Carbapenem resistance in Klebsiella pneumoniae not detected by automated susceptibility testing.Detecting [beta]-lactamase--mediated carbapenem resistance among Klebsiella pneumoniae Klebsiella pneu·mo·ni·ae n. Friedlander's bacillus. isolates and other Enterobacteriaceae is an emerging problem. In this study, 15 [bla.sub.KPC "Keeping parents clueless." See digispeak. ]-positive Klebsiella pneumoniae that showed discrepant dis·crep·ant adj. Marked by discrepancy; disagreeing. [Middle English discrepaunt, from Latin discrep results for imipenem and meropenem from 4 New York City New York City: see New York, city. New York City City (pop., 2000: 8,008,278), southeastern New York, at the mouth of the Hudson River. The largest city in the U.S. hospitals were characterized by isoelectric focusing isoelectric focusing, n the ordering and concentration of substances according to their isoelectric points. ; broth microdilution (BMD BMD In currencies, this is the abbreviation for the Bermudian Dollar. Notes: The currency market, also known as the Foreign Exchange market, is the largest financial market in the world, with a daily average volume of over US $1 trillion. ); disk diffusion (DD); and MicroScan, Phoenix, Sensititre, VITEK, and VITEK 2 automated systems. All 15 isolates were either intermediate or resistant to imipenem and meropenem by BMD; 1 was susceptible to imipenem by DD. MicroScan and Phoenix reported 1 (6.7%) and 2 (13.3%) isolates, respectively, as imipenem susceptible. VITEK and VITEK 2 reported 10 (67%) and 5 (33%) isolates, respectively, as imipenem susceptible. By Sensititre, 13 (87%) isolates were susceptible to imipenem, and 12 (80%) were susceptible to meropenem. The VITEK 2 Advanced Expert System changed 2 imipenem MIC results from [greater than or equal to] 16 [micro]g/mL to [less than or equal to] 2 [micro]g/mL but kept the interpretation as resistant. The recognition of carbapenem-resistant K. pneumoniae continues to challenge automated susceptibility systems. ********** Carbapenem resistance among the Enterobacteriaceae is emerging in the United States United States, officially United States of America, republic (2005 est. pop. 295,734,000), 3,539,227 sq mi (9,166,598 sq km), North America. The United States is the world's third largest country in population and the fourth largest country in area. , particularly on the East Coast (1-6). Resistance to the most widely used carbapenems, i.e., imipenem and meropenem, can be mediated by a variety of mechanisms, including [beta]-lactamases, porin Porin can be:
Cephalosporins are medicines that kill bacteria or prevent their growth. Purpose Cephalosporins are used to treat infections in different parts of the body—the ears, nose, throat, lungs, sinuses, and in addition to carbapenems; these [beta]-lactamases are usually plasmid encoded. Clinical microbiology Clinical microbiology The adaptation of microbiological techniques to the study of the etiological agents of infectious disease. Clinical microbiologists determine the nature of infectious disease and test the ability of various antibiotics to inhibit or kill laboratories have often found it difficult to achieve accurate susceptibility testing results for carbapenem drugs. Early studies documented false resistance to imipenem due to degradation of the drug (9); later studies with the VITEK system (bioMerieux, Durham, NC, USA) demonstrated false resistance, specifically with Proteus mirabilis Proteus mirabilis Microbiology A gram-negative pathogen linked to UTIs, wound infections Habitat P mirabilis may be found in water, soil, feces (10). Several recent proficiency testing studies have shown problems of both false resistance and false susceptibility with imipenem and meropenem among a variety of enteric enteric /en·ter·ic/ (en-ter´ik) within or pertaining to the small intestine. en·ter·ic adj. 1. Of, relating to, or within the intestine. 