Abstract
Previously, we reported the isolation of a quorum quenching protein (QQ), designated GqqA, from Komagataeibacter europaeus CECT 8546 that is highly homologous to prephenate dehydratases (PDT) (Valera et al. in Microb Cell Fact 15, 88. https://doi.org/10.1186/s12934-016-0482-y, 2016). GqqA strongly interfered with N-acyl-homoserine lactone (AHL) quorum sensing signals from Gram-negative bacteria and affected biofilm formation in its native host strain Komagataeibacter europaeus. Here we present and discuss data identifying GqqA as a novel acylase. ESI–MS–MS data showed unambiguously that GqqA hydrolyzes the amide bond of the acyl side-chain of AHL molecules, but not the lactone ring. Consistent with this observation the protein sequence does not carry a conserved Zn2+ binding motif, known to be essential for metal-dependent lactonases, but in fact harboring the typical periplasmatic binding protein domain (PBP domain), acting as catalytic domain. We report structural details for the native structure at 2.5 Å resolution and for a truncated GqqA structure at 1.7 Å. The structures obtained highlight that GqqA acts as a dimer and complementary docking studies indicate that the lactone ring of the substrate binds within a cleft of the PBP domain and interacts with polar residues Y16, S17 and T174. The biochemical and phylogenetic analyses imply that GqqA represents the first member of a novel type of QQ family enzymes.
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Introduction
Quorum sensing (QS) is very well-described process in both Gram-negative and Gram-positive bacteria2,3,4,5,6. The term QS describes the cell–cell communication within a bacterial community (mono-and multi-species) in dependence of their cell density. Thereby, bacteria synthesize and release small often diffusible molecules that allow measuring the density of a population. The different signaling molecules are sensed by other bacteria within the species or across the species. The sensing induces the coordinated transcription of genes and proteins that are of importance for the survival of the community but that are not necessarily essential at a single cell level. In general, it is assumed that through the expression of the AI synthase gene at very low level, the signal is constantly produced and not or only poorly sensed until a threshold concentration is reached. Only at higher levels, which goes in parallel with a higher cell density, then the AI can interact with the respective receptors and regulators and induce coordinated gene expression at a population wide level. Genes regulated by this phenomenon are involved in surface colonization and attachment, biofilm formation, virulence factor production, secretion, infection, conjugation, secondary metabolite production, bioluminescence, sporulation and symbiosis2,3,4,5,6.
During evolution bacteria developed a variety of different mechanisms using various QS signal molecules. Among these are N-acyl-homoserine lactones (AHLs) probably the best studied AI molecules with respect to their influence on a population wide level. AHLs in Gram-negative bacteria consist of an acyl moiety linked to an (S)-α-amino-γ-butyrolactone ring via an amide bond. The acyl chain is variable in length and frequently modified by a 3-oxo- or a 3-hydroxy-group to increase the specificity7,8,9.
Where signals are produced the destruction is one way of quenching the message. In nature signals are usually degraded over time and today we know that several bacterial enzymes exist that are involved in breakdown of AHL molecules. These enzymes are collectively called Quorum Quenching (QQ) enzymes and are summarized in recent reviews10,11,12,13. Today over 30 in part characterized enzymes are known acting on AHLs and derived from a wide range of different bacteria and also a number of non-cultivated species. Figure 1 summarizes the current phylogenetic diversity of known and biochemically characterized QQ enzymes.
Three main types of enzymes are known to act on AHLs. These are lactonases (EC. 3.1.1.-), acylases (EC 3.5.1.–) and oxidoreductases (EC 1.1.–) (Fig. 1). For each of the main enzyme classes two subclasses of enzymes are known. While a few oxidoreductases have been reported the best studied group of enzymes processing AHL molecules are hydrolases, including lactonases and acylases14,15,16. Thereby lactonases hydrolyze the lactone ring in a reversible way. One of the first QQ enzymes reported was the lactonase AiiB from Bacillus subtilis17.
Acylases (amido-hydrolases) hydrolyze the amide group and release the homoserine lactone and the carboxylic acid. The currently known acylases separate in two distinct groups: The N-terminal nucleophile aminohydrolases (Ntn hydrolases) and the α/β-hydrolases (Fig. 1). Ntn hydrolases cleave an amide bond18,19. The N-terminal fold further provides the possibility of autocatalytic processing19. The majority of the currently known AHL acting acylases belongs to the Ntn hydrolases11,20,21,22,23,24,25,26,27,28,29,30,31. Today only the Ochrobacterium sp. A44 AiiO and the Sinorhizobium NGR234 DlhR appear to be α/β-hydrolase-like acylases30. The α/β-hydrolases are an extended group of very diverse but structurally conserved enzymes. Recently, we published a newly identified QQ enzyme designated GqqA1. The gqqA gene encodes for a protein with 281 amino acid residues and a corresponding molecular mass of 30 kDa. The polypeptide sequence lacks the typical features of both, the Ntn hydrolase and the α/β-hydrolase. However, the sequence of the protein shows high similarity to predicted prephenate dehydratases (PDTs; EC 4.2.1.51), which are involved in the metabolic pathways of aromatic amino acids.
