Site-directed Mutagenesis of Glutamate 166 in Two beta -Lactamases
KINETIC AND MOLECULAR MODELING STUDIES*

(Received for publication, October 11, 1996)

Gilliane Guillaume Dagger , Marc Vanhove , Josette Lamotte-Brasseur , Philippe Ledent , Marc Jamin , Bernard Joris and Jean-Marie Frère §par

From the § Centre d'Ingénierie des Protéines and Laboratoire d'Enzymologie, Université de Liège, Institut de Chimie B6, Sart-Tilman, B-4000 Liège, Belgium

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
Acknowledgment
REFERENCES


ABSTRACT

The catalytic pathway of class A beta -lactamases involves an acyl-enzyme intermediate where the substrate is ester-linked to the Ser-70 residue. Glu-166 and Lys-73 have been proposed as candidates for the role of general base in the activation of the serine OH group. The replacement of Glu-166 by an asparagine in the TEM-1 and by a histidine in the Streptomyces albus G beta -lactamases yielded enzymes forming stable acyl-enzymes with beta -lactam antibiotics. Although acylation of the modified proteins by benzylpenicillin remained relatively fast, it was significantly impaired when compared to that observed with the wild-type enzyme. Moreover, the E166N substitution resulted in a spectacular modification of the substrate profile much larger than that described for other mutations of Omega -loop residues. Molecular modeling studies indicate that the displacement of the catalytic water molecule can be related to this observation. These results confirm the crucial roles of Glu-166 and of the "catalytic" water molecule in both the acylation and the deacylation processes.


INTRODUCTION

DD-peptidases and most beta -lactamases, belong to the superfamily of active-site serine penicillin-recognizing enzymes (1). The interaction between these proteins and beta -lactams involves the formation of an acyl-enzyme (E-S*) intermediate where the antibiotic is covalently bound to the active-site serine residue,
E+<UP>S</UP> <LIM><OP><ARROW>↔</ARROW></OP><LL>k<SUB>−1</SUB></LL><UL>k<SUB>1</SUB></UL></LIM> E<UP>S</UP> <LIM><OP><ARROW>→</ARROW></OP><UL>k<SUB>2</SUB></UL></LIM> E<UP>S</UP>* <LIM><OP><ARROW>→</ARROW></OP><UL>k<SUB>3</SUB></UL></LIM> E+P (Eq. 1)
In contrast to DD-peptidases, beta -lactamases efficiently catalyze the deacylation step (high k3 value) which regenerates the active enzyme and releases a biologically inactive product (P). Serine beta -lactamases are divided into three classes A, C, and D on the basis of their primary structures. Tertiary structures of various enzymes belonging to classes A and C have been solved by x-ray crystallography underlining similarities in the folds of all these proteins (2-6). Moreover, several conserved residues were identified, some of which appear to be essential for catalysis (7).

The mechanism by which serine beta -lactamases hydrolyze penicillins and cephalosporins has received a lot of attention and, for the class A enzymes the identity of the residue involved in the activation of the active serine (Ser-70 in the ABL numbering system (8)) has been subject of controversy. Both Lys-73 (9) and Glu-166 (10) have been proposed as potential candidates for this essential role. By contrast, the function of Glu-166 in activating the hydrolytic water molecule during the deacylation step is unanimously recognized. According to Adachi et al. (11) and Strynadka et al. (9), accumulation of an acyl-enzyme during the interaction between the TEM-1 Glu-166 right-arrow Asn mutant (E166N) and benzylpenicillin suggested that the mutation affected only the deacylation step in a severe manner. In contrast, kinetic studies of the Glu-166 right-arrow Ala mutant of the Bacillus licheniformis beta -lactamase (12) and of the Glu-166 right-arrow Asp mutant of the Bacillus cereus I beta -lactamase (13) showed that accumulation of the acyl-enzyme could result from simultaneous but different decreases of the kinetic parameters characterizing the acylation and deacylation steps.

The present paper reports the analysis of the kinetic properties of the TEM-1 E166N mutant. Methods were developed to monitor the rapid formation of the acyl-enzyme. One of the most striking results was a sharp modification of the substrate profile of the enzyme. To explain these results, the interactions between different beta -lactams and the E166N mutant were analyzed by molecular modeling. These confirmed the role of the catalytic water molecule in the mechanism and underlined the importance of the Omega -loop residues in the specificity profile. Similar kinetic data were obtained with the E166H mutant of the Streptomyces albus G class A beta -lactamase.


EXPERIMENTAL PROCEDURES

Strains and Plasmids

Escherichia coli TG1 strain (Delta (lac-pro), Sup E, thi, hsdD5/F'traD36, proA- B+, lacIq, lacZDelta M15) was used for routine transformation, DNA preparation and production of the TEM-1 beta -lactamase and as a host strain for M13 phage growth. The Streptomyces lividans TK24 strain (14) was utilized for the production of the Streptomyces albus G beta -lactamase.

