The Functional Role of a Conserved Loop in EAL Domain-Based Cyclic di-GMP-Specific Phosphodiesterase

EAL domain-based cyclic di-GMP (c-di-GMP)-specific phosphodiesterasesplay important roles in bacteria by regulating the cellularconcentration of the dinucleotide messenger c-di-GMP. EAL domainsbelong to a family of (β/ ${alpha}$ )₈ barrel fold enzymes that containa functional active site loop (loop 6) for substrate bindingand catalysis. By examining the two EAL domain-containing proteinsRocR and PA2567 from Pseudomonas aeruginosa, we found that thecatalytic activity of the EAL domains was significantly alteredby mutations in the loop 6 region. The impact of the mutationsranges from apparent substrate inhibition to alteration of oligomericstructure. Moreover, we found that the catalytic activity ofRocR was affected by mutating the putative phosphorylation site(D56N) in the phosphoreceiver domain, with the mutant exhibitinga significantly smaller Michealis constant (K_m) than that ofthe wild-type RocR. Hydrogen-deuterium exchange by mass spectrometryrevealed that the decrease in K_m correlates with a change ofsolvent accessibility in the loop 6 region. We further examinedAcetobacter xylinus diguanylate cyclase 2, which is one of theproteins that contains a catalytically incompetent EAL domainwith a highly degenerate loop 6. We demonstrated that the catalyticactivity of the stand-alone EAL domain toward c-di-GMP couldbe recovered by restoring loop 6. On the basis of these observationsand in conjunction with the structural data of two EAL domains,we proposed that loop 6 not only mediates the dimerization ofEAL domain but also controls c-di-GMP and Mg²⁺ ion binding.Importantly, sequence analysis of the 5,862 EAL domains in thebacterial genomes revealed that about half of the EAL domainsharbor a degenerate loop 6, indicating that the mutations inloop 6 may represent a divergence of function for EAL domainsduring evolution.

INTRODUCTION

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INTRODUCTION

The cyclic dinucleotide cyclic di-GMP (c-di-GMP) has emergedas a major bacterial messenger for mediating a variety of cellularfunctions that range from virulence expression and biofilm formation(5, 14, 30). The cellular concentration of c-di-GMP is controlledby the GGDEF domain proteins with diguanylate cyclase (DGC)activity and the EAL domain proteins with c-di-GMP-specificphosphodiesterase (PDE) activity. GGDEF domains catalyze thesynthesis of c-di-GMP from GTP, whereas EAL domains catalyzethe hydrolysis of c-di-GMP to generate the linear 5'-pGpG. Althougha family of HD-GYP domain proteins has also been found as c-di-GMP-specificPDEs, the overwhelmingly large number of genes encoding theEAL domains in bacterial genomes suggests that the EAL domainsare the major PDEs for maintaining the cellular c-di-GMP concentration.Remarkably, multiple copies of EAL domain-encoding genes areusually found in bacterial cells, with as many as 21 in Pseudomonasaeruginosa and 32 in Vibrio cholerae. Although many of the EALdomains were found to function as PDE domains for c-di-GMP degradation,emerging evidence suggests that some EAL domains function asligand- or protein-binding domains without catalytic activity(24, 28, 40).

The detailed structure and catalytic mechanism of the EAL domainshave started to be elucidated recently. The crystal structuresof two proteins with EAL domains, TdEAL and YkuI, have beendetermined (Protein Data Bank accession nos. 2BAS, 2R6O, and2w27) (23). EAL domains adopt a (β/ ${alpha}$ )₈ barrel fold thatcontains two extended strands, including an antiparallel strand.The (β/ ${alpha}$ )₈ barrel fold, first found in triosephosphate isomerase,has been observed in a diversity of enzymes that include manyhydrolyases and isomerases (34). Similar to other (β/ ${alpha}$ )₈barrel fold enzymes, the catalytic residues of the EAL domainare located at the C-terminal ends of the β-strands andthe beginning of the β $->$ ${alpha}$ loops connecting the β-strandsand ${alpha}$ -helices. In the proposed mechanism, EAL domains catalyzethe hydrolysis of c-di-GMP by using a Mg²⁺ ion and a generalbase catalyst (Glu) for generating the nucleophilic H₂O (28).The catalytic mechanism is supported by the crystal structureof the YkuI-substrate binary complex (Protein Data Bank accessionno. 2w27) and the model of the TdEAL-substrate complex (23,28). Both structures showed that the EAL domains bind c-di-GMPin such a configuration that the scissile phosphorus-oxygenbond aligns linearly with the attaching water and the generalbase catalyst. The catalytic mechanism can account for the lackof catalytic activity for most known inactive EAL domains, withthe loss of enzymatic activity arising from the absence of thegeneral base catalyst and/or the residues that coordinate theMg²⁺ ion (28).

