Extraction and quantification
of trehalose and trehalose-6-phosphate Trehalose from dormant and swollen conidia, germlings and mycelia was extracted and quantified as previously described [28]. In brief, ARN-509 cell line harvested fungal material was freeze-dried and homogenized using a mortar. Samples were diluted with ultra pure water, boiled, evaporated and derivatized by trimethylsilylanization Rigosertib supplier before injection into the gas chromatograph–mass spectrometer (GC–MS). Relative concentrations of α-α-trehalose were calculated as the ratio to an internal standard (α-β-trehalose) and thereafter correlated to a standard curve to obtain the absolute concentrations. All trehalose measurements were performed in biological duplicates based on the average of three technical triplicates. Extraction and quantification of T6P was performed essentially as described by
[22]. Liquid cultures were inoculated with 106 spores per ml, incubated at 25°C for 3 days at 140 rpm, and all mycelia from one culture made up one sample. Three biological replicates based on the average of three technical replicates were used for all strains. Stress tolerance and long term viability of conidia Dormant conidia from wild-type A. niger, the additional control strain pyrG+, and the deletion mutants ΔtppB and ΔtppB2 were subjected to heat stress for 20, 60, 90 and 120 min at 55°C. Dormant conidia of wild-type, pyrG + and ΔtppB were subjected to sub-lethal salt and selleck products benzoic acid stress by being spread on AMM plates containing benzoic acid or NaCl at concentrations ranging from non-effective to total growth inhibition of the control strains. For detailed description of these stress experiments see [28]. In addition,
dormant conidia from control strains and ΔtppB were subjected to oxidative stress by adding 200 mM H2O2 to freshly made conidial suspensions (approximately 250 spores/ml liquid AMM). The suspensions were incubated for 10, 20 or 40 min before being spread on AMM plates. To test Histone demethylase long-term viability, conidial suspensions (106 conidia/ml water) were stored at 4°C for a total of 8 weeks. An aliquot of the suspension was withdrawn weekly, diluted and spread on AMM plates for enumeration. Plates from all experiments were incubated at 25°C for 3–7 days before CFU were estimated, and all experiments were performed at least in triplicates (based on three technical replicates). Results Identification of genes involved in trehalose synthesis in Aspergillus niger and other fungi Known amino acid sequences of the proteins of the trehalose synthesis complex of S. cerevisiae were used as queries to identify homologous genes in the A. niger genome by searching the databases available at NCBI using blastP (http://blast.ncbi.nlm.nih.gov).