Specific Detection of Xylella fastidiosa Pierce's Disease Strains |
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Authors: | Donna Banks Rajai Albibi Jianchi Chen Olusola Lamikanra Robert L. Jarret Barbara J. Smith |
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Affiliation: | (1) Center for Viticultural Science, Florida A&M University, Tallahassee, FL 32307, USA , US;(2) USDA-ARS, Department of Plant Introduction, 1109 Experiment St., Griffin, GA 30223, USA , US;(3) USDA-ARS, Small Fruit Research Station, 306 S. High St., Poplarville, MS 39470, USA , US |
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Abstract: | ![]() Pierce's disease (PD, Xylella fastidiosa) of grapevine is the primary pathogen limiting vinifera grape production in Florida and other regions of the southeastern United States. Quick and accurate detection of PD strains is essential for PD studies and control. A unique random amplified polymorphic DNA (PD1-1-2) was isolated from a PD strain from Florida. Fragment PD1-1-2 was cloned, sequenced, and found to be 1005 bp in length. PCR primers were designed to utilize these sequence data for PD strain detection. One primer set (XF176f–XF954r) amplified a 779-bp DNA fragment from 34 PD strains including seven pathotypes of X. fastidiosa, but not from strains of Xanthomonas campestris pv. campestris, Xan. vesicatoria or Escherichia coli. A second primer set (XF176f and XF686r) amplified a 511-bp fragment specific to 98 PD strains, but not from strains of citrus variegated chlorosis, mulberry leaf scorch, oak leaf scorch, periwinkle wilt, phony peach, or plum leaf scald. Sequence analysis indicated that RAPD fragment PD1-1-2 contains a Ser-tRNA gene. The PD-specific region includes a TaqI restriction site (TCGA) and is 150 bp downstream of the Ser-tRNA gene. Received: 1 March 1999 / Accepted: 5 April 1999 |
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