It is well-known that many (β/ ${alpha}$ )₈ barrel fold enzymes containa flexible active site loop between the β6 strand and ${alpha}$ 6helix (34). Despite the diverse reactions catalyzed by (β/ ${alpha}$ )₈barrel fold enzymes, this extended loop, often referred to asloop 6, plays an important role as a functional lid for substratesequestering, solvent exclusion, and product release (15). Theloop was found to facilitate substrate binding and conformationaltransition in tryptophan synthase (3, 4) and functions as alid for substrate sequestering during catalysis in inosine 5'-monophosphatedehydrogenase (22). Notably, it was shown that the loop swaysfrom the active site in the nonactive structure of ribulose-1,5-bisphosphatecarboxylase but folds over to shield the active site from thesolvent in the activated structure (21). Similar functions havealso been proposed for loop 6 in other (β/ ${alpha}$ )₈ barrel foldenzymes, such as triosephosphate isomerase and phosphoriboxylanthranilate isomerase (15, 25, 26). Hence, it seems that thefunctional role of loop 6 has been well preserved in (β/ ${alpha}$ )₈barrel fold enzymes during evolution. The (β/ ${alpha}$ )₈ barrelfolded EAL domains also contain an eight-residue loop betweenthe β6 strand and ${alpha}$ 6 helix that seems to be critical forcatalysis. Schmidt and coworkers (32) first noticed that thecatalytically active EAL domains seem to contain a conservedmotif that was later confirmed to contain loop 6 [DFG(T/A)GYSS]and one of the residues (Asp) for Mg²⁺ binding (28, 32). Wepreviously noticed that mutation of the essential catalyticresidues is usually accompanied by the degeneration of loop6 in catalytically inactive EAL domains (28). Moreover, we observedthat the mutation of a residue interacting with loop 6 in theEAL domain-containing RocR abolished enzymatic activity, whichled us to postulate a critical role for loop 6 in catalysis(28).

To elucidate the precise role played by loop 6 in c-di-GMP hydrolysis,we examined three EAL domain-containing proteins that includeRocR, PA2567, and A. xylinus DGC2. The residues of loop 6 [DFG(A/T)SYSS]in RocR and PA2567 are well conserved, as observed in othercatalytically active EAL domains. We show that mutations inthe loop 6 region in RocR and PA2567 had significant effecton the structure and catalysis of the EAL domain. By using themethod of hydrogen-deuterium (H/D) exchange-coupled mass spectrometry,we demonstrated that a single remote mutation in the phosphoreceiverdomain of RocR caused correlated changes in loop 6 conformationand catalytic properties. We further show that the catalyticactivity of the inactive EAL domain of A. xylinus DGC2 can berecovered by restoring loop 6. The functional roles of loop6 in EAL domains in substrate binding and catalysis were discussedin conjunction with the structural data for two EAL domains.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Protein cloning, expression, and purification. The cloning, expression, and purification of RocR and PA2567have been described previously (28). All mutants were generatedusing the site-directed mutagenesis II kit (Stratagene) accordingto the manufacturer's instruction manual. The mutant proteinswere expressed and purified following the same procedure forthe wild-type proteins. The proteins were flash frozen in liquidN₂ and stored in a –80°C freezer after the measurementof concentration by the Bradford method.

For the full-length A. xylinus diguanylate cyclase 2 (DGC2),a gene construct encoding the full-length DGC2 gene from A.xylinus was commercially synthesized by GenScript Inc., amplifiedby PCR, and cloned into the expression vector pET26b(+) (Novagen)between the NdeI and XhoI restriction sites. The plasmid harboringthe gene construct and the C-terminal His₆ tag-encoding sequencewere transformed into Escherichia coli strain BL21(DE3). Forprotein expression, 2 ml of inoculum from the cell stock wasadded to 1 liter of LB medium. The bacterial culture was grownat 37°C until it reached an optical density (600 nm) of0.8 before being induced with 0.8 mM isopropyl-β-D-thiogalactopyranoside(IPTG) at 16°C for ca. 12 h. After centrifugation, the pelletswere lysed in 20 ml lysis buffer, which consists of 50 mM Tris-Cl(pH 8.0), 200 mM NaCl, 5% glycerol, 1% β-mercaptoethanol,and 1 mM phenylmethylsulfonyl fluoride. After centrifugationat 25,000 rpm for 30 min, the supernatant was filtered and thenincubated with 2 ml of Ni²⁺-nitrilotriacetic acid resin (Qiagen)for 30 min. The resin was washed with 50 ml of W1 buffer (lysisbuffer with 20 mM imidazole) and 50 ml of W2 buffer (lysis bufferwith 50 mM imidazole). The proteins were eluted using a stepgradient method with the elution buffer containing 50 mM Tris(pH 8.0), 200 mM NaCl, 5% glycerol, and 200, 300, and 500 mMimidazole. After sodium dodecyl sulfate-polyacrylamide gel electrophoresisanalysis, fractions with purity higher than 95% were pooledtogether and desalted using a PD-10 column (GE Healthcare).Proteins were first concentrated using an Amicon concentrator(Millipore) to ca. 5 mg/ml before being assayed for enzymaticactivity.

For the stand-alone EAL_DGC2 domain, an expression vector encoding306 to 574 amino acids of A. xylinus DGC2 was constructed byamplifying the corresponding gene fragment by high-fidelityPCR and cloning into pET-28(b+) (Novagen) between the NdeI andXhoI restriction sites. The plasmid harboring the gene constructwas transformed into E. coli strain BL21(DE3). The protein wasexpressed and purified in the same procedure as full-lengthA. xylinus DGC2. The triple mutant (N₄₇₃K₄₇₆I₄₇₈ $->$ D₄₇₃T₄₇₆Y₄₇₈)was generated using the site-directed mutagenesis II kit (Stratagene)according to the manufacturer's instruction manual. Mutant proteinwas expressed and purified following the same procedure describedabove.

Steady-state enzymatic activity assay. The substrate c-di-GMP used for kinetic measurement was producedenzymatically by using an engineered thermophilic DGC protein(27). The measurement of the steady-state kinetic parameterswas carried out by monitoring the formation of the product 5'-pGpGas described previously (28). The turnover number (k_cat) andMichealis constant (K_m) used for estimating enzyme efficiencyand substrate binding were obtained by fitting the initial velocitiesat various substrate concentrations to the Michaelis-Mentenequation with the exception of the two mutants that exhibitsubstrate inhibition. The kinetic data for the two mutants werefit using a model that assumes the substrate can bind to theenzyme at a productive and a nonproductive (or inhibitory) bindingsite (Fig. 1) .

