Glycosyltransferase Domain of Penicillin-Binding Protein 2a from Streptococcus pneumoniae Is Membrane Associated

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Journal of Bacteriology, May 1999, p. 2773-2781, Vol. 181, No. 9
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Glycosyltransferase Domain of Penicillin-Binding Protein 2a from Streptococcus pneumoniae Is Membrane Associated

Anne Marie di Guilmi,¹ Nicolas Mouz,¹ Lydie Martin,¹ JoAnn Hoskins,² S. Richard Jaskunas,² Otto Dideberg,¹ and Thierry Vernet¹^,^*

Institut de Biologie Structurale Jean-Pierre Ebel (CEA/CNRS), 38027 Grenoble Cedex 1, France,¹ and Lilly Research Laboratories, Eli Lilly and Company, Indianapolis, Indiana 46285-04382²

Received 23 December 1998/Accepted 26 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Penicillin-binding proteins (PBPs) are bacterial cytoplasmic membrane proteins that catalyze the final steps of the peptidoglycansynthesis. Resistance to $beta$ -lactams in Streptococcus pneumoniaeis caused by low-affinity PBPs. S. pneumoniae PBP 2a belongs tothe class A high-molecular-mass PBPs having both glycosyltransferase(GT) and transpeptide (TP) activities. Structural and functionalstudies of both domains are required to unravel the mechanismsof resistance, a prerequisite for the development of novel antibiotics.The extracellular region of S. pneumoniae PBP 2a has been expressed(PBP 2a*) in Escherichia coli as a glutathione S-transferase fusionprotein. The acylation kinetic parameters of PBP 2a* for $beta$ -lactamswere determined by stopped-flow fluorometry. The acylation efficiencytoward benzylpenicillin was much lower than that toward cefotaxime,a result suggesting that PBP 2a participates in resistance tocefotaxime and other $beta$ -lactams, but not in resistance to benzylpenicillin.The TP domain was purified following limited proteolysis. PBP2a* required detergents for solubility and interacted with lipidvesicles, while the TP domain was water soluble. We propose thatPBP 2a* interacts with the cytoplasmic membrane in a region distinctfrom its transmembrane anchor region, which is located betweenLys 78 and Ser 156 of the GTdomain.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Penicillin-binding proteins (PBPs) are components of bacterial cytoplasmic membranes that catalyze the final steps of thepeptidoglycan synthesis. These steps require three types of enzymaticactivities: the glycosyltransferase (GT), which polymerizes theglycan strand by using the lipid II as the substrate; the transpeptidase(TP), which cross-links these strands via their peptide side chains;and the D-alanine carboxypeptidase, which is believed to playa regulatory role (7). Reactions catalyzed by PBPs occur eitheron the outer surface of the cytoplasmic membrane (GT) or furtheroutside (TP and D-alanine carboxypeptidase); the major fractionof the proteins is therefore localized in the periplasm. PBPscan be divided into two groups by molecular sizes and amino acidsequence comparison (7): low-molecular-weight (low-M_r) PBPsthat catalyze D-alanine carboxypeptidase and endopeptidase reactions,and high-molecular-weight (high-M_r) PBPs that carry GT and TPactivities. Class A high-M_r PBPs are bifunctional enzymes bearingboth GT and TP activities, while class B high-M_r PBPs have sofar only been associated with the TPactivity.

Penicillin and other $beta$ -lactam antibiotics are specific inhibitors of TP and D-alanine carboxypeptidase reactions because oftheir structural similarity to the natural substrates, the stempeptides (25). When $beta$ -lactams form a covalent complex with theactive serine of TP domain enzymatic cavity, this event preventsthe cross-linking of peptide chains of the peptidoglycan, leadingto celldeath.

Streptococcus pneumoniae, a major human pathogen of the upper respiratory tract possesses six PBPs, including three that areclass A (PBPs 1a, 1b, and 2a), two that are class B (PBP 2x andPBP 2b), and a low-M_r PBP, PBP 3 (10). Individual deletion ofeither of the genes pbp2x or pbp2b is lethal for S. pneumoniae(14). However, neither the pbp1a, pbp1b, nor pbp2a gene is requiredfor growth when deleted individually, but the presence of at leasta pbp1a or pbp2a gene is essential for cell viability (12).

The increased occurrence of S. pneumoniae strains resistant to $beta$ -lactam antibiotics has become a worldwide health problem.In penicillin-resistant strains of S. pneumoniae, high-M_r PBPshave a decreased affinity for the $beta$ -lactams, driving the requirementfor a higher antibiotic dosage. The low-affinity PBP variant genesconferring resistance have a mosaic structure, in which partsof genes are replaced by equivalent parts from other bacterialsources (4, 15, 17). PBP 2b and PBP 2x constitute the mostcommon resistance determinants and confer low-level resistanceto piperacillin and cefotaxime, respectively (9). A higherlevel of resistance to these agents (but not to benzylpenicillin)is conferred by an additional alteration of PBP 2a (11), whilethe highest levels of resistance require further modificationsof PBP 1a (2, 11, 19, 22).

S. pneumoniae PBP 2a is an attractive target for antibacterial chemotherapy. Indeed, PBP 2a plays an important role in cellviability and in acquisition of $beta$ -lactam resistance. Furthermore,PBP 2a, like all class A PBPs, is a major therapeutic target,because no antibiotic usable in human therapy so far has beenable to specifically inhibit GTactivity.

The aim of this study is to gain an in-depth understanding of the mechanism of PBPs' enzymatic activities through a combinationof high-resolution three-dimensional structure and functionaldata. Solubilization of the periplasmic region of S. pneumoniaePBP 2x (18, 21), E. coli PBPs 2 and 3 (1, 6), and Staphylococcusaureus PBP 2a (23) was obtained by recombinant expression ofthe transmembrane-deleted form of the proteins. All of these proteinsbelong to the class B high-M_r PBPs. To the contrary, the extracellularregion of class A high-M_r S. pneumoniae PBP 1a was apparentlynot monomeric in solution (unpublished data), and E. coli PBP1b remained associated with the bacterial membrane even in theabsence of the transmembrane anchor (20, 26). Furthermore,low-M_r E. coli PBPs 5 and 6 are also associated with the periplasmicside of the inner membrane via a C-terminal amphiphilic helix(5, 24).

We have expressed and characterized the periplasmic region of S. pneumoniae PBP 2a (PBP 2a*) deprived of its cytoplasmic domainand transmembrane anchor. Our main finding relates to the lipophilicproperty of the GT domain and its putative association with thebacterial cytoplasmicmembrane.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials. The thiolester substrate analogue S2d (N-benzoyl-D-alanylmercaptoacetic acid) (13) was obtained from L. Christiaens (Universitéde Liège, Liège, Belgium). 4,4'-Dithiopyridine, trypsin, thrombin,glutathione, penicillin G, cefotaxime, CHAPS {3-[(3-cholamidopropyl)dimethylammonio]-1-propane-sulfonate},deoxycholic acid (DOC), Triton X-100, and phenylmethylsulfonylfluoride (PMSF) were purchased from Sigma. IPTG (isopropyl- $beta$ -D-thiogalactopyranoside)was purchased from Promega; ampicillin, leupeptin, and aprotininwere obtained from Boehringer Mannheim. A stock solution of lipid1,2-dioleoyl-sn-glycero-3-phosphocholine (DOPC) from Sigma waskept in chloroform at $-$ 20°C under nitrogengas.

