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American Society for Microbiology, Applied and Environmental Microbiology, 3(64), p. 948-954, 1998

DOI: 10.1128/aem.64.3.948-954.1998

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PCR Amplification of Ribosomal DNA for Species Identification in the Plant Pathogen Genus Phytophthora

Journal article published in 1998 by Jean B. Ristaino, Michael Madritch ORCID, Carol L. Trout, Gregory Parra
This paper is made freely available by the publisher.
This paper is made freely available by the publisher.

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Abstract

ABSTRACT We have developed a PCR procedure to amplify DNA for quick identification of the economically important species from each of the six taxonomic groups in the plant pathogen genus Phytophthora . This procedure involves amplification of the 5.8S ribosomal DNA gene and internal transcribed spacers (ITS) with the ITS primers ITS 5 and ITS 4. Restriction digests of the amplified DNA products were conducted with the restriction enzymes Rsa I, Msp I, and Hae III. Restriction fragment patterns were similar after digestions with Rsa I for the following species: P. capsici and P. citricola ; P. infestans , P. cactorum , and P. mirabilis ; P. fragariae , P. cinnamomi , and P. megasperma from peach; P. palmivora , P. citrophthora , P. erythroseptica , and P. cryptogea ; and P. megasperma from raspberry and P. sojae . Restriction digests with Msp I separated P. capsici from P. citricola and separated P. cactorum from P. infestans and P. mirabilis . Restriction digests with Hae III separated P. citrophthora from P. cryptogea , P. cinnamomi from P. fragariae and P. megasperma on peach, P. palmivora from P. citrophthora , and P. megasperma on raspberry from P. sojae. P. infestans and P. mirabilis digests were identical and P. cryptogea and P. erythroseptica digests were identical with all restriction enzymes tested. A unique DNA sequence from the ITS region I in P. capsici was used to develop a primer called PCAP. The PCAP primer was used in PCRs with ITS 1 and amplified only isolates of P. capsici , P. citricola , and P. citrophthora and not 13 other species in the genus. Restriction digests with Msp I separated P. capsici from the other two species. PCR was superior to traditional isolation methods for detection of P. capsici in infected bell pepper tissue in field samples. The techniques described will provide a powerful tool for identification of the major species in the genus Phytophthora.