2. species (11,12). Even quality control measures fail to detect all false resistance problems (13). Yigit and colleagues described the KPC-1 [beta]-lactamase in 2001 (1). The [beta]-lactamase was identified in an imipenem-resistant isolate of Klebsiella pneumoniae from the United States. Subsequently, 3 additional KPC-type [beta]-lactamases have been described from Salmonella, K. oxytoca, Enterobacter cloacae Enterobacter cloacae is a clinically significant Gram-negative, facultatively-anaerobic, rod-shaped bacterium. , and other K. pneumoniae; these differ in amino acid amino acid (əmē`nō), any one of a class of simple organic compounds containing carbon, hydrogen, oxygen, nitrogen, and in certain cases sulfur. These compounds are the building blocks of proteins. sequence from each other, typically by 1 or 2 amino acids (2-6). Bratu and colleagues reported false-susceptible results for K. pneumoniae isolates with the MicroScan WalkAway system (Dade MicroScan, Inc., West Sacramento, CA, USA), which were attributed in part to low inoculum inoculum /in·oc·u·lum/ (-ok´u-lum) pl. inoc´ula material used in inoculation. in·oc·u·lum n. pl. size (14). Similar problems with false-susceptible results were noted with the VITEK system (15). The goal of this study was to conduct a rapid assessment of currently available antimicrobial antimicrobial /an·ti·mi·cro·bi·al/ (-mi-kro´be-al) 1. killing microorganisms or suppressing their multiplication or growth. 2. an agent with such effects. susceptibility testing methods to determine whether these methods were capable of consistently detecting KPC-mediated carbapenem resistance in fresh clinical isolates of K. pneumoniae. Materials and Methods Bacterial Isolates To achieve a diversity of [beta]-lactam resistance phenotypes, we selected 15 isolates of K. pneumoniae from 4 hospitals in New York List of hospitals in New York (U.S. state), sorted by hospital name. A to H
sputum cruen´tum bloody sputum. , and urine) and obtained in a 1-month period in 2005. The carbapenem-resistant quality control isolates K. pneumoniae 1534 (containing the KPC-1 carbapenemase) and Serratia marcescens Serratia marcescens Microbiology The type-species of the gram-negative Serratia, widely present in the environment, and occasional cause of hospital-acquired infections Asssociations Contaminated fluids, equipment, cleaning solutions, hands, ↓ 525 (which contains an SME-like [beta]-lactamase) were from the Project ICARE ICARE International Cancer Alliance for Research and Education ICARE International Cancer Academy for Research and Education ICARE International Community Actively Responding to The Environment ICARE Informed Citizens Against Runway Expansion (Intensive Care Antimicrobial Resistance Epidemiology) strain collection (1,11). The imipenem MICs for the isolates and the study identification of their hospital of origin are shown in Table 1. Reference Susceptibility Testing Methods The antimicrobial susceptibility profiles of the isolates were determined by the broth microdilution method with cation-adjusted Mueller-Hinton broth (BD Diagnostic Systems [BDDS BDDS Birmingham District Dental Society (Alabama) BDDS Broadcast Data Distribution System BDDS Biliopancreatic Diversion with Duodenal Switch (baryatric surgery) ], Sparks, MD, USA), as described in the National Committee for Clinical Laboratory Standards (NCCLS NCCLS National Committee for Clinical Laboratory Standards , Wayne, PA, USA) (now known as the Clinical and Laboratory Standards Institute [CLSI CLSI Clinical and Laboratory Standards Institute (Wayne, PA) CLSI Cisco Link Services Interface ]) publication M7-A6 (16). Disk diffusion was performed as described in NCCLS document M2-A8 (17). Interpretations of MIC and disk diffusion results were made by using CLSI document M100-S15 (18). Commercial Susceptibility Testing and Molecular Methods The Etest method (AB Biodisk, Solna, Sweden) was