The lesion intensity on each mushroom was analysed using ImageJ analysis software (http://rsbweb.nih.gov/ij/): Image J converted each image to 8-bit grayscale, assigning a value of 0–255 to each pixel; the area of mushroom inoculated was selected and the average grayscale value for each pixel (the Pixel Value, PV), was calculated. On this scale, 0 = black and 255 = white, and so the data were transformed using the formula 1/PV to invert the scale, so that darker lesions AZD9291 molecular weight give higher intensity values. These transformed data are displayed in Figures 2 and 4. Visualising B. bacteriovorusand P. tolaasiiinteractions
on the mushroom surface Mushrooms under each of the five treatment conditions detailed in Table 3 were visualised using Scanning Electron Microscopy. Preparation of mushroom samples for imaging was as follows: Samples of mushroom pileus surface tissue W 5 mm × L 5 mm × D 2 mm were cut and stored in 70% ethanol. They were then dehydrated through
a graded find more series of ethanol concentrations (fresh 70% ethanol, followed by 90% ethanol, and finally 2 changes of 100% ethanol) and dried using a Polaron E3000 Critical Point Dryer. The dried samples were mounted onto aluminium stubs using silver paint, and the stubs were gold coated (~10 μm thickness) using a Polaron E5100 SEM Coating Unit. The samples were viewed and photographed under a JEOL JSM 840 Scanning Electron Microscope at 20 kV. Images were false-coloured in Adobe Photoshop by selecting P. tolaasii 2192T and B. bacteriovorus HD100 cells and using the ‘Colorize’ function in the ‘Hue/Saturation’ tool. A pale yellow colour was selected for P. tolaasii to provide optimum contrast to the mushroom surface, and blue gave a sharp contrast for the B. bacteriovorus. Enumerating P. tolaasiirecovered from
infected mushroom tissue Mushrooms were pre-treated using methods as above; B. bacteriovorus HD100 was Avelestat (AZD9668) applied at either 2.9 × 106 or 1.4 × 107 PFU 15 μl−1 before 1.7 × 106 P. tolaasii 2192T in 15 μl. Mushroom lesions were photographed in a class II containment hood after 48 hours, as above, and lesion intensities were analysed using ImageJ analysis software. Lesion tissue from each mushroom was then cut out using a sterile scalpel blade. Tissue samples were weighed and homogenised in sterile 2 mM CaCl2 25 mM HEPES pH 7.6 buffer (1 ml Calcium HEPES/0.04 g lesion tissue) using separate glass pestle and mortar sets, (pre-cleaned with ethanol and dried), for samples under each of the different treatment combinations. P. tolaasii 2192T CFU recovered from each sample were enumerated by serial dilution and plating on King’s Medium B agar, incubated at 29°C for 15 hours. Characteristic smooth, beige colonies growing on King’s Medium B were counted and recorded as P. tolaasii.