论文信息 - Infection Efficiency of Four Phytophthora infestans Clonal Lineages and DNA-Based Quantification of Sporangia - 字舞流文

Infection Efficiency of Four Phytophthora infestans Clonal Lineages and DNA-Based Quantification of Sporangia

The presence and abundance of pathogen inoculum is with host resistance and environmental conditions a key factor in epidemic development. Therefore, several spore-sampling devices have been proposed to monitor pathogen inoculum above fields. However, to make spore sampling more reliable as a management tool and to facilitate its adoption, information on infection efficiency and molecular tools for estimating airborne sporangia concentration are needed. Experiments were thus undertaken in a growth chamber to study the infection efficiency of four clonal lineages of P. infestans (US-8, US-11, US-23, and US-24) by measuring the airborne sporangia concentration and resulting disease intensity. The relationship between the airborne sporangia concentration and the number of lesions per leaf was exponential. For the same concentration, the sporangia of US-23 caused significantly more lesions than the sporangia of the other clonal lineages did. Under optimal conditions, an airborne sporangia concentration of 10 sporangia m−3 for US-23 was sufficient to cause one lesion per leaf, whereas for the other clonal lineages, it took 15 to 25 sporangia m−3 to reach the same disease intensity. However, in terms of diseased leaf area, there was no difference between clonal lineages US-8, US-23 and US-24. Also, a sensitive quantitative real-time polymerase chain reaction (qPCR) tool was developed to quantify P. infestans airborne sporangia with detection sensitivity of one sporangium. The specificity of the qPCR assay was rigorously tested for airborne inoculum and was either similar to, or an improvement on, other published PCR assays. This assay allows rapid and reliable detection and quantification of P. infestans airborne sporangia and thereby, facilitates the implementation of spores-sampling network.

Carole Beaulieu | Odile Carisse | M. Fall | C. Lévesque | O. Carisse | C. Beaulieu | H. Rocheleau | Mamadou Lamine Fall | David Mathieu Tremblay | Mélanie Gobeil-Richard | Julie Couillard | Hélène Rocheleau | Hervé Van der Heyden | Camile André Lévesque | Julie Couillard | D. Tremblay | H. Van der Heyden | Mélanie Gobeil-Richard | Hélène Rocheleau | H. van der Heyden

[1] R. Visser,et al. Applied Biotechnology to Combat Late Blight in Potato Caused by Phytophthora Infestans , 2009, Potato Research.

[2] N. Dufault,et al. Potential effects of diurnal temperature oscillations on potato late blight with special reference to climate change. , 2015, Phytopathology.

[3] C. Smart,et al. The 2009 Late Blight Pandemic in the Eastern United States - Causes and Results. , 2013, Plant disease.

[4] Laurence V. Madden,et al. The study of plant disease epidemics , 2007 .

[5] A. Gevens,et al. Novel Resistance in Heirloom Tomatoes and Effectiveness of Resistance in Hybrids to Phytophthora infestans US-22, US-23, and US-24 Clonal Lineages. , 2014, Plant disease.

[6] H. Judelson,et al. Enhanced Polymerase Chain Reaction Methods for Detecting and Quantifying Phytophthora infestans in Plants. , 2000, Phytopathology.

[7] M. Fall,et al. Spatiotemporal variation in airborne sporangia of Phytophthora infestans: characterization and initiatives towards improving potato late blight risk estimation , 2015 .

[8] H. W. Platt,et al. Development of a SNP genetic marker system based on variation in microsatellite flanking regions of Phytophthora infestans , 2010 .

[9] W. Rossing,et al. Scenario approach for assessing the utility of dispersal information in decision support for aerially spread plant pathogens, applied to Phytophthora infestans. , 2009, Phytopathology.

[10] B. Kleinhenz,et al. Effectiveness of SIMBLIGHT1 and SIMPHYT1 models for predicting Phytophthora infestans in north-eastern United States , 2012 .