Plasmid pAD25 (15) encodes both the tetracycline resistance and an isopropyl beta -D-thiogalactopyranoside-inducible TEM-1 beta -lactamase. It was used both for the mutagenesis procedure and the expression of the WT1 and mutant enzymes.

The gene encoding the S. albus G beta -lactamase was cloned into the M13tg131 phage for mutagenesis. The mutant gene was entirely sequenced, recloned into the pIJ702' Streptomyces plasmid (a gift from Dr. J. Altenbüchner, Universität-Regensburg, Germany), and expressed in S. lividans.

Nucleic Acid Techniques

Sequencing was performed by the method of Sanger et al. (16) using the Sequenase sequencing kit (U. S. Biochemical Corp.). T4 DNA ligase and kinase were purchased from Boehringer Mannheim GmbH. Oligonucleotides were purchased from Eurogentec (Liège, Belgium). Specific Streptomyces DNA manipulations, such as protoplast preparation, transformation, and plasmid extraction, were based on Hopwood et al. (17).

Mutagenesis

The E166N TEM-1 beta -lactamase mutant was obtained by inverse polymerase chain reaction mutagenesis (18) with the following oligonucleotides: 5'-AAGGCGAGTTACATGATCCCC-3'; 5'-GTAAGTCGAGGCC<UNL><B>C</B></UNL>A<UNL><B>A</B></UNL>GGTTGCTAG-3'. The latter carried the two mismatched bases designed to mutate the GAA (Glu) codon into AAC (Asn).

Amplification was performed with the Vent DNA polymerase (Biolabs) in the buffer supplied by the manufacturer to which MgSO4 was added to a final concentration of 4 mM; 30 cycles (60 s at 94 °C, 60 s at 56 °C, 270 s at 72 °C) were performed on the reaction mixture. The polymerase chain reaction product was subsequently treated as described by Imai et al. (19) and used to transform E. coli TG1.

For the E166H mutant of the S. albus G beta -lactamase, mutagenesis was performed as described by Eckstein et al. (20). The oligonucleotide used to replace the GAC (Glu) codon by CAC (His) was 5'-CTCGACCGCTGG<UNL><B>C</B></UNL>ACCCGGAGCTGAAC-3'.

Chemicals

Benzylpenicillin was from Rhône Poulenc (Paris, France), cefuroxime and ceftazidime were from Glaxo Group Research (Greenford, Middlesex, United Kingdom), cefotaxime from Hoechst-Roussel (Romainville, France). Imipenem, moxalactam, temocillin, and cefoxitin from Merck, Sharp and Dohme Research Laboratories (Rahway, NJ). Cephalosporin C and cephaloridine from Eli Lilly and Co. (Indianapolis, IN). All these compounds were kindly given by the respective companies. [14C]Benzylpenicillin (54 mCi/mmol) was purchased from Amersham International.

Isopropyl beta -D-thiogalactopyranoside and tetracycline were purchased from Sigma. Fluoresceyl-6-aminopenicillanic acid was prepared as described by Lakaye et al. (21).

Expression and Purification of Mutant beta -Lactamases

The E166H mutant of the S. albus G beta -lactamase was isolated from 3 liters of culture supernatant and purified as described by Brannigan et al. (22) with an additional chromatographic step on a Superdex 75 HR 10/30 column in 25 mM sodium phosphate buffer, pH 7.

For the production of the E166N TEM-1 mutant, E. coli TG1 was grown at 30 °C in 15 liters of M9 minimal medium supplemented with 50 µg/ml tetracycline. When the A550 value reached 0.6, 0.1 mM isopropyl beta -D-thiogalactopyranoside was added and the culture was further incubated for 3 h. Cells were collected, suspended in a 30 mM Tris-HCl buffer, pH 7, containing 27% sucrose (w/v) and lysed by lysozyme (1 mg/ml final) as described by Dubus et al. (15). Cell debris were discarded by centrifugation and the supernatant dialyzed against 10 mM Tris-HCl, pH 7.5. The enzyme was purified as described by Vanhove et al. (23). The fractions containing the enzyme were identified by submitting samples of fluoresceyl-6-aminopenicillanic acid-labeled enzyme to electrophoresis on a 15% polyacrylamide gel in the presence of SDS (24).

The purity of the different enzyme preparations was verified by Coomassie Blue staining of SDS-polyacrylamide electrophoresis gels. The TEM-1 mutant was titrated with [14C]benzylpenicillin and found to be more than 95% pure. The E166H mutant of S. albus G was only 50% pure and remained contaminated by a single, low molecular mass protein which did not interfere with the kinetic measurements.