Prephenate dehydratases are part of the phenylalanine biosynthesis pathway and catalyze the decarboxylation of prephenate to phenylpyruvate. In some bacteria, such as Escherichia coli, the PDT is part of a relatively large bifunctional P-enzyme that also has a chorismate mutase function (CM, EC 5.4.99.5). Thereby the amino acid residues 1–109 harbor the CM function and residues 101–285 the PDT activity. In addition, the structural region of amino-acid residues 286–386 contains an independent regulatory-domain (ACT-domain) that is involved in a regulatory feedback system by coordinating L-Phenylanalnine32,33. Komagataeibacter europaeus CECT 85,646 codes in its 4.1 Mb genome for a single predicted PDT, designated GqqA34. GqqA has a length of 281 amino-acid residues and shares 31% identity to the E. coli PDT enzyme. However, the K. europaeus N-terminal aa of GqqA lack homology to the chorismate mutase domain but contains the C-terminal regulatory domain, indicating that the chorismate mutase activity is encoded as a separate protein (Ga0098768_10078, tyrA1) elsewhere in the genome34 (Fig. 2A). GqqA overexpression in the host strain Komagataeibacter europaeus interfered with QS-dependent biofilm and cellulose formation and further experiments provided strong evidence that GqqA wildtype protein actively quenches AHL signaling molecules1 (Fig. 2B). Intrigued by the observation that GqqA has a rather low homology to so far known QQ enzymes, however, is sharing a high similarity with PDT enzymes, we were interested to analyze its function in terms of AHL modification. Therefore, we assayed the hydrolysis of AHLs with recombinant GqqA and applied ESI–MS–MS to identify the reaction products. We solved and refined the native GqqA three-dimensional structure to 2.5 Å resolution, utilizing SAD phases obtained from a truncated and Se modified version of GqqA. Structural data together with a phylogenetic analysis and the enzymatic characteristics implied that GqqA represents the first example of a till now unknown, third and novel subclass of acylases. They act on AHLs and modern ß-lactam antibiotics, thus adding a new and complementary functionality to the PDT family of enzymes.
Results and discussion
Recombinant GqqA is a multifunctional enzyme acting as an acylase on AHLs, ß-lactam antibiotics and complements E. coli pheA phenotype
Previously, we showed that GqqA actively quenches AHL signalling molecules using reporter strains1. GqqA is a 281 aa protein consisting of eight α-helices and 15 β-sheets (Fig. 2A). The protein reveals two major functional domains. The predicted PDT domain stretches from position 1–180 and the ACT regulatory domain stretches from aa position 194–281 (Fig. 2A). To further characterize the protein GqqA was heterologously overproduced and purified similar to the previously published protocol1. The purified protein was verified by SDS-PAGE and Western blotting with associated immune detection of the His-tagged GqqA. Purified GqqA produced a single band on SDS-PAGEs corresponding to approx. 30.5 kDa (Figure S1, A), which is in accordance with the calculated molecular mass. The SDS-PAGEs indicated that the protein was homogenous with only very minor contaminations. Experiments to access the activity, using initially either Chromobacterium violaceum CV026 and/or Agrobacterium tumefaciens NTL4 as reporter strains and 3-oxo-C8-HSL as substrate, confirmed that the purified protein was active (Fig. 2B).
The active protein was incubated with oxo-octanoyl homoserine lactone (3-oxo-C8-HSL) as substrate and the enzymatic cleavage products were analyzed using ESI–MS–MS. The employed oxo-C8-HSL has a molecular mass of 241.26 g/mol. After incubation of oxo-C8-HSL with recombinant GqqA we observed a molecular mass of 134.08 in the ESI positive mode and a molecular mass of 157.09 in the ESI negative mode. The 134.08 peak [M + MeOH + H]+ corresponded to the homoserine lactone with a MW of 101.05 g/mol and the 158.09 [M–H]− peak corresponded to 3-oxo-octanoic acid (MW of 158.09 g/mol). Further analyses implied that GqqA can transforms the four different 3-oxo-acyl homoserine lactones tested, with 3-oxo-decanoyl homoserine lactone being the preferred substrate (Table 1). Our biochemical assays implied that GqqA had a Vmax of 152 ± 6.3 U g−1 with oxo-C10–HSL and a-Vmax of 117.3 ± 12.8 using 3-oxo-C8-HSL (Table 1). This is in agreement with the structure analysis which suggests that the active site of GqqA allows to cover fatty acid residues with variable lengths. These data are also in line with our previous results using reporter strains1.
