Eagle-Type Methicillin Resistance: New Phenotype of High Methicillin Resistance under mec Regulator Gene Control

doi:10.1128/AAC.45.3.815-824.2001

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Antimicrobial Agents and Chemotherapy, March 2001, p. 815-824, Vol. 45, No. 3
0066-4804/01/$04.00+0 DOI: 10.1128/AAC.45.3.815-824.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Eagle-Type Methicillin Resistance: New Phenotype of High Methicillin Resistance under mec Regulator Gene Control

Noriko Kondo, Kyoko Kuwahara-Arai, Hiroko Kuroda-Murakami, Eiko Tateda-Suzuki, and Keiichi Hiramatsu^*

Department of Bacteriology, Juntendo University, 2-1-1 Hongo, Bunkyo-ku, Tokyo 113-8421, Japan

Received 28 February 2000/Returned for modification 23 June 2000/Accepted 8 December 2000

	ABSTRACT

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We report a novel phenotype of methicillin resistance, designated "Eagle-type" resistance, which is characteristic in itsresistance to high concentrations of methicillin (64 to 512 µg/ml)and susceptibility to low concentrations of methicillin (2 to16 µg/ml). The type of resistance was expressed in mutant strainsselected with high concentrations (e.g., 128 to 512 µg/ml) ofmethicillin from the pre-methicillin-resistant Staphylococcusaureus strain N315, whose mecA gene transcription is stronglyrepressed by the mecI gene-encoded repressor protein MecI. TheEagle-type mutant strains harbored no mutation in the mecI geneor in the operator region of mecA gene to which MecI repressoris supposed to bind. In the representative Eagle-type strain h4,repression of mecA gene transcription and penicillin-binding protein2' production were found to be released by exposing the cellsto a high concentration (128 µg/ml) of methicillin but not tolower concentrations (1 and 8 µg/ml) of methicillin. The strainh4 expressed paradoxical susceptibility (Eagle effect) to thecytokilling activity of methicillin. Experimental deletion ofmecI gene from the chromosome of h4 by mecI-specific gene substitutionconverted its Eagle-type resistance to homogeneously high methicillinresistance. We cloned two novel genes, designated hmrA and hmrB,from genomic library of h4, which conferred Eagle-type resistanceto N315 when introduced into the cell in multiple copies. Thegenes were shown to confer homogeneous methicillin resistanceto the heterogeneously methicillin-resistant strain LR5 when theywere introduced into on multicopy plasmids. This result stronglyindicated that the genetic alteration responsible for the expressionof the Eagle phenotype is identical, or equivalent in its effect,to the genetic alteration underlying heterogeneous-to-homogeneousconversion of methicillin resistance in S. aureus.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Beta-lactam resistance of methicillin-resistant Staphylococcus aureus (MRSA) is caused by the expression of penicillin-bindingprotein 2' (PBP2' or PBP2a) encoded by the mecA gene (28), whichhas low binding affinities to practically all beta-lactam antibioticsso far introduced into clinical use (11, 21, 32). Becauseof the low binding affinities, PBP2' is not inhibited by beta-lactamantibiotics and continues synthesizing cell wall in the presenceof beta-lactam antibiotics. However, it has been pointed out thatproduction of PBP2' in Staphylococcus aureus cells per se doesnot make the entire cell population resistant to methicillin but,instead makes the strain a mixture of cells with different levelsof methicillin resistance (23). This peculiar resistance phenotypehas long been recognized as heterogeneous (hetero)-methicillinresistance (19, 24). This inability of PBP2' to confer fullor homogeneous (homo) methicillin resistance has also been demonstratedusing pre-MRSA strain N315 (12, 17). Pre-MRSA is an S. aureushaving a susceptible level of methicillin MIC (<4 mg/liter) becauseof a strong repression of the mecA gene transcription exertedby mecI gene-encoded repressor protein MecI (13, 17, 30).Inactivation of MecI function in pre-MRSA strain by mecI-specificgene substitution derepresses PBP2' production but causes thestrain express only a hetero type of methicillin resistance (17).It is only after further selection with a high concentration ofmethicillin (e.g., 128 µg/ml) that the homoresistant strain, whoseentire cell population is uniformly resistant to high (126 to512 µg/ml) concentrations of methicillin, is generated (12,17). Ryffel et al. have also shown that, besides PBP2' production,a chromosomal mutation, designated chr*, is required for the hetero-to-homophenotypic conversion to occur (23). So far, no phenotypic expressionintrinsic to chr* mutation (i.e., in the absence of coexpressionof PBP2') has been identified (23). We report here that a mutantstrain of pre-MRSA N315 with a novel methicillin resistance phenotype,designated Eagle-type resistance, is considered to manifest theeffect of chr*-equivalent genetic alteration under mecI-mediatedrepression of PBP2'production.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains. Table 1 lists the bacterial strains used in this study. All of the mutant strains with various methicillin-resistance phenotypeswere obtained from N315 and its derivative strains by a one-stepselection procedure with methicillin as follows. Portions of overnightculture of N315 and its derivative strains were spread onto heartinfusion agar plates containing various concentrations (4 to 512µg/ml) of methicillin, and the plates were incubated overnightat 37°C. The grown colonies were picked as resistant mutants fromeach of the selective concentrations of methicillin. The mutantswere then streaked onto drug-free heart infusion agar plates,and single-colony isolation (colony purification) was performedbefore establishing them as strains. A mutant strain, h4, is oneof the Eagle-type resistant strains obtained as described aboveby selecting N315 with 128 µg of methicillin per ml. Strains $Delta$ Iand h4 $Delta$ I are derivatives of N315 and h4, respectively; they wereobtained by substituting their mecI genes with tetL by using thegene substitution procedure described previously (17). Mutantstrain $Delta$ I-HR expressing methicillin homoresistance was obtainedby one-step selection of $Delta$ I with 128 µg of methicillin per ml.Mutant strain h4-4R is a methicillin homoresistant strain obtainedby one-step selection of h4 with 4 µg of methicillin per ml. Mutantstrain LR5, in which mecI gene function is inactivated by a 62-bpdeletion (from nucleotide positions 130 to 191 of the mecI structuregene [13]), is a derivative of N315 expressing hetero-type methicillinresistance as described previously (1).

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TABLE 1. Bacterial strains used in this study

Plasmids. Escherichia coli-S. aureus shuttle vector pYT3 was used to construct a genomic library of strain h4. The plasmid carries atetracycline-resistant gene (tetL) and the temperature-sensitiveorigin of pE194ts and has been described previously (9, 16).Another shuttle vector, pRIT5, was used for the subcloning ofcloned DNA fragments (20).