Expression plasmid and culture conditions. The S. pneumoniae R6 pbp2a sequence had been deposited previously in the EMBL and GenBank databases under the accession no.AJ002292 (11). Cloning of the PBP 2a* gene was describedin reference 12. Briefly, the periplasmic region of the PBP2a gene was PCR amplified by using a DNA genomic preparation ofthe S. pneumoniae R6 strain. The upstream primer introduced anATG start codon beginning at Lys 78. The PCR product was clonedinto pGEX-2T plasmid (Pharmacia) in frame with glutathione S-transferase(GST), leading to a construct namedpJAH144.

Protein expression was performed with E. coli DH5 $alpha$ [ $phi$ 80dlacZ $Delta$ M15 recA1 endA1 gyrA96 thi-1 hsdR17 (r_K m_K⁺) supE44 relA1 deoR $Delta$ (lacZYA-argF)U169]. Cultures were grown inLuria-Bertani medium (10 g of tryptone, 5 g of yeast extract,10 g of NaCl per liter) (Life Technologies) supplemented with100 µg of ampicillin per ml whennecessary.

Protein solubilization and purification. A culture (1.6 liters) of DH5 $alpha$ /pJAH144 cells in Luria-Bertani medium containing 100 µg of ampicillin per ml was grown at 37°Cuntil the optical density at 600 nm (OD₆₀₀) reached 1. The fusionprotein synthesis was induced with 0.5 mM IPTG, and the culturecontinued overnight at 22°C. All of the following steps were carriedout at 0 to 4°C. Cells were harvested by centrifugation at 11,300× g for 15 min and resuspended in 40 ml of a solution of 50 mMTris-HCl (pH 8.0)-200 mM KCl containing 1 mM PMSF, 1 µg of leupeptinper ml, and 1 µg of aprotinin per ml. The resulting suspensionwas disrupted by a 2-min sonication step. The cell lysate wasthen centrifuged at 31,000 × g for 20 min, and the supernatantwas discarded. The pellet was resuspended in 20 ml of 50 mM Tris-HCl(pH 8.0)-200 mM KCl-0.5% CHAPS. The suspension was submitted torotary shaking to allow a more efficient solubilization of theGST-PBP 2a* fusion protein. The supernatant containing the fusionprotein obtained from a 15-min centrifugation at 20,800 × g waskept. The solubilization procedure was repeated twice. The resultingsupernatant was pooled and was loaded onto a 5-ml glutathione-Sepharosecolumn (Pharmacia). The column was equilibrated and washed with50 mM Tris-HCl (pH 8.0)-200 mM KCl-0.5% CHAPS. The fusion proteinwas cleaved while bound to the column in the presence of 50 Uof thrombin for 1 h at room temperature. The thrombin activitywas then inhibited by 1 mMPMSF.

Gel filtration experiments were performed with a Superdex 200 HR 10/30 column (Pharmacia). The equilibration buffer was 50mM Tris-HCl (pH 8.0)-200 mM KCl with or without 0.5% CHAPS. Theflow rate was 0.5 ml/min. Fractions (0.5 ml) were collected, and50-µl aliquots were analyzed for [³H]benzylpenicillin binding and fluorography. One hundred twentyand 60 µg of PBP 2a* and TP domain, respectively, were loadedonto thecolumn.

The concentration of PBP 2a* in the presence of detergent was measured by the bicinchoninic acid (BCA) method (Pierce BCAkit) and by OD₂₈₀.

Protease digestion of PBP 2a*. Purified PBP 2a* in 50 mM Tris-HCl (pH 8.0)-200 mM KCl-0.5% CHAPS was incubated at various trypsin/PBP 2a* ratios of 1:20to 1:500 (wt/wt) for 30 min at 37°C. Following incubation, theproteolyzed samples were subjected to a sodium dodecyl sulfate(SDS)-12.5% polyacrylamide gel for electrophoresis. The TP domainwas prepared by trypsin digestion of PBP 2a* at a trypsin/PBP2a* ratio of 1:100 (wt/wt) for 30 min at 37°C. The protease activitywas inhibited by 1 mMPMSF.

Extensive proteolysis of PBP 2a* with thrombin was performed at a thrombin/PBP 2a* ratio of 1:1 (wt/wt) for 30 min at 37°C,before addition of 1 mMPMSF.

PAGE. Native discontinuous gel electrophoresis was performed on a vertical slab apparatus by using a 3% stacking gel and an 8% separatinggel starting from a stock acrylamide solution of 29% acrylamide-1%N,N'-methylenebisacrylamide. The separating gel contained 373mM Tris-HCl (pH 8.8) and 0.64% glycerol, while the stacking gelwas buffered by 127 mM Tris-HCl (pH 6.8). Polymerization was performedwith 0.1% N,N',N',N'-tetramethylenediamine and 0.036% ammoniumpersulfate. The electrode buffer was 25 mM Tris-HCl (pH 8.3)-192mM glycine. The loading sample buffer was composed of 62.5 mMTris-HCl (pH 6.8), 10% glycerol, 0.1% bromophenol blue. Charge-shiftelectrophoresis experiments were performed on such native gels.CHAPS detergent was exchanged in PBP 2a* and TP domain solutionsfor other detergents (0.5% Triton X-100 or 0.5% Triton X-100-0.25%DOC) by 10-fold dilution and concentration of the protein solutionsto their original volume with a Microcon-30 unit(Amicon).

Discontinuous SDS-polyacrylamide gel electrophoresis (PAGE) conditions were slightly modified from the native PAGE. The separatinggel concentration was 12.5%, and 0.1% SDS was included in bothstacking and separating gels. Denaturing agents (2% SDS, 0.65M $beta$ -mercaptoethanol) were added to the sample buffer, and 0.1%SDS was included in the electrodebuffer.

N-terminal protein sequencing. Sample proteins (2 to 10 µg) were boiled in SDS-PAGE loading buffer for 5 min at 100°C and then loaded onto an SDS-12.5% polyacrylamidegel. The proteins were transferred to a Problot membrane (AppliedBiosystems) and stained according to the supplier's instructions.The protein bands were cut from the membrane and sequenced byautomated Edman degradation on an Applied Biosystem gas-phasesequencer model 477A with on-line analysis of the phenyl thiohydantoinderivatives.

