Received 17 September 2008/Returned for modification 29 October 2008/Accepted 18 November 2008

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1 JOURNAL OF CLINICAL MICROBIOLOGY, Feb. 2009, p Vol. 47, No /09/$ doi: /jcm Copyright 2009, American Society for Microbiology. All Rights Reserved. Identification of Plasmid-Mediated AmpC -Lactamases in Escherichia coli, Klebsiella spp., and Proteus Species Can Potentially Improve Reporting of Cephalosporin Susceptibility Testing Results Fred C. Tenover, 1 Shannon L. Emery, 2 Carol A. Spiegel, 3 Patricia A. Bradford, 4 Samantha Eells, 2 Andrea Endimiani, 5 Robert A. Bonomo, 5 and John E. McGowan, Jr. 2 * Division of Healthcare Quality Promotion, Centers for Disease Control and Prevention, Atlanta, Georgia ; Department of Epidemiology, Rollins School of Public Health, Emory University, Atlanta, Georgia ; Department of Pathology and Laboratory Medicine, University of Wisconsin, Madison, Wisconsin ; Wyeth Research, Pearl River, New York ; and Louis Stokes Department of Veterans Affairs Medical Center, Cleveland Ohio Received 17 September 2008/Returned for modification 29 October 2008/Accepted 18 November 2008 The goal of this study was to determine if the interpretations of extended-spectrum and advanced-spectrum cephalosporins (ESCs and ASCs, respectively) for isolates of Enterobacteriaceae would be impacted by the results of aminophenylboronic acid (APBA) testing. Fifty-three isolates of Escherichia coli,21klebsiella species, and 6 Proteus species that were resistant to at least one ESC were tested by disk diffusion with ceftazidime and cefotetan disks with and without APBA. Ceftazidime disks with and without clavulanic acid (CLAV) were also tested to confirm extended-spectrum -lactamase (ESBL) carriage. Twenty-nine (36.3%) isolates were only APBA test positive, 27 were only CLAV test positive, 2 were positive with both substrates, and 22 were negative with both substrates. Thirteen (41.9%) of the 31 APBA-test-positive isolates (all E. coli) tested susceptible to cefotaxime, ceftriaxone, or ceftazidime. Since clinical data suggest that AmpC-producing isolates should be reported as resistant to all ESCs, APBA testing can be helpful in identifying such organisms. Screening for AmpC-producing organisms using nonsusceptibility to cefoxitin and amoxicillin-clavulanate was less specific than APBA testing; it identified ESBL as well as AmpC-producing organisms. Only 18 of 31 APBA-positive isolates were positive by PCR for an AmpC -lactamase gene. Thus, testing with APBA could improve the accuracy of reporting ESCs, especially for E. coli. However, results of APBA and CLAV testing did not correlate well for isolates containing both AmpC -lactamases and ESBLs. Thus, additional data are needed before formal recommendations can be made on changing the reporting of ASC test results. Downloaded from -Lactamase-mediated resistance to penicillins and cephalosporins is a significant problem among gram-negative bacteria worldwide (2, 4, 17). -Lactamases can be divided into four major classes (A, B, C, and D) based on substrate profiles and amino acid sequences (3, 5). Class A -lactamases include enzymes that are active against penicillins and cephalosporins. Mutations in key positions in class A -lactamase genes can produce extended-spectrum -lactamases (ESBLs) that mediate resistance to extended-spectrum cephalosporins (ESCs), such as cefotaxime (CTX), ceftriaxone, and ceftazidime (CAZ), and, in some cases, the advanced-spectrum cephalosporins (ASCs) cefepime and cefpirome (2, 13, 14). Class C -lactamases, such as the AmpC enzymes, also mediate resistance to ESCs but often remain susceptible to the ASCs, which could be important information for clinicians considering therapy for gram-negative infections. Studies by Coudron (9), Jacoby et al. (12), and Yagi et al. (33) have validated the use of boronic acid derivatives to detect AmpC -lactamases in gram-negative bacilli. Coudron s study (9) included a recommendation that for isolates positive by the * Corresponding author. Mailing address: Department of Epidemiology, Rollins School of Public Health, Emory University, 1518 Clifton Rd., Atlanta, GA Phone and fax: (404) jmcgowa@sph.emory.edu. Present address: Los Angeles BioMedical