These observations implied that GqqA acts as an acylase by hydrolyzing the acyl substituent of the lactone ring, but not as lactonase (Fig. 3). Further biochemical assays implied that GqqA had a Vmax ranging from ca. 14 U mg−1 for 3-Oxo-dodecanoyl homoserine lactone to ca. 152 U mg−1 for 3-Oxo-decanoyl homoserine lactone, which were found as the less and best preferred substrate according to Vmax/Km values (see Table 1 and Figure S2).
Further we asked to which extend GqqA would be promiscuous with respect to the substrate profile. To answer this question, we investigated the degradation of various ß-lactam antibiotics by GqqA. In a disc diffusion antibiotic susceptibility test, ß-lactam antibiotics were used and the effect after incubation with GqqA on S. aureus cells was tested. These assays demonstrated that GqqA effectively degrades Penicillin G, Amoxicillin and Ampicillin (Figure S3). However, it was not active against the Cefotaxime. The latter is in contrast to the other ß-lactam antibiotics tested a 3rd generation ß-lactam antibiotic and structurally more advanced. This explains why Penicillin G, Amoxicillin and Ampicillin were cleaved. Altogether our data imply that GqqA reveals at least some promiscuity. Within this framework, it is notably, that the recently uncovered acylase MacQ has been described to be involved in QQ and antibiotic resistance. Thereby, MacQ acts against AHLs and Penicillin G and is an acylase belonging to the Ntn family21.
Since GqqA revealed surprisingly high similarities to prephenate dehydratases, we also asked if an E. coil pheA mutant could be complemented by gqqA. In the complementation assays we used the phenylalanine auxotrophic E. coli JW2580-1. This mutant carries a kanamycin gene inserted into pheA and is thus auxotrophic for phenylalanine (TABLE S1). Notably, growth of this strain could be restored in phenylalanine deficiency medium after introducing gqqA on the self-replicating plasmid pDrive. Cells carrying extra copies of gqqA usually grew within 24 h to optical densities of OD 600 nm 0.5 (Fig. 2C). Clearly, these findings imply that GqqA retains its prephenate dehydratase activities.
The observation here that GqqA has an additional acylase activity may explain some of the earlier observations that have been observed for pheA mutations in other Gram-negative bacteria but that could not be explained by the simple knockout of an amino acid biosynthesis pathway. Among those the recent observations that motility and pathogenicity, which are usually QS-dependent processes in Acidovorax citrulli35 were altered in the background of a pheA mutant. Further the increased persistence of the opportunistic pathogen Pseudomonas aeruginosa had been reported in a phe mutant and may also hint into a similar direction36.
DLS and SAXS experiments
The homogeneity of recombinant GqqA was analyzed via DLS measurements at 20 °C. A single peak was monitored corresponding to a hydrodynamic radius of 3.9 ± 0.1 nm, which is indicating a GqqA dimer of 61 kDa in solution (Fig. 4). Long-term DLS measurements at room temperature showed that the GqqA dimer remains stable for at least 4 days (Figure S4, A). Also, data obtained from SAXS experiments verified a GqqA dimer in solution. SAXS data revealed a radius of gyration of 2.7 nm and a dmax of 7.56 nm (Table S4).
Crystal structure analysis of GqqA
Crystals of GqqA and SeGqqA grew applying seeding within 3 days and belong to the space group P21 (GqqA) and P212121 (SeGqqA), respectively (Figure S4 B, C). Molecular replacement calculations using the diffraction data of native GqqA collected to 2.5 Å resolution and the most homologous protein structure deposited at pdb at that time, a prephenate dehydratase with 33% sequence identity (pdb code 2qmx), was not successful to solve the phase problem. Therefore, the crystal structure of SeGqqA was solved by single-wavelength anomalous diffraction (SAD) and refined to 1.7 Å resolution. The coordinates of the solved and refined structure of SeGqqA were suitable to solve the phase problem of native GqqA data by molecular replacement.
GqqA consists of three subdomains. Upon structure solution and refinement of SeGqqA we realized that one subdomain (residues 86–170) is missing, shown and indicated in Figure 5A. The loss of this domain, which obviously appeared by proteolysis during the crystallization process of SeGqqA, resulted in crystals with different space group and cell dimensions, compared to GqqA. However, the obtained crystals were of higher quality. Due to the fold of the polypeptide chain in GqqA the missing domain for SeGqqA is located entirely at one side of the protein and has only a few interactions with the other domains (Figure 5B). Superposition of the native GqqA on SeGqqA main chain atoms resulted in a Cα rms deviation of 0.76 Å, indicating that the missing domain of the SeGqqA structure did not change the overall fold of remaining two protein domains.
