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accessA structural study of the interaction between the Dr haemagglutinin DraE and derivatives of chloramphenicol
aSir William Dunn School of Pathology, University of Oxford, South Parks Road, Oxford OX1 3RE, England, and bDepartment of Chemistry, Chemistry Research Laboratory, 12 Mansfield Road, Oxford OX1 3TA, England
*Correspondence e-mail: susan.lea@path.ox.ac.uk
Dr adhesins are expressed on the surface of uropathogenic and diffusely adherent strains of Escherichia coli. The major adhesin subunit (DraE/AfaE) of these mediates attachment of the bacterium to the surface of the host cell and possibly intracellular invasion through its recognition of the complement regulator decay-accelerating factor (DAF) and/or members of the carcinoembryonic antigen (CEA) family. The adhesin subunit of the Dr haemagglutinin, a Dr-family member, additionally binds type IV collagen and is inhibited in all its receptor interactions by the antibiotic chloramphenicol (CLM). In this study, previous structural work is built upon by reporting the X-ray structures of DraE bound to two chloramphenicol derivatives: chloramphenicol succinate (CLS) and bromamphenicol (BRM). The CLS structure demonstrates that acylation of the 3-hydroxyl group of CLM with succinyl does not significantly perturb the mode of binding, while the BRM structure implies that the binding pocket is able to accommodate bulkier substituents on the N-acyl group. It is concluded that modifications of the 3-hydroxyl group would generate a potent Dr haemagglutinin inhibitor that would not cause the toxic side effects that are associated with the normal bacteriostatic activity of CLM.
Keywords: Dr adhesins; Dr haemagglutinin; DraE; chloramphenicol.
3D view: 2w5p,2jkn,2jkl,2jkj
PDB references: DraE–CLS, C2, 2w5p, r2w5psf; DraE–CLS, space group P3, 2jkn, r2jknsf; DraE–BRM, 2jkl, r2jklsf; DraE–THM, 2jkj, r2jkjsf
1. Introduction
Dr adhesins are thought to be important virulence factors for diffusely adherent (DAEC) and uropathogenic (UPEC) strains of Escherichia coli. Members of the Dr adhesin family include the Dr haemagglutinin, Dr-II, Afa-III and F1845 fimbriae (Servin, 2005![[Servin, A. L. (2005). Clin. Microbiol. Rev. 18, 264-292.]](../../../../../../logos/arrows/d_arr.gif "Servin, A. L. (2005). Clin. Microbiol. Rev. 18, 264-292.")
). Estimates as to the frequency of Dr-family members in DAEC isolates range from 50% to 75% (Giron et al., 1991). They are also the third most common group of colonization factors for UPEC behind type 1 and P pili (Nowicki et al., 2001), with 25–50% of cystitis isolates from children and 30% of pyelonephritis isolates in pregnant women expressing Dr adhesins (Labigne-Roussel & Falkow, 1988). In addition, infection with Dr adhesin-positive UPEC is associated with an increased risk of a recurrent urinary-tract infection (Foxman et al., 1995).
The Dr haemagglutinin, a member of the Dr adhesin family, can utilize up to four receptors to adhere to the host. The major adhesin subunit DraE recognizes decay-accelerating factor (DAF; Bernet-Camard et al., 1996) and members of the carcinoembryonic antigen (CEA) family (Guignot et al., 2000, 2009) and can trigger the bacterial mobilization of α5β1 integrin (Guignot et al., 2009). DraE also binds type IV collagen (Westerlund et al., 1989; Carnoy & Moseley, 1997). Together, these interactions are capable of orchestrating some of the host effects that are associated with the DAEC and UPEC pathotypes (reviewed by Servin, 2005).
The receptor interactions of DraE are inhibited by the antibiotic chloramphenicol (CLM). CLM inhibition of DraE was serendipitously discovered by Nowicki et al. (1988), who noticed that a CLM-contaminated reagent completely abolished DAF-mediated mannose-resistant haemagglutination (MRHA). CLM also inhibits the type IV collagen and CEA receptor interactions (Westerlund et al., 1989; Korotkova, Cota et al., 2006). In the years following the Nowicki group discovery, CLM was found to compare very effectively with other inhibitors of bacterial adhesion, its minimum (MIC) being 2 µM compared with equivalent MICs for type 1 and P pili (carbohydrate) receptor analogues of between 400 and 500 µM (Old, 1972; Svenson et al., 1983). More recently, however, novel classes of carbohydrate derivatives have been developed with affinities in the nanomolar range specifically for type 1 or P pili (Bouckaert et al., 2005; Ohlsson et al., 2005). The present work represents a first exploratory step towards CLM-based, less toxic and perhaps more specific inhibitors of DraE-mediated bacterial adhesion. For example, chloramphenicol succinate (CLS) inhibits DAF-mediated MRHA at similar levels to CLM (Nowicki et al., 1988), although the stability of CLS to hydrolysis has not been characterized and the molecule is likely to be quickly metabolized to CLM in vivo.