performed as described by the manufacturer with Mueller-Hinton agar (BDDS); tests were interpreted at 18-20 h. The MicroScan WalkAway (Dade MicroScan, Inc.), BD Phoenix (BDDS), Sensititre AutoReader (Westlake, OH, USA), VITEK Legacy (bioMerieux), and VITEK 2 (bioMerieux) systems were tested according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. manufacturers' protocols. The panels and cards used are listed in Table 2. All systems were tested with inocula from the same subculture subculture /sub·cul·ture/ (sub´kul-chur) a culture of bacteria derived from another culture. sub·cul·ture n. . All strains for which the commercial MIC results were discrepant with MIC results from the broth microdilution reference method were retested by using all methods. The carbapenem inactivation inactivation /in·ac·ti·va·tion/ (in-ak?ti-va´shun) the destruction of biological activity, as of a virus, by the action of heat or other agent. assay was performed on Mueller-Hinton agar with imipenem and meropenem disks as described by Yigit et al. (1). Isoelectric focusing was performed on crude lysates of isolates as previously described (1,2). For detection of [bla.sub.KPC] genes, a 489-bp internal gone fragment was amplified by using forward (5'-CTTGCTGCCGCTGTGCTG-3') and reverse (5'-GCAGGTTCCGGTTTTGTCTC-3') oligonucleotide Oligonucleotide A deoxyribonucleic acid (DNA) or ribonucleic acid (RNA) sequence composed of two or more covalently linked nucleotides. Oligonucleotides are classified as deoxyribooligonucleotides or ribooligonucleotides. primers where the 5' base of each primer corresponds to position 223 or 711, respectively, with regard to the translational start site ([bla.sub.KPC-1] numbering, GenBank accession no. AF297554). PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) reagents included a final concentration of 0.5 [micro]mol/L of each primer and 2 mmol/L [MgCl.sub.2]. An annealing annealing (ənēl`ĭng), process in which glass, metals, and other materials are treated to render them less brittle and more workable. temperature of 60[degrees]C was used for amplification. For DNA sequence DNA sequence Genetics The precise order of bases–A,T,G,C–in a segment of DNA, gene, chromosome, or an entire genome. See Base pair, Base sequence analysis, Chromosome, Gene, Genome. determination, a 989-bp PCR product that included the entire [bla.sub.KPC] structural gene was amplified by using oligonucleotide primers as previously described (4). Products were purified on QIAquick spin columns (Qiagen, Chatsworth, CA, USA). The nucleotide sequences of both strands of the [bla.sub.KPC] gene from isolates 4 and 11 were determined from independent amplification products by using previously described primers (1). Cycle sequencing reactions were performed in a GeneAmp PCR system 9700 thermal cycler The Thermal cycler (also known as a thermocycler, PCR machine or DNA amplifier) is a laboratory apparatus used for PCR. The device has a thermal block with holes where tubes with the PCR reaction mixtures can be inserted. with the ABI Abi (ā`bī) [short for Abijah], in the Bible, King Hezekiah's mother. (Application Binary Interface) A specification for a specific hardware platform combined with the operating system. BigDye Terminator v3.1 cycle sequencing kit (Perkin-Elmer, Applied Biosystems Applied Biosystems, Inc. (formerly NASDAQ: ABIO) is the original name of a pioneer biotechnology company founded in 1981 in Foster City, California, among the Silicon Valley cities of the southern San Francisco Bay Area. Division, Foster City, CA, USA). Products from sequencing reactions were purified on Cetri-Sep spin columns (Princeton Separations, Adelphia, NJ, USA) before analysis on an ABI 3130x1 Genetic Analyzer. DNA sequencing DNA sequencing The determination of the sequence of nucleotides in a sample of DNA. data were analyzed by using DNASIS for Windows (Hitachi Software Genetic Systems, San