Two recombinant plasmids, pHMR-A and pHMR-B, were obtained by screening the genomic library of strain h4; they had 2,063-and 2,100-base Sau3AI fragments inserted at the BamHI site ofpYT3 vector, respectively. The 1.3-kb HindIII-Sau3AI fragmentof the insert was removed from pHMR-A by restriction enzyme cleavage,followed by self-ligation, to obtain plasmid pHMR-A1 having therest of the insert (a 757-bp Sau3AI-HindIII fragment). PlasmidpHMR-A2 was constructed by subcloning the 1.3-kb HindIII-Sau3AIfragment cut out from pHMR-A into the multicloning site of plasmidvector pRIT5 in the same orientation of transcription with spagene on the vector (20). Plasmid pHMR-A3 was constructed bycloning a PCR-amplified DNA fragment into vector pYT3 as follows.A PCR reaction was performed with pHMR-A plasmid DNA as a templateand using two synthetic oligonucleotide primers: primer 1, 5'-AAAAGAGCTCAAAACCCGGGCTTATGTTTACAATTTGA-3'(the introduced SacI site is underlined), and primer 2, 5'-TTTTTGGTACCTTGATGTTCGTCCGGTTTCA-3'(the introduced KpnI site is underlined). Amplified DNA was doublydigested with SacI and KpnI and subjected to agarose gel electrophoresis.The restricted DNA fragment was purified from the agarose gelby electroelution and was ligated into the pYT3 vector predigestedwith SacI and KpnI.

Plasmid pHMR-A4 was constructed by cutting out the 850-base EcoRI DNA fragment from pHMR-A plasmid DNA and then ligating itinto the EcoRI site of vector pRIT5 in the same orientation oftranscription with the spa gene on the vector. Plasmids pHMR-A5and pHMR-A5* were constructed as follows. The DNA fragment containingthe hmrA gene was amplified by PCR with h4 genomic DNA as a templateand the following two synthetic oligonucleotides as primers: primer3, 5'-AAAAGGATCCGATCTAAACTTTCAQCATTCATTT-3' and 5'-AAAAGGATCCGAATTCCCAATTCTTAATCTCGAA-3'(the introduced BamHI sites are underlined). The amplified DNAwas cut with BamHI and ligated into the BamHI site of pYT3, generatingplasmid pHNR-A5. Plasmid pHMR-A5 was digested with NdeI (the NdeIsite is located within hmrA gene at bases 201 to 206 from thestart codon). The cohesive ends of the DNA were filled in by Klenowfragment, followed by blunt-end ligation. The plasmid pHMR-A5*thus generated possessed two additional bases in the hmrA gene,causing a shift of the reading frame and generating a prematuretermination codon at base 632 from the startingcodon.

Plasmids pHMR-B1 to pHMR-B4 were constructed by cutting out the respective restriction fragments from pHMR-B and subcloningthem into pYT3 vector; the inserts were Sau3AI-TthI fragment (pHMR-B1),SalI-Sau3AI fragment (pHMR-B2), TthI-Sau3AI fragment (pHMR-B3),and TthI-SalI fragment (pHMR-B4),respectively.

Screening of h4 gene library. Genomic DNA was extracted from h4 as described previously (13), partially digested with Sau3AI, and ligated with the BamHI-cleaveddephosphorylated pYT3 vector. The plasmid library was establishedby transforming E. coli JM109 (Takara, Tokyo, Japan) with therecombinant plasmids and by selecting transformants on the heartinfusion agar plates containing 10 µg of tetracycline per ml at37°C. A total of 2,871 transformants were obtained. Recombinantplasmids were then isolated from the transformants, purified byCsCl isopycnic centrifugation, and introduced into N315 by electroporationas described previously (17). A total of 22,580 transformantswere obtained by the selection on heart infusion agar plates containing10 µg of tetracycline per ml at 30°C (a permissive temperaturefor the replication of pYT3 vector in S. aureus cells). The transformantswere then replicated onto two heart infusion agar (Difco, Detroit,Mich.) plates containing 10 and 100 µg of methicillin per ml,respectively. The plates were then incubated at 30°C for 48 h.Transformants were sought that formed greater colonies on theplate containing 100 µg of methicillin per ml than those on theplate containing 10 µg of methicillin per ml (Eagle phenotype).Two transformants carrying plasmids pHMR-A and pHMR-B were thusobtained.

Nucleotide sequencing. The nucleotide sequence of hmrA and hmrB genes were determined using AmpliTaq Cycle Sequencing Kit (Perkin-Elmer) based onthe dideoxynucleotides termination method described by Sangeret al. (26) with synthetic oligonucleotides as primers. Sequencesof the mecI genes and mecA gene operator regions of N315 and N315-derivedmutants were determined by using the PCR-amplified DNA fragmentsas templates as described previously (17). The primers usedwere 5'-GACTTGATTGTTTCCTCTGTT-3' and 5'-GACTTGATTGTTTCCTCTGTTT-3'for mecI gene sequencing and 5'-TATACCAAACCCGACAAG-3' and 5'-CATATCGTGAGCAATGAACTG-3'for mecA operator region sequencing. The primers correspondedto the nucleotide positions 1923 to 2403, 2403 to 1983 (complementary),66 to 83, and 287 to 257 (complementary), respectively, of thereported nucleotide sequence of mecI-mecR1-mecA gene complex ofN315 (13).

Analysis of nucleotide sequences. The homology search for the deduced polypeptides encoded by hmrA and hmrB genes was performed with the nucleotide sequencesregistered in the EMBL and GenBank databases and with the proteinsequences of the SWISSPlot and NBRF data libraries. A BLAST searchwas performed to compare hmrA and hmrB gene sequences in publicS. aureus genome databases as follows: strains COL (TIGR [http://www.tigr.org/tdb/mdb/mdbinprogress.html]), NCTC8325 (University of Oklahama [http://www.genome.ou.edu/]),and EMRSA-16 and MSSA strain 476 (The Sanger Centre [http://www.sanger.ac.uk/Projects/S_aureus]).Complete nucleotide sequences of hmrA and hmrB are available underthe DDJB accession numbers D85816 and D85817,respectively.

Population analysis. Analysis of resistant subpopulations was performed with an Autoplate Model 3000 (Spiral Biotech, Inc., Bethesda, Md.). asdescribed previously (17). In brief, 50-µl aliquots of overnightculture and its 1:10 serial dilutions were inoculated onto heartinfusion agar plates containing various concentrations of methicillin.The plates were incubated at 37°C for 48 h, and then mature colonieswere counted. The number of resistant cells theoretically containedin 50 µl of the undiluted overnight culture was calculated andplotted on a bilogarithmicgraph.

Western blotting. The Western blotting to detect methicillin-induced PBP2' production in N315-derived strains has been described previously(17). In this study, three different concentrations of methicillin(1, 8, and 128 µg/ml) were used. Densitometry was performed withMaster Scan (CSPI, Billerica, Mass.).