Determination of the Kinetic Parameters

Due to the very low k3 values observed with these two mutants the determination of their kinetic parameters rested on methods similar to those used for penicillin-binding proteins rather than for regular beta -lactamases. Unless otherwise mentioned, all the kinetic assays were performed at 30 °C in 50 mM sodium phosphate buffer, pH 7.

Determination of k2/K Values

Pseudo-first order reactions are only obtained when the beta -lactam concentration is at least five times greater than that of enzyme. Due to the high k2/K values, these conditions where only fulfilled when the experiments were performed in a stopped-flow apparatus. The beta -lactam concentration was also decreased close to that of enzyme and analysis performed according to the general second order equation. Finally after the direct determination of the k2/K values for cefoxitin and cephalosporin C, those for the other compounds were determined by a competition method.

Direct Determination with Manual Mixing (Method A)

The enzyme solution was added with cefoxitin, cephalosporin C, cefotaxime, moxalactam, or ceftazidime. The total volume was 0.5 ml and the final enzyme concentration 16 µM. The antibiotic concentration was always slightly higher than that of the enzyme. Decrease of the A260 value resulting from the opening of the beta -lactam ring was monitored with the help of an Uvikon spectrophotometer connected to a COPAM PC88C microcomputer. The data were fitted to Equation 2 using the Enzfitter program (Biosoft, Cambridge, United Kingdom (25)) yielding the value of the second-order rate constant k, i.e. k2/K', where K' = (k-1 + k2)/k+1. Under conditions of similar initial enzyme and substrate concentration, the general Equation 2 prevails.
<UP>ln</UP>[(E<SUB>0</SUB>−x)/(S<SUB>0</SUB>−x)]=<UP>ln</UP>(E<SUB>0</SUB>/S<SUB>0</SUB>)+(E<SUB>0</SUB>−S<SUB>0</SUB>)k · <UP>t</UP> (Eq. 2)
where S0 and E0 are the initial concentrations of substrate and enzyme and x the concentration of E (or S) transformed at time t.

Under our experimental conditions (S0 > E0) concentrations could be replaced by absorbance values as in Equation 3, leading to Equation 4,
E<SUB>0</SUB>=(A<SUB>0</SUB>−A<SUB>∞</SUB>)/&Dgr;ϵ; <UP>S</UP><SUB>0</SUB>=(A<SUB>0</SUB>−A<SUB>∞</SUB>) · (<UP>S</UP><SUB>0</SUB>/E<SUB>0</SUB>)/&Dgr;ϵ <UP>and</UP> x=(A<SUB>0</SUB>−A<SUB>t</SUB>)/&Dgr;ϵ (Eq. 3)
where A0, At, Ainfinity , are the absorbance values at times 0, t, and at the end of the reaction and Delta epsilon is the variation of the substrate molar extinction coefficient upon hydrolysis.
(A<SUB>t</SUB>−A<SUB>∞</SUB>)/[(<UP>S</UP><SUB>0</SUB>/E<SUB>0</SUB>)(A<SUB>0</SUB>−A<SUB>∞</SUB>)−A<SUB>0</SUB>+A<SUB>t</SUB>)]=[1/(<UP>S</UP><SUB>0</SUB>/E<SUB>0</SUB>)]<UP>exp</UP>[((A<SUB>0</SUB>−A<SUB>∞</SUB>) (Eq. 4)
(1−<UP>S</UP><SUB>0</SUB>/E<SUB>0</SUB>)/&Dgr;ϵ)kt]

Stopped-flow Experiments (Method B)

The enzyme (16 µM) was mixed with increasing concentrations of cefoxitin with the help of a Biologic Stopped-flow apparatus (Grenoble, France). The S0/E0 ratio ranged from 1.2 to 25. For data analysis, Equation 2 was adapted to the stopped-flow recording conditions. Alternatively, for the highest S0/E0 ratios the pseudo-first order approximation was used, yielding identical results.

Competition Method (Method C)

The enzyme (0.9 µM) was added with a mixture of [14C]benzylpenicillin (B) and another antibiotic (I) at concentrations ranging from 2.5 × 10-6 to 1.0 × 10-4 M. After 5 min, the reaction was stopped and the protein precipitated, isolated, and the radioactivity determined as described by Martin and Waley (26). Since both antibiotic concentrations were larger than that of the enzyme and the incubation time was much shorter than the half-life of both acyl-enzymes (see below), the respective quantities of labeled (E-B* formed with [14C]benzylpenicillin) and unlabeled (E-I* formed with the other antibiotic) acyl-enzymes were given by Equation 5 as shown by Frère et al. (27),
[E<UP>I</UP>*]/[E<UP>B</UP>*]=(k<SUB>2</SUB>/K)<SUB><UP>I</UP></SUB>[<UP>I</UP>]/(k<SUB>2</SUB>/K)<SUB><UP>B</UP></SUB>[<UP>B</UP>] (Eq. 5)
The value of [EI*] was estimated as [EB*]0 - [EB*], where [EB*]0 was the quantity of acyl-enzyme formed with [14C]benzylpenicillin in the absence of competing substrate.