The Dr haemagglutinin is the only CLM-sensitive Dr adhesin-family member (Le Bouguenec et al., 1993). Our recently determined X-ray structure of the DraE–CLM complex has uncovered the molecular basis of the specificity of CLM for DraE (Pettigrew et al., 2004). Binding was observed to be dependent on a shallow hydrophobic depression on the surface of DraE defined by residues Pro40–Pro43 on strand B and Ile111, Gly113 and Tyr115 on strand E. The structure of AfaE-III (Anderson et al., 2004), a close relative of DraE with 98% sequence identity (three residue differences out of 140), demonstrates that the mutation of residue 88 from threonine (DraE) to methionine (AfaE-III) is sufficient to mask the binding pocket, thereby abolishing CLM sensitivity.
The conventional bacteriostatic activity of CLM arises from its ability to act as an inhibitor of the 50S prokaryotic ribosome (Moazed & Noller, 1987). In this context, the principal requirements for CLM activity are the 1,3-propanediol moiety and a para-substituted electron-withdrawing (nitro) group on the aromatic ring (Nagabhushan et al., 1991). The structure of CLM complexed with the 50S ribosome of Deinococcus radiodurans has demonstrated that CLM inhibits protein biosynthesis in prokaryotes by binding to the peptidyl transferase active site (Schlunzen et al., 2001). This interaction is particularly dependent on the burial of the nitrobenzene group and on hydrogen-bonding interactions between the primary hydroxyl group (3-OH) of CLM and In contrast, our X-ray structure of the complex between DraE and CLM demonstrates that this CLM interaction is somewhat different in character, being more dependent on the hydrophobic burial of the dichloromethyl group of CLM rather than the aromatic ring or the hydroxyl groups (Pettigrew et al., 2004). Since CLM is toxic in a small number of susceptible individuals, owing to its ability to traverse cell membranes and inhibit mitochondrial ribosomes (Kroon & Van den Bogert, 1983), we proposed that the DraE–CLM structure could provide a starting point for the design of an agent designed to inhibit Dr adhesion without the toxic side effects that are associated with the `normal' bacteriostatic activity of CLM.
In the present study, a number of CLM derivatives were designed, cocrystallized with DraE and examined using X-ray crystallography in order to unambiguously determine which functional groups are important for DraE binding. We present the structures of chloramphenicol succinate and bromamphenicol bound to DraE and use them to suggest possible modifications to the small molecule that could result in a safer inhibitor with a more wide-ranging action against other Dr adhesin-family members.
2. Materials and methods
2.1. Protein expression and purification
Recombinant DraE was expressed as an N-terminal hexahistidine fusion in Escherichia coli strain M15[pREP4] (Qiagen) and purified as described previously (Pettigrew et al., 2004). Briefly, DraE was purified from the supernatant using nickel-affinity followed by on an Superdex S75 Sepharose column (GE Life Sciences) to separate the trimeric form from small amounts of monomeric, dimeric and aggregated forms. The trimeric form was concentrated to 1.6 mg ml−1 and used in crystallization trials. Although the DraE trimer has previously been shown to be an artefact resulting from `domain swapping' of strand A1 (rather than strand G, as observed in native Dr fimbriae), the chloramphenicol-binding site is intact in this form of the protein (Pettigrew et al., 2004). This construct is amenable to crystallization in a number of different crystal forms, which makes it a convenient route to determining a number of CLM-derivative–DraE cocrystal structures.
2.2. Synthesis
The various CLM derivatives and their abbreviations are summarized in Fig. 1. Chloramphenicol succinate (CLS), chloramphenicol base (CLB) and thiamphenicol (THM) were obtained from commercial sources (Sigma–Aldrich, UK). All the other analogues were synthesized as described below.
![[Figure 1]](be5123fig1thm.gif) | Figure 1 Chloramphenicol derivatives studied. |
All reactions involving moisture-sensitive reagents were carried out in a nitrogen atmosphere using standard vacuum-line techniques and glassware that was flame-dried and cooled under nitrogen before use. The solvents were dried according to the procedure outlined by Grubbs and coworkers (Pangborn et al., 1996). Water was purified using an Elix UV-10 system. All other solvents were used as supplied (analytical or HPLC grade) without prior purification. was performed on aluminium plates coated with 60F254 silica. The plates were visualized using UV light (254 nm), iodine, 1% aqueous KMnO4 or 10% ethanolic phosphomolybdic acid. Melting points were recorded on a Gallenkamp Hot Stage apparatus and are uncorrected. Optical rotations were recorded on a PerkinElmer 241 polarimeter with a water-jacketed 10 cm cell. Specific rotations are reported in 10−1 deg cm2 g−1 and concentrations (c) in grams per 100 ml. NMR spectra were recorded on Bruker Avance spectrometers in the deuterated solvent stated. The field was locked by external referencing to the relevant deuteron resonance.
