Figure 3

in vivo detection of recombinant α-L-rhamnosidase activity. S. cerevisiae cells were grown at 30°C for about 5 h on SD plates containing the artificial substrate MUR. Differences in α-L-rhamnosidase activity between non permeabilized (A) and permeabilized (B) cells are shown. The names of the strains appear in panel C. Representative transformants (YR150-YR153) expressing the A. nidulans rhaE gene were tested. Strains harbouring an empty vector (YR70) or a plasmid expressing the A. aculeatus rhaA gene (YR8; [27]) were included as controls.