Direct Binding of a Labeled Antibiotic (Method D)

With the E166H mutant of the S. albus G enzyme the second-order rate constant for acylation (k2/K') was obtained by monitoring acyl-enzyme formation as a function of time (method D). The enzyme was incubated with an excess of [14C]benzylpenicillin (S0 >>  E0) and after increasing periods of time, the reaction was stopped by addition of 1% SDS. The labeled acyl-enzyme was isolated by SDS-polyacrylamide gel electrophoresis and quantified by fluorography (24).

Determination of k3

Labeled Antibiotic

The protein (1.6 µM) was reacted with an excess of [14C]benzylpenicillin (10-4 M) and the excess of free antibiotic eliminated by addition of 600 ng of the wild-type enzyme. The mixture was incubated at 30 °C and after increasing periods of time, the residual acyl-enzyme quantified after precipitation as above (26).

Unlabeled Antibiotics

After formation of the acyl-enzyme in 50 mM cacodylate buffer, pH 7, at 30 °C, the excess of unlabeled antibiotic was hydrolyzed by addition of the Zn-beta -lactamase of B. cereus (1 µM) and 100 µM ZnCl2. The acyl-enzyme was then left to decay during different time periods. 1 mM EDTA was added to inactivate the Zn-beta -lactamase and the regenerated active-serine enzyme was quantified by saturation with [14C]benzylpenicillin and precipitation as above. With both labeled and unlabeled antibiotics, the degradation of the acyl-enzyme obeyed simple first-order kinetics (28).

pH Dependence of the Enzyme Activity

The following pH range was explored: acetic acid/sodium acetate, pH 4-5.5, sodium phosphate, pH 6-8, Tris-HCl, pH 8.5-9. All the buffers were 50 mM. These experiments were performed with the help of method A for the E166N mutant and method D for the E166H mutant. For the TEM-1 wild-type enzyme, the kcat/Km value was obtained by determining initial rates (v0) at substrate concentrations well below the Km value.

The data obtained for the wild-type TEM-1 and the E166N mutant were fitted to Equation 6 by means of the Enzfitter program,
k<SUB><UP>obs</UP></SUB>=k<SUB><UP>lim</UP></SUB>/(1+[<UP>H</UP><SUP><UP>+</UP></SUP>]/K<SUB>1</SUB>+K<SUB>2</SUB>/[<UP>H</UP><SUP><UP>+</UP></SUP>])+k<SUB><UP>lim</UP>2</SUB>/(1+K<SUB>2</SUB>/[<UP>H</UP><SUP><UP>+</UP></SUP>]) (Eq. 6)
Alternatively, fitting of the same data was performed with klim2 = 0. The pH dependence of k3 characterizing the degradation rate of the E166N-[14C]benzylpenicillin adduct was investigated in the same buffers.

Thermal Denaturation Curves

Temperature-induced unfolding was monitored by recording the intrinsic fluorescence of the TEM-1 E166N as described by Vanhove et al. (29).

The cuvette containing the sample (1.4 ml) was heated at a rate of 0.9 °C/min using a thermostatically regulated circulating water bath. The enzyme unfolded reversibly in a simple co-operative fashion. Unfolding curves were analyzed according to Equation 7 by means of the nonlinear regression data analysis Enzfitter program,
F<SUB><UP>mes</UP></SUB>={(<UP>N</UP>+<UP>yT</UP>)+(<UP>U</UP>+<UP>zT</UP>)<UP>exp</UP> a}/{1+<UP>exp</UP> a} (Eq. 7)
with a = Delta Hm [(T/Tm- 1]/RT, where Tm is the midpoint at the transition and Delta Hm is the enthalpy of unfolding at Tm. The (N + yT) and (U + zT) terms were necessary to account for the linear decreases of the intrinsic fluorescences of the native and denatured states of the protein (N and U, respectively) upon increasing temperature.

Proteolysis Experiments

A mixture containing 0.2 mg of enzyme and 0.02 mg of trypsin was incubated in 100 mM Tris-HCl, pH 7.5, at 40 °C. Aliquots were removed and trypsin was inactivated by addition of 40 mg/ml soybean trypsin inhibitor (Sigma). Quantification of the mutant residual activity was performed by titration with [14C]benzylpenicillin.