Cytokilling assay. Overnight cultures of test strains in L broth were diluted to 1% (vol/vol) in fresh L broth and further cultivated with gentleshaking until an optical density at 578 nm of 0.3 (ca. 10⁸ CFU/ml) was reached. Then, 0.1 ml of the cell suspension wasinoculated into 10 ml of prewarmed L broth containing 0, 1, 8,or 128 µg of methicillin per ml in glass test tubes. The testtubes were incubated with gentle shaking, and 0.1-ml portionsof the culture were harvested at 0, 0.5, 1, 2, and 4 h after theinitiation of the culture. The sample was serially diluted withsaline and spread onto heart infusion agar plates, followed byincubation at 37°C for 18 h. Grown colonies were counted and plottedin the graph. The cultivation temperature of the test strainswas 37°C for N315, h4, h4-4R, $Delta$ I, and $Delta$ I-HR and 30°C for the transformantstrains N315(pYT3), N315(pHMR-A), and N315(pHMR-B).

	RESULTS

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Selection of Eagle-type methicillin-resistant strain h4 from pre-MRSA N315. The in vitro mutant strain h4 was obtained from N315 as a methicillin-resistant strain grown on the heart infusion agar platecontaining 128 µg of methicillin per ml. Figure 1A shows a populationanalysis of strain h4 in comparison with those of pre-MRSA strainN315 and its derivative strains with various phenotypes of methicillinresistance, $Delta$ I (hetero-type), $Delta$ I-HR (homo-type), h4-4R (homo-type),and h4- $Delta$ I (homo-type). Strain h4 showed an unusual pattern ofdistribution of resistant cell subpopulation, i.e., more cellsgrew in high concentrations than in low concentrations of methicillin(Fig. 1A). Since the pattern reminded us of the "Eagle effect"of penicillin killing (7), we designated the resistance phenotypeEagle-type resistance after him. Nucleotide sequencing of themecI gene and mecA operator region of h4 revealed no sequencealteration. This was in contrast to the derivatives of N315 withhetero-type methicillin resistance phenotypes, in which mutationsare identified either in mecI gene or in the operator region ofmecA gene (12, 17).

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FIG. 1. Population analysis of N315-derived strains with various methicillin-resistance phenotypes. The number of colonies grown on agar plates containing various concentrations of methicillin were counted after 48 h incubation at 37°C (A, C, and E) and at 30°C (B and D). (A) Comparison of N315 and its mutant and mecI-gene substituted strains. Symbols: $open circle$ , Eagle-type strain h4; $triangle$ , homo-type strain h4 $Delta$ I; $black-triangle$ , hetero-type strain $Delta$ I;

, homo-type strain $Delta$ I-HR;

, pre-MRSA strain N315;

, homo-type strain h4-4R. (B to E) Comparison of N315 and its transformants. Symbols:

, N315; $open circle$ , LR5; $black-triangle$ , N315(pYT3);

, N315(pHMR-A); $black-lozenge$ , N315(pHMR-B);

, LR5(pHMR-A); $diamond$ , LR5(pHMR-B).

To see if the Eagle-type phenotype is stably maintained during passage, h4 was serially cultivated for 7 days in drug-freemedium as well as in the medium containing 128 µg of methicillinper ml. In both cases, the cultures showed essentially the samepopulation curve, and no mutation was detectable in either mecIgene or in the operator region of mecA gene. Thus, this phenotypewas considered stable enough to be analyzed further with variousexperimentalprocedures.

There was a clear correlation between the appearance of mutants with Eagle-type resistance and the concentrations of methicillinused for the selection of the mutants. Table 2 shows that themutants with Eagle-type resistance were predominantly obtainedfrom N315 when selected with a concentration of methicillin of32 µg/ml or greater. On the other hand, lower concentrations ofmethicillin (4 to 16 µg/ml) predominantly selected heteroresistantmutants. All of the five Eagle-type mutants obtained with eachselective concentration of methicillin (32, 64, 128, 256, and512 µg/ml; Table 2) retained intact mecI gene and mecA gene operatorregion. Table 2 also shows that no mutant with homo-type methicillinresistance was obtained in the selection procedures, indicatingthat the homoresistant mutants do not emerge within the cell populationof N315 at a high frequency comparable to those with Eagle-typeor hetero-type mutants: the appearance rates for the latter werein the range of 10⁴ to 10⁵.

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TABLE 2. Phenotypic expression of methicillin resistance of the mutants obtained by selecting N315 with various concentrations of methicillin

Conversion of Eagle-type resistance to homo methicillin resistance by mecI gene inactivation. Eagle-type strain h4 was plated onto the heart infusion agar containing a low concentration of methicillin (4 µg/ml). Afterincubation overnight at 37°C, a number of colonies grew at a platingefficiency of 3.2 × 10⁴. Ten such colonies were picked, grown in drug-free medium, andsubjected to population analysis. All 10 strains had homo-typemethicillin resistance. The population curve of representativestrain h4-4R is shown in Fig. 1A. Nucleotide sequence determinationof the mecI gene of strain h4-4R revealed a point mutation thatcaused an amino acid substitution from Glu₇₄ to Gly in the MecIprotein. This observation suggested that inactivation of MecIwas responsible for the Eagle-type-to-homo-type phenotypic conversion.To prove this hypothesis, the mecI gene of h4 was substitutedby the tetL gene (17). The resultant strain h4 $Delta$ I expressed homo-typeresistance, as judged by population analysis (see Fig. 1A).

PBP2' production in Eagle-type strain in response to various concentrations of methicillin. The methicillin-induced production of PBP2' in the Eagle-type strain h4 was studied in comparison with those in other teststrains with various types of methicillin resistance (Fig. 2).The intensity of the PBP2' band of each lane was measured by densitometryand is shown under the lane as a value relative to that of $Delta$ Iwithout methicillin induction (Fig. 2A, lane 5). The amount ofPBP2' induced by methicillin was measured 1 h after exposure to1, 8, or 128 µg of methicillin per ml, respectively. Because ofthe mecI gene-mediated repression of mecA gene transcription (17),N315 produced a very-low-level amount of PBP2' before induction,which was scarcely visible in the assay (Fig. 2A, lane 1). Inductionwith 1 and 8 µg of methicillin per ml could not induce PBP2' productionappreciably (Fig. 2A, lanes 2 and 3).

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FIG. 2. PBP2' production induced by various concentrations of methicillin. (A) Western blot of PBP2' after 1 h of induction with methicillin. The strains are N315 (lanes 1 to 4), $Delta$ I (lanes 5 to 8), and $Delta$ I-HR (lanes 9 to 12). The methicillin concentrations used for induction were 0, 1, 8, and 128 µg/ml from left to right for each strain. (B) Same experiment as in panel A with strains h4 (lanes 2 to 5) and h4 $Delta$ I (lanes 6 to 9). Lane 1 is $Delta$ I without induction (the same sample for the lane 5 of panel A). (C) Comparison of PBP2' amount in strain h4 during growth in 128 µg of methicillin per ml (lane 1) and that after 1-h induction with 128 µg of methicillin per ml (lane 2). The values under the lanes are relative amounts of PBP2' as determined by densitometry to that of strain $Delta$ I without induction as a unit of comparison for panels A and B and to that of h4 for panel C.