2.2.1. N-Propyl 2,2-dichloroacetamide (NPDA)
To a stirred solution of 1-aminopropane (0.70 ml, 8.5 mmol) in CH2Cl2 (30 ml) at 273 K was added a solution of dichloroacetyl chloride (0.81 ml, 8.5 mmol) in CH2Cl2 (20 ml) dropwise. The resulting solution was stirred at 273 K for 1 h and then at room temperature (RT) for 2 h. The solution was washed successively with saturated aqueous NaHCO3 (10 ml), saturated aqueous NaCl (10 ml), dried (MgSO4) and the solvent removed with a vacuum pump (in vacuo). The crude product was recrystallized from ethyl acetate/pentane to yield the title compound as a white crystalline solid (1.16 g, 80%): melting point (m.p.) 321–323 K [literature melting point (lit. m.p.) 322–323 K; Matsumura et al., 1976]; δH (400 MHz, methanol-d4) 0.96 (3H, t, J = 7.5 Hz, CH3), 1.53–1.62 (2H, m, CH2CH3), 3.22 (2H, t, J = 7.1 Hz, CONHCH2), 6.24 (1H, s, COCHCl2).
2.2.2. (1′R,2′R)-2,2-Dibromo-N-[1′,3′-dihydroxy-1′-(4′′-nitrophenyl)propan-2′-yl]acetamide (bromamphenicol/BRM)
To a stirred solution of dibromoacetic acid (0.21 ml, 2.3 mmol) in tetrahydrofuran (THF, 20 ml) under N2 at 273 K was added triethylamine (0.32 ml, 2.3 mmol) and then trimethylacetyl chloride (0.28 ml, 2.3 mmol) dropwise. The resulting suspension was stirred at 273 K for 1 h. The supernatant solution was decanted and added dropwise to a stirred solution of (1R,2R)-2-amino-1-(4′-nitrophenyl)propane-1,3-diol (490 mg, 2.3 mmol) at 273 K. The resulting solution was stirred at 273 K for 1 h and then RT for 2 h and was then quenched with saturated aqueous ammonium chloride (5 ml). The organic phase was separated and the aqueous phase was extracted with ethyl acetate (2 × 20 ml). The combined organic extracts were washed successively with saturated aqueous NaHCO3 (10 ml) and saturated aqueous NaCl (10 ml), dried (MgSO4) and the solvent was removed in vacuo. The crude product was purified by recrystallization from methanol/diethyl ether to give the title compound as a white crystalline solid (590 mg, 62%): m.p. 321–323 (lit. m.p. 325–326 K; Moersch, 1955); [α]D22 +22.4 (c 1.0, EtOH) {lit. [α]D25 +19.6 (c 1.0, EtOH) (Moersch, 1955)}; δH (400 MHz, methanol-d4) 3.62 [1H, dd, J = 10.8, 6.0 Hz, C(3′)H2A], 3.83 [1H, dd, J = 10.8, 7.4 Hz, C(3′)H2B], 4.12–4.16 [1H, m, C(2′)H], 5.19 [1H, d, J = 2.3 Hz, C(1′)H], 6.19 [1H, s, C(1)H], 7.67 [2H, d, J = 8.4 Hz, Ar(2′′)H and Ar(6′′)H], 8.20 [2H, d, J = 8.4 Hz, Ar(3′′)H and Ar(5′′)H].
2.2.3. (1′R,2′R)-N-[1′,3′-Dihydroxy-1′-(4′′-nitrophenyl)propan-2′-yl]isobutyramide (methamphenicol/MEM)
To a stirred solution of (1R,2R)-2-amino-1-(4′-nitrophenyl)propane-1,3-diol (500 mg, 2.4 mmol) in THF (20 ml) at 273 K was added triethylamine (0.33 ml, 2.4 mmol) and then a solution of isobutyryl chloride (0.25 ml, 2.4 mmol) in THF (20 ml) dropwise. The resulting solution was stirred at 273 K for 1 h and then RT for 2 h. The solvent was removed in vacuo and the residue was taken up in ethyl acetate (30 ml). The solution was washed successively with 10% aqueous HCl (10 ml), saturated aqueous NaHCO3 (10 ml), saturated aqueous NaCl (10 ml), dried (MgSO4) and the solvent was removed in vacuo. The crude product was recrystallized from ethyl acetate/pentane to yield the title compound as a white crystalline solid (450 mg, 68%): m.p. 301–303 K (lit. m.p. 304.5–306 K; Shirahata et al., 1972); [α]D22 −56.4 (c 1.1, EtOH) {lit. [α]D25 −61 (c 1.0, EtOH) (Shirahata et al., 1972)}; δH (400 MHz, methanol-d4) 0.89 (3H, d, J = 6.9 Hz, CHMe2), 1.01 (3H, d, J = 6.8 Hz, CHMe2), 2.39–2.48 (1H, m, CHMe2), 3.61 [1H, dd, J = 10.8, 5.9 Hz, C(3′)H2A], 3.81 [1H, dd, J = 10.8, 7.4 Hz, C(3′)H2B], 4.19–4.23 [1H, m, C(2′)H], 5.18 [1H, d, J = 2.6 Hz, C(1′)H], 7.66 [2H, d, J = 8.5 Hz, Ar(2′′)H and Ar(6′′)H], 8.21 [2H, d, J = 8.5 Hz, Ar(3′′)H and Ar(5′′)H].