Optimized Structures of the Substrates

The structures of the beta -lactam molecules were optimized by the AM1 semi-empirical method (Dewar et al. (30)). CNDO charges were adopted for these ligands. The bond lengths, bond angles, and ring dihedral angles of the antibiotics were constrained to the AM1 values.

Molecular Modeling

Models of the mutant enzymes were obtained from the x-ray structures of the wild-type proteins (5) and the local conformational space of the mutated amino acid was searched by a minimum perturbation approach (31).

The system was solvated by cubes of standard "Monte Carlo" water molecules and the positions of these molecules after minimization were compared to those in the crystal structures. The geometry of the protein was optimized with the AMBER 4.1 set of programs (32) using a distance-dependent dielectric constant.

The beta -lactam molecules were docked in the modeled active sites with the beta -lactam amide oxygen atom oriented into the oxyanion-hole formed by the main chain nitrogen atoms of Ser-70 and Ala-237. Hydrogen bonds appeared to be formed between the C7 side chain amide group and the Ndelta 2 amide nitrogen atom of Asn-132 and the main chain oxygen atom of Ala-237. The energy of the Michaelis complexes thus obtained was minimized using AMBER (32).


RESULTS

Production and Purification

About 16 mg of the TEM-1 E166N mutant were obtained per liter of culture. The protein was purified to 95% homogeneity with a yield of 45%. For the S. albus G mutant, the culture and purification yields were 20 mg/liter and 25%, respectively; as stated above, the final preparation was only 50% pure. Attempts to eliminate the low molecular mass contaminant by various chromatographic procedures, including molecular sieve filtration, remained unsuccessful.

Kinetic Properties

The values of the rate constants obtained for the TEM-1 E166N mutant are reported in Table I. As expected and in agreement with the observations of Adachi et al. (11) and Strynadka et al. (9), the rates of deacylation (k3) were exceedingly low.

Table I.

Acylation rate constants (k2/K') and deacylation rate constants (k3) of the TEM-1 E166N mutant and wild-type enzymes with various beta -lactams

For the WT enzyme, the k2/K' are the kcat/Km values and kcat supplies a minimum k3 value when it has not been independently measured. The method used for determining the k2/K' values of the mutant protein is indicated between parentheses. The kinetic parameters for the WT enzyme are from Raquet et al. (37), Fisher et al. (48), Christensen et al. (49), and Raquet (50).
Compound k2/K' WT k2/K' E166N Mutant/WT k3 WT k3 E166N

M-1 s-1 s-1
Benzylpenicillin 84  × 106 450  × 103(C) 0.005 1500 5.2  × 10-6
Cephalosporin C 90  × 103 2  × 103(A+C) 0.022 >36 0.71  × 10-6
Cephaloridine 2.24  × 106 15  × 103(C) 0.007 >1500 0.76  × 10-6
Cefoxitin 6 4.5  × 103(A+C) 750 4 × 10-3  ---a
Moxalactam 16 3.5  × 103(A) 219  ---a  --- a
Temocillin *b 500(C) >150  ---a  --- a
Cefotaxime 1.5  × 103 2.5  × 103(A) 1.7 >9 0.91  × 10-6
Cefuroxime 6  × 103 6  × 103(C) 1 >6 0.63  × 10-6
Ceftazidime 70 400(A) 5.7 >0.34 2.1  × 10-6
Imipenem 2  × 103 30  × 103 (C) 15 >2 × 10-2  --- a

a  Not determinated.
b  No hydrolysis detected (3).

Different strategies were utilized to determine the second-order rate constant (k2/K'), characteristic of the acylation rate. Rapid acylation could not be monitored by the usual methods. With [14C]benzylpenicillin, the reaction was so rapid that it could not be followed by manual mixing methods. In consequence, the first experiments were performed with compounds exhibiting lower acylation rates and whose modifications upon acyl-enzyme formation could be directly monitored by spectrophotometric methods. The manual method A allowed the determination of the k2/K' values for cephalosporin C, cefoxitin, cefotaxime, and ceftazidime. That Equation 2 applied was confirmed by the fact that similar k2/K' values were obtained at cefoxitin concentrations ranging from 20 to 40 µM. The stopped-flow method, which required much larger quantities of proteins was only utilized with cefoxitin. Here the antibiotic concentrations were as high as 400 µM. An average k2/K' value of 2200 ± 440 M-1 s-1 was found, in fair agreement with that obtained in the manual mixing experiments (4500 ± 130 M-1 s-1). The values for the other compounds were obtained by the competition method C. First, competitions between [14C]benzylpenicillin and cephalosporin C or cefoxitin were performed, allowing the computation of the k2/K' value for the 14C-labeled compound. Subsequently, the values for all the other beta -lactams were derived from competition experiments with [14C]benzylpenicillin.