DLS and SAXS measurements indicated a GqqA dimer in solution, which is also present in the crystal structure with a rather extended interface area of approx. 2230 Å2 between the monomers (Figure 6). A GqqA monomer itself consists of three domains. Two of them, the N-terminal and middle domain form the functional unit, which is homologous to the catalytic PBP domain of the prephenate dehydratase (pdb code: 2qmx), whereas the C-terminal domain is homologous to the regulatory ACT domain. The N-terminal and middle domain of GqqA consist of a mixed five-stranded β-sheet with three parallel strands, surrounded by three α-helices. The C-terminal ACT domain is formed by a four-stranded anti-parallel β-sheet and two helices. The symmetry related mate of the ACT domain complements an extended central β-sheet structure of the functional homodimer (Figure 6). In the C-terminal regions of both monomers within the dimer interface we identified two L-Phe molecules. Bound L-Phe molecules were also identified in the E. coli prephenate dehydratase structure (pdb code 2qmx), where they are assigned to be responsible for feedback regulation37, triggering allosteric events by changing the relative orientation of the ACT-domains in the homodimer. L-Phe is also bound in the truncated SeGqqA.
Comparison of GqqA and the homologous prephenate dehydratase
Overall, the structure of GqqA is highly homologous to known structures of PDT enzymes. A DALI38 search identified the highest structural similarity of GqqA and a PDT from Bifidobacterium adolescentis (PDB: 3luy), with a sequence identity of 22.7% and Cα rms value of 2.5 Å (Figure 7A). A sequence comparison of GqqA with various prephenate dehydratases showed that the PBP domain is more conserved than the ACT domain (Figure 7B). Superposition with the prephenate dehydratase structure of Chlorobium tepidum TLS (2qmx) which shares 33% sequence identity and rmsd of 2.3 Å on Cα-atoms, revealed that the catalytic and the regulatory domains of the proteins share the same fold, but the catalytic domains have slightly different orientations to each other. In GqqA the loop formed by residues 181–192 is slightly shorter than the corresponding loop of the Chlorobium tepidum TLS prephenate dehydratase (PDB: 2qmx, residues 178–192) and has a different conformation (Figure 8).
The active site of GqqA
Crystal structures of GqqA closely related enzymes with bound substrates or inhibitors are not published. Our efforts to get substrate or inhibitor complexes of GqqA by co-crystallization with N-acyl homoserine lactones or soaking native crystals with substrates or inhibitors failed. The electron density maps of several diffraction datasets revealed no electron density to localize a putative active site.
The PBP domain is folded into two structurally similar subdomains which form a cleft for the putative active site. Regarding other structures which share PBP domains, we suggest an active site in a cleft between the subdomains of the catalytic PBP domain. The DALI server38 was used to find the most homologous structure with a bound substrate. An ATP phosphoribosyltransferase (pdb code: 1nh8) shares 12% sequence identity with GqqA and a rmsd of 4.3 Å on Cα-atoms. This protein has an AMP bound in the above-mentioned cleft of the PBP domain39. GqqA possess a highly hydrophobic cleft between these domains which gave a suitable environment for the hydrophobic part of N-AHLs.
Docking studies applying the native GqqA structure and the potential substrate N-octanoyl-L-homoserine lactone suggest that the lactone ring most probably binds to the polar residues Y16, S17 and T174 located in the cleft typical for the subdomains of PDT (Figure 9). A minor binding site of the ligand has been identified on the surface of GqqA (Figure 9A). The polarity of the cleft is enhanced by the helical dipoles of three α-helices pointing with their N-termini into the cleft. Also, the C-termini of the parallel β-sheet of the catalytic domain point towards the cleft. The nonpolar alkyl chain of AHL is directed to the entrance of the active site of GqqA, allowing to cover fatty acid residues with variable lengths.
For prephenate dehydratases structures an open and a closed conformation has been observed, which is regulated by phenylalanine binding37. In the open conformation the putative active site region is more solvent accessible. According to this data the GqqA crystal structure we analysed corresponds to a closed conformation.
Overall, the structural homology of GqqA with structures of PDTs implies that GqqA evolved from a prephenate dehydratase and the substrate specificity was enhanced, due to mutations in its active site region. In the E. coli prephenate dehydratases four amino acid residues were identified to be important for prephenate dehydratase catalytic activities32,33. However only two were conserved in GqqA (N206 and L215). Further in E. coli the two amino acids E159 and E232 appear to be important for substrate binding33. These two amino acid positions are conserved in GqqA and correspond to E55 and E127.
Notably, the above-described complementation studies (Figure 2C) strongly imply that GqqA has retained its native prephenate dehydratase activities. Growth of the E. coli PDT mutant would not be possible without a functional PDT activity of GqqA.