2.3. Crystallization
Cocrystallization of a number of CLM-analogue–DraE complexes was attempted using a crystallization robot (Tecan, Zurich, Switzerland) to generate a large number of ammonium sulfate concentration versus small-molecule concentration grid screens at pH 7.0 (0.1 M Na HEPES).
DraE–CLS cocrystals in P3 were obtained in 2 M ammonium sulfate, 0.1–20 mM CLS and 0.1 M Na HEPES pH 7.0. One unique crystal crystallized in C2 in a drop containing 10 mM CLS but could not be reproduced. Owing to the low solubility of bromamphenicol (BRM) and thiamphenicol (THM), soaks of these small molecules into preformed CLS cocrystals were also attempted. CLS cocrystals were transferred to a mother-liquor solution without CLS and left for 15–20 min to reduce the occupancy of the small molecule in the binding site. Longer backsoaking, which, in principle, would have been needed to soak the ligand out (Collins et al., 2007), led to visible damage to the crystals and could not be afforded. The crystal was then placed in a mother-liquor solution saturated with either BRM or THM and soaked for a further 15 min.
2.4. Data collection and processing
X-ray diffraction data were collected in-house and on beamline ID-29 at the European Synchrotron Radiation Facility (ESRF). Crystals were cryoprotected in 25% ethylene glycol plus mother liquor or soaking solution before being mounted in a fibre loop and flash-frozen at 100 K. The data-reduction and are summarized in Table 1. Two crystal forms were obtained for successful CLM-derivative–DraE cocrystals: trigonal (P3) and monoclinic (C2). Within MOSFLM (Collaborative Computational Project, Number 4, 1994), initial autoindexing solutions based on two sets of five diffraction images (φ = 90° apart) were used to screen for successful small-molecule-bound derivatives. Crystals that initial indexing revealed as belonging to the orthorhombic polymorph deposited as PDB entry 1ut1 (space group P212121, unit-cell parameters a = 68.88, b = 108.51, c = 119.62 Å) were immediately discarded as packing interactions make the CLM-binding site inaccessible in this crystal form; these crystals must therefore form by favouring the subunit–subunit interaction over the subunit–ligand interaction and are useless for the present study. Prior to the start of the DraE–BRM data collection, an scan was taken to locate the bromine peak absorption wavelength (0.91947 Å). Data were collected at this wavelength to maximize the anomalous difference signal from the Br atoms of BRM. Data reduction was performed using SCALA (Evans, 2006). The Friedel pairs were kept separate for the BRM data set and were merged for the others.
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2.5. Structure solution and refinement
2.5.1. P3 data sets
of the CLM-derivative data sets in P3 (CLS, BRM and THM) were performed using the program autoBUSTER (Vonrhein et al., 2006). As the unit-cell parameters (a = b = 119.6, c = 57.8 Å) and symmetry were those of our previously determined of the DraE–CLM complex (space group P3; a = b = 119.0, c = 57.4 Å; PDB code 1usq ), this model, minus CLM, was used as a starting point for The binding site was excluded from the automatic addition of waters. The small-molecule conformation was then interpreted from an Fo − Fc map after all the other density had been explained. For each CLM derivative, the program CORINA (Sadowski et al., 1994) was used to generate a coordinate file with appropriate bond lengths and angles. The program XPLO2D (Kleywegt & Jones, 1997) was used to generate a TNT stereochemical restraints dictionary from the resulting coordinate file. Soft (NCS) restraints were then used in refining the atomic positions and temperature factors of the six NCS-related copies of the CLM derivative.
For the CLS–DraE data set in P3, an NCS-averaged 2Fo − Fc density map was produced after the CLS molecule had been built and refined in the absence of the succinate tail, since the succinate moiety was not visible in the initial difference map. The coordinates of the small molecule and the binding site (comprised of residues 37–45, 84–88 and 110–116) were used to define a 5 Å radius mask around the atoms using the program NCSMASK (Collaborative Computational Project 4, Number 4, 1994). The NCS operators and the mask were used as input for the program MAPROT (Collaborative Computational Project 4, Number 4, 1994) to produce the NCS-averaged 2Fo − Fc density map. Three conformers for the succinate tail, each at an occupancy of 0.3, were built. 15 cycles of manual (NCS-restrained) BUSTER-TNT with all six copies of CLS in place generated three energy-minimized succinate conformers.
For the BRM data set in P3, an anomalous difference map was calculated using the phases from the final refined model in the absence of small molecule. Inspection of this map unambiguously confirmed that the small-molecule density was a superposition of CLS and BRM. After the initial placement of CLS (minus the succinate tail) and BRM into the Fo − Fc map (each at 50% occupancy), an occupancy of the small molecules determined the relative composition of each binding site. The small-molecule parameters were allowed to refine independently of NCS restraints as each binding site had a different occupancy.