For good substrates of the wild-type enzyme (benzylpenicillin and cephaloridine), the E166N mutation resulted in a decrease of the acylation rates by 2-3 orders of magnitude. This was, however, much less drastic than for the k3 value. The most striking results concerned the modification of the substrate profile.

In contrast to what occurred with the good substrates, the k2/K' for the poorest WT substrates (i.e. temocillin, cefoxitin, and moxalactam which bear a methoxy side chain on the alpha -face of the beta -lactam ring) were increased by several orders of magnitude. With the oxyiminocephems, the k2/K' value was not much affected. In consequence the k2/K' values of the mutant only spanned 3 (from 400 to 400 × 103) versus 7 orders of magnitude for the wild-type protein.

With benzylpenicillin and the S. albus G E166H mutant, similar results were obtained, involving a significant decrease of k2/K' accompanied by a much more drastic decrease of k3 (Table II).

Table II.

Acylation (k2/K') and deacylation rate constants (k3) of the S. albus G beta -lactamase E166H mutant and of the wild-type enzyme with benzylpenicillin

The k2/K' values for the mutant were determined by direct binding of a labeled antibiotic (method D). For the WT values see the footnote to Table I.
pH E166H k2/K' WT kcat/Km E166H k3 WT k3

M1 s-1 s-1
5 6,000 1,950  × 103 1.8  × 10-3 >3,800
7 10,000 3,000  × 103 3.9  × 10-4 >3,400
9 32,000 2,300  × 103 4.5  × 10-4 >2,800

Effect of the pH on Catalytic Parameters

The pH dependence of the acylation rate of the E166N mutant by cefoxitin was studied using method A (see Fig. 1). The pH dependence of the k2/K' value could be fitted to Equation 6 with pK1 and pK2 values of 6.0 and 8.5, respectively. With the wild-type enzyme pK values of 7.2 and 9 were found. The mutation thus resulted in a shift of the curve to lower pH values, with a more significant effect to the acid limb. The k3 constant was not significantly influenced by the pH value (not shown).


Fig. 1. pH dependence of the second-order acylation rate constant (k2/K') of the TEM-1 E166N and wild-type enzymes. bullet , WT; and open circle , E166N mutant. Above pH 10.5, spontaneous hydrolysis of the antibiotic did not allow precise measurements. S.D. values were below 20%. The solid line was obtained by fitting data to Equation 6. Fitting with klim2 = 0 lead a somewhat poorer fit in the low pH range. It was, however, not possible to be certain that this was statistically meaningful.
[View Larger Version of this Image (15K GIF file)]


The k2/K' value of the E166H mutant of the S. albus G beta -lactamase (Table II) exhibited a new pH dependence which seemed to indicate that the base form of the His-166 side chain was adequately oriented to actively participate in the acylation step. By contrast, the k3 value at pH 5 was higher than at pH 7 or 9. This suggested that the His-166 residue of the mutant enzyme was not involved in the deacylation step as a general base catalyst.

Stability of the E166N TEM-1 Mutant

The melting temperature (Tm) and the enthalpy (Delta Hm) of unfolding obtained by fitting the experimental curves to Equation 7 were: 51.1 ± 0.2 °C and 112 ± 7 kcal/mol °C, 43 ± 1.4 °C and 87 ± 5 kcal/mol °C for the wild-type and the E166N mutant proteins, respectively. This result highlighted a significant destabilization of the mutant which was corroborated by the proteolysis experiments in which the pseudo-first order rate constants (ki) characterizing trypsin-mediated inactivation were 0.29 min-1 and 0.012 min-1 for the TEM-1 E166N and WT proteins (33), respectively.

Models of the Mutant Enzymes

The strong hydrogen bonds found between the carboxylic group of Glu-166 and the side chain nitrogen atoms of Lys-73 and Asn-170 of TEM-1 disappeared in the E166N mutant, allowing free rotation of these residues. In the most stable structure obtained by conformational analysis, the Asn-170 acyl group was rotated by 180° around the Cbeta -Cgamma bond with respect to the orientation found in the WT enzyme. A similar rotation was observed in the structure of the E166A mutant of the B. licheniformis beta -lactamase (34). There was no change in the position of Lys-73 relative to its WT position. All calculations were performed considering both the protonated and unprotonated states of Lys-73 and yielded similar results.

The position of the "catalytic" water molecule in the mutant was found to be the same whether it was generated by a Monte Carlo simulation or minimized from the position found in the WT structure. The water hydrogen atoms were oriented toward the Asn-166 and Asn-170 Odelta s, respectively. By comparison with the WT structure, it was shifted by 1.3 Å away from Ser-70 with which it no longer formed a H-bond (Fig. 2).


