison of bioassays and laboratory assays for apple stem grooving virus.

Author

Kirby MJ, Guise CM, and Adams AN

Subjects

Base Sequence, Fruit virology, Genome, Viral, Indicators and Reagents, Molecular Sequence Data, Plant Viruses genetics, Polymerase Chain Reaction, Sequence Alignment, Trees virology, Virus Latency, Plant Diseases virology, Plant Viruses isolation & purification

Abstract

The standard field double-budding assay with the indicator Virginia Crab and the glasshouse test with the indicator Malus micromalus, were compared with ELISA and immunocapture PCR for the detection of Apple stem grooving virus (ASGV) in 102 apple trees and three oriental pear. Twenty-two trees were positive for ASGV by both ELISA and IC-PCR but three of these trees were negative by Virginia Crab, three were negative by M. micromalus and one was negative by both these bioassays. The infected trees were re-tested by IC-PCR and ELISA in a second year; the IC-PCR results were confirmed but two of the 22 infected trees were negative by ELISA. On this evidence, IC-PCR is a more reliable assay for ASGV than the slow and expensive bioassays.

Published

2001

9. Differentiation of closely related but biologically distinct cherry isolates of Prunus necrotic ringspot virus by polymerase chain reaction.

Author

Hammond RW, Crosslin JM, Pasini R, Howell WE, and Mink GI

Subjects

DNA Restriction Enzymes metabolism, DNA, Viral metabolism, Electrophoresis, Polyacrylamide Gel, Ilarvirus genetics, Polymorphism, Restriction Fragment Length, Reverse Transcriptase Polymerase Chain Reaction methods, Fruit virology, Ilarvirus classification, Ilarvirus isolation & purification, Trees virology

Abstract

Prunus necrotic ringspot ilarvirus (PNRSV) exists as a number of biologically distinct variants which differ in host specificity, serology, and pathology. Previous nucleotide sequence alignment and phylogenetic analysis of cloned reverse transcription-polymerase chain reaction (RT-PCR) products of several biologically distinct sweet cherry isolates revealed correlations between symptom type and the nucleotide and amino acid sequences of the 3a (putative movement protein) and 3b (coat protein) open reading frames. Based upon this analysis, RT-PCR assays have been developed that can identify isolates displaying different symptoms and serotypes. The incorporation of primers in a multiplex PCR protocol permits rapid detection and discrimination among the strains. The results of PCR amplification using type-specific primers that amplify a portion of the coat protein gene demonstrate that the primer-selection procedure developed for PNRSV constitutes a reliable method of viral strain discrimination in cherry for disease control and will also be useful for examining biological diversity within the PNRSV virus group.

Published

1999

10. Development of a multiplex immunocapture RT-PCR assay for detection and differentiation of tomato and tobacco mosaic tobamoviruses.

Author

Jacobi V, Bachand GD, Hamelin RC, and Castello JD

Subjects

Enzyme-Linked Immunosorbent Assay methods, Solanum lycopersicum virology, Molecular Sequence Data, Plant Extracts, Plant Viruses genetics, Plant Viruses isolation & purification, Sensitivity and Specificity, Tobacco Mosaic Virus classification, Tobacco Mosaic Virus genetics, Tobacco Mosaic Virus immunology, Tobamovirus classification, Tobamovirus genetics, Tobamovirus immunology, Polymerase Chain Reaction methods, Tobacco Mosaic Virus isolation & purification, Tobamovirus isolation & purification, Trees virology

Abstract

Immunocapture (IC) RT-PCR assays were developed for detection of tomato (ToMV) and tobacco mosaic (TMV) tobamoviruses in spruce and pine extracts. When purified viruses were diluted in root or needle extracts of virus-free conifer seedlings, both IC-RT-PCR assays detected their respective target viruses at concentrations of 10-100 fg ml(-1). This compared to ELISA detection sensitivities of 1 ng ml(-1). Primers were designed from regions of high sequence diversity. Specificity of all primer pairs was confirmed by sequencing of PCR products. PCR distinguished more reliably between the two viruses than ELISA. Moreover, a multiplex IC-RT-PCR assay for the simultaneous detection and differentiation of TMV and ToMV was developed. When root extracts were seeded with both viruses simultaneously, the multiplex assay detected each virus at concentrations of 1-10 pg ml(-1). Six TMV and 18 ToMV isolates from various hosts, water samples and a soil sample were amplified and differentiated by multiplex IC-RT-PCR. No amplifications were observed against pepper mild mottle and ribgrass mosaic tobamoviruses and against six viruses belonging to other taxonomic groups.

Published

1998

11. The use of short and long PCR products for improved detection of prunus necrotic ringspot virus in woody plants.

Author

Rosner A, Maslenin L, and Spiegel S

Subjects

DNA, Complementary chemistry, Fruit, Ilarvirus chemistry, Nuts, RNA, Viral chemistry, RNA-Directed DNA Polymerase, Templates, Genetic, Trees virology, Ilarvirus isolation & purification, Polymerase Chain Reaction methods

Abstract

The reverse transcriptase-polymerase chain reaction (RT-PCR) was used for detection of prunus necrotic ringspot virus (PNRSV) in dormant peach and almond trees by the application of two different pairs of primers yielding a short and a long product, respectively. The relative amount of the short (200 base pair, bp) product was higher than the longer (785 bp) product. PNRSV was detected better in plant tissues with a low virus concentration (e.g. dormant trees) by amplification of the short PCR product, whereas the long product was product was produced at higher virus titers. Simultaneous amplification of both short and long products was demonstrated using a three-primer mixture in a single reaction tube. In this assay, amplification of either PCR product indicated the presence of PNRSV-specific sequences in the plant tissue examined, thus covering a wide range of virus concentrations in a single test. Dilution of the RNA extracted from infected plant material resulted in a steep decline in the amplification of both short and long PCR products. In contrast, serial dilutions of the intermediate cDNA template differentially affected the amplification patterns: the relative amount of the short product increased whereas that of the long product decreased. These results may explain the preferential amplification of the short PCR product observed in samples containing low virus concentrations.

Published

1997