2.5.2. C2 data set
Initial phases for the CLS data in C2 were determined by searching with the DraE–CLM trimer in MOLREP, again with the CLM molecules omitted. 12 cycles of (monomer) rigid-body were run using BUSTER-TNT (Blanc et al., 2004) with no nonbonded restraints. Next, autoBUSTER was used to refine the model with soft NCS restraints and to add waters. After four rounds of rebuilding and using XtalView/Xfit and BUSTER-TNT, respectively, the Fo − Fc map was inspected to confirm the presence of CLS in the binding site.
3. Results
Previously, we reported the structure of DraE bound to CLM (Pettigrew et al., 2004). In this structure, CLM binding was observed to be focused on the chlorine `tail' rather than the nitrobenzene `head' of the molecule. The presence of CLM in the crystallization mother liquor results in a change of from the apo orthorhombic (P212121) crystal form to the `drug-bound' trigonal (P3) crystal forms. This is a consequence of the binding site being involved in a crystal contact in the orthorhombic crystal form (see §3.4 below for details of this crystal contact).
In the present work, a number of CLM analogues were tested in order to determine which functional groups of CLM are important for DraE interaction (Fig. 1). Cocrystals were very difficult to obtain for most of the small molecules owing to their extremely poor aqueous solubility, while soaks of the required CLM derivative into pre-formed CLM/CLS cocrystals were complicated by residual CLM/CLS in the binding site. Therefore, this route to was only attempted for small molecules with easily identifiable functional groups (such as the anomalous scatterers of BRM or the para-substituted methyl sulfone group of THM).
All the cocrystals described in this work belong to the P3 form (with the exception of a single irreproducible C2 DraE–CLS crystal that grew in 10 mM CLS); both C2 and P3 crystals contain DraE trimers, as did the apo P212121 crystals (and the related AfaE-III cubic and trigonal crystals). The physiological intersubunit interactions that give rise to the adhesin fibres in vivo are those described in the published NMR study of DraE (Anderson et al., 2004), while the crystals contain strand-swapped trimers (Pettigrew et al., 2004): as explained in the latter study, the trimers in these crystals arise from inter-subunit strand swapping and have no physiological relevance, but the nonphysiological intersubunit strand swapping does not affect the CLM ligand binding as it occurs at a site distal with respect to the site of fibre and trimer formation. This was proved by the NMR mapping upon CLM titration, which agreed with the CLM-binding site of the crystal structures and was conducted on the donor-strand exchanged DraE construct that does not give rise to trimers (Pettigrew et al., 2004). Also entirely crystal-related and therefore of no physiological relevance is the intertrimer that describes the packing of the trimers; for this reason, we do not describe the packing nor the in detail (suffice here to say that in both crystal forms the trimers are arranged in slabs laying in the ab planes and are stacked along the c direction, both the a and c unit-cell axes being of similar length in the two forms; see Table 1).
3.1. N-Propyldichloroacetamide and chloramphenicol base
The observed mode of CLM binding to DraE suggested that the interaction is focused on the burial of the chlorines. In order to investigate this in more detail, two CLM fragments consisting of the aliphatic `tail' (N-propyldichloroacetamide; NPDA) and the aromatic `head' (chloramphenicol base; CLB) groups were studied (Fig. 1). Unfortunately, NPDA abolished the crystallization of DraE at small-molecule concentrations greater than 0.1 mM and only the apo crystals were obtained for lower concentrations. This could imply that NPDA bound in the CLM-binding pocket. In this scenario, crystallization would be abolished by the inability of the small molecule to stabilize the appropriate crystal contacts in the trigonal crystal form. Alternatively, NPDA may have bound nonspecifically to the protein, thereby perturbing crystal contacts elsewhere. Crystallization mother liquors containing CLB at concentrations of up to 1 mM generated the apo orthorhombic crystal form. Since the concentration of CLB did not appear to influence the crystallization of the apo crystal form, we concluded that CLB did not interact specifically with the CLM-binding site or nonspecifically with a portion of DraE that was involved in a crystal contact. This hypothesis is supported by the observation that CLB is unable to inhibit the haemagglutination of erythrocytes (Nowicki et al., 1988).
3.2. Chloramphenicol succinate
In order to establish whether substitution at the primary hydroxyl of CLM influences the binding of the small molecule to DraE, the structure of a DraE–CLS complex was determined. CLS cocrystals in P3 were reproducibly obtained using small-molecule concentrations between 1 and 15 mM. In this crystal form, the unbiased Fo − Fc difference map showed CLM-like density in the region of the physiological binding site (Fig. 2a). The aliphatic `tail' and the nitro-benzene `head' group were traced within this electron density. Positional and temperature (B) factor confirmed that CLS was present in the binding site at full occupancy, with an average B factor of 32 Å2. No difference density was resolved for the succinate tail, implying that these atoms adopted a number of alternate conformers that were not resolved at 1.9 Å resolution. However, an NCS-averaged 2Fo − Fc map revealed weak density for three possible low-energy succinate conformers (Fig. 2b). With each conformer set to an occupancy of 30%, the B factors refined to an average value of 49 Å2 for the succinate atoms, compared with an average value of 40 Å2 for the rest of the small molecule.