Analysis of different mutations of GqqA
To obtain functional insights about the dimerization we analyzed the dimer interface region and identified essential interactions and amino-acid residues stabilizing the dimer. To address these regions, five GqqA mutants (Figure 2) were generated. The correctness of the different mutations was verified by sequencing and the constructs were transformed into the overexpression strain E. coli BL21 (DE3), purified and assayed for their function (Figure 2B).
In GqqA_F261S (M1), this mutation probably reduced essential hydrophobic interaction within the dimer interface and as a result GqqA_F261S (M1) was inactive, when assayed with the Chromobacterium violaceum reporter strain CV026 (Figure 2B). The second mutation (GqqA_Δ279-281) (M2) truncated the C-terminus without effects on the enzymatic activity. The GqqA_R25S (M3) mutant affected the dimerization resulting again in a loss of activity (Figure 2B). A fourth mutation (GqqA_P187A_ΔP188_ΔP189-190_P191S) (M4) was introduced with the goal to remove the most divergent loop, at residues 187–191. This mutant was not active. A fifth mutation (M5) was introduced and targeted the threonine at position 118 and which was changed to a valine. This mutant was active implying that the threonine 118 was not involved in the catalysis.
Conclusions
Earlier we have identified GqqA in the cellulose overproducer and biofilm-forming bacterium K. europaeus CECT 8546, interfering with QS signals of AHLs from Gram-negative bacteria1,34. GqqA acts as an acylase on AHL and the amido hydrolyzing mechanism is unambiguously characterized by ESI–MS/MS analysis, identifying homoserine lactone and the fatty acid as products. The crystal structure confirmed that GqqA can be assigned to be a first member of a novel type of acylases, since GqqA has no homology to currently known Ntn hydrolases or alpha/beta hydrolases. Instead, the structure has a high homology to prephenate dehydratases, indicating that GqqA developed from this class of enzymes, which are all active as dimers. While the mutational analyses in combination with the structural data gave a first insights into the function of this remarkable and bifunctional enzyme future research will have to address additional questions. Thereby, the most immediate steps will be a mutational verification of the substrate binding site and gaining a better understanding on the mechanisms involved in substrate specificity versus promiscuity.
Materials and methods
Bacterial strains, plasmids, primers and growth conditions
Bacterial strains and plasmids utilized in terms of the investigations are summarized in Table S1. Escherichia coli strains were cultivated in LB or M9 medium at 37 °C. Antibiotics were added to the cultures, when required, with appropriate concentrations.
Overexpression and purification of GqqA
The gene encoding GqqA, isolated from Komagataeibacter europeaus, was integrated in pET21a with a C-terminal TEV-protease cleavage site (ENLYFQS) and a His6-tag, as described before by1. GqqA was produced by gene overexpression in E. coli strain BL21 (DE3). The culture was grown in LB medium with ampicillin (final concentration 100 µg ml−1) inoculated with 25 ml pre-culture at 37 °C. When the cells reached the exponential growth phase (OD600nm), protein expression was induced by supplementation of 1 mM IPTG (isopropyl-β-D-1-thiogalactopyranoside). After 3 h of incubation the cells were harvested by centrifugation applying 4000 g at 277 K for 30 min. The pellet was resuspended in lysis buffer (50 mM NaH2PO4, 300 mM NaCl, 10 mM imidazole, pH 8.0). The cells were disrupted by 5 × 1 min sonification and centrifuged with 17000 g at 277 K for 1 h. The supernatant containing the His6-tagged target protein was incubated on a Ni–NTA agarose column for 1 h on a rotary shaker at 277 K. The sample was washed twice with wash buffer (50 mM NaH2PO4, 300 mM NaCl, 20 mM imidazole, pH 8.0) and eluted with 5 ml elution buffer (50 mM NaH2PO4, 300 mM NaCl, 250 mM imidazole, pH 8.0). The sample was concentrated by centrifugation applying amicon filters and loaded onto a size-exclusion chromatography column (Superose6Increase, GE Healthcare) in a buffer consisting of 0.1 M K2HPO4, pH 5.0, 150 mM NaCl. Fractions containing the pure protein were pooled and concentrated to 10 mg ml−1. The purity of the protein was verified by Coomassie stained SDS-PAGE (FIGURE S1 A), which shows a dominant band at approximately 30 kDa, consistent with monomeric GqqA (30.5 kDa).
To solve the crystallographic phase problem the 8 methionines of GqqA were substituted by selenomethionines40. The preculture was centrifuged with 17,000 g at 4 °C for 20 min. and resuspended in 5 ml M9-medium. The culture was grown in M9-medium with Ampicillin (final concentration 100 µg ml−1) inoculated with 1.25 ml resuspended pellet at 37 °C. When the cells reached the exponential growth phase (OD600nm), they were supplemented with 20 ml selenomethionine (SeMet) (1 g l−1) and 5 ml of an amino acid mixture (TABLE S2). After 15 min protein expression was induced by supplementation of 1 mM Isopropyl-β-D-thiogalactopyranoside (IPTG) and after 3 h of incubation at 37 °C the cells were harvested by centrifugation with 4,000 g at 4 °C for 30 min. The selenomethionine-variant of GqqA (SeGqqA) was purified following the same procedures as applied for GqqA.