Determination of kinetic parameters. PBPs interact with $beta$ -lactam antibiotics according to the three-step scheme

k1 k2 k3

E+I → EI → EI* → E+P

k−1

where E is the PBP enzyme, I is the $beta$ -lactam antibiotic, EI is the Michaelis-Menten complex, EI* is the acyl-enzyme covalentcomplex, and P is the product of the reaction (degraded $beta$ -lactamantibiotic). K, the dissociation constant of the enzyme-substratecomplex, is equal to k₁/k₁.

The k₂/K parameter, accounting for the acylation step efficiency, was determined by monitoring the decrease in the intrinsicfluorescence of the protein in the presence of antibiotic at 37°Cby using spectrofluorometric measurements coupled with a BiologicSFM3 stopped-flow apparatus. The excitation wavelength specificfor tryptophan was 280 nm, and emission was measured in the 305-to 360-nm range. PBP 2a* at a concentration of 2 µM in 10 mM sodiumphosphate (pH 7.0)-200 mM KCl was incubated with concentrationsof $beta$ -lactam antibiotic ranging from 200 µM to 1mM.

The activity of the TP domain of PBP 2a* was measured in terms of its ability to hydrolyze the S2d molecule, a synthetic thiolesteranalogue of cell wall stem peptide, according to the method describedby Zhao et al. (27). The assays were performed at 37°C. Proteinconcentrations were determined with the BCA detection kit (Pierce)with bovine serum albumin (BSA) as astandard.

The titration of functional PBP and determination of k₃ were performed with [³H]benzylpenicillin (20 Ci/mmol, 1 mCi/ml; Amersham). PurifiedPBP 2a* (2 µM) in 50 mM Tris-HCl (pH 8.0)-200 mM KCl was incubatedat 37°C with different concentrations of [³H]benzylpenicillin for 15 min, at which time, the reaction wascompleted. The samples were then subjected to SDS-PAGE electrophoresis.[³H]benzylpenicillin bound to proteins was monitored by two differentprocedures. The gel was stained with Coomassie blue, destained,incubated with Amplify (Amersham), dried, and either exposed toa film for 16 h or cut around the protein bands. In the lattercase, the radioactivity of the gel slice was measured by usinga liquid scintillation analyzer (Packard model 2100TR) after beingmixed with 10 ml of LSC cocktail (Picofluor 15;Packard).

The deacylation reaction obeys the following equation: $-$ k₃t = ln [EI*]_t/[EI*]₀, where [EI*]₀ is the initial concentrationof acyl-enzyme and [EI*]_t is its concentration at time t. Determinationof k₃ was performed as follows. A 2 µM concentration of purifiedPBP was labelled with 1 µM [³H]benzylpenicillin during 15 min at 37°C. Cold benzylpenicillin(15 mM) was added, and the incubation was continued at 37°C. Sampleswere removed at various times and loaded onto an SDS gel, andthe amount of radioactivity was measured in the protein bandsas mentionedabove.

Lipid vesicle reconstitution. DOPC solution in chloroform was dried under argon, and the lipids were then redissolved to a final concentration of 15 mMin 50 mM Tris-HCl (pH 8.0)-200 mM KCl-10% CHAPS. The lipid suspensionwas subsequently sonicated. The purified PBP 2a* protein, TP domain,and PBP 2a* thrombin-digested product were reconstituted intophospholipid bilayer vesicles by removal of detergent by dialysis.PBP 2a* and TP domain concentrations were adjusted to 1 mg perml in 50 mM Tris-HCl (pH 8.0)-200 mM KCl-3% CHAPS. The PBP 2a*thrombin-digested product was used at 0.07 mg per ml in the samebuffer. DOPC (15 mM) was added to make molar protein/DOPC ratiosof 1:50 to 1:1,000. The mixtures (20 to 100 µl) were extensivelydialyzed against 50 mM Tris-HCl (pH 8.0)-200 mM KCl for at least24 h at 4°C. The proteoliposome formation was assayed by PAGEunder nativeconditions.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

PBP 2a sequence and topology. The open reading frame of the pbp2a gene encodes a 731-amino-acid protein which contains all of the features characteristicof class A high-M_r PBPs (Fig. 1A) (11). PBP 2a includes a cytoplasmicN-terminal region (Met 1 to Arg 51) and a hydrophobic 26-amino-acidregion (Tyr 52 to Ala 77), which likely functions as a membraneanchor (Fig. 2A). The periplasmic region is divided into two domains:the 25-kDa GT domain and the 50-kDa TP domain. Conserved motifsin the GT and TP domains are indicated in Fig. 1A (11).

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FIG. 1. (A) Alignment sequence of class A high-M_r PBPs S. pneumoniae PBP 1a, PBP 2a (11, 12), and E. coli PBP 1b. The conserved motifs in the GT domain are underlined and in boldface, and are numbered according to the system used in reference 8. The active-site conserved motifs in the TP domain are underlined. Arrowheads indicate the N-terminal positions of the PBP 1a TP domain (Ser 264) (3) and T1 and T2 tryptic products of PBP 2a (this work). The underlined residues in italics correspond to the permissive site found in E. coli PBP 1b delineating the GT and TP junction domains (16). Vertical bars indicate the C terminus of TP domains (reference 3 and this work). Stars indicate the first residue of the detergent-free soluble proteins (reference 26 and this work). (B) Schematic representation of the proteolytic fragments. The molecular mass of each fragment was measured by SDS-PAGE. The N-terminal sequence of the fragments was experimentally determined. The C terminus of T2 is derived from mass spectrometry measurements. The position of the active-site serine 410 is indicated (S*).

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FIG. 2. Schematic diagrams of S. pneumoniae PBP 2a. (A) Topology of the native PBP 2a protein. The solid and hatched boxes indicate the N-terminal cytoplasmic region and the membrane anchor, respectively. (B) Construction of the GST-PBP 2a* fusion protein. The active-site serine 410 is indicated in both figures. The peptide at the GST-PBP 2a* junction includes sequences specific for thrombin and factor Xa cleavage, as well as the polyhistidine tag. The N-terminal sequence of PBP 2a* is presented in boldface.

Expression and purification of PBP 2a*. The successful expression and characterization of the periplasmic region of S. pneumoniae PBP 2x and PBP 1a (3, 18) promptedus to produce a soluble form of the periplasmic domain of PBP2a as a GST fusion protein (Fig. 2B). Cleavage sites specificfor thrombin and factor Xa have been added between GST and theN terminus of PBP 2a*. A stretch of eight histidines was addedfollowing the thrombin cleavagesite.

