Synthesis and biological activity of fluorescent yeast pheromones

The mating pheromones of Saccharomyces cerevisiae and derivatives of these pheromones have been synthesized and tested for biological activity in a solution-phase assay. The effects of native alpha-factor and a-factor on the growth of target cells in these assays were identical. A derivative of alpha-factor in which the amino terminus was modified with the fluorescent probe, 6-amino-N-(7-nitrobenz-2-oxa-1,3-diazol-4-yl)hexanoyl, was only slightly less active than the unmodified pheromone. Derivatives of a-factor that contain various alkyl groups in place of the farnesyl moiety of the native pheromone were also synthesized and tested for biological activity. A derivative in which the farnesyl moiety is substituted with an unbranched decyl group exhibited activity identical to that of the natural pheromone, whereas a derivative that contains an unbranched pentyl group exhibited significantly lower biological activity than native a-factor. The derivatives of a-factor have in addition been modified to incorporate 6-amino-N-(7-nitrobenz-2-oxa-1,3-diazol-4-yl) at the terminus of the alkyl chains. A derivative with the probe attached to a decyl chain displayed activity similar to that of the native pheromone, whereas the same modification on a pentyl chain produced a derivative with very low activity. The fluorescence spectra of the modified alpha-factor and a-factors were measured in methanol, aqueous solution, and aqueous solution containing phospholipid vesicles. The fluorescence of the probes depends on the environment of the pheromones and can be used to monitor the association of the pheromones with the lipid bilayer.