4.7 Article

Dirhamnose-lipid production by recombinant nonpathogenic bacterium Pseudomonas chlororaphis

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APPLIED MICROBIOLOGY AND BIOTECHNOLOGY
卷 99, 期 10, 页码 4333-4342

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SPRINGER
DOI: 10.1007/s00253-015-6433-4

关键词

Biosurfactant; Microbial glycolipid; Pseudomonas chlororaphis; Rhamnolipid; Rhamnosyltransferases; Surface tension

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We previously discovered that Pseudomonas chlororaphis NRRL B-30761 produces monorhamnolipids (R(1)Ls) with predominantly 3-hydroxydodecenoyl-3-hydroxydecanoate (C-12:1-C-10) or 3-hydroxydodecanoyl-3-hydroxydecanoate (C-12-C-10) as the lipid moiety under static growth conditions only. We have now cloned, sequenced, and analyzed in silico the gene locus of NRRL B-30761 containing the putative coding sequences of rhamnosyltransferase chain A (rhlA (Pch) , 894 bps), rhamnosyltransferase chain B (rhlB (Pch) , 1272 bps), and N-acyl-homoserine lactone-dependent transcriptional regulatory protein (rhlR (Pch) , 726 bps). The putative gene products RhlA(Pch) (297 amino acid residues or a.a.), RhlB(Pch) (423 a.a.), and RhlR(Pch) (241 a.a.) only have between 60 and 65 % a.a. identities to their respective closest matched homologs in P. aeruginosa. Polymerase chain reaction (PCR)-based assay did not detect the presence of rhamnosyltransferase C gene (rhlC) in P. chlororaphis, suggesting a genetic basis for the lack of dirhamnose-lipid (R2L) synthesis in this organism. We thus genetically constructed an R2L-synthesizing P. chlororaphis by expressing a rhamnosyltransferase C (rhlC) gene of P. aeruginosa using an expression vector (pBS29-P2-gfp) containing a Pseudomonas syringae promoter. The R2L/R1L ratio is 2.4 in the rhamnolipid (RL) sample isolated from the genetically engineered (GE) P. chlororaphis [pBS29-P2-rhlC], in contrast to undetectable R2L in the GE P. chlororaphis [pBS29-P2-gfp] control cells based on LC-MS analysis. The critical micelle concentrations of the R2L and R1L samples from GE P. chlororaphis [pBS29-P2-rhlC] and the control [pBS29-P2-gfp] cells were ca. 0.1 mM, and their minimum surface tensions were ca. 26 mN/m with no significant difference.

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