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Copyright 1994-2008
The American Phytopathological Society
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First Report of Dieback and Leaf Lesions on
Rhododendron sp. Caused by Phytophthora hedraiandra in the United
States. B. W. Schwingle, J. A. Smith, R.
A. Blanchette, S. Gould, and B. L. Blanchette, Department of Plant Pathology,
University of Minnesota, St. Paul 55108; J. Pokorny, USDA Forest Service,
Northeastern Area State and Private Forestry, St. Paul, MN 55108; and S. D.
Cohen, USDA, APHIS, PPD, Riverdale, MD 20737. Plant Dis. 90:109, 2006; published
on-line as DOI: 10.1094/PD-90-0109A. Accepted for publication October 25, 2005.
Surveys for Phytophthora ramorum in
Minnesota nurseries revealed the presence of P. hedraiandra de Cock & Man
in’t Veld and several other Phytophthora species but not P. ramorum.
Symptomatic leaf and stem tissues from diseased Rhododendron and
Quercus species were cultured on PARP, a selective growth medium for
Phytophthora (3). The Phytophthora isolates obtained were later
identified by sequencing the internal transcribed spacer (ITS) region of the
rDNA and comparing the sequences with those in GenBank using BLAST searches (1).
The ITS sequences of six cultures (GenBank Accession Nos. DQ139804-DQ139809),
isolated during 2003 from various Rhododendron cultivars exhibiting leaf
lesions and shoot dieback, showed 100% identity with the ITS sequence of P.
hedraiandra (GenBank Accession No. AY707987) (2). This is a recently
described pathogenic species from the Netherlands responsible for causing leaf
spots on Viburnum spp. Since the ITS sequence of P. hedraiandra
differs little from that of P. cactorum (2), we verified one isolate to
be P. hedraiandra by sequencing the mitochondrial cytochrome c
oxidase subunit I gene (cox1) (GenBank Accession No. DQ139810).
Comparison of this sequence with the P. hedraiandra voucher specimen in
GenBank (Accession No. AY769115) showed 99% identity, which was the closest
match. Reproductive structures were measured on V8 juice agar. The average
oogonium diameter for three isolates was 29 µm with a range of 26 to 32 µm,
while the average antheridium length was 13 µm (11 to 15 µm). Sporangium length
and width averages on crushed hemp seeds were 32 µm (28 to 36 µm) and 26 µm (21
to 30 µm), respectively, with the average length to width ratio of 1.25 (1.23 to
1.29). Pathogenicity tests on Rhododendron cv. Mikkeli were carried out
using three of our P. hedraiandra isolates. Spore suspensions of 2 × 10(^4)
zoospores per ml were used to mist-spray shoots of five, 3-year-old plants for
each isolate. Five controls were mist sprayed with water. After inoculation,
plants were placed in plastic bags in a dark growth chamber (22°C) for 7 days
and then moved to a greenhouse. Leaf blotches and shoot dieback were apparent 5
days after inoculation, and P. hedraiandra was reisolated from those
symptomatic tissues and identified by an exact match of the ITS sequence.
Necrotic areas lengthened from the shoot tips to the main stems of the plants
while expanding into petioles and leaves. No symptoms were observed on control
plants. To our knowledge, this is the first report of P. hedraiandra in
the United States as well as the first report of Koch’s postulates performed
with P. hedraiandra on Rhododendron cv. Mikkeli. The significance
of this disease to other woody plants in nurseries or the landscape is unknown,
and further study is needed to determine the host range and extent of the
disease that may occur from this introduction.
References: (1) S. F. Altschul et al. J. Mol. Biol. 215:403, 1990. (2) A.
W. A.M de Cock and C. A. Lévesque. Stud Mycol 50:481, 2004. (3) D. C. Erwin and
O. K. Ribeiro. Phytophthora Diseases Worldwide. The American
Phytopathological Society, St. Paul, MN, 1996.
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