Characterization and PCR-based detection of benzimidazole-resistant isolates of Monilinia laxa in California

Zhonghua Ma; Michael A Yoshimura; Brent A Holtz; Themis J Michailides

doi:10.1002/ps.982

Characterization and PCR-based detection of benzimidazole-resistant isolates of Monilinia laxa in California

Pest Manag Sci. 2005 May;61(5):449-57. doi: 10.1002/ps.982.

Authors

Zhonghua Ma¹, Michael A Yoshimura, Brent A Holtz, Themis J Michailides

Affiliation

¹ Department of Plant Pathology, University of California, Davis, Kearney Agricultural Center, 9240 South Riverbend Ave, Parlier, CA 93648, USA. zhma@uckac.edu

PMID: 15816017
DOI: 10.1002/ps.982

Abstract

Monilinia laxa is a pathogen of brown rot of stone fruit and almond in California, causing blossom blights and fruit rots. In this study, low-level resistance to the benzimidazole fungicides benomyl and thiophanate-methyl was detected in field isolates of M laxa collected from stone fruits and almonds in California. Low-resistant (LR) isolates grew in potato dextrose agar (PDA) plates amended with benomyl and thiophanate-methyl at 1 and 5 microg ml(-1), respectively, but not in plates amended with benomyl at 5 microg ml(-1) or thiophanate-methyl at 50 microg ml(-1). The benzimidazole LR isolates were characterized by temperature sensitivity and the DNA sequence of the beta-tubulin gene. The LR isolates showed high-temperature sensitivity, being sensitive to 1 microg ml(-1) of benomyl at 28 degrees C but resistant at 8-24 degrees C. Analysis of the DNA sequence of the beta-tubulin gene showed that the LR isolates had a point mutation at the amino-acid position 240, causing substitution of leucine by phenylalanine. Based on the point mutation, a pair of allele-specific PCR primers was developed for rapid detection of LR isolates of M laxa. In addition, a pair of PCR primers specific to M laxa was developed on the basis of the differences in the DNA sequence of the intron 6 of beta-tubulin gene from M laxa, M fructicola and other fungal species. The primer pair amplified the expected 376-bp DNA fragment from all M laxa isolates tested, but not from 14 other fungal species isolated from stone fruit and almond crops. The restriction endonuclease BsmA I recognized the sequence GTCTCC in the PCR products from sensitive (S) isolates only, but not the GTTTCC sequence in the PCR products from LR isolates. The endonuclease digested the 376-bp PCR products from S isolates to produce two bands (111 and 265 bp) on agarose gels. Thus, both allele-specific PCR and the PCR-restriction fragment length polymorphism (PCR-RFLP) methods could be useful for rapidly detecting benzimidazole-resistant isolates of M laxa from stone fruit and almond crops in California.

Publication types

Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

Ascomycota* / genetics
Base Sequence
Benzimidazoles*
California
Drug Resistance, Fungal*
Fungicides, Industrial*
Molecular Sequence Data
Plant Diseases / microbiology
Polymerase Chain Reaction
Polymorphism, Restriction Fragment Length
Sequence Alignment
Sequence Homology, Nucleic Acid
Temperature
Tubulin / genetics

Substances

Benzimidazoles
Fungicides, Industrial
Tubulin