Fig. 2. Active site of the TEM-1 beta -lactamase E166N mutant. The position of the W1 water molecule in the wild-type enzyme is shown as oplus . The backbone atoms are represented as filled circles.
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In the E166H mutant, the plane of the imidazole side chain was rotated by 75° with respect to that formed by the glutamate carboxylate in the WT enzyme. The catalytic water molecule slightly (0.8 Å) moved to the bottom of the cavity away from its initial position and was thus further from Ser-70. The lengths of the hydrogen bonds were 3.12 and 2.85 Å with an unprotonated and protonated Lys-73 residue, respectively, as previously shown in the model of the E166D mutant of the S. albus G enzyme (35). The N170 side chain was more outward-oriented due to a 30° rotation around the Calpha -Cbeta bond.

Modeled Interactions of the E166N Mutant with beta -Lactam Substrates

Three cephalosporins: cephaloridine, cefuroxime, and cefoxitin, respectively, good, bad, and very bad substrates of the WT TEM-1 but of similar properties with the mutant were chosen as models for the study of the specificity of the E166N mutant. Benzylpenicillin was also studied (not shown), yielding results similar to those obtained with cephaloridine (Fig. 3A).


Fig. 3. Modeling of the Michaelis complexes formed by the TEM-1 E166N beta -lactamase with cephaloridine (A), cefuroxime (B), and cefoxitin (C). The antibiotic molecules are represented by filled circles and black lines. The arrows indicate the oxyimino group and the C7 alpha -methoxy groups of cefuroxime and cefoxitin, respectively.
[View Larger Version of this Image (28K GIF file)]


The optimized structures of the Michaelis complexes were not very different from those found in the case of the WT enzyme. In all the complexes, the catalytic water molecule remained positioned as in the free mutant (Fig. 3B), so that it was not perturbed by the C7-methoxy group of cefoxitin, a situation very different from that observed with the WT enzyme. With cefuroxime the main additional observation was a decrease of the steric hindrance between the oxyimino group and the N170 side chain (Fig. 3C). Deprotonation of Lys-73 only resulted in a slight increase of the distance between the water and the Ser-70.

Interaction of the E166H Mutant with Benzylpenicillin

The optimized Henri-Michaelis complex was not very different from that computed for the wild-type enzyme (Fig. 4). The major difference was that the NH-CO bond of the C-6 substituent of penicillin was now closer to the N170 side chain due to the displacement of the latter (about 3 Å).


Fig. 4. Modeling of the Michaelis complex formed by the E166H mutant of beta -lactamase of S. albus G and benzylpenicillin. The antibiotic molecule is represented by filled circles and black lines.
[View Larger Version of this Image (26K GIF file)]



DISCUSSION

Both mutant proteins were more poorly produced than the WT enzymes. This might be related to the relative instability of the mutant proteins which increases their sensitivity to proteases as shown for the TEM-1 E166N mutant. With this protein, utilization of a minimal medium and a lower temperature significantly improved the production yield. This instability might due to an increased mobility of the Omega -loop as shown for various other TEM-1 mutants (36, 37).

On the basis of a preliminary study of the TEM-1 E166N mutant, Adachi et al. (11) concluded that the deacylation rate was severely decreased while the acylation reaction was unimpaired. Since the first conclusion was in disagreement with the data of Gibson et al. (13) and Leung et al. (38), however, obtained with different Glu-166 mutants of another enzyme, a careful kinetic study of the TEM-1 E166N protein was performed. As expected and with all substrates, our results indicated extremely large decreases of the k3 value, a 109 factor for benzylpenicillin. This result underlined the pivotal role of the Glu-166 in the deacylation step, a feature on which a general consensus has been reached. By contrast, with the good substrates, the k2/K' value, which characterizes the efficiency of acylation and corresponds to the kcat/Km of the WT enzyme, was decreased by 2 or 3 orders of magnitude indicating a non-negligible, although less pivotal role of Glu-166 in the acylation step. This was, however, not true for all substrates since the acylation rates by poorer substrates were unchanged or even slightly increased and for the very bad substrates, cefoxitin and other compounds exhibiting a methoxy group on the alpha -face, acylation was significantly facilitated.

