First Report of Bulb Disease of Onion Caused by Pantoea ananatis in New York

First Report of Bulb Disease of Onion Caused by Pantoea ananatis in New York

In winter 2007, disease symptoms were observed in stored yellow onion bulbs (Allium cepa) grown in New York (NY) in 2006. Similar symptoms were observed in bulbs produced in 2007, 2008, and 2009. Symptoms were associated with one to three bulb scales near the midsection. Infected scales were light b...

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Veröffentlicht in:Plant disease 2010-07, Vol.94 (7), p.916-916
Hauptverfasser: Carr, E.A, Bonasera, J.M, Zaid, A.M, Lorbeer, J.W, Beer, S.V
Format: Artikel
Sprache:eng
Schlagworte:
Allium cepa
bacterial diseases of plants
Burkholderia cepacia
disease diagnosis
Gram-negative bacteria
internal transcribed spacers
microbial genetics
molecular sequence data
new geographic records
onions
Pantoea ananatis
pathogen identification
pathogenicity
plant pathogenic bacteria
polymerase chain reaction
postharvest diseases
postharvest losses
ribosomal DNA
sequence analysis
signs and symptoms (plants)
vegetable crops
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Zusammenfassung:In winter 2007, disease symptoms were observed in stored yellow onion bulbs (Allium cepa) grown in New York (NY) in 2006. Similar symptoms were observed in bulbs produced in 2007, 2008, and 2009. Symptoms were associated with one to three bulb scales near the midsection. Infected scales were light brown to brown, not macerated, and lacking foul odors typical of onion bulbs infected with Burkholderia cepacia. Onion grower-packers located in Orange County, NY were concerned that onion lots were rejected following grading by inspectors who cut bulbs to check market quality. Extent of the problem statewide is not currently clear. Isolation attempts were made from symptomatic tissues onto nutrient agar plates (3), with incubation for 24 h at 26 to 28°C, and PA-20 (2), a semiselective medium for the isolation of Pantoea ananatis, with similar incubation for 4 to 6 days. Most strains that grew on PA-20 were gram negative and yellow pigmented with dark centers. Isolated strains were tentatively identified as P. ananatis on the basis of growth on PA-20, a positive indole and negative oxidase test, positive tests for catalase, fermentation of glucose, Voges-Proskauer, and citrate utilization; negative for phenylalanine deaminase, urease, nitrate reductase, methyl red tests, and hypersensitive response induction in tobacco. The BIOLOG (Hayward, CA) system indicated that all presumptive strains of P. ananatis utilized d-mannose, d-cellobiose, d-melibiose, l-inositol, d-arabinose, cellulose, glycerol, d-arabitol, and sucrose, but not glycogen, N-acetyl-d-galactosamine, malonic acid, l-fucose, or xylitol. Strains of P. ananatis recovered from diseased onions in Georgia (GA) (1) were included in all tests as positive controls. We used PCR primers suggested by R. D. Gitaitis (University of Georgia): PanITS1 (5'-GTC TGA TAG AAA GAT AAA GAC-3') and AS2b (5'-TTC ATA TCA CCT TAC CGG CGC-3'). Together, they amplify the 16S-23S rDNA internal transcribed spacer region of 398 bp; the nucleotide sequences of six NY and three GA strains are identical to each other and 99.3% identical to P. ananatis LMG 20103 (GenBank CP001875) and 93.3% identical to P. stewartii (AJ311838). Pathogenicity tests were done in onion leaves. For inoculation, strains were grown on nutrient agar for 24 h and bacterial suspensions of ~10 CFU/ml were prepared in sterile water. Tips of healthy, greenhouse-grown onion leaves were cut and inoculum was applied to the cut surfaces with cotton swabs. Plants were
ISSN:0191-2917
1943-7692
DOI:10.1094/PDIS-94-7-0916B