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First Report of Bacterial Wilt of Annual Bluegrass Caused by Xanthomonas
translucens pv. poae in Montana. N. A. Mitkowski, Department of
Plant Sciences, University of Rhode Island, Kingston 02881. Plant Dis. 89:1016,
2005; published on-line as DOI: 10.1094/PD-89-1016B. Accepted for publication 10
June 2005.
During August 2003, a golf course putting green sample composed of Poa annua
from the Buffalo Hill Country Club in Kalispell, MT exhibiting symptoms of
general decline, wilting, and necrosis was submitted to the University of Rhode
Island Turfgrass Disease Diagnostic Laboratory. No pathogenic fungi were
observed or cultured from affected plants. Bacterial streaming was observed from
cut leaves. Cut leaves were surface disinfested for 5 min in a 0.6% sodium
hypochlorite solution and plated on yeast dextrose calcium carbonate (YDC) agar
media. A single yellow, mucoid colony type composed of rod-shaped bacteria was
isolated from all leaves. Bacteria were gram negative, lacked anaerobic growth,
did not fluorescence on King’s medium B, and were able to grow at 33°C on
YDC. Colonies were transferred to YDC for 10 days, DNA was extracted and a
2,190-bp region encompassing the 16S rRNA, ITS, and 5(prime) end of the 23S rRNA
was amplified via polymerase chain reaction (PCR) using previously published
protocols (1). Sequence comparisons of the resulting 2,190-bp PCR product
revealed a 99.7% sequence similarity with X. translucens pv. poae
(American Type Culture Collection [ATCC] no. 33804) and a 99.8% sequence
similarity with X. translucens pv. poae M-1 (Torrington, CT). No
higher sequence similarity could be identified from a BLAST search. The Montana
isolate and the previously described M-1 isolate were inoculated onto four
replicates of 5-month-old P. annua var. annua plants by dipping
cut leaves into a bacterial suspension adjusted to 10(^9) CFU/ml in 0.9% NaCl.
Control plants were dipped into 0.9% NaCl without the presence of the bacteria.
All plants were placed in the greenhouse at an average daytime temperature of
approximately 24°C and 12 h of sunlight. After 8 weeks, the plants were
assessed for disease and checked for bacterial streaming. This experiment was
repeated once. The Montana isolate caused approximately 68 and 70% leaf death
and the M-1 isolate caused 21 and 25% leaf death in the two experiments.
Bacterial streaming was observed in approximately 50 and 80% of the examined
leaves inoculated with the M-1 and Montana isolates, respectively. Control
plants showed no leaf mortality or bacterial streaming. Although this pathogen
was originally identified in the United States in Michigan (2) and has been
prevalent in the northeastern United States for the past 10 to 15 years, to our
knowledge, this is the first report of the disease in the northwestern United
States.
References: (1) N. A. Mitkowski et al. Plant Dis. 89:469, 2005. (2)
D. L. Roberts et al. Phytopathology 75:1289, 1985.
Erratum
A correction was made to this note on October 10, 2005. In the text, the
correct name of the pathogen is X. translucens pv. poae.
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