Research Institute, Torrance, CA Published ahead of print on 26 November boronic acid test all cephalosporin test results be reported as resistant, similar to the Clinical and Laboratory Standards Institute (CLSI) ESBL reporting algorithm. It is not clear if Coudron s recommendation included changing the results with regard to ASCs. The other two studies did not comment on the issue of how to interpret cephalosporin results. CLSI has yet to establish a testing and reporting algorithm specifically for organisms containing AmpC -lactamases. CLSI s algorithm to detect and confirm the presence of ESBLs is limited to isolates of Klebsiella pneumoniae, Klebsiella oxytoca, Escherichia coli, and Proteus mirabilis (6 8). Using the algorithm is critical for accurate test reporting since ESBLproducing organisms often test susceptible to one or more ESCs even though these drugs are not clinically active against infections caused by ESBL-producing organisms (20, 21). Thus, confirmation of the presence of an ESBL in an isolate of E. coli, P. mirabilis, or a Klebsiella species indicates that all penicillin and cephalosporin results should be reported as indicating resistance. However, resistance to ESCs in E. coli, Enterobacter species, and several other species of Enterobacteriaceae can also be the result of mutations that upregulate production of chromosomal AmpC -lactamases or can be the result of acquisition of plasmid-encoded AmpC enzymes among organisms that do not contain a chromosomal AmpC -lactamase gene (24, 32). Pai and colleagues (19) have indicated that organisms that produce AmpC -lactamases, similar to those that produce ESBLs, may test as susceptible to ESCs, on August 14, 2018 by guest 294

2 VOL. 47, 2009 BORONIC ACID TESTING FOR AmpC -LACTAMASES 295 Organism No. of isolates tested g TABLE 1. Results of APBA, CLAV, and AmpC PCR tests for all study isolates No. of isolates positive by APBA test by substrate (family) a CAZ only CTT only CAZ and CTT No. of isolates positive with CLAV and APBA (family) No. of isolates positive with CLAV only b No. of isolates negative with both ABPA and CLAV Escherichia coli 53 7 (2 CIT, 5 NEG c ) 1(1NEG d ) 17 (4 CIT, 1 DHA, 2 (1 EBC, 1 NEG f ) FOX, 5 MOX, 6 NEG e ) Klebsiella oxytoca 7 1 (CIT) 6 0 Klebsiella pneumoniae 14 3 (2 FOX, 1 MOX) 10 1 Proteus mirabilis 1 1 Proteus penneri 1 1 Proteus vulgaris 4 4 Total a Multiplex PCR was performed as described by Perez-Perez and Hanson (23) only on isolates that were positive in the APBA disk diffusion test. NEG, negative PCR assay. PCR results represent families of AmpC genes, not individual determinants (See Materials and Methods). b Organisms were tested previously with CAZ and CTT with and without CLAV per CLSI criteria (7). Results of ESBL production were consistent with previous results. c pi values of -lactamases determined by aief of five PCR negative isolates: (i) 8.5; (ii) 8.9, 8.1, 7.7, 7.0, 6.5; (iii) 9.0; (iv) 9.0; (v) 9.0, 8.8, 5.4. d pi values of -lactamases determined by aief of PCR negative isolate, 6.4. e aief of six PCR negative isolates: (i) 8.4, 5.4; (ii) 8.4, 5.4; (iii) 8.9; (iv) 8.4, 5.3; (v) 9.0, 8.4, 8.0, 7.6, 7.0, 6.4; (vi) 9.2, 8.0, 6.8, 5.4. f aief of PCR negative isolate, 7.3. g All ESBL screen test positive. thus producing misleading clinical information. This suggests that the identification of AmpC -lactamases among E. coli, P. mirabilis, or a Klebsiella species could also increase the accuracy of antimicrobial susceptibility test reports for ESCs if the results were used to modify the interpretations of cephalosporin results. As noted above, in contrast to bacterial isolates containing ESBLs, isolates containing AmpC -lactamases typically remain susceptible to ASCs (13, 14, 26, 27, 31). Although the occurrence is rare, AmpC -lactamases, such as CMY-19, show modest cefepime hydrolyzing activity (31) even though the organisms carrying this -lactamase remain fully susceptible to both cefepime and cefpirome in vitro. Thus, there may be clinical relevance to distinguishing between bacterial isolates containing ESBLs, for which ASC results should be reported as resistant, and those containing AmpC -lactamases, for which ESC results would be reported as resistant but the ASC results would be reported as