Francisco San Francisco (săn frănsĭs`kō), city (1990 pop. 723,959), coextensive with San Francisco co., W Calif., on the tip of a peninsula between the Pacific Ocean and San Francisco Bay, which are connected by the strait known as the Golden , CA, USA). Results Carbapenem Testing with VITEK Legacy Initial imipenem and meropenem susceptibility test results for 15 isolates of K. pneumoniae tested with the VITEK Legacy system with GNS GNS GEOnet Names Server (NIMA) GNS Global Network Services (INMARSAT) GNS Guinea Franc GNS Get Nearest Server (component of IPX and SAP) GNS Global Navigation System 122 and 127 panels (flex system) in 1 hospital laboratory in New York City in a 1-month period in 2005 yielded a range of imipenem and meropenem MICs from susceptible (MIC [less than or equal to] 4 [micro]g/mL) to resistant (MIC [greater than or equal to] 16 [micro]g/mL) (data not shown). One isolate was imipenem resistant (MIC >16 [micro]g/mL) but meropenem susceptible ([less than or equal to] 4 [micro]g/mL) on day 1, but on retesting the following day was meropenem resistant (16 [micro]g/mL) and imipenem susceptible ([less than or equal to] 4 [micro]g/mL). Imipenem Etest results, which were set up to arbitrate the conflicting results, were difficult to interpret because of variable numbers of colonies within the ellipses Ellipses is the plural form of either of two words in the English language:
[FIGURE OMITTED] Characterization of [bla.sub.KPC]-containing K. pneumoniae Strains By using the broth microdilution reference method, all the isolates were either intermediate or resistant to both imipenem and meropenem (Table 2). Two known imipenem-resistant isolates, K. pneumoniae 1534 and S. marcescens 525, were included as controls. Eight of 15 isolates from the 4 hospitals had the same pulsed-field gel electrophoresis gel electrophoresis n. Electrophoresis performed in a gel composed of agarose, polyacrylamide, or starch. (PFGE PFGE Pulsed-Field Gel Electrophoresis ) type (data not shown), although their antibiograms varied for several antimicrobial agents Antimicrobial agents Chemical compounds biosynthetically or synthetically produced which either destroy or usefully suppress the growth or metabolism of a variety of microscopic or submicroscopic forms of life. (data not shown). Two isolates had a similar pattern but because of a 3-band difference were designated as type B. The remaining isolates showed patterns unrelated to types A or B (Table 1). All 15 isolates demonstrated 5 [beta]-lactamase bands by isoelectric focusing (pIs = 5.4, 6.8, 7.0, 8.1, and 8.2), 1 of which was consistent with a KPC [beta]-lactamase (pI = 6.8) (1,2). A 489-bp gene fragment was amplified from all 15 carbapenem-resistant K. pneumoniae isolates by using [bla.sub.KPC]-specific oligonucleotide primers. DNA sequence analysis of purified PCR products that included the entire coding region The coding region of a gene is the portion of DNA that is transcribed into mRNA and translated into proteins. This does not include such regions as a recognition site, initiator sequence, or termination sequence, only the region that will directly code for amino acid linkage. of the [bla.sub.KPC] genes of isolates 4 and 11 (which had unique PFGE profiles) identified the [beta]-lactamase genes as [bla.sub.KPC-2] and [bla.sub.KPC-3], respectively. The 15 isolates were tested for imipenem and meropenem resistance by disk diffusion, Etest, MicroScan WalkAway, BD Phoenix, Sensititre AutoReader, VITEK, and VITEK 2 panels and cards. The results of testing are summarized in Table 2. MicroScan WalkAway reported 1 isolate as susceptible to both imipenem and meropenem, whereas the Phoenix system called 2 isolates susceptible to both imipenem and meropenem. VITEK called 7 isolates (representing 3 different PFGE profiles) susceptible to both imipenem and meropenem, 3 isolates resistant to imipenem but susceptible to meropenem, 