However, consensus GGA motifs for binding of the RNA binding prot

However, consensus GGA motifs for binding of the RNA binding proteins [49–51] were detected upstream of the mbo and mgo operons (Figure 2C). It must be taken into account that the described

consensus sequence is from P. protegens[49], and nothing is known yet about the recognition site of RNA binding proteins in P. syringae. Figure 2 Transcriptional analysis and mbo operon promoter activity. mboA, mboC and mboE (A), belonging to the mbo operon and mgoB and mgoA (B), belonging to the mgo operon Captisol supplier transcript levels in the wild type strain P. syringae pv. syringae UMAF0158 and mgoA and gacA mutants. (C) Comparison of the described consensus motif (5′-CANGGANG-3′) for P. fluorescens[49–51]: The search was done in front of each start codon of the mgo and mbo genes. (D) β-galactosidase activity of the mbo operon promoter in the wild-type strain UMAF0158 and mgoA, gacS and gacA mutants. These H 89 Strains were transformed with the mbo operon promoter named pMP::P mboI and the empty promoter-probe vector pMP220 was used as a control. The different mutants were also transformed with the vector pLac-mgoBCAD. Log2RQ represents the expression

levels of the studied genes by relative quantification scores. Values below 0 indicates lower expression Doramapimod solubility dmso than the housekeeping gene used for normalization of data. The results are average of three independent experiments however performed in triplicate. Error bars indicate standard deviation. Data were analysed for significance using an arcsine square root transformation with analysis of variance followed by Fisher’s least significant

difference test (P = 0.05). Values of bars with different letter designations represent a statistically significant difference. As the transcription of the mgo operon was substantially lower in the gacA mutant (Figure 2B), we subsequently tested whether introduction of extra copies of the mgo operon in the gacS or gacA mutant could restore mangotoxin production. When the mgo operon was introduced in the mgoA mutant mangotoxin production was restored, which was not the case for the mboA, gacA and gacS mutants (Table 2). Table 2 Toxic activity of P. syringae pv syringae UMAF0158 mutants and mgo operon complemented strains Strains E. coliinhibition assay   Mangotoxin production   PMS PMS + ornithine   Wild type strain and derivative mutants       UMAF0158 + – Yes mboA – -* -* No ΔmgoA – - No gacA – - – No gacS – - – No Transformed with empty vector       UMAF0158 + – Yes mboA – -* -* No ΔmgoA – - No gacA – - – No gacS – - – No Transformed with pLac-mgoBCAD       UMAF0158 ++ – Yes mboA – -* -* No ΔmgoA ++ – Yes gacA – - – No gacS – - – No The results are indicated as follows: – absence of inhibition halo, + inhibition halo between 5-10 mm, ++ inhibition halo bigger 10 mm, -* slight toxicity which did not revert in presence of ornithine.

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