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FIG. 1. Kinetic model for mutants that exhibit substrate inhibition. The model assumes that the substrate can bind to the enzyme at a productive binding site and a nonproductive (inhibitory) binding site. Abbreviations: E, enzyme; P, product; S, substrate; k_c, rate constant for the chemical step.

The curves were obtained by fitting the kinetic data to thefollowing equation derived from the model based on the steady-stateand rapid equilibrium assumptions. In the following equation,K_i is the inhibition constant, ${alpha}$ and β are the factors bywhich the K_m, K_i, and V_max change when the second substrateis bound at the nonproductive site, v is initial velocity, and[S] is the concentration of the substrate.

Formula 1 (1)

Size exclusion chromatography. Gel filtration was performed at 4°C using the AKTA FPLC(fast protein liquid chromatography) system (GE Healthcare)equipped with a Superdex 200 HR 16/60 column (Amersham Biosciences).The buffer used for gel filtration is comprised of 20 mM Tris-HCl(pH 8.0), 0.5 M NaCl, 5% glycerol, and 0.5 mM dithiothreitol.

Amide hydrogen-deuterium exchange by mass spectrometry. The apparatus for H/D exchange was similar to the setup describedelsewhere (13, 19, 29). The purified RocR or D56N mutant wasexchanged into 100 mM sodium phosphate buffer (pH 7.0) thatcontains 150 mM sodium chloride and 1 mM dithiothreitol. Thepeptides generated by pepsin digestion were first identifiedby a tandem mass spectrometry experiment. The H/D exchange reactionswere initiated by adding 10 µl of newly thawed proteinsolution to 90 µl of D₂O. After incubation for varioustime lengths (1/3, 1, 5, 15, 30 and 60 min), the exchange reactionwas rapidly quenched by lowering the pH to 2.4 and loweringthe temperature to 0°C, and followed by pepsin digestion.The resulting peptides were passed through a homemade capillaryreverse-phase C₁₈ high-performance liquid chromatography (HPLC)column and eluted into the quadruple time-of-flight mass spectrometer(Applied Biosystems/MDX Sciex QSTAR Elite system) equipped withan IonSpray source. The peptides were eluted at a flow rateof 20 µl/min using a step gradient (7.5, 10, 12.5, 15,17.5, 20, 22.5, 25, 30, 40, and 80% acetonitrile in 0.1% formicacid). The time from the initiation of digestion to the elutionof the last peptide was approximately 22 min. Analyst QS softwarewas used for spectrum analysis and data extraction, and theH/D exchange data were processed by using the program HX-Express(42). Zero time point control or the "artifactual in-exchange"control was performed by adding the quenching buffer to theprotein solution before exposure to D₂O (13). Measured peptidemasses were corrected for artifactual in-exchange at t = 0,normalized to 100% D₂O, and corrected for back exchange followingthe empirical method described by Hoofnagle et al. (13). Thetime-dependent H/D exchange data were fit by nonlinear least-squaresfitting to the equation shown below.

Formula 2 (2)
where N is the total number of deuterons incorporatedover the observed course for each peptide, and A, B, and C correspondto the number of amides exchanging with the rate constants k₁,k₂, and k₃, respectively (13) (20). The number of nonexchangingamides is calculated from the total number of the backbone amides(N_H) in the peptide, excluding proline residues.

Bioinformatic analysis and structural modeling. The Stockholm-format alignment of 5,862 sequences in the EAL(PF00563) family was downloaded from the PFAM database (http://pfam.sanger.ac.uk//family/EAL).Two PERL scripts were used to search for sequences that containthe essential catalytic residues (equivalent to E175, N233,E265, D295, and E352 in RocR) and the motif DFG(A/S/T)(A/G)(Y/F)(S/T)(S/T/G/A/N)that constitutes loop 6. On the basis of the search results,the 5,862 sequences were divided into four groups as we discussbelow in the Discussion. For homology modeling, the structuralmodel for the EAL domain of RocR was constructed with the coordinatesof the TdEAL structure (Protein Data Bank accession no. 2R6O)as the template in SWISS-MODEL (1). The structural model forthe response receiver (RR) domain of RocR was built using thestructure of the RR domain of CheB (Protein Data Bank accessionno. 1A2O) as the template.

RESULTS

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RESULTS

Catalytically active EAL domains require four residues for bindingthe essential Mg²⁺ ion and a general base catalyst for activatingthe nucleophilic water (28). In addition, a conserved loop,loop 6, which contains the motif DFG(T/A)GYSS, was found inmost known active EAL domains (32). Considering that a largenumber of EAL domains in the genomes contain a degenerate loop6, elucidation of the functional role of loop 6 may yield cluesto the functions of these EAL domains.