GST-PBP 2a* is expressed in E. coli cells in large amounts as a major 90-kDa species (Fig. 3, lane 2). The fusion moleculepartitions into a minor soluble pool and a much larger insolublefraction (Fig. 3, lanes 3 and 4). Attempts at purifying activePBP 2a* from the soluble fraction were unsuccessful due to thesensitivity of the protein to proteolytic degradation during thepurification procedure. Solubilization of the insoluble fractionfrom the cell debris with urea followed by in vitro refoldingled to a heterogeneous nonfunctional GST-PBP 2a*. Solubilizationof the insoluble fraction with a series of detergents, includingTriton X-100, $beta$ -octylglucoside, and CHAPS was efficient, providedthat the E. coli cultures were grown at 22°C (Fig. 3, lane 4).A concentration of 0.5% CHAPS was selected for the rest of thiswork for its high critical micellar concentration (0.25%), allowingeasy detergent removal or exchange. GST-PBP 2a* solubilized withCHAPS was purified by affinity chromatography and cleaved withthrombin directly on the glutathione column. The eluted fractionincluded a dominant species with an apparent molecular mass of71 kDa, which is in good agreement with the calculated value ofPBP 2a* (71.8 kDa), and a 63-kDa minor species (Fig. 3, lane 5).Both molecules were functional with respect to [³H]benzylpenicillin binding (Fig. 4B, lane 2). The N-terminal sequencesof the dominant and minor PBP 2a* forms were determined by Edmandegradation to be Lys-Ser-Thr-Asn and Ser-Gly-Gly-Gly-Ser-Thr,respectively (Fig. 1B). Therefore, thrombin proteolysis occurredefficiently downstream of the expected site, at the junction betweenfactor Xa cleavage sequence and the N-terminal portion of PBP2a* (Fig. 1B and 2B). The secondary minor cleavage between Arg155 and Ser 156 is reminiscent of a similar site within the PBP1a* sequence (3). After a single chromatography step, the purificationyield was around 2 to 3 mg/liter of E. coli culture, with theminor cleavage product acting as the sole source of heterogeneityin the preparation.

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FIG. 3. Analysis of solubilization and purification of PBP 2a*. Proteins were separated by SDS-12.5% PAGE and stained with Coomassie blue. The numbers to the left indicate the sizes of standard molecular mass markers. Lanes: 1, molecular mass markers; 2, total cell proteins; 3, soluble supernatant; 4, 0.5% CHAPS soluble extract; 5, PBP 2a* eluted from glutathione Sepharose after thrombin cleavage.

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FIG. 4. Trypsin cleavage of PBP 2a* leading to TP domain isolation. (A) Proteins were separated by SDS-12.5% PAGE and stained with Coomassie blue. The N-terminal sequence of each product is indicated on the right. (B) Fluorogram of a dried gel from SDS-12.5% PAGE of proteins (2 µg) labelled with [³H]benzylpenicillin prior to the migration. Digestions were performed at 37°C for 30 min. Lanes: 1, molecular mass markers; 2, undigested PBP 2a*; 3, trypsin/PBP 2a* ratio of 1:500 (wt/wt); 4, trypsin/PBP 2a* ratio of 1:100 (wt/wt); 5, trypsin/PBP 2a* ratio of 1:50 (wt/wt); 6, trypsin/PBP 2a* ratio of 1:20 (wt/wt).

Determination of PBP 2a* kinetic parameters. Quantitative binding of [³H]benzylpenicillin was performed to titrate the active site in PBP 2a*. The protein concentrationswere identical, whether determined by active-site titration orby the BCA method (data not shown), showing that all proteinswere functional in the preparation. The kinetic properties ofPBP 2a* were then determined by using the cephalosporin and penicillinclasses of antibiotics and the S2d substrate analogue (Table 1).A second-order rate constant of acylation (k₂/K) of 7,700 ± 600M¹ s¹ was measured with cefotaxime. The very small fluorescent quenchof PBP 2a* with benzylpencillin during the 5 s of the experimentimpaired accurate determination of k₂/K. This shows that benzylpenicillinacylates PBP 2a* with a very low efficiency. This observationis not contradictory with the complete labeling of PBP 2a* by[³H]benzylpenicillin in fluorography experiments when a much longerincubation time (15 min) was used. The efficiency of hydrolysisof S2d thiolester by PBP 2a* is close to values reported for PBP1a and the PBP 2x of the resistant clinical strain of S. pneumoniae328, (R-PBP 2x*) (Table 1). The k₃ deacylation rate of PBP 2a*for benzylpenicillin is in the same range as those reported forother PBPs (Table 1).

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TABLE 1. Kinetic parameters of S. pneumoniae PBP 2a^*

Limited trypsin proteolysis of PBP 2a* releases the TP domain. Proteolysis of purified PBP 2a* with a trypsin/protein ratio ranging from 1:100 to 1:20 (wt/wt) results in the productionof two major protein fragments, T1 and T2, with molecular massesof 43 and 39.5 kDa, respectively (Fig. 4A). Both fragments arecompetent for [³H]benzylpenicillin binding (Fig. 4B), showing that they encompassthe TP domain. N-terminal sequencing revealed that the T1 fragmentstarts at position Asp 264, whereas the T2 fragment begins atIle 301 (Fig. 1 and 4), leading to calculated molecular massesfor T1 and T2 of 51,301 and 47,176 kDa, respectively. The calculatedmass value and amino acid sequence analysis indicate that trypsincleavage also occurred at the C terminus of PBP 2a*, probablyafter Arg 678 for both the T1 and T2 fragments. This cleavagesite location has been confirmed by mass spectrometry analysisof fragment T2 (41,236 ± 1.5 Da) (Fig. 1). Conditions limitingthe production of the T2 fragment (trypsin/protein ratio of 1:100[wt/wt]) were used for the remainder of thisstudy.

The lipophilic character of PBP 2a* is due to its GT domain. The requirement for detergent to recover and purify PBP 2a* from bacterial extracts shows that the molecule or a region ofthe molecule displays a hydrophobic character. Since the lipidII substrate for the GT activity is membrane bound, this raisesthe possibility that PBP 2a* is still membrane associated. Totest the lipophilic character of functional domains of PBP 2a*,we have relied upon three independent biochemical approaches usingfull-length PBP 2a* and the TP domain obtained by limitedproteolysis.

PBP 2a* and TP domain were prepared in the presence of 0.5% CHAPS and analyzed by gel filtration in either the presence orabsence of the detergent. Protein fractions from each eluted peakwere characterized with respect to their ability to bind to [³H]benzylpenicillin (Fig. 5). In the presence of CHAPS, PBP 2a*elutes as a protein with an apparent molecular mass of 116 kDa(Fig. 5A). This value is larger than the monomeric 72-kDa PBP2a*, probably due to the formation of a complex with the detergentmicelles. In the absence of CHAPS in the column equilibrationbuffer, PBP 2a* is excluded from the gel matrix (Fig. 5B). Therefore,PBP 2a* requires a detergent to remain soluble. The solubilityof the TP domain is independent of the presence of the detergent(compare Fig. 5C and D). Under both conditions, TP protein peakscorrespond to a 45- to 48-kDa species compatible with the 43-kDameasured mass for the T1 fragment (Fig. 4). Comparable profileswere obtained when the TP domain was extensively dialyzed to removeCHAPS prior to gel filtration analysis (data not shown). Peptidefragments lacking penicillin binding activity and eluting as aseries of slowly migrating peaks (range, 3,600 to 7,600 Da), likelyoriginate from the trypsin cleavage of the GT domain (Fig. 5Cand D). Overall, these results indicate that the solubility ofTP domain is detergent independent, while PBP 2a* requires CHAPSfor its solubility.