In contrast, N315 was found to produce detectable amount of PBP2' when 128 µg of methicillin per ml was used for the induction(Fig. 2A, lane 4). The amount of induced PBP2' was comparableto that in $Delta$ I without induction (lane 5), but the amount was only12% of that produced in $Delta$ I after induction with 128 µg of methicillinper ml (compare lanes 4 and 8). This induction profile of N315greatly contrasted with those of strains $Delta$ I (Fig. 2A, lanes 5to 8) and $Delta$ I-HR (Fig. 2A, lanes 9 to 12), in which productionof PBP2' was derepressed because of the absence of the mecI gene.The PBP2' production in $Delta$ I was still partially suppressed, presumablydue to the presence of the blaI-blaRI regulatory complex carriedby the penicillinase plasmid (8), and was increased by 4.4,5.8, and 6.2 times upon induction with 1, 8, and 128 µg of methicillinper ml, respectively. Elimination of the penicillinase plasmidfrom $Delta$ I made it a constitutive producer of PBP2', whose PBP2'amount was comparable to those in $Delta$ I after methicillin induction(data notshown).

It was noticed that the amounts of PBP2' produced in $Delta$ I-HR, a methicillin-selected homoresistant derivative of $Delta$ I, exceededthose of $Delta$ I by 6.2 times before induction (compare lanes 5 and9) and by 1.4- to 2.3 times upon methicillin induction (comparelanes 6 to 8 and 10 to 12). However, the "induction ratio" (definedby dividing the PBP2' amount produced after induction by thatbefore induction) of $Delta$ I-HR (1.4 to 1.6) was smaller than thatof $Delta$ I (4.4 to 6.2).

PBP2' production in h4 in response to methicillin was essentially the same as in N315 (Fig. 2B, lanes 2 to 5). PBP2' productionwas strongly repressed both before and after induction with 1or 8 µg of methicillin per ml. However, PBP2' induction was evidentafter exposure to 128 µg of methicillin per ml, and an amountof PBP2' comparable to that of N315 was produced (compare lane5 in Fig. 2B with lane 4 in Fig. 2A). The amount, however, wasstill only 24% of that produced by the homoresistant strain h4 $Delta$ Ibefore methicillin induction (Fig. 2B, lane 6). Strain h4 $Delta$ I hada pattern of PBP2' induction (lanes 6 to 9) which was quite similarto that of $Delta$ I-HR. PBP2' production in h4 $Delta$ I was derepressed muchfurther than in the heteroresistant strain $delta$ I, and, as in $Delta$ I-HR,the "induction ratio" (1.7 to 1.8) was smaller than that in $Delta$ I.

Figure 2C shows the comparison of PBP2' amounts produced by the strain h4 after cultivation for 1 and 12 h in the heart infusionbroth containing 128 µg of methicillin per ml. The amount of PBP2'produced in h4 after prolonged culture in methicillin-containingmedium was comparable to, and only slightly greater than, thatproduced after 1 h exposure tomethicillin.

Paradoxical effect of methicillin in the cytokilling activity against Eagle-type strain h4. Figure 3 illustrates short-time killing curves of N315 and is derivative strains with various methicillin resistance phenotypes.N315 cells were killed by methicillin in a dose-dependent manner,i.e., the viable cell count decreased from 7.9 × 10⁵ CFU at time zero to 1.9 × 10⁵ CFU at 4 h in the presence of 8 µg of methicillin per ml andto 4.9 × 10⁴ CFU at 4 h in the presence of 128 µg of methicillin per ml (Fig.3A). The heteroresistant strain, $Delta$ I, showed resistance to 8 µgof methicillin per ml (the cell count increased at 4 h; Fig. 3B).However, it showed an enhanced susceptibility to 128 µg of methicillinper ml: the cell count decreased by 3 log₁₀ units (from 1.1 ×10⁶ CFU at time zero to 1.1 × 10³ CFU at 4 h; Fig. 3B). This enhanced susceptibility of $Delta$ I to ahigh concentration of methicillin disappeared in its homo-convertedmutant strain $Delta$ I-HR (Fig. 3C). No apparent decrease in the viablecell count was observed with the strain after a 4-h exposure to128 µg of methicillin per ml.

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FIG. 3. Methicillin time-kill study of N315 and its derivative strains with various methicillin-resistance phenotypes. The tested strains were N315 (A), $Delta$ I (B), $Delta$ I-HR (C), h4 (D), h4 $Delta$ I (E), h4-4R (F), N315(pYT3) (G), N315(pHMR-A) (H), and N315(pHMR-B) (I). Cytokilling was performed in the presence of methicillin at concentrations of 0 ( $open circle$ ), 1 (

), 8 (

), and 128 ( $black-triangle$ ) µg/ml. Viable cell counts were done at 1, 2, and 4 h after the start of culture. The incubation temperature was 37°C for panels A to F and 30°C for panels G to I. Note that the cytokilling activity of methicillin at 128 µg/ml was remarkably decreased with the strains with the Eagle-type or the homo-type methicillin resistance and with the transformant strains harboring multiple copies of hmrA or hmrB genes.

Eagle-type strain h4 (Fig. 3D) showed almost equivalent susceptibility with that of N315 to 8 µg of methicillin per ml (84%decrease; from 1.4 × 10⁶ CFU at time zero to 2.2 × 10⁵ CFU at 4 h; compare closed-square lines in panels A and D). However,h4 exhibited reduced susceptibility to the cytokilling activityof methicillin at 128 µg/ml; no reduction in the cell count wasobserved at 4 h (1.4 × 10⁶ CFU) compared to that at time zero (1.4 × 10⁶ CFU) (Fig. 3D). The mecI-inactivated strain h4 $Delta$ I showed resistanceto all the tested concentrations of methicillin as shown in Fig.3E, which was also the case with h4-4R (Fig. 3F).

Isolation of N315 transformants with Eagle-type methicillin resistance. To identify a responsible gene involved in the expression of Eagle-type methicillin resistance, in screening 22,580 N315 transformantsby replica plating as described in Materials and Methods, we obtainedthree transformant strains whose colony sizes were greater onthe plate containing 100 µg of methicillin per ml than on theplate containing a 10-µg/ml concentration of the antibiotic (Eaglephenotype; see above). By restriction mapping analysis of therecombinant plasmids extracted from the transformants, two ofthe three had an identical restriction pattern. Therefore, thetwo different plasmids were designated pHMR-A and pHMR-B, respectively.The plasmids, amplified in E. coli JM109, were then introducedinto strain N315 and the hetero-type strain LR5, and their methicillinresistance phenotypes were evaluated by population analysis (Fig.1B to E). The analysis was performed both at 30°C (Fig. 1B andD; the copy number of plasmid is 14) and at 37°C (Fig. 1C andE; the copy number is 1). When introduced into N315, both plasmidscaused Eagle-type methicillin resistance, although the sizes ofhighly methicillin-resistant subpopulations were different inthe two transformants, and they changed depending on thetemperature.

