Identification and Regulation of Genes from a Biocontrol Strain of Fusarium oxysporum

Differential display with three time points revealed that thiram altered expression of numerous genes in the biocontrol fungus Fusarium oxysporum CS‐20. Of the 101 bands purified from the differential display gel, 86 were successfully cloned, and 64 sequenced. Based on nucleic acid sequences, homology to known products was found using BLASTn for 26 sequences and homology to hypothetical proteins was found for six sequences, also from Gibberella zeae . One band (BM1 24‐1) showed homology to an ABC transporter from three different fungi. Because of its association with detoxification functions, the ABC transporter was selected for further study. Mycelia of CS‐20 were exposed to 25  μ g active ingredient (a.i.) thiram in liquid culture for various times from 0 to 8 h. Quantitative real‐time PCR was used to evaluate gene expression. At 30 min after treatment with thiram, the ABC transporter was upregulated 20‐ to 25‐fold relative to the control treatment. The ABC transporter was upregulated 15‐fold at 1 h after treatment and 10‐fold at 2 h. At 8 h after treatment, there was no difference between treated and non‐treated for expression of the ABC transporter. Transcription of the gene encoding EST BM1 24‐1 is induced in response to thiram treatment and may function in providing resistance in F. oxysporum isolate CS‐20 to fungicides and other toxins. Tolerance to toxins may be critical to the successful inclusion of CS‐20 in disease control strategies in cropping systems.