A total of 523 hygromycin-resistant colonies were obtained, but some of the transformants appeared unstable and pSH75 might not have integrated into genomic DNA of host cells. To confirm stability, the transformants
were transferred five times to PDA containing 200 μg mL−1 hygromycin. Surviving transformants were subsequently grown on PDA without hygromycin for 3 days prior to being transferred to PDA with 200 μg mL−1 hygromycin. HDAC inhibitor In total, 323 transformants retained their resistance to hygromycin, and this indicated that they were stable. The colony morphology of these transformants changed as compared with the original strain of B. eleusines, and 98.4% of transformants were showed reduced growth for 1–3 days (Fig. 1). About 42.1% of colonies were grey to white compared with original black colonies of the fungus. Additionally, a small number of transformants did not sporulate (Table 1). Growth of transformant B014 was retarded after 1 day, colonies were grey and spore production was reduced to 50% of that of wild-type B. eleusines. Protoplasts of the wild-type B. eleusines were successfully transformed by linear plasmid DNA from the vector pSH75. When using circular plasmid DNA Staurosporine molecular weight without the restriction
enzyme, no transformant was obtained. The addition of XboI to the linear plasmid also showed a low transformation rate. However, addition of BamHI and HindIII to the linear plasmid significantly increased transformation efficiency, resulting in transformation rates of up to 4–5 transformants μg−1 plasmid (Table 2). Six toxin-deficient transformants were obtained. Mycelial growth of R. solani was effectively inhibited by the cell-free culture filtrate of wild-type B. eleusines, with Erlotinib mw a relative inhibitory rate of 89% (Table 3). However, the filtrate of the transformant B014 showed less inhibition and the colony diameter
of R. solani was close to that of the control after 24 h. This suggests that transformant B014 is deficient of the toxins. When sprayed with the filtrate of wild-type B. eleusines, barnyard grass was yellow 5 days after treatment (data not shown). However, when treated with the filtrate of transformant B014, no significant effect was observed in comparison with control. This result further demonstrated that B014 was no longer be able to produce phytotoxic metabolites against barnyard grass and therefore might be considered a toxin-deficient mutant of B. eleusines. Other transformants showed similar or only slightly reduced efficacy against barnyard grass relative to the wild-type. The metabolite chromatographic peaks in the wild-type sample (Fig. 2b) and five toxin-deficient mutants (data not shown) were close to the retention time (7.798 min) of the ophiobolin A standard (Fig. 2a, 7.778 min). The retention times were highly reproducible, varying by < 0.2 min. However, there was no detectable peak in the transformant B014 sample (Fig.