001 mg kg−1. The levels of DON, 3ADON, 15ADON, and NIV were determined in pooled grain samples by GC-MS as previously described by Eskola et al. (2001). Each pooled sample (100 g) contained kernels pooled from c. 500 wheat heads per sample. Each sample was analyzed once. The limits of quantitation were 0.01 mg kg−1 for DON and its derivatives and 0.03 mg kg−1 for NIV. The relationships between the quantitated DNA

and trichothecene concentrations in grain samples were determined by Pearson’s correlation analysis CH5424802 using statistica software (Data Analysis Software System, version 6.1; StatSoft Inc., 2003, http://www.statsoft.com). The quantitation of transcripts of tri4, tri5, and tri11 genes located in the 12-gene core tri cluster (Brown et al., 2004) was evaluated using TaqMan probes. The proposed

trichothecene biosynthetic pathway in Fusarium has been presented in Foroud & Eudes (2009). The analyzed genes encode the first steps of the type B trichothecene biosynthesis pathway and are representative of the initial flux of the biosynthetic pathway. Tables 2 and 3 show fold-change values representing tri up-regulation in F. graminearum isolates treated with azoles as compared to nontreated control. The tri transcript levels were always higher in cultures supplemented with sublethal concentrations of azoles, although in some cases, fold-change values were not significantly C59 wnt price altered [P(H1) = 0.001]. Among the tri transcripts analyzed of all studied isolates, the amount of tri4 transcript was the highest during the culture process followed by tri11 and tri5 (data not shown). It should be noted that the tri transcript levels in nontreated samples differed among the tested DON and NIV chemotypes. The tri transcript levels of DON chemotypes were at a similar and higher level than in the NIV chemotype (data PLEKHB2 not shown). Notably, the tri transcript levels seemed to be related to the type of azole used. Within DON chemotypes, the amount of tri transcripts treated with tebuconazole was higher compared to samples treated with propiconazole; however, such a relation was not clear

for the NIV chemotype (Tables 2 and 3). In an independent experiment, the levels of trichothecenes (DON, 3ADON, 15ADON, NIV, and 4ANIV) were determined in 14-day-old cultures supplemented or not with different concentrations of azoles (Table 2 and 3). Isolate 1002T, identified with qPCR assay as 3ADON genotype, accumulated DON and higher amounts of 3ADON. Isolate 1001T, determined to be of the 15ADON genotype, produced DON and lower amounts of 3ADON and 15ADON. Isolate 0357, predicted with qPCR assay as an NIV producer, accumulated NIV, 4ANIV. For 3ADON chemotype, an increase in DON and 3ADON was revealed in samples treated with all sublethal concentrations of propiconazole. However, all samples of 15ADON chemotype exhibited decreased accumulation of trichothecenes as compared to N.T.C.