The BEC were thereafter re-suspended in PBS to obtain a concentration of 1 × 105 cells/ml by haemocytometer counting. For the adhesion assay, 0.5 ml of BEC and 0.5 ml of Candida suspension following brief exposure to the drugs were mixed gently in tubes and incubated at 37 °C for 1 h. Thereafter, the Candida/BEC suspension selleck chemicals llc was diluted in 4 ml of sterile PBS. The BEC was harvested onto 12 μm pore size polycarbonate filters and washed gently with sterile PBS to remove unattached Candida cells. Thereafter, each filter was placed on a glass slide and removed gently after 10 s. The preparation
on the glass slide was air-dried and stained with Gram’s stain. The number of adherent yeast cells was quantified by light microscopy at ×400 magnification. Fifty sequential BEC will be observed for adherent Candida cells. Clumped, folded or overlapping selleck compound BEC was to be excluded as done in
previous experiments.[19, 20] A previously used method for germ tube induction was performed.[22, 23] RPMI 1640 medium with l-glutamine (Sigma) was chosen for the assay because it effectively induces GT formation. For GT induction, 250 μl of Candida suspension, obtained after drug removal, was added to 1 ml RPMI 1640 medium with l-glutamine and incubated at 37 °C for 90 min. Afterwards, the tube was vortex mixed for 10 s and a drop of each cell suspension was placed on a Neubauer’s haemocytometer chamber and covered with a cover slip for quantification of germ tubes. Thereafter, 300 Candida cells in contiguous fields were counted (under ×40 magnification) and percentage of GT forming cells calculated. A previously used criterion was used for counting.[22, 23] The criteria used: (1) only Candida cells with a GT, without constriction at the junction between the cell and the elongation were counted; (2) clumped cells with GT were excluded; Phospholipase D1 (3) pseudo-hyphae-forming Candida cells were excluded. A
biphasic aqueous-hydrocarbon assay previously used for the assessment of CSH on oral Candida species was used in this study.[24, 25] In brief, 2.5 ml of yeast suspension obtained after exposure to the drug and subsequent drug removal and re-suspended in sterile PBS was vortex mixed and its absorbance was measured at 520 nm. For each organism tested (with and without exposure to nystatin), 2.5 ml volumes of suspension was added to two sterile glass test tubes (16 × 150 mm; 20 ml), representing one test and one control. In addition, a test and a control were prepared of the suspending medium alone as spectrophotometer blanks. 0.5 ml of xylene was added to each test suspension. The test and the controls were placed in an incubator at 37 °C for 10 min to equilibrate, then taken in turn and vortex mixed for 30 s and returned to the incubator for a further 30 min to allow the immiscible xylene and aqueous phases to separate. The lower, aqueous phase of the sample was carefully removed using a pipette and transferred to a clean test tube.