![[Figure 2]](be5123fig2thm.gif) | Figure 2 The physiological ligand-binding site. (a, b, c) Maps and models for chloramphenicol succinate: the refined model of CLS is shown [with the succinate tail ini (b) and without it in (a)]. (a) Unbiased Fo − Fc map (data set DraE–CLS.2) contoured at 2.5σ showing the CLS density in the hydrophobic pocket (P3 crystal form). (b) The NCS-averaged 2Fo − Fc electron density in the binding pocket (P3 crystal form, averaged over all six copies of the density in the ASU) reveals three possible lowest energy conformers for the succinate tail. (c) Unbiased Fo − Fc map (blue mesh, data set DraE–CLS.1) contoured at 2.3σ, showing that in the C2 crystal form the aromatic head group and the succinate tail are disordered. (d) The same view as in (a) for the BRM derivative, with the unbiased Fo − Fc difference map (contoured at 2.2σ) shown as a blue mesh. (e) Anomalous difference map (purple mesh) for the BRM derivative calculated in the resolution range 25–1.9 Å using phases from the protein model only (contoured at 3.5σ). It clearly reveals the presence of two bromines in the CLM-binding site. The final refined BRM model (20% occupancy) is also shown. The final refined CLS model is not shown for reasons of clarity, but it adopts an identical conformation. Figures were rendered in PyMOL (DeLano, 2004 ). |
A unique CLS cocrystal in C2 was obtained at a small-molecule concentration of 10 mM and could not be reproduced. In this crystal form, the unbiased Fo − Fc map revealed density for the dichloroacetyl moiety of CLS in the physiological binding site (Fig. 2c). However, even after temperature-factor and occupancy with the dichloroacetyl group in place, density for the nitrobenzene head group was not visible in any of the NCS-related binding sites. Ordering of the whole ligand in the P3 forms is helped by crystal contacts from a neighbouring protein molecule (Gln47 and Leu49) to the ligand atoms C7 and C8 (in the phenyl ring) and one of the O atoms on the nitro moiety (the atom labelled O9B); this crystal contact is missing in the C2 form and the `head group' of CLS adopted a number of conformations that were not traceable. Overall, the CLS–DraE complex structures imply that (i) substitutions at the primary hydroxyl do not significantly affect the mode of CLM binding and (ii) the nitrobenzene group is not required to bind DraE.
3.3. Bromamphenicol and methamphenicol
To investigate the contribution of the aliphatic tail to the small-molecule interaction, attempts were made to cocrystallize DraE with methamphenicol (MEM; less hydrophobic than CLM) and BRM (more hydrophobic than CLM) (Fig. 1). MEM was tested at comparable concentrations to CLM (up to 1 mM). Despite this, only the apo crystal form was obtained. Therefore, the reduced size and hydrophobicity of the acetyl group of MEM relative to the dichloroacetyl group of CLM significantly reduced or abolished the DraE–small molecule interaction. BRM was nearly insoluble and even saturated BRM mother liquors were unable to produce anything other than the apo crystal form. At such negligible BRM concentrations it was impossible to reach any conclusions about the relative affinities of BRM and CLM for DraE.
BRM soaks into CLS cocrystals were performed and the anomalous signal of the bromines was exploited in order to unambiguously determine the location of the small molecule. The fluorescence scan showed a clear in the region of the K of bromine (data not shown). This confirmed that some BRM had been dissolved despite the low solubility of the molecule. The anomalous difference map revealed two peaks in the density at a position in the physiological binding site that was previously seen to be occupied by the chlorines of CLM/CLS (Fig. 2e). The f′′ value for chlorine is low at the wavelength used in the experiment (0.26 compared with 3.82 for bromine at 0.91947 Å). Hence, the anomalous difference peaks in the binding site must arise from the presence of the bromines of BRM. In addition, the unbiased Fo − Fc difference map showed CLM-like density in the same region (Fig. 2d). The entire BRM molecule was traced within this map. However, BRM did not refine at full occupancy, as strong negative residual peaks were observed in the region of the two bromines. After occupancy of BRM, strong positive residuals were observed for all the small-molecule atoms except for the bromines. Therefore, the binding pocket contained a superposition of CLS and BRM in identical orientations. Repeated rounds of alternating occupancy and positional refinements revealed that BRM and CLS were present at between 20–30% and 50–70% occupancy, respectively, in the six NCS-related copies of the binding site. This structure demonstrated that the binding pocket of DraE can accommodate larger chemical groups.
The anomalous difference map revealed two bromines at a secondary BRM-binding site which was defined by the interface between two copies of DraE. The small molecule bridged a crystal contact, but the area of contact between molecules is too small for it to be of significance (300 Å2; 3.8% of the monomer's surface); this second binding site was therefore assumed to be an artefact of crystal packing. Moreover, CLM inhibition has been mapped to the area of surface close to the main binding site (Pettigrew et al., 2004); henceforth, this site is referred to as the `nonphysiological' binding site. The 2Fo − Fc and unbiased Fo − Fc maps in this region showed electron density corresponding to the dibromoacetyl moiety of BRM (data not shown). Difference density for the 1,3-propanediol moiety was only resolved after of the dibromoacetyl group. Even after with the aliphatic `tail' in place, the aromatic `head' group could not be resolved in the 2Fo − Fc map or the Fo − Fc map. This implied that the aromatic group adopted a number of alternate conformers that could not be resolved at 1.9 Å resolution. The average temperature factor of the BRM fragment was 33 Å2, suggesting that the nonphysiological BRM-binding site was fully occupied. As an entire THM molecule was found in an identical orientation in the same nonphysiological binding site, the relevant protein–small molecule contacts are discussed below. Fig. 3 illustrates this second binding site and the orientation of the ligand in it.
