Abstract:
The study included specimens from OPD and IPD patients of all age groups and
both sexes. Specimens were cultured on suitable media. Isolates were identified by
biochemical methods, both in house and by VITEK 2. Susceptibility to carbapenem
drugs (imipenem, meropenem and ertapenem), as well as ampicillin, amoxycillinclavulanate,
ampicillin-sulbactam, piperacillin-tazobactam, cephalothin, cefoxitin,
cefotaxime, ceftazidime, cefepime, aztreonam, gentamicin, amikacin, ciprofloxacin,
levofloxacin, co-trimoxazole, tetracycline, tigecycline, chloramphenicol, and colistin
performed by Kirby-Bauer disc diffusion method.
A total of 1544 isolates of Gram negative bacilli were studied from different
specimens, of which 184 were resistant to one or more carbapenem drugs.
Acinetobacter calcoaceticus baumannii complex (104 isolates; 52%) was the dominant
species, followed by Pseudomonas aeruginosa (31 isolates; 15.5%). Among the 49
isolates of Enterobacteriaceae, K. pneumoniae was the commonest with 17 (34.6 %)
isolates, followed by E. coli with 15 (30.6 %) isolates.
Most carbapenem-resistant GNB came from the intensive care units and the
neurosurgery ward. The largest numbers of carbapenem-resistant isolates were isolated
from pus, urine, and endotracheal tube aspirates.
Carbapenem-resistant isolates were generally also resistant to most other
antimicrobials except tigecycline and colistin.
False-positive carbapenem-resistance
Six (10.9%) Enterobacteriaceae isolates appeared to be carbapenem-resistant
upon testing with the Kirby-Bauer disc diffusion technique with discs procured from
HiMedia. These isolates later turned out to be sensitive when retested with the Kirby-Bauer disc diffusion technique with discs procured from Rosco Diagnostica, Denmark, and also by the Etest method, resulting in a false-positivity rate of 10.9% for disc diffusion.
In addition, four isolates of Stenotrophomonas maltophilia and six isolates of Elizabethkingia meningoseptica had to be left out of the study because they are intrinsically resistant to carbapenem
Minimum Inhibitory Concentration
The Etest method for minimum inhibitory concentration (MIC) showed that the carbapenem MICs of most resistant isolates were ≥32 μg/ml.
The remaining 184 isolates were then tested for carbapenemase enzymes and efflux pumps by phenotypic and genotypic methods.
PHENOTYPIC METHODS
Modified Hodge Test (MHT)
Of the 184 isolates tested by MHT, only 22 tested positive.
Rosco KPC and MBL detection kit
Of the 49 Enterobacteriaceae isolates, 40 were MBL positive, 2 were both MBL and KPC positive and the remainder did not produce any of the enzymes and were presumed to be resistant by other mechanisms.
Rosco Rapid CARB Blue kit
43 (41.3%) Acinetobacter, 13 (41.9%) P. aeruginosa & 39 (79.5%) Enterobacteriaceae isolates showed the presence of carbapenemases by this kit.
Rosco Neo Rapid CARB kit
The Enterobacteriaceae and Pseudomonas isolates were then tested by Rosco neo rapid CARB kit. 40 (81.6%) Enterobacteriaceae isolates and 16 (51.6 %) P. aeruginosa isolates were tested positive as carbapenemase producers
Carba NP test, CarbAcineto NP and Blue Carba tests with modifications
Overall 45 (91.8%) Enterobacteriaceae and 19 (61.2%) P. aeruginosa isolates were found to be positive for carbapenemase production by Carba NP and Blue Carba tests
Overall 84.6% Acinetobacter calcoaceticus baumannii were positive by CarbAcineto NP and Blue Carba test for the carbapenemase detection.
In terms of modifications, no difference in results was found regarding the source of imipenem while in three (6.25 %) Enterobacteriaceae isolates carbapenemase production was found to be inducible by imipenem
Carbapenem inactivation method (CIM)
Of the resistant isolates, 73 (70.1%) Acinetobacter spp., 15 (48.3%) P. aeruginosa and 38 (77.5%) Enterobacteriaceae isolates were tested positive for carbapenemase activity by this test.
GENOTYPIC METHODS
Detection of different carbapenemase genes
Majority of the isolates showed the presence of NDM-1 carbapenemase gene. In addition to NDM-1gene, the isolates also showed the presence of VIM and OXA-48 genes. Majority (83.3 %) of the VIM positive were P. aeruginosa.
OXA-48 was detected in only K. pneumoniae isolates. None of the study isolate found to be positive for KPC gene.
EFFLUX PUMP ACTIVITY
The presence of efflux was detected by two methods namely ethidium bromide cartwheel method and agar dilution method using reserpine as efflux inhibitor
Ethidium bromide cartwheel method
On performing the efflux protocol 27 isolates were found to be positive. i.e. (the strains showing little or no fluorescens under UV light)
Reserpine as efflux pump inhibitor
Only 20 isolates showed a decrease in the MIC of meropenem when reserpine was added.