1 isolate susceptible to imipenem but resistant to meropenem, and 2 isolates susceptible to imipenem but intermediate to meropenem. Of the final 2 isolates, 1 was resistant to imipenem and intermediate to meropenem, and the other was resistant to both antimicrobial agents. Thus, 10 (67%) of 15 isolates were interpreted on initial testing as susceptible to imipenem, and 10 were susceptible to meropenem. When the VITEK 2 system was used, 5 (33%) of 15 isolates were reported as susceptible to imipenem. The VITEK 2 Advanced Expert System (AES) used the imipenem results to predict meropenem results; thus, these same 5 isolates were called meropenem susceptible. In addition, as a result of the AES's recognizing unusual susceptibility results in the antibiograms of 2 K. pneumoniae isolates, AES did not report an interpretation for meropenem for 2 isolates. Finally, the VITEK 2 reported 2 isolates as imipenem resistant and 1 isolate as imipenem intermediate, although the MICs reported by AES were listed as [less than or equal to] 2 [micro]g/mL. Aside from these, all AES categorical interpretations were in agreement with the original VITEK 2 MIC results. When Sensititre panels were used, 10 (67%) of 15 isolates were reported as susceptible to both imipenem and meropenem, 2 isolates were reported as imipenem intermediate and meropenem susceptible, and 3 isolates were reported as imipenem susceptible and meropenem intermediate. Thus, on initial testing, 13 (87%) of 15 isolates were reported as imipenem susceptible, and 12 (80%) of 15 were meropenem susceptible. Repeat testing of strain 4 yielded imipenem- and meropenem-resistant results for MicroScan, BD Phoenix, VITEK Legacy, and VITEK 2. However, the Sensititre AutoReader results showed the isolate as susceptible to imipenem and meropenem. Retesting of strain 14 on the BD Phoenix showed the isolate as resistant to imipenem and meropenem. However, with VITEK Legacy, the isolate remained susceptible to imipenem, but the response to meropenem switched from 8 [micro]g/mL (intermediate) to [less than or equal to] 4 [micro]g/mL (susceptible), which confirmed the observations of flip-flopping (i.e., reversing) results from the New York City laboratory. The Sensititre AutoReader results for strain 14 remained susceptible on repeat testing; MicroScan results remained resistant. Discussion Detecting KPC-mediated carbapenem resistance in K. pneumoniae isolates remains a challenge for many automated susceptibility testing systems. Although we used a total of only 17 isolates in this study (including 1 S. marcescens and 1 K. pneumoniae control), the isolates and controls represented 4 different carbapenemases (KPC-1, KPC-2, KPC-3, and an SME-like [beta]-lactamase), 7 PFGE types, and variable imipenem and meropenem resistance profiles. Indeed, an important observation of this study is that the carbapenem-resistance profiles of the isolates varied from day to day, sometimes reversing from imipenem resistant/ meropenem susceptible to imipenem susceptible/meropenem resistant. Although in our study the MicroScan and BD Phoenix systems produced results that were more consistent with those with the reference testing systems than those with the VITEK and Sensititre AutoReader systems, problems detecting carbapenem resistance were still evident with the former systems. Bratu et al. suggested that part of the variability in detecting imipenem resistance with automated systems was a result of underinoculating the panels (14,15). Repeat testing of isolate 4 in our study with careful attention to inoculum appeared to improve results, which suggests that appropriate inoculum size is, indeed, a critical factor for achieving accurate results. The problem of the VITEK 2 AES reporting imipenem-resistant results as [less than or equal to] 2 [micro]g/mL has apparently been corrected in software version R04.02. Although we included the Etest method in