they test. The major goals of this study were to determine (i) whether testing 3-aminophenylboronic acid hemisulfate (APBA) in conjunction with CAZ and cefotetan (CTT) disks could improve the reporting of results for ESCs and ASCs by indicating which strains contained AmpC -lactamases, (ii) whether using the combination of resistance to amoxicillin-clavulanate and cefoxitin as a surrogate had equivalent sensitivity and specificity to the APBA assay for identifying AmpC -lactamase-producing organisms, (iii) whether organisms containing both ESBLs and AmpC -lactamases would be consistently detected with both clavulanic acid (CLAV) and APBA, and (iv) whether a disk diffusion test using APBA dissolved in water gave comparable results to dissolving the free acid compound in dimethyl sulfoxide (DMSO). With regard to the last goal, one of the drawbacks to using boronic acid is the requirement to dissolve the free acid in DMSO, a toxic chemical not often used in microbiology laboratories. Thus, we hypothesized that a boronic acid compound that did not have to be dissolved in DMSO could improve the general acceptance of the test in clinical laboratories. MATERIALS AND METHODS Bacterial strains. A total of 80 clinical isolates of E. coli, Klebsiella species, and Proteus species collected during a 5-year period from 15 hospitals in the United States that participate in Project ICARE (Intensive Care Antimicrobial Resistance Epidemiology) (11) were tested (Table 1). Sixty-one isolates were previously characterized for ESBL production (18, 28, 30). All isolates were resistant to at least one ESC (i.e., CTX, CAZ, ceftriaxone, or ceftizoxime). The study was conducted in three phases. In phase I, all 80 isolates were tested. In phase II, a subset of 24 isolates from phase I (21 E. coli, 1K. oxytoca, and 2 K. pneumoniae isolates), which had been collected prospectively at the University of Wisconsin because they were nonsusceptible to both cefoxitin (FOX) and amoxicillinclavulanate, were further examined (Table 2). In phase III, an additional 11 isolates (8 E. coli and 2 K. pneumoniae isolates and 1 P. mirabilis isolate) containing multiple -lactamases from the Wyeth Research collection were tested (Table 3). Isolates from phase I were identified using Vitek 2 (biomérieux, Durham, NC) or standard biochemical methods (10). Isolates from phase II were identified using Vitek, conventional biochemical tests, and phenotypic tests, and isolates in phase III were identified using API-20E strips (biomérieux). All isolates were stored at 70 C prior to testing. Each isolate was subcultured on Trypticase soy agar supplemented with 5% sheep blood (BD BioSciences, Sparks, MD) twice before testing. Control strains were kindly provided by the following individuals: E. coli TG1 containing the -lactamase FOX-1 was from George Jacoby (Lahey Clinic, Boston, MA); E. coli isolates containing the DHA-1 and ACC-1 -lactamases were obtained from Nancy Hanson (Creighton University School of Medicine, Omaha, NB); K. pneumoniae containing the CMY-8 was from Jing-Jou Yan (National Cheng Kung University Medical College, Taiwan); and Salmonella enterica AM03430 containing a CMY-2 -lactamase was obtained from Jean Whichard (Centers for Disease Control and Prevention, Atlanta, GA). Disk diffusion testing. BBL Sensi-Disc (6 mm) disks containing 30 g of either CTT, 30 g of CAZ, or 30 g of CAZ plus 10 g of CLAV were purchased from BD BioSciences (Sparks, MD). APBA hemisulfate (120 mg) was dissolved in 6 ml of distilled H 2 O, and 100 mg of APBA was dissolved in DMSO; 30 l of either solution was added to CAZ and CTT disks. Disks were dried for 30 min prior to use or stored at 4 C for up to 1 month without loss of activity. Organisms were suspended in Mueller-Hinton broth to the turbidity of a 0.5 McFarland standard and inoculated onto 150-mm Mueller-Hinton agar plates (BD Biosciences) as for disk diffusion (7). Disks containing 30 g of CTT, 30 g of CAZ, 30 g ofctt plus 600 g of APBA, 30 g of CAZ plus 600 g of APBA, and 30 g of CAZ plus 10 g of CLAV were placed on the plate. (All isolates had previously been