Effects of mutations in the loop 6 region. The P. aeruginosa protein RocR is a response regulator thatcontains a RR domain and a catalytically active EAL domain (18,28). RocR catalyzes the hydrolysis of c-di-GMP with a turnovernumber (k_cat) of 0.67 ± 0.03 s^–1 and Michaelisconstant (K_m) of 3.2 ± 0.3 µM under the enzymaticassay conditions. We previously found that the mutation of Glu²⁶⁸,a highly conserved residue that was suggested to stabilize loop6, significantly altered the catalytic properties of RocR (Fig.2) (28). The E268A mutation reduced the enzyme activity to belowthe measurable level, whereas the E268Q mutation decreased K_mto 0.31 ± 0.1 µM and caused a 446-fold reductionin k_cat. We found that the mutation of Phe²⁹⁷, a residue onloop 6 (DF²⁹⁷GASYSS), reduced k_cat to 0.02 ± 0.1 s^–1and K_m to 0.73 ± 0.2 µM (Table 1) . Size exclusionchromatography showed that mutant enzymes with the E268A mutation,enzymes with the F297A mutation, and the majority of enzymeswith the E268Q mutation formed high-molecular-weight oligomer(HMWO) and eluted in the void volume (data not shown). The changein oligomeric state for the three mutants indicated that loop6 is crucial for maintaining the quaternary structure of RocR.This is in line with the observation that loop 6 is locatedat the dimer interface as we discuss later. In addition, theside chain of loop residue Ser³⁰² (DFGAGYSS³⁰²) interacts withGlu²⁶⁸ through hydrogen bonding according to the EAL_RocR structuralmodel and the TdEAL structure (Fig. 2A). Remarkably, the eliminationof the single hydrogen bond by the S302A mutation caused theenzyme to exhibit strong substrate inhibition kinetics withan inhibition constant of 10.9 ± 3.0 µM withoutaltering the oligomeric structure (Fig. 2B). The substrate inhibitionstrongly suggested that binding of c-di-GMP is sensitive tothe change of the loop conformation. Finally, the first residueof the loop (Asp²⁹⁶) may be involved in the binding of c-di-GMPaccording to the structural model (28). The D296A mutation causedsignificant changes in catalytic parameters without alteringthe oligomeric structure, by causing a decrease in k_cat by 33.5-foldand an increase of K_m to 8.6 ± 2.8 µM.

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FIG. 2. Loop 6 of RocR and the effects of mutations on catalysis. (A) Structural model of EAL_RocR with the residues of loop 6 and Glu²⁶⁸ highlighted. The hydrogen bonds formed between Glu₂₆₈ and the loop residues Gly³⁰⁰ and Ser³⁰² are represented by the broken lines. The Mg²⁺ ion is shown as the ball. (B) Effects of the mutations in the loop 6 region on the steady-state kinetics of RocR. The curves were generated by fitting the data to the Michaelis-Menten equation with the exception of the S302A mutant, for which the curve was generated by fitting the kinetic data to equation 1.

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TABLE 1. Steady-state kinetic parameters for RocR and its mutants^a

A large number of EAL domain proteins contain a widely occurringGGDEF-EAL didomain unit. PA2567 from P. aeruginosa is such aprotein; PA2567 contains a catalytically active EAL domain alongwith the GAF and GGDEF domains (28, 35) (Fig. 3). Site-directedmutagenesis and kinetic measurements were performed to determinewhether loop 6 plays similar roles in PA2567. Surprisingly,the single mutations of Phe⁴⁹³ and Ser⁴⁹⁸, which are the equivalentsof Phe²⁹⁷ and Ser³⁰² in RocR, caused the protein to form inclusionbodies during protein expression. Meanwhile, the mutation ofGlu⁴⁶⁴, the equivalent of Glu²⁶⁸ in RocR, caused strong substrateinhibition at high substrate concentration, with an inhibitionconstant of 30.4 ± 12.0 µM (Fig. 4 and Table 2).The mutation E464A did not perturb the oligomeric state of thedimeric PA2567 according to size exclusion chromatography. Theresults from the study of PA2567 and RocR seemed to suggestthat loop 6 plays crucial roles in stabilizing the overall proteinstructure and participating in catalysis, probably through mediatingsubstrate binding.

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FIG. 3. Domain organization of the RocR protein, the PA2567 protein from P. aeruginosa PAO-1, and the DGC2 protein from A. xylinus (AxDGC2).

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FIG. 4. Effect of the E464A mutation on the steady-state kinetics of PA2567. The curves were generated by fitting the kinetic data of the wild-type and mutant enzyme to the Michaelis-Menten equation and equation 1, respectively.

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TABLE 2. Steady-state kinetic parameters for PA2567 and its mutants^a

Effect of the D56N mutation on catalytic activity and loop 6 conformation in RocR. Because the small phosphor donors acetyl phosphate, carbamoylphosphate, and phosphoramidite did not phosphorylate RocR inour in vitro phosphorylation assay, we were not able to examinethe effect of phosphorylation on the catalytic activity of theEAL domain. In an effort to probe how the modification of theputative phosphorylation site (Asp⁵⁶) may affect EAL domainactivity, we found that the D56N mutation caused significantchanges in the steady-state kinetic parameters (Table 1). Themost significant change is in the Michaelis constant K_m, whichis 0.20 ± 0.03 µM for the D56N mutant, representinga 16-fold decrease from that of RocR (3.2 ± 0.3 µM).Meanwhile, the D56N mutant exhibits a k_cat value only slightlysmaller (0.13 s^–1) than that of RocR (0.67 s^–1).To probe the structural changes in the mutant that account forthe small K_m, the method of H/D exchange-coupled mass spectrometrywas used, because this method has been used increasingly asa sensitive tool for detecting changes in protein conformationand mobility (13). H/D exchange of RocR and the mutant D56Nenzyme were performed by following an established protocol (6,13, 19, 20). In total, 21 pairs of peptides generated from pepsindigestion were identified by a tandem mass spectrometry experimentand chosen for H/D exchange analysis. The 21 pairs of peptidesencompass 93% of the protein sequences for RocR and the D56Nmutant, including peptides 1 to 6 from the RR domain, peptide7 from the linker region, and peptides 8 to 21 from the EALdomain (Fig. 5A). The deuteration pattern of each pair of peptidesfrom RocR and the D56N mutant was compared by examining thetime-dependent deuteration plots. While about two-thirds ofthe peptides exhibited similar H/D exchange patterns, 8 outof 21 pairs of peptides exhibited notable differences in exchangerate and final deuteration level as we discuss below.