Consequently, the "activity" profile of the enzyme was deeply modified, with a spectacular leveling effect. According to Strynadka et al. (9), the position of the Omega -loop was not strongly modified in the mutant. The situation was the same with the B. licheniformis E166A mutant but quite different with the TEM-1 E166Y (39) and S. aureus D179N (40) proteins where the loop was disordered. Here the most striking structural modifications were the displacement of the water molecule W1 away from the active site Ser-70 side chain and the disappearance of several strong hydrogen bonds. It should be noted that this water molecule has been hypothesized to serve as a relay in the activation of the Ser-70 hydroxyl group by the Glu-166 side chain acting as a general base in the acylation process. However, an alternative mechanism has been proposed by Strydnaka et al. (9), where the general base would be the unprotonated side chain of Lys-73 and the Glu-166 carboxylate in the acylation and deacylation steps, respectively. Although it would explain the properties of E166X mutants which would catalyze the acylation reaction with the same efficiency as the wild-type enzyme but would fail to deacylate, this hypothesis also implies a significantly decreased pKa value for the alkylammonium group of the lysine 73 side chain in the wild-type enzyme. A recent NMR titration of the Lys-73 residue in the TEM-1 protein failed to supply evidence for such unusual pKa value (41). Other Glu-166 mutants have been prepared with other enzymes (12, 38, 42). Whenever detailed kinetic studies were performed, both acylation and deacylation rates appeared to be decreased by the mutation, although deacylation was sometimes much more severely impaired. Moreover, the K73R mutant of the B. cereus 569/H beta -lactamase I (13) was significantly more active than its E166D counterpart. The drastic substrate profile modifications observed in this present study suggest that the acylation of the mutant might rely on an alternative mechanism. One can hypothesize that, as proposed by Lamotte-Brasseur et al. (10) and Matagne et al. (43), the very low acylation rates of the WT enzyme by cefoxitin, moxalactam, and temocillin are due to a displacement of W1 by the methoxy side chain of the substrates. With the mutant, the Lys-73 side chain might replace Glu-166 as the general base as in acetoacetate decarboxylase (44) and as suggested by Strynadka et al. (9) for the WT beta -lactamase. The disappearance of the negative Glu-166 charge would explain a decrease of the Lys-73 pKa when compared to the WT enzyme.

This alternative acylation mechanism would be significantly less efficient for good substrates but, since it would not involve W1, the reaction rates with cefoxitin and similar compounds would be increased. Finally, the unchanged acylation rates with oxyiminocephalosporins would result from the same negative factor as with the good substrates compensated by a positive effect due to the increased mobility of the omega loop as observed for example with the Arg-164 mutants of the TEM-1 enzyme (37).

Note that an unprotonated Lys-73 may not be necessary to act as a proton relay. The softness of the electronic atmosphere of the nitrogen atom allows an easy adaptation to environmental modifications such as the binding of a ligand. It is finally interesting to note that the acylation rates observed with the E166N mutant are of the same order of magnitude as those measured with several penicillin-binding proteins. The Actinomadura R39 (45) DD-peptidase and B. licheniformis PBP1 (46) contain all the residues constituting the conserved elements of the class A beta -lactamases with the exception of the Omega -loop and, in consequence, have no equivalent of Glu-166 as shown by the three-dimensional structures of the homologous Streptococcus pneumoniae PBP2x (47) and Streptomyces K15 DD-peptidase.2

The results obtained with the S. albus G enzyme generally support these conclusions. In this case, the k3 value is also strongly decreased and this residue does not appear to act as a general base in the deacylation reaction, as indicated by the absence of significant variation of k3 between pH 5 and 9. By contrast, the k2/K' value significantly increases with increasing pH values and, although a real titration curve is not observed, this might suggest that the base form of this residue might participate in the acylation reaction.

These results underline a major role of the W1-Glu-166 pair in the enzymatic acylation-deacylation process and indicate that although Glu-166 is involved in both acylation and deacylation reactions in class A beta -lactamases, these two reactions are not necessarily "mirror" images of each other since the disappearance of Glu-166 affects the two steps in a different way. A careful kinetic analysis of mutant enzymes is thus a prerequisite to meaningful mechanistic conclusions.


FOOTNOTES

*   This work was supported, in part by the Belgian government, as Pôles d'attraction interuniversitaires Grant PAI 19, an Action concertée with the Belgian government convention 89/94-130), and Fonds de la recherche scientifique médicale Contract 3.4537.88). The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Dagger    Fellow of the Fonds pour la Formation à la Recherche dans l'Industrie et dans l'Agriculture (F.R.I.A., Brussels, Belgium).
par    To whom correspondence should be addressed. Tel.: 32-4-3663398; Fax: 32-4-3663364; E-mail, jmfrere@ULG.AC.BE.
   Chercheur qualifié of the Fonds National de la Recherche Scientifique (FNRS, Brussels, Belgium).
1    The abbreviation used is: WT, wild type.
2    E. Fonzé and P. Charlier, personal communication.

Acknowledgment

We thank Dr. X. Raquet for many fruitful discussions.


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