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FIG. 5. Gel filtration of PBP 2a* and the TP domain in the presence or absence of 0.5% CHAPS. Chromatography conditions were described in Materials and Methods. Each peak aliquot was assayed for [³H]benzylpenicillin binding (dotted line). (A and B) PBP 2a*. (C and D) TP domain.

The detergent-binding property of PBP 2a* and the TP domain was assayed by using a modified version of the charge-shift electrophoresistechnique described in reference 26. The migration of proteinsthat bind detergents is altered upon variation of the ionic compositionof the detergents, whereas the electrophoretic mobility of solubleproteins is not altered by the presence of detergent. The zwitterionicdetergent CHAPS present in the preparation of PBP 2a* and theTP domain was exchanged against Triton X-100 (a nonionic detergent)or a mixture of Triton X-100 and DOC (an anionic detergent) priorto analysis on a native polyacrylamide gel. The migration of PBP2a* is extensively shifted in the presence of Triton X-100-DOCcompared to the migration in the presence of Triton X-100 or CHAPS(compare lanes 1 to 3 in Fig. 6). Under identical experimentalconditions, the migration of the TP domain remains unchanged,for the major species (compare Fig. 6, lanes 4 and 5), a behavioralso found for the soluble protein, BSA, used as a control (Fig.6, lanes 6 and 7). This experiment shows that the GT domain isrequired for the binding of detergents to PBP 2a*.

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FIG. 6. Charge-shift migration on native polyacrylamide gel. Proteins (5 µg) in the presence of 0.5% Triton X-100 or in a mixture of 0.5% Triton X-100-0.25% DOC were separated by native 8% PAGE and stained with Coomassie blue. Lanes: 1 to 3, PBP 2a* in 0.5% CHAPS, 0.5% Triton X-100, and 0.5% Triton X-100-0.25% DOC, respectively; 4, TP domain (star) in 0.5% Triton X-100; 5, TP domain in 0.5% Triton X-100-0.25% DOC; 6, BSA in 0.5% Triton X-100; 7, BSA in 0.5% Triton X-100-0.25% DOC.

The requirement for detergent during solubilization of PBP 2a* implies that the molecule is membrane associated in S. pneumoniae.To further test the lipophilic character of PBP 2a*, we have comparedthe abilities of PBP 2a* and the TP domain to incorporate intolipid vesicles. The phospholipid DOPC was added at various protein/lipidmolar ratios, and the mixtures were extensively dialyzed to removethe detergent. The efficiency of liposome formation under theseexperimental conditions was verified by electron microscopy (datanot shown). PBP 2a* within reconstituted liposomes exhibited amodification of electrophoretic migration in a native gel whichwas correlated with the PBP 2a*/lipid molar ratios (Fig. 7A, lanes3 to 5). As the relative lipid concentration increased, the migrationof PBP 2a* became considerably and progressively retarded. Themore slowly migrating species was absent when the dialysis wasconducted in the absence of lipids (Fig. 7A, compare lane 2 withlanes 3 to 5); under these experimental conditions, PBP 2a* wasnot aggregated as it entered the gel (Fig. 7A, lane 2). This controlshows that retarded migration does not originate from aggregationof PBP 2a* following removal of the detergent, but correspondsto a specific association of PBP 2a* with DOPC. Contrary to PBP2a*, the electrophoretic behavior of the TP domain was not affectedby the presence of lipid (Fig. 7A, lanes 6 to 10). This observationconfirms the lipophilic character of the GT domain within PBP2a*. The GT domain of PBP 2a* reconstituted in lipid vesicleswas still sensitive to trypsin digestion (data not shown). Thisshows that the GT domain is not embedded in the vesicle bilayerbut interacts with the lipids via a small region.

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FIG. 7. Reconstitution of proteins in lipid vesicles. Proteins were reconstituted into lipid vesicles as described in Materials and Methods. The vesicles were analyzed by native 8% PAGE. (A) PBP 2a* and the TP domain. Proteins (10 µg) were stained with Coomassie blue. Lanes: 1, PBP 2a* in 3% CHAPS; 2 to 5, PBP 2a* in the presence of molar protein/lipid ratios of 0, 1/50, 1/200, and 1/500, respectively; 6, TP in 3% CHAPS; 7 to 10, TP in the presence of molar protein/lipid ratios of 0, 1/50, 1/200, and 1/500, respectively. (B) PBP 2a* thrombin-digested product. Protein detection (0.7 µg) was performed by [³H]benzylpenicillin labelling. Lanes: 1, thrombin-digested PBP 2a* in 3% CHAPS; 2 to 5, thrombin-digested PBP 2a* in the presence of molar protein/lipid ratios of 0, 1/200, 1/500, and 1/1,000, respectively.

Extensive thrombin digestion of PBP 2a* (protease/PBP 2a* ratio of 1:1 [wt/wt]) releases a major 63-kDa species starting atSer 156 according to N-terminal sequencing (Fig. 3, lane 5). Thisshorter form of PBP 2a* offered us the opportunity to delineatemore accurately the lipophilic region of PBP 2a*. The abilityof the 63-kDa species to bind lipids was monitored by native gelelectrophoresis. The functional protein was revealed by [³H]benzylpenicillin labelling (Fig. 7B). The migration of the 63-kDaspecies was unchanged whether the protein was preincubated withlipids (Fig. 7B, lanes 3 to 5) or not (Fig. 7B, lanes 1 and 2).Thus the membrane association site in PBP 2a* is likely to residebetween residues Lys 78 (start of the putative periplasmic region)and Ser 156, for a span of 78 amino acids (Fig. 1).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Recent genetic studies have suggested that S. pneumoniae PBP 2a is important in cell viability (12). Moreover, the enzymeplays a role as a cefotaxime resistance determinant (11). Eventhough this dual character identifies PBP 2a as a potential targetfor antibiotherapy, the molecule has not yet been studied froma biochemical and structural point of view. Therefore, we haveexpressed in E. coli cells, purified, and characterized the recombinantperiplasmic region of PBP 2a (PBP 2a*), which encompasses theGT and TPdomains.