our study, determining resistance and susceptibility for both imipenem and meropenem with Etest was difficult because colonies were present within the zones of inhibition. Since we could not achieve consensus on the interpretations among several readers who viewed the results, we did not include the Etest data in our analysis. Ertapenem Etest strips and disks were not tested in this study. This lack of consensus on reading Etest method, which is often used as a secondary testing method to confirm questionable results generated by automated methods, raises the question of which, if any, of the methods are reliable enough to be used for confirmation testing of carbapenem nonsusceptibility, particularly in K. pneumoniae isolates. Our data suggest that disk diffusion, especially with meropenem disks, may be used to confirm a carbapenem nonsusceptible result in K. pneumoniae isolates, which would warrant further testing. Whether this recommendation will hold true for other species of Enterobacteriaceae will require further study. Our data also suggest that if the interpretations of MIC or disk diffusion results for imipenem and meropenem for K. pneumoniae are discrepant, isolates should be retested with particular attention to using an adequate inoculum size. If treatment failure with carbapenems is observed for isolates of K. pneumoniae that were previously reported as susceptible to carbapenems, repeat testing with a nonautomated method, such as disk diffusion, may be warranted. Acknowledgment We thank Bette Jensen and Linda McDougal for assistance with PFGE. Phase 5 of Project ICARE is supported in part by unrestricted grants to the Rollins School of Public Health The Rollins School of Public Health (RSPH) is the public health school of Emory University. Founded in 1990, RSPH has more than 850 students pursuing master's degrees (MPH/MSPH) and over 100 students pursuing doctorate degrees (PhD). of Emory University Emory University (ĕm`ərē), near Atlanta, Ga.; coeducational; United Methodist; chartered as Emory College 1836, opened 1837 at Oxford. It became Emory Univ. in 1915 and in 1919 moved to Atlanta. by Astra-Zeneca Pharmaceuticals, bioMerieux, Incorporated, Elan Pharmaceuticals, and Pfizer Incorporated. References (1.) Yigit H, Queenan AM, Anderson GJ, Sanchez-Sanchez AD, Biddle JW, Steward CD, et al. Novel carbapenem-hydrolyzing [beta]-lactamase, KPC-1, from a carbapenem-resistant strain of Klebsiella pneumoniae. Antimicrob Agents Chemother. 2001;45:1151-61. (2.) Yigit H, Queenan AM, Anderson GA, Biddle JW, Steward CD, Domenech-Sanchez A, et al. Characterization of a carbapenem-resistant strain of Klebsiella oxytoca Klebsiella oxytoca is a Gram-negative, rod-shaped bacterium that is closely related to K. pneumoniae, from which it is distinguished by being indole-positive; it also has slightly different growth characteristics in that it is able to grow on melezitose, but not harboring the KPC-2 carbapenemase. Antimicrob Agents Chemother. 2003;47:3881-9. (3.) Bradford PA, Bratu S, Urban C, Visalli M, Mariano N, Landman D, et al. Emergence of carbapenem-resistant Klebsiella klebsiella Any of the rod-shaped bacteria that make up the genus Klebsiella. They are gram-negative (see gram stain), thrive better without oxygen than with it, and do not move. K. spp. possessing the class A carbapenem-hydrolyzing KPC-2 and inhibitor resistant TEM-30 beta-lactamases in New York City. Clio Infect Dis. 2004;39:55-60. (4.) Smith Moland E, Hanson ND, Herrera VL, Black JA, Lockhart TJ, Hossain A, et al. Plasmid-mediated, carbapenem-hydrolysing [beta]-lactamase, KPC-2, in Klebsiella pneumoniae isolates. J Antimicrob Chemother. 