[11] Y. Cohen,et al. RESISTANCE TO PHENYLAMIDE FUNGICIDES: a case study with phytophthora infestans involving mating type and race structure. , 1996, Annual review of phytopathology.

[12] James G. Horsfall,et al. Plant Pathology, an Advanced Treatise. , 1960 .

[13] D. Cooke,et al. Markers, old and new, for examining Phytophthora infestans diversity , 2004 .

[14] C. Gachon,et al. DNA barcoding of oomycetes with cytochrome c oxidase subunit I and internal transcribed spacer , 2011, Molecular ecology resources.

[15] S. Restrepo,et al. The Plant Pathogen Phytophthora andina Emerged via Hybridization of an Unknown Phytophthora Species and the Irish Potato Famine Pathogen, P. infestans , 2011, PloS one.

[16] H. W. Platt,et al. Genetic Composition of Phytophthora infestans in Canada Reveals Migration and Increased Diversity. , 2012, Plant disease.

[17] D. Ebert,et al. Quantitative PCR to detect, discriminate and quantify intracellular parasites in their host: an example from three microsporidians in Daphnia , 2006, Parasitology.

[18] D. Caldiz,et al. Early management of late blight (Phytophthora infestans) by using systemic fungicides applied to seed-potato tubers , 2006 .

[19] William W. Kirk,et al. Containment of existing potato late blight (Phytophthora infestans) foliar epidemics with fungicides , 2002 .

[20] N. Grünwald,et al. The biology of Phytophthora infestans at its center of origin. , 2005, Annual review of phytopathology.

[21] M. Fall,et al. Bremia lactucae Infection Efficiency in Lettuce is Modulated by Temperature and Leaf Wetness Duration Under Quebec Field Conditions. , 2015, Plant disease.

[22] M. Coffey,et al. Species Tree Estimation for the Late Blight Pathogen, Phytophthora infestans, and Close Relatives , 2012, PloS one.

[23] P. Tooley,et al. Development of PCR primers from internal transcribed spacer region 2 for detection of Phytophthora species infecting potatoes , 1997, Applied and environmental microbiology.

[24] Y. Cohen. Local and systemic control of Phytophthora infestans in tomato plants by DL-3-amino-n-butanoic acids , 1994 .

[25] Jonathan D. G. Jones,et al. Genome sequence and analysis of the Irish potato famine pathogen Phytophthora infestans , 2009, Nature.

[26] David G. Schmale,et al. Tracking the potato late blight pathogen in the atmosphere using unmanned aerial vehicles and Lagrangian modeling , 2011 .

[27] B. Llorente,et al. A quantitative real‐time PCR method for in planta monitoring of Phytophthora infestans growth , 2010, Letters in applied microbiology.

[28] R. Hamelin,et al. Molecular Detection of Phytophthora ramorum by Real-Time Polymerase Chain Reaction Using TaqMan, SYBR Green, and Molecular Beacons. , 2007, Phytopathology.

[29] W. Werf,et al. Multi-scale modeling of potato late blight epidemics , 2008 .

[30] K. Gindro,et al. Development of a TaqMan real-time PCR assay for quantification of airborne conidia of Botrytis squamosa and management of botrytis leaf blight of onion. , 2009, Phytopathology.

[31] G. Danies,et al. Phenotypic Characterization of Recent Clonal Lineages of Phytophthora infestans in the United States. , 2013, Plant disease.

[32] Fenguangzhai Song. CD , 1992 .

[33] Murray Logan,et al. Biostatistical Design and Analysis Using R: A Practical Guide , 2010 .

[34] Rhys A. Farrer,et al. Genome Evolution Following Host Jumps in the Irish Potato Famine Pathogen Lineage , 2010, Science.

[35] G. Forbes,et al. Genetic Diversity of Phytophthora infestans sensu lato in Ecuador Provides New Insight Into the Origin of This Important Plant Pathogen. , 2004, Phytopathology.

[36] A. Lees,et al. Development of a quantitative real-time PCR assay for Phytophthora infestans and its applicability to leaf, tuber and soil samples , 2012 .