3 296 TENOVER ET AL. J. CLIN. MICROBIOL. TABLE 2. Isolates presumptively positive for AmpC beta-lactamases using cefoxitin and amoxicillin-clavulanic acid screening Organism No. of isolates (n 24) PCR result a result with Cephalosporin phenotype b APBA-positive CAZ CTX CRO FEP CAZ/CTT c E. coli 1 MOX R R R S CAZ, CTT E. coli 2 MOX R I R S CAZ, CTT E. coli 3 MOX R I I S CAZ, CTT E. coli 1 CIT R I R S CAZ, CTT E. coli 1 CIT R S I S CAZ E. coli 2 Negative I S S S CAZ, CTT E. coli 1 Negative R I I S CAZ E. coli 1 Negative R S S S CAZ E. coli 2 Negative I S S S CAZ E. coli 1 Negative R I I S CTT E. coli 1 Negative R R R I Both negative d E. coli 1 Negative S R R I Both negative d E. coli 4 Negative S S S S Both negative K. pneumoniae 1 MOX R I R S CAZ, CTT K. pneumoniae 1 FOX R R I S CAZ, CTT K. oxytoca 1 CIT R R R S CAZ, CTT a The AmpC gene family is indicated for positive results. b CRO, ceftriaxone; FEP, cefepime. Results were interpreted using CLSI criteria (8). R, resistant; I, intermediate; S, susceptible. c Organisms were tested using the disk diffusion method. d ESBL positive. Organism screened for ESBL production by disk diffusion with both CAZ and CTX, with and without CLAV. Thus, in this study we screened only with disks containing CAZ and CAZ plus CLAV to ensure that the ESBL type was consistent with previous results. All ESBL results were consistent). Plates were incubated for 18 to 20 h in ambient air at 35 C. Zone diameter differences of 5 mm between the CTT or CAZ disks without APBA and those supplemented with APBA were considered positive for AmpC -lactamases, as previously described (9, 12, 33). Positive control strains for APBA and PCR testing are listed above. Negative controls for APBA testing included K. pneumoniae ATCC (the ESBLpositive control strain) and E. coli ATCC ESBL testing was performed using CAZ with and without CLAV, as described by CLSI (6). Molecular characterization of -lactamase genes. Organisms were tested for the presence of six families of plasmid-mediated AmpC -lactamase genes using the multiplex PCR assay described by Perez-Perez and Hanson (23). This included the genes within the following families: ACC, CIT (including LAT-1 to LAT-4, CMY-2 to CMY-7, and BIL-1), DHA (DHA-1 and DHA-2), EBC (including MIR-1T and ACT-1), FOX (including FOX-1 to FOX-5b), and MOX (including MOX-1, MOX-2, CMY-1, and CMY-8 to CMY-11). Positive- and negative-control organisms were included in each assay. aief. Analytical isoelectric focusing (aief) was performed to determine the pis of ß-lactamases from isolates, as previously described (22, 34). Briefly, electrophoresis was performed on precast polyacrylamide gels, either ph 3 to ph 10 (Bio-Rad Inc.) or ph 3.5 to 9.5 (GE Healthcare Bio-Sciences AB, Uppsala, Sweden). Isoelectric points were determined by placing filter paper soaked in nitrocefin (500 g/ml; BD Biosciences) on top of the focused gel. Control enzymes included TEM-1 (pi 5.4), TEM-12 (pi 5.25), KPC-2 (pi 6.7), SHV-1 (pi 7.6), SHV-2 (pi 7.6), and CMY-2 (pi 9.0) RESULTS APBA testing. The five AmpC control organisms and the ESBL-positive control (K. pneumoniae ATCC ) and an AmpC -lactamase-negative E. coli isolate were tested in parallel with disks containing CAZ and CTT in combination with either APBA dissolved in DMSO or the APBA hemisulfate salt dissolved in water. The zone diameters around the corresponding pairs of disks containing APBA dissolved in either water or DMSO were within 1 mm for all organisms, and all of the interpretations (positive or negative for AmpC -lacta- TABLE 3. Test results for isolates containing both ESBL and AmpC beta-lactamases -Lactamases ESBL detected using CLAV AmpC detected using APBA Interpretation of susceptibility testing to (method): a Cefepime (MIC/ disk diffusion) E. coli CTX-M-5, CTX-M-28, ACT-1 Yes No R/R R E. coli CTX-M-2, ACT-1 Yes No R/R R E. coli CTX-M-5, ACT Yes No R/R R E. coli CTX-M-2, CTX-M-28, ACT-1 Yes No R/R R P. mirabilis CTX-M-15, DHA No Yes S/S R E. coli CTX-M-15, ACT-1 Yes No R/R R E. coli CTX-M-3, ACT-1 No No R/I R K. pneumoniae SHV-type, b CTX-M-2, DHA No Yes S/S S c E. coli SHV-5, CTX-M-2, CMY No Yes S/S I E. coli TEM-1, SHV-7, CMY-2 Yes Yes R/S R K. pneumoniae TEM-1, TEM-10, SHV-7, ACT-1 No Yes S/S R Ceftriaxone (MIC) a R, resistant; I, intermediate; S, susceptible. b Positive for SHV-type -lactamase by PCR assay, but DNA sequence was not determined. c Ceftriaxone MIC of 4 g/ml.