The hydrolytic activity of PBP 2a* with the S2d thiolester is comparable to that of PBP 1a* (3) and PBP 2x from S. pneumoniaeclinical isolate 328 (R-PBP 2x*), but is about 20-fold lower thanthe activity of the R6 S. pneumoniae strain (S-PBP 2x*) (18).This pattern of activity correlates well with the acylation efficienciestoward cefotaxime. Extensive incubation of PBP 2a* with [³H]benzylpenicillin leads to complete acylation of the protein.However, binding of benzylpenicillin to PBP 2a* was so inefficient,that we were unable to measure its acylation rate by stopped-flowfluorometry accurately. This behavior is reminiscent of that ofR-PBP 2x* (18). Therefore, it is unlikely that PBP 2a participatesin benzylpenicillin resistance. This is further supported by theobservation that the PBP 2a sequences from penicillin-resistantclinical isolate 328 and susceptible strain R6 are identical (12).The involvement of PBP 2a in resistance to other $beta$ -lactams cannotbe excluded, since the molecule was found to be a resistance determinantfollowing selection with cefotaxime, a cephalosporin $beta$ -lactam(11).

The functional TP domain, which is the target for $beta$ -lactams, was delineated by limited proteolysis. This led to the identificationof the PBP 2a* interdomain hinge region (linking the GT and TPdomains), which is located in a region similar to that of S. pneumoniaePBP 1a* (3) (Fig. 1A). Insertion mutations in E. coli PBP 1b(16) were used to propose a boundary between the GT and TP domains,located 20 amino acids downstream from the N-terminal TP domainsof S. pneumoniae PBP 1a and 2a (Fig. 1A). These results, obtainedby different experimental approaches, strengthened the proposedGT/TP domain boundary localization in these three class A PBPs.In a recent review discussing the domain structure of PBPs (8),Goffin and Ghuysen localized the intermodule junction in motif6 (Fig. 1A) by analogy with the S. pneumoniae PBP 2x structure(21). As shown in Fig. 1A, the N termini of the PBP 1a and PBP2a TP domains, defined by trypsin digestion, are located betweenmotifs 5 and6.

The initial attempts to produce PBP 2a* in E. coli at 37°C led to a highly aggregated protein, which could not be recoveredas a functional protein after solubilization with urea followedby in vitro refolding. Reduction of the temperature of the E.coli culture and solubilization of the PBP 2a* fusion with nondenaturingdetergents allowed the recovery of a protein with TP activity.Treatment of insoluble PBP 2a* with a high salt concentrationfailed to solubilize the protein, an indication that hydrophobicinteractions prevail over electrostatic interactions in PBP 2a*insolubility. Using three independent methods, we have mappedthe region of association with detergents and DOPC lipid to theGT domain of PBP 2a*. We have localized the hydrophobic regionin the 78 N-terminal residues of the GT domain, between Lys 78and Ser 156. Remarkably, this finding is similar to that of classA PBP 1b from E. coli (20). Wang et al. (26) have locatedin E. coli PBP 1b a second membrane association site, distinctfrom the transmembrane stretch, within the first 163 amino acidsof the GT domain, from position 88 (the start of the putativeperiplasmic domain) to position 251 (Fig. 1A). Gel filtrationrevealed that recombinant class A S. pneumoniae PBP 1a* formssmall aggregates. This property is also linked to the GT domain,since the TP domain isolated by trypsin digestion remains monomeric(unpublished data). We have also reported that the presence ofmoenomycin, an amphiphilic GT-specific inhibitor, increased PBP1a* solubility (3).

Taken together, these observations underline the general lipophilic properties of the GT domain of class A PBPs. Computationalanalyses of the GT sequence did not predict hydrophobic stretchesor amphiphilic helices, which could account for the membrane associationof the domain. This putative membrane association of class A PBPsGT domain is, however, consistent with the transmembrane locationof its lipid IIsubstrate.

	ACKNOWLEDGMENTS

This work was supported by the Infectious Diseases Division, Lilly ResearchLaboratories.

We thank C. Vénien-Bryan for electron microscopy, J.-P. Andrieu for N-terminal sequence determination, and Y. Pétillot formass spectroscopyanalysis.

	FOOTNOTES

^* Corresponding author. Mailing address: Institut de Biologie Structurale Jean-Pierre Ebel, Laboratoire d'Ingénierie des Macromolécules,41 Avenue des Martyrs, 38027 Grenoble Cedex 1, France. Phone:33-04 76 88 96 81. Fax: 33-04 76 88 54 94. E-mail: vernet{at}ibs.fr.

This is publication no. 630 of the Institut de Biologie Structurale Jean-PierreEbel.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Adachi, H., T. Ohta, and H. Matsuzawa. 1987. A water-soluble form of penicillin-binding protein 2 of Escherichia coli constructed by site-directed mutagenesis. FEBS Lett. 226:150-154[Medline].

2. Coffey, T. J., M. Daniels, L. K. McDougal, C. G. Dowson, F. C. Tenover, and B. G. Spratt. 1995. Genetic analysis of clinical isolates of Streptococcus pneumoniae with high-level resistance to expanded-spectrum cephalosporins. Antimicrob. Agents Chemother. 39:1306-1313[Abstract].

3. Di Guilmi, A. M., N. Mouz, J.-P. Andrieu, J. Hoskins, S. R. Jaskunas, J. Gagnon, O. Dideberg, and T. Vernet. 1998. Identification, purification, and characterization of transpeptidase and glycosyltransferase domains of Streptococcus pneumoniae penicillin-binding protein 1a. J. Bacteriol. 180:5652-5659[Abstract/Free Full Text].

4. Dowson, C. G., A. Hutchison, and B. G. Spratt. 1989. Extensive re-modelling of the transpeptidase domain of penicillin-binding protein 2B of a penicillin-resistant South African isolate of Streptococcus pneumoniae. Mol. Microbiol. 3:95-102[Medline].

5. Ferreira, L. C., U. Schwarz, W. Keck, P. Charlier, O. Dideberg, and J. M. Ghuysen. 1988. Properties and crystallization of a genetically engineered, water-soluble derivative of penicillin-binding protein 5 of Escherichia coli K12. Eur. J. Biochem. 171:11-16[Medline].

6. Fraipont, C., M. Adam, M. Nguyen-Disteche, W. Keck, J. Van Beeumen, J. A. Ayala, B. Granier, H. Hara, and J. M. Ghuysen. 1994. Engineering and overexpression of periplasmic forms of the penicillin-binding protein 3 of Escherichia coli. Biochem. J. 298:189-195.

7. Ghuysen, J. M. 1994. Molecular structures of penicillin-binding proteins and beta-lactamases. Trends Microbiol. 2:372-380[Medline].

8. Goffin, C., and J.-M. Ghuysen. 1998. Multimodular penicillin-binding proteins: an enigmatic family of orthologs and paralogs. Microbiol. Mol. Biol. Rev. 62:1079-1093[Abstract/Free Full Text].

9. Grebe, T., and R. Hakenbeck. 1996. Penicillin-binding proteins 2b and 2x of Streptococcus pneumoniae are primary resistance determinants for different classes of $beta$ -lactam antibiotics. Antimicrob. Agents Chemother. 40:829-834[Abstract].