2003;51:711-4. (5.) Bratu S, Landman D, Alam M, Tolentino E, Quale qua·le n. pl. qua·li·a A property, such as whiteness, considered independently from things having the property. [From Latin qu J. Detection of KPC carbapenem-hydrolyzing enzymes in Enterobacter spp. from Brooklyn, New York New York, state, United States New York, Middle Atlantic state of the United States. It is bordered by Vermont, Massachusetts, Connecticut, and the Atlantic Ocean (E), New Jersey and Pennsylvania (S), Lakes Erie and Ontario and the Canadian province of . Antimicrob Agents Chemother. 2005;49:776-8. (6.) Woodford N, Tierno PM Jr, Young K, Tysall L, Palepou MF, Ward E, et al. Outbreak of Klebsiella pneumoniae producing a new carbapenem-hydrolyzing class A beta-lactamase, KPC-3, in a New York Medical Center. Antimicrob Agents Chemother. 2004;48:4793-9. (7.) Yigit H, Anderson GJ, Biddle JW, Steward CD, Rasheed JK, Valera LL, et al. Carbapenem resistance in a clinical isolate of Enterobacter aerogenes Enterobacter aerogenes is a Gram-negative, oxidase negative, catalase positive, rod-shaped bacterium. E. aerogenes is a nosocomial pathogen that causes opportunistic skin and tissue infections. is associated with decreased expression of OmpF and OmpC analogs. Antimicrob Agents Chemother. 2002;46:3817-22. (8.) Villar HE, Danel F, Livermore DM. Permeability to carbapenems of Proteus mirabilis mutants selected for resistance to imipenem or other beta-lactams. J Antimicrob Chemother. 1997;40:365-70. (9.) White RL, Kays MB, Friedrich LV, Brown EW, Koonce JR. Pseudoresistance of Pseudomonas aeruginosa Pseudomonas aeruginosa A normal soil inhabitant and human saprophyte that may contaminate various solutions in a hospital, causing opportunistic infection in weakened Pts Clinical Infective endocarditis in IVDAs, RTIs, UTIs, bacteremia, meningitis, 'malignant' resulting from degradation of imipenem in an automated susceptibility testing system with pre-dried panels. J Clin Microbiol. 1991;29:398-400. (10.) Doern GV, Brueggemann AB, Perla R, Daly J, Halkias D, Jones RN, et al. Multicenter laboratory evaluation of the bioMerieux VITEK antimicrobial susceptibility testing system with 11 antimicrobial agents versus members of the Family Enterobacteriaceae Noun 1. family Enterobacteriaceae - a large family of Gram-negative rod-shaped bacteria of the order Eubacteriales Enterobacteriaceae bacteria family - a family of bacteria and Pseudomonas aeruginosa. J Clin Microbiol. 1997;35:2115-9. (11.) Steward CD, Wallace D, Hubert SK, Lawton R, Fridkin SK, Gaynes RP, et al. Ability of laboratories to detect emerging antimicrobial resistance in nosocomial nosocomial /noso·co·mi·al/ (nos?o-ko´me-il) pertaining to or originating in a hospital. nos·o·co·mi·al adj. 1. Of or relating to a hospital. 2. pathogens: a survey of Project ICARE laboratories. Diagn Microbiol Infect Dis. 2000;38:59-67. (12.) Steward CD, Mohammed JM, Swenson JM, Stocker SA, Williams PP, Gaynes RP, et al. Antimicrobial susceptibility testing of carbapenems: multicenter validity testing and accuracy levels of five antimicrobial test methods for detecting resistance in Enterobacteriaceae and Pseudomonas aeruginosa isolates. J Clin Microbiol. 2003;41: 351-8. (13.) Carmeli Y, Eichelberger K, Soja D, Dakos J, Venkataraman L, deGirolami P, et al. Failure of quality control measures to prevent reporting of false resistance to imipenem, resulting in a pseudo-outbreak of imipenem-resistant Pseudomonas aeruginosa. J Clin Microbiol. 1998;36:595-7. (14.) Bratu S, Mooty M, Nichani S, Landman D, Gullans C, Pettinato B, et al. Emergence of KPC-possessing Klebsiella pneumoniae in Brooklyn, New York: epidemiology and recommendations for detection. Antimicrob Agents Chemother. 