4 VOL. 47, 2009 BORONIC ACID TESTING FOR AmpC -LACTAMASES 297 mase genes) were the same for each pair. Thus, the results for the APBA hemisulfate salt dissolved in water were comparable to the results of the free acid dissolved in DMSO (data not shown). The remainder of the testing was performed using the APBA hemisulfate salt dissolved in water. In phase I, a total of 80 clinical isolates of E. coli, Klebsiella species, and Proteus species that were resistant to one or more ESCs were tested by disk diffusion with CAZ and CTT disks with and without APBA and with CAZ disks with and without CLAV. As shown in Table 1, 29 (36.3%) isolates were positive only with APBA (an increase in zone diameter of 5 mm with either CAZ only [7 isolates], CTT only [1 isolate], or both drugs [21 isolates]), 27 were positive only with CLAV (indicating ESBL production), 2 were positive with both substrates, and 22 were negative with both substrates. The CLAV-positive results for the 27 isolates were consistent with those of our previous studies on ESBL production (18, 28, 30). Of the 31 APBA-positive isolates (including the two that were also CLAV positive), 13 (41.9%, all E. coli) tested as susceptible to at least one ESC. The other 18 isolates were intermediate or resistant to CTX, CAZ, ceftriaxone, and cefpodoxime. Twentyeight of the 29 (96.5%) APBA-positive isolates that were CLAV negative tested susceptible to the ASC cefepime (MIC 8 g/ml) (data not shown). Surprisingly, only 18 of the 31 APBA-positive isolates were positive for an AmpC gene product by PCR (Table 1) although all 31 had an IEF product compatible with either the -lactamase gene identified or a pi 8.3 (33) (Table 1). The genes present encoded -lactamases in the CIT, DHA, EBC, FOX, and MOX families (see Materials and Methods for lists of -lactamases included in each family). Screening for AmpC-containing organisms using cefoxitin and amoxicillin-clavulanate results. In the second phase of the study, we evaluated whether an alternate strategy to APBA testing, i.e., using nonsusceptibility to both cefoxitin and amoxicillin-clavulanate, was an accurate indicator of AmpC -lactamase-producing organisms. Twenty-four isolates, all of which had been collected prospectively at a single institution, were evaluated. The organisms included 21 E. coli and 2 K. pneumoniae isolates and 1 K. oxytoca isolate that were intermediate or resistant to cefoxitin and amoxicillin-clavulanate and intermediate or resistant to at least one ESC by Vitek testing (Table 2). Two E. coli isolates that were intermediate to either cefoxitin or amoxicillin-clavulanate were positive for ESBLs by CLAV testing and negative with APBA. Four additional E. coli isolates, although resistant to cefoxitin and amoxicillin-clavulanate, were susceptible to CAZ, ceftriaxone, CTX, and cefepime by broth microdilution reference testing and gave negative test results with APBA. The remaining 18 isolates, which included the three Klebsiella species isolates, were resistant to both cefoxitin and amoxicillin-clavulanate and intermediate or resistant to at least one ESC; all gave a positive APBA test (Table 2), indicating AmpC -lactamase carriage. There were seven different cephalosporin resistance phenotypes among the 15 E. coli isolates. While all of the APBApositive E. coli isolates were either intermediate or resistant to CAZ, four remained susceptible to CTX, ceftriaxone, or both; however, all were susceptible to cefepime (MIC of 8 g/ml). Twelve of 18 APBA-positive isolates (which include the three Klebsiella species isolates) were APBA positive with both CAZ and CTT disks, 5 E. coli isolates were APBA positive with only the CAZ disk, and 1 E. coli isolate was APBA positive with only the CTT disk. Among the 18 isolates that were APBA positive, 7 contained a MOX family -lactamase gene (6 E. coli isolates and 1 K. pneumoniae isolate), 1 K. oxytoca and 1 E. coli isolate each contained a CIT family -lactamase gene, and 1 K. pneumoniae isolate contained a FOX family gene. Isolates harboring multiple -lactamases. In addition to the