Heteroresistant strain LR5 had a higher level of resistance at 30°C than at 37°C but showed typical hetero-type methicillinresistance at both temperature (compare Fig. 1B and C). When pHMR-Awas introduced into LR5, homo-type methicillin resistance wasexpressed at both temperatures (Fig. 1B and C). On the other hand,introduction of plasmid pHMR-B into LR5 could not confer completehomo-type methicillin resistance to LR5, although it did increasethe level of methicillin resistance significantly at both temperatures(Fig. 1D and E). Introduction of vector plasmid pYT3 did not changethe pattern of resistance of N315 or LR5 (Fig. 1B toE).

Localization of ORFs responsible for Eagle-type resistance. Restriction maps and the location of open reading frames (ORFs) found in the inserted DNAs of pHMR-A and pHMR-B are illustratedin Fig. 4. To localize the function conferring the Eagle phenotype,subcloning of the inserted DNAs was performed either by restrictionenzyme cleavage or by PCR amplification of a part of the inserts.The constructed recombinant plasmids were introduced into N315,and their ability to confer Eagle-type resistance to N315 wasevaluated by population analysis. The correlation between thetested DNA fragments and their ability to confer Eagle phenotypesto N315 is summarized in Fig. 4. For the orf1 of pHMR-A, we constructedplasmid pHMR-A5* that carried a single frameshift mutation atNdeI site. The plasmid did not cause Eagle phenotype when introducedin N315 (Fig. 4A). With these studies, the activity to conferEagle phenotype to N315 was localized to one ORF of each plasmid;the ORF of pHMR-A was designated hmrA (standing for high methicillinresistance), and that of pHMR-B was designated hmrB.

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FIG. 4. Restriction map and functional assignment of pHMR-A and pHMR-B insert DNAs. Restriction maps and distribution of ORFs of pHMR-A (A) and pHMR-B (B) inserts are shown. Abbreviations for restriction enzymes: S, Sau3AI; E, EcoRI; H, HindIII; N, NcoI; T, Tth111I; Sal, SalI, B, BamHI. The locations of the subcloned fragments and their capability of conferring Eagle phenotype (denoted as +) to N315 are illustrated to the right of the recombinant plasmid names harboring the fragments. See Materials and Methods for the detailed method of constructing each recombinant plasmid. In the case of pHMR-A5*, a frameshift mutation was introduced at the NdeI site (indicated by a closed arrowhead) of orf1; the location of the premature stop codon generated by this procedure is indicated by an open arrowhead. Dotted arrows show the direction of transcription of the ORFs. The function to confer Eagle-type resistance to strain N315 was confined to orf1 in pHMR-A and orf2 in pHMR-B; they were designated hmrA and hmrB, respectively.

Deduced amino acid sequences encoded by hmrA and hmrB. The predicted amino acid sequences, HmrA and HmrB, encoded by hmrA and hmrB, respectively, are shown in Fig. 5. The aminoacid sequences of HmrA and HmrB were aligned with those of theextant proteins having the highest homology score. The proteinwith the highest homology score to HmrA was AmiB of Mycobacteriumtuberculosis that showed 33% amino acid identity to HmrA overthe 380 aligned sequences (Fig. 5A). AmiB is a probable amidohydrolaseprotein of M40 family with unknown physiological function. Figure5B shows that HmrB had the highest homology score to constitutiveacyl-carrier protein of Rhizobium leguminosarum; the amino acididentity was 66% over 72 aligned sequences. A characteristic prostheticgroup attachment site serine of acyl-carrier protein was alsopresent in HmrB (indicated by the arrow in Fig. 5B).

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FIG. 5. Deduced amino acid sequences of HmrA and HmrB. Amino acid sequence of HmrA is aligned with AmiB (a probable aminohydrolase) of M. tuberculosis (A), and that of HmrB is aligned with the ACP of R. leguminosarum (B). Amino acid residues identical and similar between the two peptides are indicated by asterisks and dots, respectively. The boxed sequences, a to d, are parts of sequences that were well conserved among amidohydrolase proteins of the M40 family. The serine residue implicated as the attachment site for prosthetic group of the ACP is indicated by an arrow in panel B.

The nucleotide sequencing of hmrA and hmrB genes in N315 and h4 was performed to reveal that they were identical between thetwo strains in both coding frames, as well as in promoter regions.A BLAST search was performed to identify the genes in other S.aureus strains. The genes were found as unique genes in all thefour strains whose genomic sequence data are available (i.e.,strains COL, NCTC8325, E-MRSA-16, and MSSA 146). The amino acidsequences of HmrB of the four S. aureus strains were identical.On the other hand, HmrA of N315 and h4 differed by one amino acidsubstitution from that of EMRSA-16 (Gly₇₁ to Asp) and from thoseof COL, NCTC8325, and strain 476 (Pro₂₇₆ toArg).

The hmr genes confer high-dose tolerance to methicillin. Figures 3G to I illustrate the cytokilling curves of the N315-derived transformants harboring plasmids pYT3 (Fig. 3G), pHMR-A(Fig. 3H), and pHMR-B (Fig. 3I). The control transformant N315(pYT3)responded dose dependently to the killing activity of methicillinin the same manner as N315 (Fig. 3A). On the other hand, the transformantsN315(pHMR-A) and N315(pHMR-B) had remarkably reduced susceptibilityto the killing effect of methicillin at 128 µg/ml, a finding whichwas comparable to that observed with N315-derived Eagle-type mutantstrain h4. Thus, both hmr genes encoded the function that conferN315 high-dose tolerance or the paradoxical phenotype to methicillin-inducedkilling.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

It is well established that PBP2' production is prerequisite for the expression of methicillin resistance (18). Since Eagle-typestrain h4 was capable of growth in the presence of high concentrationsof methicillin (Fig. 1), it was predictable that PBP2' was induciblewith a high concentration of methicillin. The amount of PBP2'induced in h4, however, was several times smaller than those expressedin hetero- or homoresistant strains. In contrast, the methicillin-heteroresistantstrain $Delta$ I produced a far greater amount of PBP2' than h4 but didnot grow in the presence of 128 µg of methicillin per ml (Fig.1). This reconfirms the previous reports that high productionof PBP2' alone is not enough for the high-level or homoresistanceexpression of MRSA, and expression of some factor other than mecAgene referred to as chr* is involved in the hetero-to-homo conversionof methicillin resistance (2). Ryffel et al. (23), however,did not look for a phenotypic expression of chr* mutation alone,i.e., a phenotypic change caused by chr* mutation itself in theabsence of the combined function of PBP2'.

In this study, we observed that there was a significant difference between N315 and h4 in terms of vulnerability of cellsto methicillin-induced cytokilling (Fig. 3). Pre-MRSA strain N315was killed by methicillin dose dependently, whereas the Eagle-typestrain h4 was paradoxically resistant to high concentrations ofmethicillin. This resembles the "high-dose tolerance" or "paradoxicaleffect" observed first by Eagle and Musselman (7). We considerthat the tolerance to a high concentration of methicillin is thephenotypic expression of chr* mutation in the genetic backgroundof pre-MRSA strain N315, i.e., under mecI gene-mediated mecA generepression.

