Quorum Quenching by an
            <i>N</i>
            -Acyl-Homoserine Lactone Acylase from
            <i>Pseudomonas aeruginosa</i>
            PAO1

Sio, Charles F.; Otten, Linda G.; Cool, Robbert H.; Diggle, Stephen P.; Braun, Peter; Bos, Rein; Daykin, Mavis; Cámara, Miguel; Williams, Paul; Quax, Wim J.

doi:10.1128/iai.74.3.1673-1682.2006

Cited by 279 publications

(269 citation statements)

References 60 publications

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“…This is consistent with the observation in the present study, that a pvdQ mutant produces precursors with myristic or myristoleic acid still bound to the L-Glu residue. The physiological function of PvdQ is therefore not in the deacylation of the quorum sensing molecule 3-oxo-C12 as previously suggested [14] but in the deacylation of the PVDI precursor isolated in the present work.…”

Section: Discussionsupporting

confidence: 57%

“…This precursor has been purified and was proposed to be a substrate of PvdQ [8], providing a direct link between PvdQ and the mechanism of myristate group removal by PvdQ before Abbreviations: PVDI, pyoverdine I; PVDIq, PVDI precursor produced by PAO1pvdQ; NRPS, non-ribosomal peptide synthetases; CA, collision activation; HPLC-MS, high performance liquid chromatography-mass spectrometry secretion into the extracellular milieu. PvdQ belongs to the NTN hydrolase family [13] and was identified as a periplasmic quorum-quenching protein that cleaves acyl homoserine lactones [14]. Transport of newly synthesized PVDI from the periplasm into the extracellular medium involves PvdRT-OpmQ, an ATP-dependent efflux pump [15].…”

Section: Introductionmentioning

confidence: 99%

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Biosynthesis of the pyoverdine siderophore of Pseudomonas aeruginosa involves precursors with a myristic or a myristoleic acid chain

et al. 2011

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a b s t r a c tPyoverdine I (PVDI) is the major siderophore produced by Pseudomonas aeruginosa to import iron. Biosynthesis of this chelator involves non-ribosomal peptide synthetases and other enzymes. PvdQ is a periplasmic enzyme from the NTN hydrolase family and is involved in the final steps of PVDI biosynthesis. A pvdQ mutant produces two non-fluorescent PVDI precursors with a higher molecular mass than PVDI. In the present study, we describe the use of mass spectrometry to determine the structure of these PVDI precursors and show that they both contain a unformed chromophore like ferribactin, and either a myristic or myristoleic chain that must be removed before PVDI is secreted into the extracellular medium.

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Section: Discussionsupporting

confidence: 57%

Section: Introductionmentioning

confidence: 99%

Biosynthesis of the pyoverdine siderophore of Pseudomonas aeruginosa involves precursors with a myristic or a myristoleic acid chain

et al. 2011

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“…Interestingly, homologues of AiiD were also found in various other Ralstonia and Pseudomonas spp. (46), and these bacteria were later confirmed to also possess AHL acylase activity (42,44,45,47,51,52). Biochemical analysis of the fate of 3OC10HSL incubated with purified AiiD protein confirmed that AiiD functions as an AHL acylase, releasing HSL and 3-oxodecanoic acid as the major degradation products (46).…”

Section: Enzymatic Degradation and Inactivation Of Ahlsmentioning

confidence: 88%

Exploiting Quorum Sensing To Confuse Bacterial Pathogens

LaSarre

Federle

2013

Microbiol Mol Biol Rev

665

556

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SUMMARY Cell-cell communication, or quorum sensing, is a widespread phenomenon in bacteria that is used to coordinate gene expression among local populations. Its use by bacterial pathogens to regulate genes that promote invasion, defense, and spread has been particularly well documented. With the ongoing emergence of antibiotic-resistant pathogens, there is a current need for development of alternative therapeutic strategies. An antivirulence approach by which quorum sensing is impeded has caught on as a viable means to manipulate bacterial processes, especially pathogenic traits that are harmful to human and animal health and agricultural productivity. The identification and development of chemical compounds and enzymes that facilitate quorum-sensing inhibition (QSI) by targeting signaling molecules, signal biogenesis, or signal detection are reviewed here. Overall, the evidence suggests that QSI therapy may be efficacious against some, but not necessarily all, bacterial pathogens, and several failures and ongoing concerns that may steer future studies in productive directions are discussed. Nevertheless, various QSI successes have rightfully perpetuated excitement surrounding new potential therapies, and this review highlights promising QSI leads in disrupting pathogenesis in both plants and animals.