10. Hakenbeck, R., T. Briese, H. Ellerbrok, G. Laible, C. Martin, C. Metelmann, H.-M. Schier, and S. Tornette. 1988. Targets of $beta$ -lactams in Streptococcus pneumoniae, p. 390-399. In P. Actor, L. Daneo-Moore, M. L. Higgins, M. R. J. Salton, and G. D. Shockman (ed.), Antibiotic inhibition of bacterial cell surface assembly and function. American Society for Microbiology, Washington, D.C.

11. Hakenbeck, R., A. König, I. Kern, M. van der Linden, W. Keck, D. Billot-Klein, R. Legrand, B. Schoot, and L. Gutmann. 1998. Acquisition of five high-M_r penicillin-binding protein variants during transfer of high-level $beta$ -lactam resistance from Streptococcus mitis to Streptococcus pneumoniae. J. Bacteriol. 180:1831-1840[Abstract/Free Full Text].

12. Hoskins, J. A., G. Zhao, T. I. Meier, P. Matsushima, D. L. Mullen, J. Tang, T. I. Nicas, and R. S. Jaskunas. Unpublished observations.

13. Jamin, M., R. Hakenbeck, and J. M. Frere. 1993. Penicillin binding protein 2x as a major contributor to intrinsic beta-lactam resistance of Streptococcus pneumoniae. FEBS Lett. 331:101-104[Medline].

14. Kell, C. M., U. K. Sharma, C. G. Dowson, C. Town, T. S. Balganesh, and B. G. Spratt. 1993. Deletion analysis of the essentiality of penicillin-binding proteins 1A, 2B and 2X of Streptococcus pneumoniae. FEMS Microbiol. Lett. 106:171-175[Medline].

15. Laible, G., B. G. Spratt, and R. Hakenbeck. 1991. Interspecies recombinational events during the evolution of altered PBP 2x genes in penicillin-resistant clinical isolates of Streptococcus pneumoniae. Mol. Microbiol. 5:1993-2002[Medline].

16. Lefevre, F., M. H. Rémy, and J.-M. Masson. 1997. Topographical and functional investigation of Escherichia coli penicillin-binding protein 1b by alanine stretch scanning mutagenesis. J. Bacteriol. 179:4761-4767[Abstract/Free Full Text].

17. Martin, C., C. Sibold, and R. Hakenbeck. 1992. Relatedness of penicillin-binding protein 1a genes from different clones of penicillin-resistant Streptococcus pneumoniae isolated in South Africa and Spain. EMBO J. 11:3831-3836[Medline].

18. Mouz, N., E. Gordon, A. M. Di Guilmi, I. Petit, Y. Petillot, Y. Dupont, R. Hakenbeck, T. Vernet, and O. Dideberg. 1998. Identification of a structural determinant for resistance to beta-lactam antibiotics in Gram-positive bacteria. Proc. Natl. Acad. Sci. USA 95:13403-13406[Abstract/Free Full Text].

19. Munoz, R., C. G. Dowson, M. Daniels, T. J. Coffey, C. Martin, R. Hakenbeck, and B. G. Spratt. 1992. Genetics of resistance to third-generation cephalosporins in clinical isolates of Streptococcus pneumoniae. Mol. Microbiol. 6:2461-2465[Medline].

20. Nicholas, R. A., D. R. Lamson, and D. E. Schultz. 1993. Penicillin-binding protein 1B from Escherichia coli contains a membrane association site in addition to its transmembrane anchor. J. Biol. Chem. 268:5632-5641[Abstract/Free Full Text].

21. Pares, S., N. Mouz, Y. Petillot, R. Hakenbeck, and O. Dideberg. 1996. X-ray structure of Streptococcus pneumoniae PBP2x, a primary penicillin target enzyme. Nat. Struct. Biol. 3:284-289[Medline].

22. Reichmann, P., A. Konig, A. Marton, and R. Hakenbeck. 1996. Penicillin-binding proteins as resistance determinants in clinical isolates of Streptococcus pneumoniae. Microb. Drug Resist. 2:177-181. [Medline]

23. Roychoudhury, S., J. E. Dotzlaf, S. Ghag, and W. K. Yeh. 1994. Purification, properties, and kinetics of enzymatic acylation with beta-lactams of soluble penicillin-binding protein 2a. A major factor in methicillin-resistant Staphylococcus aureus. J. Biol. Chem. 269:12067-12073[Abstract/Free Full Text].

24. Siligardi, G., F. Harris, and D. A. Phoenix. 1997. Alpha-helical conformation in the C-terminal anchoring domains of E. coli penicillin-binding proteins 4, 5 and 6. Biochim. Biophys. Acta 1329:278-284[Medline].

25. Tipper, D. J., and J. L. Strominger. 1965. Mechanism of action of penicillins: a proposal based on their structural similarity to acyl-D-alanyl-D-alanine. Proc. Natl. Acad. Sci. USA 54:1133-1141[Free Full Text].

26. Wang, C. C., D. E. Schultz, and R. A. Nicholas. 1996. Localization of a putative second membrane association site in penicillin-binding protein 1B of Escherichia coli. Biochem. J. 316:149-156.

27. Zhao, G., W.-K. Yeh, R. H. Carnahan, J. Flokowitsch, T. I. Meier, W. E. Alborn, Jr., G. W. Becker, and S. R. Jaskunas. 1997. Biochemical characterization of penicillin-resistant and -sensitive penicillin-binding protein 2x transpeptidase activities of Streptococcus pneumoniae and mechanistic implications in bacterial resistance to $beta$ -lactam antibiotics. J. Bacteriol. 179:4901-4908[Abstract/Free Full Text].