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FIG. 5. Comparison of amide H/D exchange between RocR and the D56N mutant. (A) Sequence coverage map of RocR with the 21 peptides generated from pepsin digestion represented by the bars below the sequence. The peptides from the mutant exhibiting decrease in deuteration are colored blue, whereas the peptides showing significant and moderate increase in deuteration are colored red and yellow, respectively. (B) Structural models of the EAL and REC domains of RocR. The peptides exhibiting decrease in deuteration are colored blue, and the peptides showing significant and moderate increase in deuteration are colored red and yellow, respectively. The linker between the RR and EAL domains is represented by the brown broken line. (C) Time-dependent H/D exchange plots for the peptides in the EAL domain that exhibit changes in deuteration (RocR [•] and D56N mutant [ ${circ}$ ]). The curves were generated by fitting the data to equation 2 to obtain the total number of incorporated deuterons (N) as well as the exchange rate constants k₁, k₂, and k₃. (D) Time-dependent H/D exchange plots for the peptides in the phosphoreceiver (REC) domain and linker region that exhibit changes in deuteration (RocR ([•] and D56N mutant [ ${circ}$ ]). The phosphorylated site (Asp⁵⁶) and two putative residues (Ser⁸³ and Phe¹⁰⁵) involved in signal transduction are shown as sticks in panel B.

In the EAL domain, 4 out of the 14 peptides in the D56N mutantexhibited different deuteration pattern from their counterpartsin RocR (Fig. 5B and C). The most prominent one is peptide 16,which exhibited faster exchange and higher deuteration levelin the mutant. Peptide 16 includes four residues (LAMD²⁹⁵) fromthe β6 strand that contains the conserved Asp²⁹⁵ for Mg²⁺coordination and the D²⁹⁶FGAGYSS motif that constitutes loop6. In addition to peptide 16, two peptides (peptides 9 and 19)showed moderate elevation in deuteration in the mutant. Peptide9 contains the first two β strands of the (β/ ${alpha}$ )₈ barreland forms part of the substrate-binding pocket, whereas peptide19 encompasses half of the ${alpha}$ 7 helix residing at the dimer interface.The fourth peptide (peptide 11) contains helix ${alpha}$ 2 and forms alid on the top of the substrate-binding pocket. Peptide 11 inthe mutant showed slightly faster exchange but a lower levelof deuteration at the end of the exchange (Fig. 5C). The resultingcrossover of the two exchange curves is likely to reflect achange in protein mobility (20). These results support a picturein which the D56N mutation induces rather localized structuralchanges in the EAL domain, with the most significant changesrestricted to the region near loop 6 and the end of the β6strand.

Since Asp²⁹⁶ is most likely to be the residue directly interactingwith the substrate and the D296A mutation increases K_m to 8.6± 2.8 µM, we further examine whether the effectof the D56N mutation on catalysis is exerted through Asp²⁹⁶.The D56N D296A double mutant was prepared and found to exhibitkinetic parameters similar to those of the D296A mutant, withk_cat of (1.2 ± 0.3) x 10^–2 s^–1 and elevatedK_m of 9.4 ± 2.8 µM. Together with the H/D exchangeresults, the resemblance of the catalytic properties of thedouble mutant to the D296A mutant, rather than the D56N mutant,suggested that the "regulatory signal" originated from the RRdomain probably exerts its effect on substrate binding and catalysisthrough Asp²⁹⁶ and the adjacent residues in loop 6.

In addition to the four peptides in the EAL domain, four peptidesresiding in the RR domain and linker region also exhibited alteredH/D exchange patterns (Fig. 5D). Most notably, the peptide spanningthe linker region and the end of the ${alpha}$ 5' helix (peptide 7) showeda significant increase in deuteration in the mutant protein.The deuteration level for peptide 7 is already relatively high(75%) in comparison with other peptides in RocR, indicatinga flexible and solvent-exposed linker region. The deuterationlevel of peptide 7 increased to 90% for the D56N mutant, suggestingthat the solvent accessibility of the linker region has beenfurther increased. Moreover, the two peptides (peptides 1 and4) that contain parts of the ${alpha}$ 1' and ${alpha}$ 4' helices showed lowerexchange rates and lower deuteration levels in the mutant, whereasthe adjacent peptide, peptide 6, which contains the β5'strand, part of the ${alpha}$ 5' helix, and the ${alpha}$ 5'-β5' loop showsmoderate increases in deuteration and exchange rate. Together,the changes in solvent accessibility in the RR domain indicatedthat the most significant structural changes caused by the mutationD56N occur within the linker and the ${alpha}$ 4'-β5'- ${alpha}$ 5' region.