2005;49:3018-20. (15.) Bratu S, Landman D, Haag R, Recco R, Eramo A, Alam M, et al. Rapid spread of carbapenem-resistant Klebsiella pneumoniae in New York City. Arch Intern intern /in·tern/ (in´tern) a medical graduate serving in a hospital preparatory to being licensed to practice medicine. in·tern or in·terne n. Med. 2005;165:1430-5. (16.) National Committee for Clinical Laboratory Standards (NCCLS). Methods for dilution antimicrobial susceptibility tests for bacteria that grow aerobically; approved standard--sixth edition. NCCLS document M7-A6. Wayne (PA): The Committee; 2003. (17.) National Committee for Clinical Laboratory Standards (NCCLS). Performance standards for antimicrobial disk susceptibility tests; approved standard--eighth edition. NCCLS document M2-A8. Wayne (PA): The Committee; 2003. (18.) Clinical and Laboratory Standards Institute. Performance standards for antimicrobial susceptibility testing; Fifteenth informational supplement M100-S15. Wayne (PA): The Institute; 2005. Fred C. Tenover, * Rajinder K. Kalsi, ([dagger]) Portia P. Williams, ([double dagger double dagger n. A reference mark (  ) used in printing and writing. Also called diesis.Noun 1. ]) Roberta B. Carey, * Sheila Stocker, * David Lonsway, * J. Kamile Rasheed, * James W. Biddle, * John E. McGowan Jr., ([double dagger]) and Bruce Hanna ([dagger]) * Centers for Disease Control and Prevention, Atlanta, Georgia, USA; ([dagger]) Bellevue Hospital Bellevue Hospital, municipal hospital, in New York City. America's oldest public hospital, Bellevue developed from a "Publick Workhouse and House of Correction" commissioned in 1734. , New York, New York, USA; and ([double dagger]) Rollins School of Public Heath, Emory University, Atlanta, Georgia, USA Address for correspondence: Fred C. Tenover, Division of Healthcare Quality Promotion, Centers for Disease Control and Prevention, 1600 Clifton Rd, Mailstop G08, Atlanta, GA 30333, USA; email: fnt1@cdc.gov
Table 1. Carbapenem susceptibility and strain typing results for
isolates tested in the study *
Imipenem broth Meropenem
microdilution broth
MIC ([dagger]) microdilution MIC
([micro]g/mL) and ([micro]g/mL)and
Organism CLSI interpretation CLSI interpretation
1 Klebsiella
pneumoniae 8 I 16 R
2 K. pneumoniae 16 R >16 R
3 K. pneumoniae 16 R 16 R
4 K. pneumoniae 8 I 8 I
5 K. pneumoniae 16 R >16 R
6 K. pneumoniae 16 R 16 R
7 K. pneumoniae 16 R 16 R
8 K. pneumoniae 32 R 16 R
9 K. pneumoniae 16 R >16 R
10 K. pneumoniae 16 R >16 R
11 K. pneumoniae 16 R 16 R
12 K. pneumoniae 16 R 16 R
13 K. pneumoniae 16 R 16 R
14 K. pneumoniae 16 R >16 R
15 K. pneumoniae 16 R >16 R
K. pneumoniae
1534 (control) 16 R >16 R
Serratia
marcescens 525
(control) >16 R >16 R
Hospital
PFGE identification
Organism profile no.
1 Klebsiella
pneumoniae A 1
2 K. pneumoniae A 1
3 K. pneumoniae A 2
4 K. pneumoniae A 2
5 K. pneumoniae A 2
6 K. pneumoniae A 2
7 K. pneumoniae A 3
8 K. pneumoniae A 4
9 K. pneumoniae B 1
10 K. pneumoniae B 1
11 K. pneumoniae C 4
12 K. pneumoniae D 1
13 K. pneumoniae E 4
14 K. pneumoniae F 1
15 K. pneumoniae F1 4
K. pneumoniae
1534 (control) NA NA
Serratia
marcescens 525
(control) NA NA
* CLSI, Clinical and Laboratory Standards Institute; PFGE,
pulsed-field gel electrophoresis; NA, not applicable.
([dagger]) Interpretations of MIC results used CLSI criteria (18); I,
intermediate; R, resistant.
Table 2. Summary of antimicrobial susceptibility testing results for 15
test isolates *
Imipenem results (n = 15)
Method Card/panel Resistant Intermediate Susceptible
(software)
Broth In-house 13 2 0
microdilution frozen panel
Disk diffusion BDDS disks 3 11 1
MicroScan Negcombo 7 7 1
(LabProl.51, 32
Alert 1.50)
Phoenix NMIC/ ID- 5 8 2
(4.05W/3.81 A) 104
Sensititre GN2F 0 2 13
AutoReader
(3.0.8 SP2)
VITEK (R10.01) Superflex 5 0 10
GNS 122
and 127
VITEK 2 * GN07 4 6 5
(R04.01)
Meropenem results (n = 15)
Method Card/panel Resistant Intermediate Susceptible
(software)
Broth In-house 14 1 0
microdilution frozen panel
Disk diffusion BDDS disks 10 5 0
MicroScan Negcombo 13 1 1
(LabProl.51, 32
Alert 1.50)
Phoenix NMIC/ ID- 12 1 2
(4.05W/3.81 A) 104
Sensititre GN2F 0 3 12
AutoReader
(3.0.8 SP2)
VITEK (R10.01) Superflex 2 3 10
GNS 122
and 127
VITEK 2 * GN07 4 4 5
(R04.01)
* No meropenem interpretations were given by the Advanced Expert
System for 2 organisms.
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