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	ALL ASM JOURNALS

1.	Adachi, H., T. Ohta, and H. Matsuzawa. 1987. A water-soluble form of penicillin-binding protein 2 of Escherichia coli constructed by site-directed mutagenesis. FEBS Lett. 226:150-154[Medline].
2.	Coffey, T. J., M. Daniels, L. K. McDougal, C. G. Dowson, F. C. Tenover, and B. G. Spratt. 1995. Genetic analysis of clinical isolates of Streptococcus pneumoniae with high-level resistance to expanded-spectrum cephalosporins. Antimicrob. Agents Chemother. 39:1306-1313[Abstract].
3.	Di Guilmi, A. M., N. Mouz, J.-P. Andrieu, J. Hoskins, S. R. Jaskunas, J. Gagnon, O. Dideberg, and T. Vernet. 1998. Identification, purification, and characterization of transpeptidase and glycosyltransferase domains of Streptococcus pneumoniae penicillin-binding protein 1a. J. Bacteriol. 180:5652-5659[Abstract/Free Full Text].
4.	Dowson, C. G., A. Hutchison, and B. G. Spratt. 1989. Extensive re-modelling of the transpeptidase domain of penicillin-binding protein 2B of a penicillin-resistant South African isolate of Streptococcus pneumoniae. Mol. Microbiol. 3:95-102[Medline].
5.	Ferreira, L. C., U. Schwarz, W. Keck, P. Charlier, O. Dideberg, and J. M. Ghuysen. 1988. Properties and crystallization of a genetically engineered, water-soluble derivative of penicillin-binding protein 5 of Escherichia coli K12. Eur. J. Biochem. 171:11-16[Medline].
6.	Fraipont, C., M. Adam, M. Nguyen-Disteche, W. Keck, J. Van Beeumen, J. A. Ayala, B. Granier, H. Hara, and J. M. Ghuysen. 1994. Engineering and overexpression of periplasmic forms of the penicillin-binding protein 3 of Escherichia coli. Biochem. J. 298:189-195.
7.	Ghuysen, J. M. 1994. Molecular structures of penicillin-binding proteins and beta-lactamases. Trends Microbiol. 2:372-380[Medline].
8.	Goffin, C., and J.-M. Ghuysen. 1998. Multimodular penicillin-binding proteins: an enigmatic family of orthologs and paralogs. Microbiol. Mol. Biol. Rev. 62:1079-1093[Abstract/Free Full Text].
9.	Grebe, T., and R. Hakenbeck. 1996. Penicillin-binding proteins 2b and 2x of Streptococcus pneumoniae are primary resistance determinants for different classes of $beta$ -lactam antibiotics. Antimicrob. Agents Chemother. 40:829-834[Abstract].
10.	Hakenbeck, R., T. Briese, H. Ellerbrok, G. Laible, C. Martin, C. Metelmann, H.-M. Schier, and S. Tornette. 1988. Targets of $beta$ -lactams in Streptococcus pneumoniae, p. 390-399. In P. Actor, L. Daneo-Moore, M. L. Higgins, M. R. J. Salton, and G. D. Shockman (ed.), Antibiotic inhibition of bacterial cell surface assembly and function. American Society for Microbiology, Washington, D.C.
11.	Hakenbeck, R., A. König, I. Kern, M. van der Linden, W. Keck, D. Billot-Klein, R. Legrand, B. Schoot, and L. Gutmann. 1998. Acquisition of five high-M_r penicillin-binding protein variants during transfer of high-level $beta$ -lactam resistance from Streptococcus mitis to Streptococcus pneumoniae. J. Bacteriol. 180:1831-1840[Abstract/Free Full Text].
12.	Hoskins, J. A., G. Zhao, T. I. Meier, P. Matsushima, D. L. Mullen, J. Tang, T. I. Nicas, and R. S. Jaskunas. Unpublished observations.
13.	Jamin, M., R. Hakenbeck, and J. M. Frere. 1993. Penicillin binding protein 2x as a major contributor to intrinsic beta-lactam resistance of Streptococcus pneumoniae. FEBS Lett. 331:101-104[Medline].
14.	Kell, C. M., U. K. Sharma, C. G. Dowson, C. Town, T. S. Balganesh, and B. G. Spratt. 1993. Deletion analysis of the essentiality of penicillin-binding proteins 1A, 2B and 2X of Streptococcus pneumoniae. FEMS Microbiol. Lett. 106:171-175[Medline].
15.	Laible, G., B. G. Spratt, and R. Hakenbeck. 1991. Interspecies recombinational events during the evolution of altered PBP 2x genes in penicillin-resistant clinical isolates of Streptococcus pneumoniae. Mol. Microbiol. 5:1993-2002[Medline].
16.	Lefevre, F., M. H. Rémy, and J.-M. Masson. 1997. Topographical and functional investigation of Escherichia coli penicillin-binding protein 1b by alanine stretch scanning mutagenesis. J. Bacteriol. 179:4761-4767[Abstract/Free Full Text].
17.	Martin, C., C. Sibold, and R. Hakenbeck. 1992. Relatedness of penicillin-binding protein 1a genes from different clones of penicillin-resistant Streptococcus pneumoniae isolated in South Africa and Spain. EMBO J. 11:3831-3836[Medline].
18.	Mouz, N., E. Gordon, A. M. Di Guilmi, I. Petit, Y. Petillot, Y. Dupont, R. Hakenbeck, T. Vernet, and O. Dideberg. 1998. Identification of a structural determinant for resistance to beta-lactam antibiotics in Gram-positive bacteria. Proc. Natl. Acad. Sci. USA 95:13403-13406[Abstract/Free Full Text].
19.	Munoz, R., C. G. Dowson, M. Daniels, T. J. Coffey, C. Martin, R. Hakenbeck, and B. G. Spratt. 1992. Genetics of resistance to third-generation cephalosporins in clinical isolates of Streptococcus pneumoniae. Mol. Microbiol. 6:2461-2465[Medline].
20.	Nicholas, R. A., D. R. Lamson, and D. E. Schultz. 1993. Penicillin-binding protein 1B from Escherichia coli contains a membrane association site in addition to its transmembrane anchor. J. Biol. Chem. 268:5632-5641[Abstract/Free Full Text].
21.	Pares, S., N. Mouz, Y. Petillot, R. Hakenbeck, and O. Dideberg. 1996. X-ray structure of Streptococcus pneumoniae PBP2x, a primary penicillin target enzyme. Nat. Struct. Biol. 3:284-289[Medline].
22.	Reichmann, P., A. Konig, A. Marton, and R. Hakenbeck. 1996. Penicillin-binding proteins as resistance determinants in clinical isolates of Streptococcus pneumoniae. Microb. Drug Resist. 2:177-181. [Medline]
23.	Roychoudhury, S., J. E. Dotzlaf, S. Ghag, and W. K. Yeh. 1994. Purification, properties, and kinetics of enzymatic acylation with beta-lactams of soluble penicillin-binding protein 2a. A major factor in methicillin-resistant Staphylococcus aureus. J. Biol. Chem. 269:12067-12073[Abstract/Free Full Text].
24.	Siligardi, G., F. Harris, and D. A. Phoenix. 1997. Alpha-helical conformation in the C-terminal anchoring domains of E. coli penicillin-binding proteins 4, 5 and 6. Biochim. Biophys. Acta 1329:278-284[Medline].
25.	Tipper, D. J., and J. L. Strominger. 1965. Mechanism of action of penicillins: a proposal based on their structural similarity to acyl-D-alanyl-D-alanine. Proc. Natl. Acad. Sci. USA 54:1133-1141[Free Full Text].
26.	Wang, C. C., D. E. Schultz, and R. A. Nicholas. 1996. Localization of a putative second membrane association site in penicillin-binding protein 1B of Escherichia coli. Biochem. J. 316:149-156.
27.	Zhao, G., W.-K. Yeh, R. H. Carnahan, J. Flokowitsch, T. I. Meier, W. E. Alborn, Jr., G. W. Becker, and S. R. Jaskunas. 1997. Biochemical characterization of penicillin-resistant and -sensitive penicillin-binding protein 2x transpeptidase activities of Streptococcus pneumoniae and mechanistic implications in bacterial resistance to $beta$ -lactam antibiotics. J. Bacteriol. 179:4901-4908[Abstract/Free Full Text].