Recovery of the c-di-GMP-specific phosphodiesterase activity of an inactive EAL domain. DGC2 is a cytoplasmic protein involved in the regulation ofcellulose biosynthesis in Acetobacter xylinus (37). A. xylinusDGC2 contains a PAS-like domain at the N terminus and the GGDEF-EALdidomain at the C terminus (Fig. 3). It was found that the GGDEFdomain of A. xylinus DGC2 is an active DGC domain capable ofsynthesizing c-di-GMP and that the EAL domain is catalyticallyinactive for hydrolyzing c-di-GMP (37). Examination of the sequenceof A. xylinus DGC2 suggested that the EAL domain contains theessential general base catalyst (Glu⁵²⁹) and the residues (Glu³⁵⁰,Asn⁴⁰⁹, Glu⁴⁴¹, and Asp⁴⁷²) for Mg²⁺ binding, and thus, is apotentially active PDE domain (28). Indeed, we found that A.xylinus DGC2 was capable of hydrolyzing several nonphysiologicalPDE substrates, such as thymidine-5-monophosphate-p-nitrophenylester (thymidine-pNPP) and bis-(p-nitrophenyl) phosphate (bis-pNPP)(Y. Qi, F. Rao, and Z.-X. Liang, submitted for publication).The stand-alone EAL domain of A. xylinus DGC2 (DGC2_306-574)was cloned and expressed to further determine whether the activityof the EAL domain is repressed by the PAS and GGDEF domains.We found that the stand-alone EAL domain was active toward thenonphysiological substrates described above, but still not c-di-GMP.

Although it contains all the catalytic residues for Mg²⁺ ionbinding and general base catalysis, the EAL domain of A. xylinusDGC2 contains a highly degenerate loop 6, consisting of N⁴⁷³FGKGITVL⁴⁸¹,in contrast to the DFG(T/A)GYSS loop in active EAL domains.The observed catalytic activity toward the synthetic substratesindicated that the lack of activity toward c-di-GMP is probablycaused by the binding of c-di-GMP in an unproductive configuration.To examine whether the loss of activity is due to the degenerationof loop 6, we partially "restored" the loop by mutating threeresidues in the stand-alone EAL domain. We found that the triplemutant (Asn⁴⁷³Lys⁴⁷⁶Ile⁴⁷⁸ $->$ Asp⁴⁷³Thr⁴⁷⁶Tyr⁴⁷⁸) of the EAL domainwas capable of hydrolyzing c-di-GMP (Fig. 6A). Steady-statekinetic characterization revealed that the triple mutant catalyzesthe hydrolysis of c-di-GMP with a k_cat of (5.9 ± 0.2)x 10^–4 s^–1 and K_m of 13.0 ± 1.2 µMunder the enzymatic assay conditions (Fig. 6B). The observedcatalytic activity toward nonphysiological substrates for thewild-type A. xylinus DGC2 and the recovered activity towardc-di-GMP for the EAL domain provided further support for theproposed roles of the catalytic residues (28). In addition,the observations also suggested that the degeneration of loop6 is at least partially responsible for the lack of activityagainst c-di-GMP for A. xylinus DGC2, and maybe some other EALdomain proteins as well.

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FIG. 6. Enzymatic activity assay for the EAL domain of A. xylinus DGC2. (A) HPLC analysis of the enzymatic activity of the full-length A. xylinus DGC2, stand-alone EAL domain, and the triple mutant with three mutations (Gln⁴⁷³Lys⁴⁷⁶Ile⁴⁷⁸ $->$ Asp⁴⁷³Thr⁴⁷⁶Tyr⁴⁷⁸) in the EAL domain. The enzymes were incubated with c-di-GMP and Mg²⁺ for 90 min. Abs (mAU), absorbance (milliabsorbance units). (B) Steady-state kinetics of the triple mutant of the stand-alone EAL domain. The curve was generated by fitting the data to the Michaelis-Menten equation.

DISCUSSION

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DISCUSSION

It is common to find flexible loops in the vicinity of the activesites of enzymes. The loops play important roles in substratebinding and positioning, as well as shielding the substratefrom the bulk solvent. The results of extensive structural andbiochemical studies suggested that a functional loop (loop 6)has been preserved during evolution in (β/ ${alpha}$ )₈ barrel foldenzymes (15, 34). Despite the diverse reactions catalyzed by(β/ ${alpha}$ )₈ barrel fold enzymes, flexible loop 6 plays variousfunctional roles assisting catalysis by undergoing significantstructural changes during substrate binding and catalysis. Theresults presented here seem to support an equally importantrole for loop 6 in the hydrolysis of c-di-GMP for the (β/ ${alpha}$ )₈barrel folded EAL domains.

The single mutations in the loop 6 region exerted profound impacton the structure and enzymatic activity of RocR. The mutationof the loop residue Phe²⁹⁷ and the loop-stabilizing Glu²⁶⁸ causedthe formation of HMWO and significantly changed both k_cat andK_m. The fact that the Glu₂₆₈ and Phe₂₉₇ mutations increasedthe propensity of RocR to form HMWO suggested that loop 6 playsa critical structural role in maintaining the quaternary structureof the protein. The change in oligomeric state is likely tobe a result of disruption of the dimer interface, as inferredfrom the observation that loop 6 is located at the dimer interfacein the crystal structure of TdEAL and EAL_YkuI. The observedantiparallel loop-loop interaction between the residues fromloop 6 may stabilize the dimeric structure (23). It is conceivablethat the mutation of Glu²⁶⁸ or the residues on the loop maydisrupt the loop-loop interaction and result in the dissociationof the dimer and the formation of HMWO. On the other hand, themutation of Asp²⁹⁶ and Ser³⁰², two residues of loop 6 in RocR,led to significant changes in catalytic parameters without alteringthe oligomeric structure. The S302A mutant exhibited strongsubstrate inhibition with an inhibition constant (K_i) of 10.9± 3.0 µM, while for the D296A mutant, K_m (8.6 ±2.8 µM) was greater and k_cat (0.02 s^–1) was smaller.The observed substrate inhibition and greater K_m indicated thatthe perturbation of the loop could lead to the alteration ofthe binding affinity for c-di-GMP. Similar results were obtainedwith the GGDEF-EAL didomain-containing PA2567. The mutationof Glu⁴⁶⁴, the equivalent of Glu²⁶⁸ in RocR, resulted in strongsubstrate inhibition, whereas the other two mutations seemedto affect protein folding, presumably due to the destabilizationof the dimer structure. The effects of the mutations in RocRand PA2567 support the view that loop 6 plays important structuraland catalytic roles in EAL domains.