![[Figure 3]](be5123fig3thm.gif) | Figure 3 The nonphysiological THM-binding site. (a) The 2Fo − Fc map contoured at 1.3σ (calculated after of the entire THM molecule) in the region of the nonphysiological binding site clearly shows the tetrahedral density of the sulfonyl group. (b) LIGPLOT (Wallace et al., 1995 ) representation of THM at the same site. The number of each residue involved is given, together with the chain designation of the DraE subunit it originates from (D or F). An identical THM-binding site is also observed between copies B and C. |
3.4. Thiamphenicol
Preparation of THM–DraE cocrystals was attempted in order to determine whether para substitutions of the nitro group affected the interaction with DraE. The aromatic `head' group of THM comprises a para-substituted methyl phenyl sulfone moiety (Fig. 1). Soaks of THM into CLS cocrystals were attempted based on the assumption that the tetrahedral methyl sulfone group of THM could be distinguished from the planar nitro group of CLS in the electron density.
Inspection of the unbiased Fo − Fc difference density in the region of the physiological binding pocket revealed a planar rather than a tetrahedral group at the para position of the benzene ring (data not shown). Indeed, CLS refined successfully at full occupancy and no residual peaks were observed in the difference map. Therefore, we concluded that THM was unable to enter the CLM-binding pocket of DraE in the P3 crystal form. Steric interference between the protein and the methylsulfonyl group of THM is the most likely reason for this.
As mentioned above, THM occupied the same nonphysiological binding site as BRM. 2Fo − Fc and Fo − Fc maps were calculated using phases from the protein, the CLS models in the physiological binding site and the dichloroacetyl group of THM in the nonphysiological binding site. The para-substituted tetrahedral moiety of THM was clearly observed in the nonphysiological binding site in both density maps. The entire THM molecule was traced within this difference density and no negative peaks were observed in the difference map after with 100% THM occupancy (Fig. 3). The average B factor (33 Å2) was comparable to the average nonprotein B factor (27 Å2). Therefore, the two nonphysiological binding sites in the ASU were fully occupied.
The principal contacts between THM and the protein are given in Fig. 3. The two THM molecules in the ASU adopt a similar conformation to CLM in the physiological binding site and are positioned at the interface between two subunit copies. In Fig. 3 this is illustrated by subunits D and F (in the crystal the same binding site exists between the subunits labelled B and C). This predominately electrostatic interaction is mediated by residues within the loop between the first and third strand on one subunit (labelled D in Fig. 3) and by residues within a loop between the sixth and ninth β-strand on the other (labelled F). In more detail, hydrogen bonds are formed between the carbonyl of THM and the main-chain amide of Val105, the primary hydroxyl group OH(3) of THM forms hydrogen bonds to the side-chain atoms of Asp104 on one subunit (chains F and C) and Thr36 on the other (chains D and B), and a hydrogen bond occurs between the main-chain carbonyl of Gly33 and the amide within the aliphatic tail of THM. Van der Waals contacts are also formed between atoms of the aliphatic tail and residues within both DraE subunits. Only minor van der Waals contacts are observed between the para-substituted methyl phenyl sulfone moiety and the protein.
4. Discussion
There is an urgent need for novel therapeutics to combat the emergence of antibiotic-resistant strains of pathogenic bacteria (Breithaupt, 1999). An attractive approach is the use of agents that interfere with the ability of the bacterium to adhere to the host. As adhesion is an absolute requirement for successful colonization, prevention of adhesion at an early stage should prevent infection. Furthermore, since anti-adhesive agents do not kill or inhibit bacterial growth, it is expected that strains which are resistant to these agents will emerge at a much lower rate than those which are resistant to antibiotics (Ofek et al., 2003). Studies on anti-adhesives for UPEC have focused on the use of carbohydrate-receptor analogues, which aim to competitively inhibit bacterial adhesion via the lectin domains of type 1 and P pili (reviewed by Sharon, 2006). As UPEC strains express more than one type of adhesin (Hacker, 1992), any therapeutic cocktail against UTIs must include an effective agent against Dr adhesins. One lead candidate is the antibiotic chloramphenicol (CLM), which abolishes the adhesion of the Dr haemagglutinin DraE to DAF, CEA and type IV collagen (Nowicki et al., 1988; Westerlund et al., 1989). All the derivatives of CLM studied here are expected to inhibit fimbrial adhesion in the same way as CLM does, given that they bind at the same site and that CLM binding at that site has previously been shown to disturb receptor adhesion (Pettigrew et al., 2004).