ESI–MS/MS analysis
For enzyme assays 3-oxo-octanoyl homoserine lactone (oxo-C8-HSL) as substrate was used in 5 mM N-2-hydroxyethylpiperazine-N’-3-propanesulfonic acid (EPPS) buffer, pH 8.0. Prior to use a 100 mg/ml stock solution of oxo-C8-HSL in dimethyl sulfoxide (DMSO) was prepared. If otherwise not indicated, reactions were performed, in triplicates and corrected for non-enzymatic transformation, at—70° and in 5 mM EPPS buffer, pH 8.0. The assays were conducted according to the following steps. One milliliter of 5 mM EPPS buffer, pH 8.0, was introduced into a 1.5 ml Eppendorf tube that was closed tightly. The substrate oxo-C8-HSL was then added to a final concentration of 0.5 mg/ml (from a 100 mg/ml stock solution in DMSO). Finally, the protein was immediately added to a final concentration of 10 µg/ml (from a stock solution of 5 mg/ml in 40 mM HEPES, pH 7.0). Aliquots were taken at different time intervals, and the reaction products were analyzed by Mass Spectrometry (MS) experiments, performed in a hybrid quadrupole-time of flight mass spectrometer (QTOF, QSTAR pulsar i, ABSciex) equipped with a micro electrospray ion source (in positive and negative mode). Samples were dissolved in methanol (0.1 ml sample plus 0.9 ml methanol) and introduced in the spectrometer using a syringe infusion pump with a 10 ul/min flow. N2 was employed in the collision cell. MS experiments in TOFMS mode were registered to identify the reaction products. The experiments were performed with positive ion detection. The instrumental parameters were set as follows: mass range 50–2000 Dalton; ion spray voltage (IS): 4500 V; ion source gas pressure (GS1): 10 psi; curtain gas pressure (Cur): 20 psi; declustering potential (DP): 30 V; focusing potential (FP): 210 V; declustering potential 2 (DP2): 15 V; collision gas: 3. Substrates and products used and generated are listed in TABLE S3 together with their molecular mass.
Dynamic light scattering measurements
Prior to SAXS and crystallization experiments the homogeneity of GqqA and SeGqqA in solution (3.6 mg ml−1 in 0.1 M K2HPO4 pH 5.0, 150 mM NaCl) was verified performing dynamic light scattering (DLS) measurements at 20 °C. 15 µl of purified GqqA suspension were measured in Helma cuvettes applying the SpectroSize 300 DLS system (Xtal Concepts, Germany).
Small angle X-ray scattering
Small angle X-ray scattering data for GqqA were collected at 20 °C at beamline P12 (PETRA III, EMBL, Hamburg, Germany). Three different protein concentrations (4, 2 and 0.8 mg ml−1) were measured applying an automated robotic sample changer and a Dectris 2D photon-counting detector (PILATUS-6 M) with 3.1 m sample to detector distance. Scattering data for all three concentrations were collected, integrated, and averaged applying the SasTool software (EMBL, Hamburg, Germany) (Franke 2017. Guinier analysis and radius of gyration (RG) values were calculated using PRIMUS41. The pair distribution functions P(r) and forward scattering intensities I(0) were processed with GNOM42 and PRIMUS. Data collection statistics and results are summarized in TABLE S4.
Crystallization
Initial screening of GqqA and SeGqqA was performed applying the sitting-drop vapor-diffusion method and 96-well plates utilizing a Honeybee crystallization robot (Genomic Solutions, USA) and using the commercial kit JCSG-plus (Molecular Dimensions, UK). Thin GqqA crystals were identified after 3 days with 0.8 M succinic acid at pH 7.0 as reservoir solution. To obtain larger and X-ray suitable crystals streak seeding was applied to seed a droplet of 2 µl protein solution (10 mg ml−1) and 2 µl reservoir solution using 24-well linbro plates (FIGURE S1, C and D). Seed suspensions were prepared according to the protocol of HAMPTON Research (HAMPTON Research, US). SeGqqA crystals were obtained in 10% PEG3350. Final crystallization conditions are summarized in TABLE S5.
GqqA diffraction data collection, structure solution, and refinement
For native GqqA and SeGqqA X-ray diffraction data were collected at 100 K at beamline P11 (PETRA III, DESY, Hamburg). The diffraction data were indexed, integrated and scaled using the XDS software package43.