Figure 6 summarizes the proposed evolutionary status of Eagle-type resistance described in this study in correlation withother phenotypes of methicillin resistance. There are two alternateevolutionary pathways for pre-MRSA to acquire the homo-type methicillinresistance, and Eagle-type resistance is assigned to the intermediatestage in one of the evolutionary pathways. Since mecI gene inactivationis common in both pathways, the genetic event underlying the conversionfrom pre-MRSA to the Eagle phenotype is considered to be equivalentto that underlying the hetero-to-homo phenotypic conversion, thelatter having been designated as chr* mutation by Ryffel et al.(23). This hypothetical equation was further supported by oursuccessful cloning of hmr genes that conferred both pre-MRSA-to-Eagleand hetero-to-homo conversions to the host strain with respectivephenotype.

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FIG. 6. Two pathways of acquisition of homo-type methicillin resistance by pre-MRSA strain N315. Two sequencial genetic alterations, mecI inactivation and chr* mutation (see the text) are required for N315 to achieve homo-type methicillin resistance. We propose that the phenotypic expression of chr* mutation in the pre-MRSA genetic background corresponds to the Eagle phenotype.

It is noteworthy that the heteroresistant strain $Delta$ I producing a high amount of PBP2' exhibited much greater susceptibilityto 128 µg of methicillin per ml than did N315 (Fig. 3B). The reasonfor this hypersusceptibility is unknown, but it could be due todeleterious effect of PBP2' overproduction on the cell wall synthesisof S. aureus cell. PBP2' is reported to be an inefficient transpeptidasein S. aureus cell (6). Therefore, overexpression of the exogenousPBP2 might have caused a decrease in the cross-linkage of thecell wall, resulting in the increased susceptibility to beta-lactamaction. In that sense, the chr* mutation may be considered asa "counter mutation" to complement the weakness of the host cellwall produced by the expression of PBP2'. In this hypothesis,derepression production of PBP2' would be regarded as an "internalselective pressure" for the evolution of hostcells.

Many genes, designated fem or aug, have been reported whose genetic alteration affect the expression of homo-type methicillinresistance in MRSA (2). Most of the genes have been identifiedby transposon mutagenesis of S. aureus strains expressing homo-typemethicillin resistance. They are the genes whose partial or completeinactivation lead to the decrease in the methicillin resistance,and most of the genes encode enzymes involved in the cell wallsynthesis of S. aureus cell. We approached this problem from adifferent direction, i.e. we adopted the Eagle phenotype as theassay for cloning the genes responsible for hetero-to-homo conversionof methicillinresistance.

With regard to the fem and aug genes, little is known about how frequently these genes are involved in the hetero-to-homoconversion of methicillin resistance. In the case of hmr genes,we have recently analyzed 10 each of the N315-derived mutant strainswith Eagle- and homo-type methicillin resistance. We found thatthe hmrA overexpression, defined as such when the amount of hmrAtranscript in the mutant strain exceeded that in N315(pHMR-A)at 37°C as measured by quantitative reverse transcription-PCR(4), was found in one strain (10%) of Eagle-type and two strains(20%) of homo-type resistance (H. Kuroda-Murakami et al., unpublishedresults). On the other hand, no strain with hmrB overexpressionwas found among the mutant strains. Curiously, overexpressionof hmrA or hmrB gene was not observed in strain h4. Therefore,it is probable that some other alternate genetic mechanisms existthat cause the expression of homo- and Eagle-type methicillinresistance.

The mechanism how chr* mutation causes high-dose tolerance to methicillin will become clear through the study of hmr genefunction. HmrA had a considerable homology to the amidohydrolaseof M40 family, into which many enzymes of diverse physiologicalor unknown functions are classified, e.g., AmiB of M. tuberculosis,hippuricase of Campylobacter jejuni (10), N-carbamyl-L-aminoacid aminohydrolase of Pseudomonas species (34), N-acyl-L-aminoacid amidohydrolase of Bacillus stearothermophilus (25), andthermostable carboxypeptidase of Sulfolobus solfataricus (5).At this moment, we cannot infer any plausible function of HmrAto lead to the tolerance to methicillin caused by itsexpression.

HmrB, on the other hand, turned out to be the S. aureus homologue of acyl carrier protein (ACP). The hmrB gene homologue foundin the Bacillus subtilis genome corresponded to the unique ACPgene acpA (accession no. CAB 13465). hmrB corresponds to the uniqueACP gene homologue in N315 chromosome based on a homology searchover the complete nucleotide sequence of N315 genome (K. Hiramatsu,unpublished data). ACP is a small acidic protein having multiplefunctions in the biosynthesis of macromolecules in bacteria. Theprotein is involved in the synthesis of fatty acids (33), phospholipids(22), aromatic polyketides (14), membrane-derived oligosaccharides(31), and lipopolysaccharides such as lipid A (3). The importanceof ACP-dependent protein acylation has also been demonstratedin posttranslational protoxin activation in bacteria, e.g., inthe conversion of prohemolysin into hemolysin in pathogenic E.coli (15). It is tempting to speculate that overproduction ofACP in the cell may cause tolerance through the stabilizationof the autolytic activity by increasing the synthesis of lipoteichoicacid, which is known as a stabilizer of autolysin in S. aureus(29). Alternatively, ACP may function through enhancing cellwall synthesis of S. aureus, since an increased amount of ACPmay lead to the increased production of undecaprenol, the membranelipid known as the carrier of murein monomer precursors (27).A study is under way to clarify the molecular mechanism how HmrAand HmrB confer high methicillin resistance to S. aureus.

In conclusion, we have described Eagle-type resistance as a novel phenotype of methicillin resistance. We propose that itis the phenotype caused by chr* mutation responsible for the hetero-to-homoconversion of methicillin resistance under the mec regulator genecontrol of mecA genetranscription.

	ACKNOWLEDGMENTS

This work was supported by Core University Program under Japan Society for the Promotion of Science, coordinated by the Universityof Tokyo, Graduate School of Medicine and Universiti Sains Malaysia,School of Medical Sciences, and by Specially Designated ResearchPromotion of Monbusho,Japan.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Bacteriology, Juntendo University, 2-1-1 Hongo, Bunk-yo-ku, Tokyo 113-8421,Japan. Phone: 81-3-5802-1040. Fax: 81-3-5684-7830. E-mail: hiram{at}med.juntendo.ac.jp.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Asada, K., Y. Inaba, E. Tateda-Suzuki, K. Kuwahara-Arai, T. Ito, and K. Hiramatsu. 1995. Evolution and resistance expression of MRSA: evaluation of beta-lactam antibiotics against a set of isogenic strains with different types of phenotypic expression. Acta Biochim. Polon. 42:517-524[Medline].

2. Berger-Bachi, B., and M. Tschierske. 1998. Role of Fem factors in methicillin resistance Drug Resist. Updates 1:325-335.

3. Brozek, K. A., and C. R. H. Raetz. 1990. Biosynthesis of lipid A in Escherichia coli:acyl carrier protein-dependent incorporation of laurate and myristate. J. Biol. Chem. 265:15410-15417[Abstract/Free Full Text].

