Comparison of Monoclonal Antibodies and Polymerase Chain Reaction Assays for the Typing of Isolates Belonging to the D and M Serotypes of Plum Pox Potyvirus

Candresse, Thierry; Cambra, M.; Dallot, Sylvie; Lanneau, M.; Asensio, M.; Gorris, M. T.; Revers, Frédéric; Macquaire, G.; Olmos, Antonio; Boscia, D.; Quiot, J. B.; Dunez, Jean

doi:10.1094/phyto.1998.88.3.198

Cited by 99 publications

(80 citation statements)

References 22 publications

Supporting

Mentioning

Contrasting

Unclassified

Order By: Relevance

“…However, we are cautious about the rates of mixed infection in Ankara. We assume that most of the mixed infections identified by Elibüyük (2011) could be PPV-T, similar to the misinterpretation of PPV-T as PPV-M, because T isolates could also react to PPV-D-specific antibodies Candresse et al, 1998;Myrta et al, 1998). Other than D isolates in Ankara, PPV-D occurrence has not been reported in other regions in Turkey.…”

Section: Discussionmentioning

confidence: 87%

“…Sequence analysis is accepted as the most reliable method to identify the virus. Similar to other plant viruses, PPV has been mostly analyzed by sequencing the viral CP gene (Bousalem et al, 1994;Candresse et al 1998). Typing methods for the P3-6K1 region have also been developed, and the P3-6K1 region has been used for PPV variability studies, allowing PPV subgroup discrimination independent of the CP (Glasa et al, 2002).…”

mentioning

confidence: 99%

See 1 more Smart Citation

Strain identification and sequence variability of plum pox virus in Turkey

Gürcan¹,

Ceylan²

2016

Turk J Agric For

View full text Add to dashboard Cite

IntroductionPlum pox virus (PPV) is considered to be the most devastating disease of Prunus spp. (Cambra et al., 2006), and it is one of the 10 most studied plant viruses in molecular plant pathology (Scholthof et al., 2011). PPV is a member of the genus Potyvirus, which encompasses approximately 30% of the currently known plant viruses (Gibbs et al., 2008). The virus causes reduced fruit quality and premature fruit drop in susceptible stone fruit crops (peach, apricot, plum, and Japanese plum). After the onset of the viral infection, controlling the virus has been very difficult in stone fruit-producing regions (Cambra et al., 2006).PPV has a single molecule of a positive, single-sense, RNA genome, approximately 9.7 kb. RNA viruses exhibit rapid evolution and have high mutation rates with large population sizes, resulting in high genetic diversity within the virus populations (Domingo and Holland, 1997). Like other RNA viruses, PPV shows high variability, with nine strains identified to date: Ancestor Marcus (An), Cherry (C), Cherry Russian (CR), Dideron (D), Marcus (M), El Amar (EA), Recombinant (Rec), Turkey (T), and Winona (W). This large number of strains is greater than for any other Potyvirus (Garcia et al., 2014). Among the nine strains, PPV-M and PPV-D are considered the two most prevalent groups (Candresse et al., 1998). PPV-M prevalence has been reported throughout southern, eastern, and central Europe (Myrta et al., 2001;Capote et al., 2010). PPV-M identification with reliable sequence analysis was not reported outside of Europe (Garcia et al., 2014). PPV-D is the most prevalent strain in Europe and worldwide and it has been reported in more than 40 countries (Garcia and Cambra, 2007;James et al., 2013). PPV-Rec is a recombination product of the M and D strains, carrying mostly a PPV-D-like genome and known to be present in central and south-central Europe (Cervera

show abstract

Section: Discussionmentioning

confidence: 87%

mentioning

confidence: 99%

Strain identification and sequence variability of plum pox virus in Turkey

Gürcan¹,

Ceylan²

2016

Turk J Agric For

View full text Add to dashboard Cite

show abstract

“…The most frequently targeted region in PPV analysis is the highly variable 5'-terminal part of the CP gene. Many strain-specific primers targeting this and other parts of the PPV genome have been developed for single or mixed infection detection (Candresse et al, 1995;Candresse et al, 1998;Nemchinov & Hadidi, 1998;Glasa et al, 2002b;Šubr et al, 2004;Glasa et al, 2005;Glasa et al, 2013). PPV strains can also be discriminated by PCR-RFLP analysis, but some isolates may be mistakenly classified.…”

Section: Plum Pox Virus Strain Variabilitymentioning

confidence: 99%

Plum pox virus strains: Diversity and geographical distribution in Serbia

Jevremović

Paunović

2014

Pesticidi i fitomedicina

View full text Add to dashboard Cite

Plum pox virus (PPV) is the causal agent of Sharka disease. Since its discovery, Sharka has been considered as a calamity in plum orchards. PPV is present worldwide in many Prunus species, causing great economic losses. In highly susceptible plum varieties, such as Pozegaca, PPV causes a premature fruit drop and reduces fruit quality, which leads to total yield loss. Eight PPV strains (PPV-M, PPV-D, PPV-EA, PPV-C, PPV-Rec, PPV-W, PPV-T and PPVCR) have been recognized so far. Three major strains (PPV-M, PPV-D and PPV-Rec) are the most widely dispersed and occur frequently in many European countries. Other strains are of minor importance due to their limited host preferences or geographic distribution. So far, all three major strains have been identified in Serbia. In this paper, we provide a comprehensive overview of the research into Plum pox virus variability in Serbia. [Projekat Ministarstva nauke Republike Srbije, br TR-20013A i br. TR-31064. This study was partially supported by the ECONET grant no. 10159PL, the FP7 project SharCo]

show abstract

“…Reasonably "universal" primers have been developed for some virus families, genera, and "species" targeted to taxon-specific sequences (35,91,150). RT-PCR clearly differentiates between some strains of common viruses: for example, between PPV strains D and M (27) and SMV strains G2 and G7 (131) The methods mentioned above are all limited by their reliance on a minute fraction of a taxon's many defining features. For nucleic acid-based methods, the accuracy of the comparison to some degree will be proportional to the length of the fragment (and/or the site) used in the analysis.…”

Section: Comparison and Validation Of Current Microbial Forensic Idenmentioning

confidence: 99%

Plant Pathogen Forensics: Capabilities, Needs, and Recommendations

Fletcher

Bender

Budowle

et al. 2006

Microbiol Mol Biol Rev

163

View full text Add to dashboard Cite

SUMMARY A biological attack on U.S. crops, rangelands, or forests could reduce yield and quality, erode consumer confidence, affect economic health and the environment, and possibly impact human nutrition and international relations. Preparedness for a crop bioterror event requires a strong national security plan that includes steps for microbial forensics and criminal attribution. However, U.S. crop producers, consultants, and agricultural scientists have traditionally focused primarily on strategies for prevention and management of diseases introduced naturally or unintentionally rather than on responding appropriately to an intentional pathogen introduction. We assess currently available information, technologies, and resources that were developed originally to ensure plant health but also could be utilized for postintroduction plant pathogen forensics. Recommendations for prioritization of efforts and resource expenditures needed to enhance our plant pathogen forensics capabilities are presented.

show abstract

Comparison of Monoclonal Antibodies and Polymerase Chain Reaction Assays for the Typing of Isolates Belonging to the D and M Serotypes of Plum Pox Potyvirus

Cited by 99 publications

References 22 publications

Strain identification and sequence variability of plum pox virus in Turkey

Strain identification and sequence variability of plum pox virus in Turkey

Plum pox virus strains: Diversity and geographical distribution in Serbia

Plant Pathogen Forensics: Capabilities, Needs, and Recommendations

Contact Info

Product

Resources

About