Initial structure solution was possible applying diffraction data of a single SeMet-labelled GqqA (SeGqqA) crystal collected at a wavelength of 0.98 Å. This crystal diffracted up to 1.7 Å resolution and diffraction data were used for single-wavelength anomalous phasing (SAD), performed using the Autorickshaw-Server44. Based on eight located Se-positions phasing was possible and initial electron densities allowed model building of SeGqqA applying the program Coot45. Subsequent refinement was performed utilizing the program Refmac546. Interestingly this structure contained only two of the three GqqA protein domains.
Diffraction data to 2.5 Å resolution were collected for native GqqA at a wavelength of 1.03 Å. The obtained SeGqqA structure was used for molecular replacement to obtain initial phases of the native GqqA structure using the program Phaser47. The native structure was subsequently completed by building amino-acid residues 85–170 of the missing domain into the 2Fo-Fc electron density maps. The following structure refinement was performed using the program Phenix48. In later stages of the refinement the Phenylalanine co-factor and solvent molecules were introduced and refined. Data collection statistics and refinement results are summarized in Table 2. The refined GqqA and SeGqqA structures were deposited in the Protein Data Bank with pdb codes 7AM0 and 7ALZ.
In silico ligand docking
Docking approaches were performed with the freely available docking software SwissDock49,50. The software searches possible target cavities in proteins by calculating the binding energies of small molecules. N-octanoyl-L-homoserine lactone was chosen as putative ligand due to previous experiments1 and provided in mol2 format. The GqqA dimer was used without solvent molecules but with bound L-Phe in the regulatory domain. The best hits are clustered and are visualized in Figure 8A.
Construction of GqqA mutants
For the exchange of individual amino acids in GqqA, site-directed mutagenesis was used. For this purpose, the mutations were carried out using the phusion DNA polymerase, the construct pET21a::gqqA as template and the following mutation-specific primers:
GqqA_M1_for (5’ CGAACTTTCGTCCTTTTCGGAACAGCAGGAGATC 3’), GqqA_M1_rev (5’ TCCAGCGCACGCGCCAGT 3’), GqqA_M2_for (5’ CTCGAGCACCACCACCACC 3’), GqqA_M2_rev (5’ CCGGAAGGGCGATGCGGG 3’), GqqA_M3_for (5’ CATGCAAGGTCCGAATAGGCCCCGGCAGGCCTCGCCCGGCTGGA 3’), GqqA_M3_rev (5’ CATGCAAGGTCCGAATAGGCCC 3’), GqqA_M5_for (5’ CGGCATCATTGTCGAACTGGGACTGGACCCAG 3’), GqqA_M5_rev (5’ CGCACCTGCGCCATGGCG 3’). The GqqA_Mut4 construct was generated by using a synthesized gene fragment containing the substitution and deletion side. To remove the template DNA, the PCR product was digested with DpnI (30 min 37 °C, 10 min heat inactivation at 75 °C). After digestion, a phosphate group was added to the amplicon polynucleotide phosphokinase using the manufacturer's protocol (Thermo Scientific, Bremen, Germany). With the added phosphate group, the linear amplicon could be ligated with the T4 ligase by adding 1 µL 10 mM ATP. The ligation was carried out at alternating between 10 °C and 30 °C for 60 min. A heat inactivation step was followed by heat shock transformation into E. coli DH5α. Positive clones were verified by sequencing and transformed into the overexpression strain E. coli BL21(DE3).
In vivo QQ enzyme assays
For a functional AHL-degrading assay, the reporter strain C. violaceum CV026 was used as previously described and with minor modifications1,52. For this purpose, E. coli BL21 (DE3) strains containing the pET-21a::gqqA wt or the pET21a::gqqA M1-M5 mutant constructs were grown in a preculture. Fresh LB medium was inoculated with 1% (vol/vol) of the precultures and cultured at 37 °C until an OD600 of 0.6 was reached. Following this cells were induced with 0.1 mM IPTG and proteins were expressed for 16 h. After this fresh LB medium containing ampicillin and 10 µM oxo-C8-HSL was inoculated with the expression strains at a ratio of 2% (vol/vol) and incubated at 37 °C for 6 h. The culture supernatant was collected by centrifugation and 30 µL was used for bioassay. For this, a grown CV026 culture was mixed with 24-fold volume of LB agar and poured into plates. Sterile filter papers were placed on the plates. The CV026 plates with the supernatants of the cultures were incubated for 24 h at 28 °C. If CV026 cells turned purple, AI molecules were present; and if CV026 cells remain colourless, the AI molecules were degraded.
β-lactamase activity assay
The β-lactamase activity of GqqA was determined via a disc diffusion antibiotic susceptibility test. Ampicillin 10 µg (AMP), Amoxicillin 10 µg (AML), Cefotaxime 30 µg (CTX 30) and Penicillin G 10 µg (P) sensitivity discs (Thermo Fischer Scientific, Waltham, MA, USA) were incubated for 30 min at 28 °C with 30 µL of 0.1 M potassium phosphate buffer pH 8 containing 40 µg of GqqA. A control without enzyme was included. The antibiotic susceptibility test was performed on LB agar plates with S. aureus cells. After overnight incubation at 37 °C the halo formation indicates a degradation of the antibiotic.