4. Christiane, G., C. Silvia, G. B. Manfred, D. Gerd, B. Konrad, and W. Christiane. 2000. Direct quantitative transcript analysis of the agr regulon of Staphylococcus aureus during human infection in comparison to the expression profile in vivo. Infect. Immun. 68:1304-1311[Abstract/Free Full Text].

5. Colombo, S., S. De Auria, P. Fusi, L. Zecca, C. A. Raia, and P. Tortora. 1992. Purification and characterization of a thermostable carboxypeptidase from the extreme thermophilic archaebacterium Sulfolobus solfataricus. Eur. J. Biochem. 206:349-357[Medline].

6. De Jonge, B. L. M., and A. Tomasz. 1993. Abnormal peptidoglycan produced in a methicillin-resistant strain of Staphylococcus aureus grown in the presence of methicillin: functional role for penicillin-binding protein 2A in cell wall synthesis. Antimicrob. Agents Chemother. 37:342-346[Abstract/Free Full Text].

7. Eagle, H., and A. D. Musselman. 1948. The rate of bactericidal action of penicillin in vitro as a function of its concentration, and its paradoxically reduced activity at high concentrations against certain organisms. J. Exp. Med. 88:99-131[Abstract].

8. Hackbarth, C. J., and H. F. Chambers. 1993. blaI and blaR1 regulate beta-lactamase and PBP2a production in methicillin-resistant Staphylococcus aureus. Antimicrob. Agents Chemother. 37:1144-1149[Abstract/Free Full Text].

9. Hanaki, H., K. Kuwahara-Arai, S. Boyle-Vavra, R. S. Daum, H. Labischinski, and K. Hiramatsu. 1998. Activated cell-wall synthesis is associated with vancomycin resistance in methicillin-resistant Staphylococcus aureus clinical strains Mu3 and Mu50. J. Antimicrob. Chemother. 42:199-209[Abstract/Free Full Text].

10. Hani, E. K., and V. L. Chan. 1995. Expression and characterization of Campylobacter jejuni benzoylglycine amidohydrolase (Hippuricase) gene in Escherichia coli. J. Bacteriol. 177:2396-2402[Abstract/Free Full Text].

11. Hartman, B. J., and A. Tomasz. 1984. Low-affinity penicillin-binding protein associated with beta-lactam resistance in Staphylococcus aureus. J. Bacteriol. 158:513-516[Abstract/Free Full Text].

12. Hiramatsu, K. 1995. Molecular evolution of MRSA. Microbiol. Immunol. 39:531-543[Medline].

13. Hiramatsu, K., K. Asada, E. Suzuki, K. Okonogi, and T. Yokota. 1991. Molecular cloning and nucleotide sequence determination of the regulator region of mecA gene in methicillin-resistant Staphylococcus aureus (MRSA) FEBS Lett. 298:133-136.

14. Hopwood, D. A., and D. H. Sherman. 1990. Molecular genetics of polyketides and its composition to fatty acid biosynthesis. Annu. Rev. Genet. 24:37-66[CrossRef][Medline].

15. Issartel, J.-P., V. Koronakis, and C. Hughes. 1991. Activation of Escherichia coli prohaemolysin to the mature toxin by acyl carrier protein-dependent fatty acylation. Nature 351:759-761[CrossRef][Medline].

16. Katayama, Y., T. Ito, and K. Hiramatsu. 2000. A new class of genetic element, Staphylococcus Cassette Chromosome mec, encodes methicillin resistance in Staphylococcus aureus. Antimicrob. Agents Chemother. 44:1549-1555[Abstract/Free Full Text].

17. Kuwahara-Arai, K., N. Kondo, S. Hori, E. Tateda-Suzuki, and K. Hiramatsu. 1996. Suppression of methicillin resistance in a mecA-containing pre-methicillin-resistant Staphylococcus aureus strain is caused by the mecI-mediated repression of PBP2' production. Antimicrob. Agents Chemother. 40:2680-2685[Abstract].

18. Matthews, P., and A. Tomasz. 1990. Insertional inactivation of the mec gene in a transposon mutant of a methicillin-resistant clinical isolate of Staphylococcus aureus. Antimicrob. Agents Chemother. 34:1777-1779[Abstract/Free Full Text].

19. Matthews, P. R., and P. R. Stewart. 1984. Resistance heterogeneity in methicillin-resistant Stapylococcus aureus. FEMS Microbiol. Lett. 22:161-166[CrossRef].

20. Nilsson, B., L. Abrahmsen, and M. Uhlen. 1985. Immobilization and purification of enzymes with staphylococcal protein A gene fusion vectors. EMBO J. 4:1075-1080[Medline].

21. Reynolds, P. E., and C. Fuller. 1986. Methicillin-resistant strains of Staphylococcus aureus: presence of identical additional penicillin-binding protein in all strains examined. FEMS Microbiol. Lett. 33:251-254[CrossRef].

22. Rock, C., and S. Jackowski. 1982. Regulation of phospholipid synthesis in Escherichia coli. Composition of the acyl-acyl carrier protein pool in vivo. Biol. Chem. 257:10759-10765[Abstract/Free Full Text].

23. Ryffel, C., A. Strassle, F. H. Kayser, and B. Berger-Bachi. 1994. Mechanism of heteroresistance in methicillin-resistant Staphylococcus aureus. Antimicrob. Agents Chemother. 38:724-728[Abstract/Free Full Text].

24. Sabath, L. D., and S. J. Wallace. 1971. Factors influencing methicillin resistance in staphylococci. Ann. N. Y. Acad. Sci. 182:258-266[Medline].

25. Sakanyan, V., L. Desmarez, C. Legrain, D. Charlier, I. Mett, A. Kochikyan, A. Savchenko, P. Falmagne, A. Pierard, et al. 1993. Gene cloning, sequence analysis, purification, and characterization of thermostable aminoacylase from Bacillus stearothermophilus. Appl. Environ. Microbiol. 59:3878-3888[Abstract/Free Full Text].

26. Sanger, F., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain-terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].

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28. Song, M. D., M. Wachi, M. Doi, F. Ishino, and M. Matsuhashi. 1987. Evolution of an inducible penicillin-target protein in methicillin-resistant Staphylococcus aureus by gene fusion. FEBS Lett. 221:167-171[CrossRef][Medline].

29. Sugai, M. 1997. Peptidoglycan hydrolases of the staphylococci J. Infect. Chemother. 3:113-127.

30. Tesch, W., C. Ryffel, A. Strassle, F. H. Kayser, and B. Berger-Bachi. 1990. Evidence of a novel staphylococcal mec-encoded element (mecR) controlling expression of penicillin-binding protein 2'. Antimicrob. Agents Chemother. 34:1703-1706[Abstract/Free Full Text].

31. Therisod, H., and E. P. Kennedy. 1987. The function of acyl carrier protein in the synthesis of membrane-derived oligosaccharides does not require its phosphopanthetheine prosthetic group. Proc. Natl. Acad. Sci. USA 84:8235-8238[Abstract/Free Full Text].