original 80 isolates tested, eight E. coli, one P. mirabilis, and three K. pneumoniae isolates that had previously been shown to express both ESBLs and AmpC -lactamases were tested using both APBA and CLAV (Table 3). One E. coli isolate containing a known ESBL (CTX-M-3) and an AmpC -lactamase (ACT-1) gave false-negative results for both ABPA and CLAV. A second E. coli isolate containing TEM-1, SHV-7, and CMY-2 gave true-positive results for both APBA and CLAV. Four additional E. coli isolates, each containing a combination of a CTX-M and ACT-1 -lactamases, gave truepositive results for the CLAV test but were falsely negative with APBA. All four also tested resistant to cefepime by MIC and disk diffusion. On the other hand, two K. pneumoniae isolates and an E. coli isolate that each contained an SHV and AmpC -lactamase in conjunction with either a CTX-M or TEM -lactamase gave false-negative CLAV results but truepositive APBA results (Table 3). All three organisms were cefepime susceptible by both MIC and disk diffusion testing. Thus, the results of APBA and CLAV testing rarely correlated with isolates containing both AmpC -lactamases and ESBLs. DISCUSSION Pai et al. (19) have shown that AmpC -lactamase-producing K. pneumoniae isolates did not respond clinically to ESCs even when in vitro test results indicated susceptibility to those agents. Our study of a convenience sample of 80 selected isolates of E. coli, Klebsiella species, and Proteus species indicated that 41.9% of APBA test-positive, CLAV test-negative isolates remained susceptible to at least one ESC, indicating the potential for misclassifying isolates of these three species as susceptible to ESCs to which they may not respond clinically. Using the boronic acid test, the accuracy of which has been validated by multiple laboratories (9, 12, 33), to confirm the presence of an AmpC -lactamase could improve the accuracy of test results for the ESCs by reporting these cephalosporin results as resistant. This would be consistent with the CLSI algorithm for ESBL testing and reporting (8). Thus, laboratories should consider performing APBA testing in conjunction with ESBL testing on E. coli, Klebsiella species, and Proteus species to improve the accuracy of susceptibility testing results for all ESCs. An important difference between ESBL- and AmpC-containing organisms is that those containing only AmpC -lactamases often remain susceptible to ASCs, such as cefepime and cefpirome (13, 15, 26, 27). CLSI recommends changing ASC results, such as for cefepime, from susceptible to resistant for organisms in which an ESBL has been identified by CLAV testing (6, 7). We presumed that a positive APBA test for a cefepime-susceptible isolate of E. coli, Klebsiella species, and Proteus species would indicate that the results for ASCs should not be changed to resistant since ASCs usually retain activity

5 298 TENOVER ET AL. J. CLIN. MICROBIOL. against AmpC-producing isolates. Reporting test results of susceptible to ASCs for strains of E. coli, Klebsiella species, and Proteus species could decrease unnecessary use of carbapenems. However, the data from organisms containing both ESBLs and AmpC -lactamases, some of which tested as APBA positive but falsely CLAV negative, raise a potential concern for this strategy since an ESBL may still be present in these organisms even though they test as susceptible to cefepime. In addition, a recent report of the acquisition of a new ESBL gene by an organism that initially harbored only an AmpC -lactamase (and thus initially appeared to be cefepime susceptible), which ultimately led a cefepime treatment failure, also has to be considered (29). Another issue that impacts the decision regarding the reporting of ASCs is the clinical relevance of the inoculum effect (i.e., the presence of large quantities of -lactamase-producing organisms at the site of infection) that has been observed with cefepime and other cephalosporins with isolates containing AmpC -lactamases. In several studies, MIC results for the cephalosporins rose dramatically when the