The comparison of the H/D exchange pattern between the peptidesfrom RocR and the D56N mutant revealed intriguing structuralchanges in both the RR and EAL domains as an effect of the singlemutation. The most significant and intriguing changes in theEAL domain are in loop 6 and the end of β6 strand (Fig.5B and C). The enhanced H/D exchange reflects increased solventaccessibility in loop 6 region resulting from conformationalchange. The slightly higher deuteration for the dimerizationhelix ${alpha}$ 7 (peptide 19), along with the great increase in solventaccessibility in the linker region (peptide 7), probably reflectsa rearrangement of the dimer interface. Such an interface conformationchange could be coupled to the local conformational change inloop 6, since part of loop 6 is located at the interface aswell. The coupling of domain rearrangement and movement of Asp²⁹⁵has been suggested to be critical for controlling EAL domainactivity by comparing the structures of YkuI and TdEAL (23).Together with the change in K_m caused by the D56N mutation,the observed change in solvent accessibility seemed to suggestthat catalysis is sensitive to conformational changes in thesubstrate-binding pocket, especially in the vicinity of loop6. Moreover, the comparison of H/D exchange patterns also revealedsignificant changes in solvent accessibility in the linker andthe ${alpha}$ 4'-β5'- ${alpha}$ 5' region of the RR domain. Interestingly, structuraland biochemical studies have shown that the ${alpha}$ 4'-β5'- ${alpha}$ 5' regionundergoes conformational changes upon activation by phosphorylationor the binding of the phosphoryl mimic beryllium fluoride (BeF₃^–)in other RR domains (8, 12). The observed conformational changesin the ${alpha}$ 4'-β5'- ${alpha}$ 5' face raised the tantalizing possibilitythat the D56N mutant might bear some resemblance to the activatedform of RocR. However, this remains speculative before the comparisonbetween the mutant and phosphorylated RocR proteins in the future.Another underlying implication of these observations is thatthe control of catalysis through loop 6 might be used by EALdomains as a regulatory mechanism.

In contrast to RocR and PA2567, the EAL domain of A. xylinusDGC2 represents one of the EAL domains that contains all theessential residues for Mg²⁺ binding and general base catalysisbut has a highly degenerate loop 6. The observation that DGC2is active against nonphysiological PDE substrates indicatedthat the loss of activity toward c-di-GMP is most likely dueto alteration of substrate specificity. This idea is furthersupported by the recovery of activity for the triple mutantof EAL_DGC2 domain by partially "restoring" the degenerate loop.Although the catalytic rate for the triple mutant is low comparedto those of RocR and PA2567, the small K_m of the triple mutant(13.0 ± 1.2 µM) indicates that the triple mutanthas reasonable binding affinity for c-di-GMP. These observationsconfirmed the importance of loop 6 in catalysis and furthersuggested that the restoration of loop 6 enables the EAL domainto bind c-di-GMP in a productive configuration for hydrolysis.

The functional roles of loop 6 in EAL domains can be rationalizedin light of the structural data for TdEAL and the YkuI-substratecomplex. Although the catalytic activity has not been experimentallyvalidated, the TdEAL domain is most likely to be an active PDEdomain with a conserved loop 6 and catalytic residues. In contrast,the EAL domain of YkuI, which contains a degenerate loop 6 (NIGKESS),is catalytically inactive despite its ability to bind c-di-GMP(23). The comparison of the structures of the active (TdEAL)and inactive (YkuI) EAL domain structures revealed some intriguingdifferences for loop 6 (Fig. 7A). One of the major differencesis that the "anchor" residue Glu¹²⁵ (Glu²⁶⁸ in RocR) is no longertucked under loop 6 in YkuI. As a result, the loop adopts avery different conformation with the residues shifted away fromthe catalytic Mg²⁺ ion. The catalytically indispensable residueAsp¹⁵² (Asp²⁹⁵ of RocR) in YkuI is too far away to coordinatethe catalytic Mg²⁺ ion as suggested by Minasov and coworkers(23). In addition, the residue Asn¹⁵³ (Asp²⁹⁶ in RocR) thatis involved in the binding of c-di-GMP is now pulled away fromthe substrate. On the basis of these observations, we proposethat loop 6 is crucial not only for stabilizing the dimer interfacebut also for the binding of Mg²⁺ ions and c-di-GMP. The conformationalchange in loop 6 caused by mutation or regulatory signal willimpact catalysis in one of the following ways. First, the conformationalchange in the loop can affect the dimerization of the protein,which would result in a change of oligomeric structure and evenprotein stability. Second, binding of c-di-GMP can be affectedas a result of the alternation of the interaction between c-di-GMPand the loop. Both structural and biochemical data suggestedthat the loop may interact with c-di-GMP directly (or indirectlythrough a second Mg²⁺ ion [28]) through the conserved Asp (Asp²⁹⁶of RocR). Hence, mutations that affect the interactions betweenloop 6 and substrate or that impede the ability of loop 6 toundergo conformational change for effective substrate bindingwould affect catalysis. Third, change in the loop conformationcan severely hamper catalysis by dislocating the essential Mg²⁺ion-binding residue (Asp²⁹⁵ in RocR). The reduced binding affinityfor Mg²⁺ can have catastrophic effect on the catalytic activityas demonstrated by the detrimental effect of the D295N mutationin RocR (28). Given the sensitivity of the catalytic activityto the loop conformation and the position of the Mg²⁺-bindingresidue, we postulate that some EAL domains could be regulatedthrough controlling the conformation of loop 6.

