We also evaluated the possible existence of an alternative promoter after the mgoB gene, which would explain the production of mangotoxin by the mutant UMAF0158::mgoB. However, during 5′RACE experiment (Figure 3) only a single transcription start site was located, eliminating the possibility of another promoter downstream of mgoB. Therefore there must be something different NVP-HSP990 clinical trial between the mutant and wild-type strain, which is probably the plasmid integration. In reviewing the process by which the mgo mutants were obtained, we observed that UMAF0158::mgoB was not easy to obtain. The size of mgoB is 777 bp, and the cloned sequence in pCR2.1
was 360 bp of mgoB. The integration of pCR::mgoB into mgoB occurred by single-crossover homologous recombination as it was confirmed. During this process, the plasmid could be integrated into mgoB sequence maintaining an important part of the gene. In this circumstances mgoB or sufficient fragment of it, and the remarkably other three genes of the mgo operon, could be under the influence of a promoter located in
plasmid polylinker, lacZ promoter, allowing a reduced transcript expression (Figure 2) and mangotoxin production (Tables 1 and 2). To determine the insert position, a PCR was performed in which the forward primer annealed to the lacZ gene (M13F primer) and the reverse primer annealed to the 5′-end of the mgoC gene, with wild-type UMAF0158 used as the negative control. The amplicon obtained from the mutant UMAF0158::mgoB selleck products had a size of 1000 bp, confirming that the plasmid pCR::mgoB was integrated and the lacZ promoter is close to mgoB fragment (Additional file 1: Figure S1). Because the chemical structure of mangotoxin is unknown [13], it is difficult to establish a hypothesis concerning Ureohydrolase the role of the mgo genes in mangotoxin biosynthesis or to determine whether they are related to the regulation of mangotoxin production. Recent studies in P. entomophila have focussed on the pvf gene cluster, which is homologous to the mgo operon, and suggest that the gene cluster
serves as a regulator of certain virulence factors in pathogenic strains of AR-13324 solubility dmso Pseudomonas spp. The pvf gene cluster may be a new regulatory system that is specific to certain Pseudomonas species [21]. In the present study, extract complementation restored mangotoxin production in the UMAF0158ΔmgoA mutant only when the culture medium was supplemented with an extract from wild-type UMAF0158. Polar effects of the deleted mgoA on mgoD expression were excluded because the construction of the deletion mutant preserved the reading phase of protein translation. Mangotoxin production was restored in the miniTn5 mutants, which contain disrupted regulatory genes, when their cultures were complemented with a wild-type extract.