32. Utsui, Y., and T. Yokota. 1985. Role of an altered penicillin-binding protein in methicillin- and cephem-resistant Staphylococcus aureus. Antimicrob. Agents Chemother. 28:397-403[Abstract/Free Full Text].

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34. Watanabe, K., T. Ishikawa, Y. Mukohara, and H. Nakamura. 1992. Cloning and sequencing of the genes involved in the conversion of 5-substituted hydantoins to the corresponding L-amino acids from the native plasmid of Pseudomonas sp. strain NS671. J. Bacteriol. 174:962-969[Abstract/Free Full Text].

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1.	Asada, K., Y. Inaba, E. Tateda-Suzuki, K. Kuwahara-Arai, T. Ito, and K. Hiramatsu. 1995. Evolution and resistance expression of MRSA: evaluation of beta-lactam antibiotics against a set of isogenic strains with different types of phenotypic expression. Acta Biochim. Polon. 42:517-524[Medline].
2.	Berger-Bachi, B., and M. Tschierske. 1998. Role of Fem factors in methicillin resistance Drug Resist. Updates 1:325-335.
3.	Brozek, K. A., and C. R. H. Raetz. 1990. Biosynthesis of lipid A in Escherichia coli:acyl carrier protein-dependent incorporation of laurate and myristate. J. Biol. Chem. 265:15410-15417[Abstract/Free Full Text].
4.	Christiane, G., C. Silvia, G. B. Manfred, D. Gerd, B. Konrad, and W. Christiane. 2000. Direct quantitative transcript analysis of the agr regulon of Staphylococcus aureus during human infection in comparison to the expression profile in vivo. Infect. Immun. 68:1304-1311[Abstract/Free Full Text].
5.	Colombo, S., S. De Auria, P. Fusi, L. Zecca, C. A. Raia, and P. Tortora. 1992. Purification and characterization of a thermostable carboxypeptidase from the extreme thermophilic archaebacterium Sulfolobus solfataricus. Eur. J. Biochem. 206:349-357[Medline].
6.	De Jonge, B. L. M., and A. Tomasz. 1993. Abnormal peptidoglycan produced in a methicillin-resistant strain of Staphylococcus aureus grown in the presence of methicillin: functional role for penicillin-binding protein 2A in cell wall synthesis. Antimicrob. Agents Chemother. 37:342-346[Abstract/Free Full Text].
7.	Eagle, H., and A. D. Musselman. 1948. The rate of bactericidal action of penicillin in vitro as a function of its concentration, and its paradoxically reduced activity at high concentrations against certain organisms. J. Exp. Med. 88:99-131[Abstract].
8.	Hackbarth, C. J., and H. F. Chambers. 1993. blaI and blaR1 regulate beta-lactamase and PBP2a production in methicillin-resistant Staphylococcus aureus. Antimicrob. Agents Chemother. 37:1144-1149[Abstract/Free Full Text].
9.	Hanaki, H., K. Kuwahara-Arai, S. Boyle-Vavra, R. S. Daum, H. Labischinski, and K. Hiramatsu. 1998. Activated cell-wall synthesis is associated with vancomycin resistance in methicillin-resistant Staphylococcus aureus clinical strains Mu3 and Mu50. J. Antimicrob. Chemother. 42:199-209[Abstract/Free Full Text].
10.	Hani, E. K., and V. L. Chan. 1995. Expression and characterization of Campylobacter jejuni benzoylglycine amidohydrolase (Hippuricase) gene in Escherichia coli. J. Bacteriol. 177:2396-2402[Abstract/Free Full Text].
11.	Hartman, B. J., and A. Tomasz. 1984. Low-affinity penicillin-binding protein associated with beta-lactam resistance in Staphylococcus aureus. J. Bacteriol. 158:513-516[Abstract/Free Full Text].
12.	Hiramatsu, K. 1995. Molecular evolution of MRSA. Microbiol. Immunol. 39:531-543[Medline].
13.	Hiramatsu, K., K. Asada, E. Suzuki, K. Okonogi, and T. Yokota. 1991. Molecular cloning and nucleotide sequence determination of the regulator region of mecA gene in methicillin-resistant Staphylococcus aureus (MRSA) FEBS Lett. 298:133-136.
14.	Hopwood, D. A., and D. H. Sherman. 1990. Molecular genetics of polyketides and its composition to fatty acid biosynthesis. Annu. Rev. Genet. 24:37-66[CrossRef][Medline].
15.	Issartel, J.-P., V. Koronakis, and C. Hughes. 1991. Activation of Escherichia coli prohaemolysin to the mature toxin by acyl carrier protein-dependent fatty acylation. Nature 351:759-761[CrossRef][Medline].
16.	Katayama, Y., T. Ito, and K. Hiramatsu. 2000. A new class of genetic element, Staphylococcus Cassette Chromosome mec, encodes methicillin resistance in Staphylococcus aureus. Antimicrob. Agents Chemother. 44:1549-1555[Abstract/Free Full Text].
17.	Kuwahara-Arai, K., N. Kondo, S. Hori, E. Tateda-Suzuki, and K. Hiramatsu. 1996. Suppression of methicillin resistance in a mecA-containing pre-methicillin-resistant Staphylococcus aureus strain is caused by the mecI-mediated repression of PBP2' production. Antimicrob. Agents Chemother. 40:2680-2685[Abstract].
18.	Matthews, P., and A. Tomasz. 1990. Insertional inactivation of the mec gene in a transposon mutant of a methicillin-resistant clinical isolate of Staphylococcus aureus. Antimicrob. Agents Chemother. 34:1777-1779[Abstract/Free Full Text].
19.	Matthews, P. R., and P. R. Stewart. 1984. Resistance heterogeneity in methicillin-resistant Stapylococcus aureus. FEMS Microbiol. Lett. 22:161-166[CrossRef].
20.	Nilsson, B., L. Abrahmsen, and M. Uhlen. 1985. Immobilization and purification of enzymes with staphylococcal protein A gene fusion vectors. EMBO J. 4:1075-1080[Medline].
21.	Reynolds, P. E., and C. Fuller. 1986. Methicillin-resistant strains of Staphylococcus aureus: presence of identical additional penicillin-binding protein in all strains examined. FEMS Microbiol. Lett. 33:251-254[CrossRef].
22.	Rock, C., and S. Jackowski. 1982. Regulation of phospholipid synthesis in Escherichia coli. Composition of the acyl-acyl carrier protein pool in vivo. Biol. Chem. 257:10759-10765[Abstract/Free Full Text].
23.	Ryffel, C., A. Strassle, F. H. Kayser, and B. Berger-Bachi. 1994. Mechanism of heteroresistance in methicillin-resistant Staphylococcus aureus. Antimicrob. Agents Chemother. 38:724-728[Abstract/Free Full Text].
24.	Sabath, L. D., and S. J. Wallace. 1971. Factors influencing methicillin resistance in staphylococci. Ann. N. Y. Acad. Sci. 182:258-266[Medline].
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