4.1. Substitution at the primary hydroxyl of CLM does not perturb binding
The CLS structure in P3 proves that substitutions at the primary hydroxyl 3-OH do not affect the mode of CLM binding to DraE. In contrast, the 3-hydroxyl group is essential for ribosome inhibition; both chloramphenicol phosphotransferase and chloramphenicol acetyltransferase abolish the bacteriostatic activity of CLM by (Mosher et al., 1995) and acetylation (Murray & Shaw, 1997), respectively, at this position. Therefore, we hoped that increased DraE specificity could be gained from substitution at the primary hydroxyl group; unfortunately, the CLS succinate in this study did not fit the surface with a single conformation and alternative substituents to the succinyl moiety will need exploring. In addition, the disordered nitrobenzene group in the DraE–CLS structure in C2 implies that the interaction with DraE is focused on the burial of the chlorines rather than the benzene ring. This raises the possibility that the nitrobenzene group is not required for DAF inhibition. Conversely, in the CLM–ribosome complexes the interaction is focused on the burial of the benzene ring and not the chlorines (Hansen et al., 2003; Schlunzen et al., 2001). DraE specificity could therefore be gained by modifying the aromatic ring or by dispensing with it altogether. However, although the nitrobenzene group is not required to bind to DraE, it may be important for inhibition. Therefore, functional studies are necessary to determine the precise requirements for drug inhibition with regard to the aromatic ring.
4.2. The CLM-binding pocket is able to accommodate bulkier substituents
The BRM structure demonstrates that the CLM-binding pocket of DraE is able to accommodate larger substituents on the N-acyl group. This raises the possibility that a more hydrophobic molecule could be used to displace the Met88 side chain from the binding pocket of AfaE-III, thereby providing a means of inhibiting Afa-III and the Dr haemagglutinin. In this respect, the structure of an AfaE-III–BRM complex would be highly informative. However, our attempts to resolve this have so far been unsuccessful.
4.3. Possible mechanisms of chloramphenicol inhibition
A major obstacle to the design of an effective Dr adhesin inhibitor is our lack of understanding of the mechanism of DAF inhibition. CLM binds to a region of DraE that is involved in binding to CEA (Korotkova, Cota et al., 2006) and possibly type IV collagen (Carnoy & Moseley, 1997), suggesting that CLM acts as a competitive inhibitor of both these receptor interactions. However, the attenuation of DAF binding is more puzzling. Mutagenesis (Van Loy et al., 2002), surface plasmon resonance (Korotkova, Le Trong et al., 2006) and NMR mapping (Anderson et al., 2004) studies have enabled the primary DAF-binding site to be identified as a negatively charged depression on a surface of DraE that is remote from the CLM-binding site (Fig. 4). Therefore, CLM must act as a noncompetitive inhibitor of DAF binding. This raises two possible mechanisms for DAF inhibition by CLM: either the small molecule disturbs the binding site indirectly and prevents rigid-body association or it prevents the conformational equilibrium of DraE from being pulled towards the DAF-bound state. The former possibility can be discounted, since CLM creates only local perturbations that do not involve residues implicated in DAF binding (Pettigrew et al., 2004). The latter possibility is supported by the observation that DAF induces structural perturbations throughout the entire AfaE-III–DSC molecule (Anderson et al., 2004). Therefore, CLM may lock DraE in its isolated solution state, thereby preventing it from undergoing the `induced-fit' modifications required for DAF interaction. The structure of DraE bound to DAF would potentially offer new insights into how CLM inhibits noncompetitively. This would greatly facilitate our search for a more potent and specific Dr adhesin inhibitor.
![[Figure 4]](be5123fig4thm.gif) | Figure 4 Receptor-binding sites on DraE. Solvent-accessible surface representation of a single DraE subunit, together with the location of CLM. Residues which have been reported to be important for DAF (red), collagen (blue and purple) and CLM (purple) binding are coloured (Van Loy et al., 2002 ; Carnoy & Moseley, 1997). Note: Asp52 has not been implicated in collagen binding. The asterisk marks the site of the secondary nonphysiological THM and BRM binding. |
Supporting information
3D view: 2w5p,2jkn,2jkl,2jkj
PDB references: DraE–CLS, C2, 2w5p, r2w5psf; DraE–CLS, space group P3, 2jkn, r2jknsf; DraE–BRM, 2jkl, r2jklsf; DraE–THM, 2jkj, r2jkjsf
Acknowledgements
Thanks to Dr Kim Watson for access to the Rigaku FRD X-ray generator at the University of Reading, the staff of the ESRF, beamlines ID14-3 and ID29, to Dr Ed Lowe and Professor E. Garman for assistance with in-house data collection in Oxford, and to Jenny Gibson and Marc Morgan for assistance with crystallization robots. Thanks also to Gerard Bricogne for access to beta versions of BUSTER-TNT and autoBUSTER programs. DP was funded by a Medical Research Council studentship and PR was funded by a Medical Research Council grant (G0400389) to SML.
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