Complementation assays with an auxotrophic strain of Escherichia coli
A complementation test was performed with the phenylalanine auxotrophic E. coli strain JW2580-1. The strain was obtained from the Coli Genetic Stock Center (http:// www.cgsc.biology.yale.edu) and carries an in-frame, single-gene knockout from the Keio Collection51. JW2580-1 was grown in LB medium overnight at 37 °C. Phenylalanine auxotrophy was verified to the complementation tests by growth on minimal medium M9 supplemented with and without L-phenylalanine (2 μM) (Sigma-Aldrich, Heidelberg, Germany). gqqA was amplified using the primers gqqA_comp_f (5’ ATGAACGGGGAACGCATCATCGC 3’) and gqqA comp_rev (5’ TCAGGGTTTGCGCCGGAG 3’) and the fragment was cloned into the pDrive vector. The resulting pDrive::gqqA vector was sequenced to verify the correctness of the sequence and was then transformed into JW2580-1 by electroporation. The transformed strain as well as the auxotrophic strain were grown in LB medium overnight at 37 °C and at 120 rpm; then, 5 ml of each culture was centrifuged, and cells were washed three times with M9 medium. 5 ml M9 medium with or without phenylalanine (2 µM) was inoculated with 50 µl of the washed cells and incubated up to 72 h at 37 °C.
Substrate specificity analysis
Conversion rate (Vmax) ) and affinity (Km) for 3-oxo-hexanoyl-, 3-oxo-octanoyl-, 3-oxo-decanoyl-, and 3-oxo-dodecanoyl- homoserine lactones, all from Merck Life Science S.L.U. (Madrid, SPAIN), was calculated using a pH indicator assay in 96-well plates, at 30 °C and pH 8.0 in a Synergy HT Multi-Mode Microplate Reader in continuous mode at 550 nm over 20 min, as described53. For enzyme assays, conditions were as detailed previously: [protein]: 10 μg ml-1; [3-oxo acyl homoserine lactone]: 0–65 mM; reaction volume: 200 μl; buffer: 5 mM EPPS buffer pH 8.0 containing 0.5 mM Phenol Red; T: 30 °C; and pH: 8.0. The absorbance readings in all wells were measured immediately after the plate was gently shaken for 3 s. The rate of hydrolysis in each triplicate assay was recorded at 15 s intervals over 20 min. The absorbance readings for the reaction steady state (within the first minute of the assay) were used to generate a progress curve (arbitrary absorbance units vs. time) from which a line slope value was determined, and enzyme units calculated as described53. All values, in triplicate, were corrected for non-enzymatic transformation, with absence of activity defined as at least a two-fold background signal as described53.
Data availability
The coordinates and structure factors of crystal structures of GqqA and SeGqqA have been deposited in the PDB with accession codes 7AM0 and 7ALZ, respectively. All other data generated or analyzed during this study are included in this article and its supplementary Information files.
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Acknowledgements
The authors acknowledge support by BMBF via project number 05K13GUA, the EU project INMARE and via the Cluster of Excellence 'Advanced Imaging of Matter' of the Deutsche Forschungsgemeinschaft (DFG)—EXC 2056—project ID 390715994 and the DFG project STR 451/7-1. MF acknowledges the support by EU H2020 grant INMARE (agreement no. 634486), and grants PCIN-2017-078 (within the Marine Biotechnology ERA-NET; GA no.: 604814 funded under the FP7 ERA-NET scheme) and BIO2017-85522-R from the Ministerio de Economía, Industria y Competitividad, Agencia Estatal de Investigación (AEI), Fondo Europeo de Desarrollo Regional (FEDER) and European Union (EU), and the grant 2020AEP061 from the Agencia Estatal CS.
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W.R.S. designed the study, coordinated manuscript writing and bioassays. Ch.B. contributed to planning and evaluation X-ray structural investigations, and manuscript preparation. N.W, W. H., S.F. and M.P. contributed to planning and evaluation X-ray structural investigations. K.P. contributed to protein expression, mutational and phylogenetic analyses. P.P.G and J.C performed ß lactam assays. CV was involved in mutational analyses, complementation studies and manuscript writing. M. F, L. F-L, performed the ESI–MS analyses.
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Werner, N., Petersen, K., Vollstedt, C. et al. The Komagataeibacter europaeus GqqA is the prototype of a novel bifunctional N-Acyl-homoserine lactone acylase with prephenate dehydratase activity. Sci Rep 11, 12255 (2021). https://doi.org/10.1038/s41598-021-91536-1
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DOI: https://doi.org/10.1038/s41598-021-91536-1
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