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“…Other enzymes exhibited more flexibility in their requirements for substrate side chain structure. The substrate side chain of PGA can be an aromatic or aliphatic carboxyl group with 2-6 carbons (with k cat range from 4 to 15 s Ϫ1 , supplemental Table S1), whereas that of PvdQ can be 4 -14 carbons long (40). Because these enzymes lack the special residue, which controlled the cleavage site shift in CA, covalent binding of the spacer became more important for the second cleavage.…”

Section: Discussionmentioning

confidence: 99%

“…Specific Binding and Covalent Binding for the Second Cleavage-In the previous studies, besides CA, PGA and PvdQ were confirmed to be Ntn hydrolases that require two-step proteolysis for activation, releasing spacers consisting of 54, 22, or 23 aa, respectively (39,40) (Table 4). The long distances between the second cleavage sites and the Ntn Ser residues were also observed in the respective crystal structures (7,41).…”

Section: Discussionmentioning

confidence: 99%

The N-terminal Nucleophile Serine of Cephalosporin Acylase Executes the Second Autoproteolytic Cleavage and Acylpeptide Hydrolysis

Yin

Deng

Zhao

et al. 2011

Journal of Biological Chemistry

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Cephalosporin acylase (CA) precursor is translated as a single polypeptide chain and folds into a self-activating pre-protein. Activation requires two peptide bond cleavages that excise an internal spacer to form the mature ␣␤ heterodimer. Using Q-TOF LC-MS, we located the second cleavage site between Glu 159 and Gly 160 , and detected the corresponding 10-aa spacer 160 GDPPDLADQG 169 of CA mutants. The site of the second cleavage depended on Glu 159 : moving Glu into the spacer or removing 5-10 residues from the spacer sequence resulted in shorter spacers with the cleavage at the carboxylic side of Glu. The mutant E159D was cleaved more slowly than the wild-type, as were mutants G160A and G160L. This allowed kinetic measurements showing that the second cleavage reaction was a firstorder, intra-molecular process. Glutaryl-7-aminocephalosporanic acid is the classic substrate of CA, in which the N-terminal Ser 170 of the ␤-subunit, is the nucleophile. Glu and Asp resemble glutaryl, suggesting that CA might also remove N-terminal Glu or Asp from peptides. This was indeed the case, suggesting that the N-terminal nucleophile also performed the second proteolytic cleavage. We also found that CA is an acylpeptide hydrolase rather than a previously expected acylamino acid acylase. It only exhibited exopeptidase activity for the hydrolysis of an externally added peptide, supporting the intra-molecular interaction. We propose that the final CA activation is an intramolecular process performed by an N-terminal nucleophile, during which large conformational changes in the ␣-subunit C-terminal region are required to bridge the gap between Glu 159 and Ser 170 .

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Quorum Quenching by an N -Acyl-Homoserine Lactone Acylase from Pseudomonas aeruginosa PAO1

Cited by 279 publications

References 60 publications

Biosynthesis of the pyoverdine siderophore of Pseudomonas aeruginosa involves precursors with a myristic or a myristoleic acid chain

Biosynthesis of the pyoverdine siderophore of Pseudomonas aeruginosa involves precursors with a myristic or a myristoleic acid chain

Exploiting Quorum Sensing To Confuse Bacterial Pathogens

The N-terminal Nucleophile Serine of Cephalosporin Acylase Executes the Second Autoproteolytic Cleavage and Acylpeptide Hydrolysis

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