susceptibility tests were performed with an inoculum of 10 6 or 10 7 CFU/ml instead of the usual 10 5 CFU/ml (16, 19, 25). Thus, the issue of whether APBA-test-positive, CLAV-test-negative isolates should be reported as susceptible to ASCs will require further study. Screening for AmpC -lactamases with cefoxitin and amoxicillin-clavulanate, which is easier to implement in a laboratory than APBA testing, detects isolates with a variety of AmpC -lactamases but includes ESBL-containing isolates and isolates that are susceptible to all the ESCs by broth microdilution reference testing (although these organisms were originally reported to be resistant to at least one ESC by Vitek testing). Thus, an algorithm that uses cefoxitin and amoxicillin-clavulanate to screen for AmpC-containing isolates would have to include criteria of full resistance (not intermediate results) to both of these antimicrobial agents and resistance to at least one ESC to increase the specificity of the testing algorithm. Other approaches to AmpC -lactamase identification, such as the EDTA disk test proposed by Black et al. (1), may be more effective than testing cefoxitin and amoxicillin-clavulanate. Only about 58% of the APBA-positive isolates in our study gave a positive result in the AmpC multiplex PCR assay although aief results were consistent with AmpC carriage. This suggests that the diversity of AmpC -lactamase genes continues to expand beyond those contained in the six families of genes covered by the multiplex assay. Finally, in this study we used the hemisulfate salt of APBA, which can be dissolved in water, rather than DMSO. This makes the use of the test more practical for a clinical laboratory since DMSO can be toxic and requires special handling in the laboratory. In summary, APBA testing may improve the accuracy of susceptibility test results for E. coli, Klebsiella species, and Proteus species by indicating that ESC results should be reported as resistant. The caveats of hidden ESBL carriage among APBA-positive, CLAV-negative organisms and of potential inoculum effects require additional data before any formal recommendations can be made on changing the reporting of ASC results for these organisms. ACKNOWLEDGMENTS We thank Y. Arakawa for the suggestion of using the hemisulfate salt of APBA and J. Kamile Rasheed, David Livermore, and Ronald Jones for helpful discussions. We also thank Portia Williams, Kitty Anderson, Lesley McGee, and Jared Fisher for technical assistance. Phase 5 of Project ICARE is supported in part by unrestricted research grants to the Rollins School of Public Health of Emory University by Astra-Zeneca Pharmaceuticals, Wilmington, DE; Elan Pharmaceuticals, San Diego, CA; Johnson & Johnson Pharmaceutical Research and Development, LLC, Raritan, NJ; Pfizer Incorporated, New York, NY; and 3 M Health Care Products, St. Paul, MN. A.E. is supported by a grant from AstraZeneca. R.A.B. is supported by the VISN 10 Geriatric Research Education and Clinical Center (GRECC), the Merit Review Program of the Department of Veterans Affairs, and the National Institutes of Health (R01 AI ). The findings and conclusions in this report are those of the authors and do not necessarily represent the official position of the Centers for Disease Control and Prevention. REFERENCES 1. Black, J. A., E. S. Moland, and K. S. Thomson AmpC disk test for detection of plasmid-mediated AmpC -lactamases in Enterobacteriaceae lacking chromosomal AmpC -lactamases. J. Clin. Microbiol. 43: Bradford, P. A Extended-spectrum -lactamases in the 21st century: characterization, epidemiology, and detection of this important resistance threat. Clin. Microbiol. Rev. 14: Bush, K Metallo-beta-lactamases: a class apart. Clin. Infect. Dis. 27(Suppl 1):S48 S Bush, K New -lactamases in gram-negative bacteria: diversity and impact on the selection of antimicrobial therapy. Clin. Infect. 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6 VOL. 47, 2009 BORONIC ACID TESTING FOR AmpC -LACTAMASES Oliver, A., L. M. Weigel, J. K. Rasheed, J. E. McGowan, Jr., P. Raney, and F. C. Tenover Mechanisms of decreased susceptibility to cefpodoxime in Escherichia coli. Antimicrob. Agents Chemother. 