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FIG. 7. Summary of EAL domains. (A) Comparison of loop 6 in active and inactive EAL domains. Loop 6 of TdEAL (Protein Data Bank accession no. 2r6o) and YkuI (Protein Data Bank accession no. 2w27) were highlighted in orange and cyan, respectively. The Mg²⁺ ion in the TdEAL structure is shown as a green ball, and c-di-GMP is shown as a stick. The corresponding residues of Asp²⁹⁵, Asp²⁹⁶, and Glu²⁶⁸ of RocR are highlighted and labeled (Asp⁶⁴⁶, Asp ⁶⁴⁷, and Glu⁶¹⁹ for TdEAL; Asp¹⁵², Asn¹⁵³, and Glu¹²⁵ for YkuI). (B) Comparison of the sequences of the loop among characterized EAL domains. The EAL domains shown are from the following proteins: PA2567, BifA, and FimX from Pseudomonas aeruginosa (indicated by the Pa suffix after the hyphen and protein) (16, 17, 31); TdEAL from Thiobacillus denitrificans (TdEAL-Td); VieA from Vibrio cholerae (VieA-Vc) (38); CC3396 from Crescentus caulobacter (CC3396-Cc) (9); YcgF, YahA, Dos, YciR, CsrD, and YegE from Escherichia coli (indicated by the Ec suffix after the hyphen and protein) (11, 32, 36, 40, 41); BphG from Rhodobacter sphaeroides (BphG-Rs) (39); PdeA1, DGC1, DGC2, and DGC3 from Gluconacetobacter xylinus (indicated by the Gx suffix after the hyphen and protein) (7, 37); HmsP from Yersinia pestis (Hmsp-Yp) (2); GcpC from Salmonella enterica (GcpC-Se) (10); STM1344 and STM3375 from Salmonella enterica serotype Typhimurium (indicated by the St suffix after the hyphen and protein)(33); and LapD from Pseudomonas fluorescens Pf0-1 (LapD-Pf) (24). The sequences were aligned using MultAlin (http://bioinfo.genopole-toulouse.prd.fr/multalin/multalin.html), and the figure was generated using ESPript 2.2 (http://espript.ibcp.fr/ESPript/ESPript/). (C) Pie chart summary of the classification of the 5,862 EAL domains from bacterial genomes according to the conservation of catalytic residues and loop 6.

Comparison of the sequences of EAL domains revealed that allthe characterized inactive EAL domains harbor a degenerate loop6 (Fig. 7B). Further sequence analysis of the 5,862 EAL domainsfound in bacterial genomes revealed that 4,809 of them containthe catalytic residues that include the general base catalystand four essential residues for Mg²⁺ coordination. Among the4,809 EAL domains, 2,895 of them contain a conserved loop 6[DFG(A/S/T)(G/A)(Y/F)(S/A/T)(S/A/G/V/T)] and 1,914 of them containa degenerate loop 6 (Fig. 7C) (see supplemental material). The2,895 EAL domains are likely to be catalytically active PDEdomains, whereas the functions of the 1,914 EAL domains witha degenerate loop 6 remain uncertain, as exemplified by theEAL domains of YkuI and A. xylinus DGC2. The EAL domains ofYkuI and A. xylinus DGC2 were found to be catalytically inactivetoward c-di-GMP by in vitro enzymatic assay (Qi et al., submitted).However, it remains to be seen whether the EAL domain can be"activated" by the putative regulatory domains in YkuI and A.xylinus DGC2. In addition to the 4,809 EAL domains, 1,053 EALdomains were found to lack one or more of the essential catalyticresidues (Fig. 7C). Among the 1,053 EAL domains, the majorityof them (990) do not contain a conserved loop 6. These 1,053EAL domains are most likely to be catalytically inactive. Thispostulation is supported by previously characterized inactiveEAL domains as well as two recently reported EAL domain proteins.The EAL domain of the protein LapD from Pseudomonas fluorescensPf0-1 contains a highly degenerate loop 6 (QRFGGRFSM) and lacksan essential residue for Mg²⁺ binding. It was proposed thatLapD functions as a c-di-GMP-binding receptor rather than aPDE domain (24). The E. coli protein YcgF contains an EAL domainthat was initially assumed to be a c-di-GMP-hydrolyzing domain.However, the EAL domain contains a Met residue at the positionof the general base catalyst and a highly degenerate loop 6(QVGRDLQI). Recent studies showed that the EAL domain does notexhibit PDE activity but participates in protein-protein interactioninstead (40). Given the strong correlation between the divergencsof loop 6 sequences and catalytic activity, we hope that theclassification of EAL domains described here can provide someassistance in elucidating the evolution and biological functionsof the versatile EAL domains.

ACKNOWLEDGMENTS

This work is supported by Singapore Biomedical Research Councilthrough a BMRC grant (06/1/22/19/464) and the Ministry of Educationof Singapore through a URC grant (RG151/06).

We thank Thomas Lee (University of Wisconsin, Madison) for hiskind assistance with the HPLC column packing for our H/D exchangeexperiment.

FOOTNOTES

* Corresponding author. Mailing address: School of Biological Sciences, Nanyang Technological University, 60 Nanyang Drive, Singapore 637551. Phone: 65 63167866. Fax: 65 67913856. E-mail: zxliang{at}ntu.edu.sg

Published ahead of print on 17 April 2009.

Supplemental material for this article may be found at http://jb.asm.org/.

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