46: Pai, H., C. I. Kang, J. H. Byeon, K. D. Lee, W. B. Park, H. B. Kim, E. C. Kim, M. D. Oh, and K. W. Choe Epidemiology and clinical features of bloodstream infections caused by AmpC-type- -lactamase-producing Klebsiella pneumoniae. Antimicrob. Agents Chemother. 48: Paterson, D. L., W. C. Ko, A. Von Gottberg, S. Mohapatra, J. M. Casellas, H. Goossens, L. Mulazimoglu, G. Trenholme, K. P. Klugman, R. A. Bonomo, L. B. Rice, M. M. Wagener, J. G. McCormack, and V. L. Yu Antibiotic therapy for Klebsiella pneumoniae bacteremia: implications of production of extended-spectrum beta-lactamases. Clin. Infect. Dis. 39: Paterson, D. L., W. C. Ko, A. Von Gottberg, S. Mohapatra, J. M. Casellas, H. Goossens, L. Mulazimoglu, G. Trenholme, K. P. Klugman, R. A. Bonomo, L. B. Rice, M. M. Wagener, J. G. McCormack, and V. L. Yu International prospective study of Klebsiella pneumoniae bacteremia: implications of extended-spectrum beta-lactamase production in nosocomial infections. Ann. Intern. Med. 140: Paterson, D. L., L. B. Rice, and R. A. Bonomo Rapid method of extraction and analysis of extended-spectrum beta-lactamases from clinical strains of Klebsiella pneumoniae. Clin. Microbiol. Infect. 7: Perez-Perez, F. J., and N. D. Hanson Detection of plasmid-mediated AmpC -lactamase genes in clinical isolates by using multiplex PCR. J. Clin. Microbiol. 40: Philippon, A., G. Arlet, and G. A. Jacoby Plasmid-determined AmpCtype -lactamases. Antimicrob. Agents Chemother. 46: Queenan, A. M., B. Foleno, C. Gownley, E. Wira, and K. Bush Effects of inoculum and -lactamase activity in AmpC- and extended-spectrum -lactamase (ESBL)-producing Escherichia coli and Klebsiella pneumoniae clinical isolates tested by using NCCLS ESBL methodology. J. Clin. Microbiol. 42: Reeves, D. S., M. J. Bywater, and H. A. Holt The activity of cefpirome and ten other antibacterial agents against 2858 clinical isolates collected from 20 centres. J. Antimicrob. Chemother. 31: Sader, H. S., and R. N. Jones In vitro antimicrobial activity of cefpirome against ceftazidime-resistant isolates from two multicenter studies. Eur. J. Clin. Microbiol. Infect. Dis. 13: Schwaber, M. J., P. M. Raney, J. K. Rasheed, J. W. Biddle, P. Williams, J. E. McGowan, Jr., and F. C. Tenover Utility of NCCLS guidelines for identifying extended-spectrum -lactamases in non-escherichia coli and non- Klebsiella spp. of Enterobacteriaceae. J. Clin. Microbiol. 42: Song, W., E. S. Moland, N. D. Hanson, J. S. Lewis, J. H. Jorgensen, and K. S. Thomson Failure of cefepime therapy in treatment of Klebsiella pneumoniae bacteremia. J. Clin. Microbiol. 43: Steward, C. D., J. K. Rasheed, S. K. Hubert, J. W. Biddle, P. M. Raney, G. J. Anderson, P. P. Williams, K. L. Brittain, A. Oliver, J. E. McGowan, Jr., and F. C. Tenover Characterization of clinical isolates of Klebsiella pneumoniae from 19 laboratories using NCCLS extended-spectrum -lactamase detection methods. J. Clin. Microbiol. 39: Wachino, J., H. Kurokawa, S. Suzuki, K. Yamane, N. Shibata, K. Kimura, Y. Ike, and Y. Arakawa Horizontal transfer of bla CMY -bearing plasmids among clinical Escherichia coli and Klebsiella pneumoniae isolates and emergence of cefepime-hydrolyzing CMY-19. Antimicrob. Agents Chemother. 50: Walther-Rasmussen, J., and N. Hoiby Plasmid-borne AmpC betalactamases. Can. J. Microbiol. 48: Yagi, T., J. Wachino, H. Kurokawa, S. Suzuki, K. Yamane, Y. Doi, N. Shibata, H. Kato, K. Shibayama, and Y. Arakawa Practical methods using boronic acid compounds for identification of class C -lactamaseproducing Klebsiella pneumoniae and Escherichia coli. J. Clin. Microbiol. 43: Yigit, H., A. M. Queenan, G. J. Anderson, A. Domenech-Sanchez, J. W. Biddle, C. D. Steward, S. Alberti, K. Bush, and F. C. Tenover Novel carbapenem-hydrolyzing -lactamase, KPC-1, from a carbapenem-resistant strain of Klebsiella pneumoniae. Antimicrob. Agents Chemother. 45: Downloaded from on August 14, 2018 by guest

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