Dear Editor:
Raoultella spp., a bacterium named after Didier Raoult, is a Gram-negative belonging to the Enterobacteriaceae family. There have been described 4 species: Raoultella planticola, Raoultella ornithinolytica, Raoultella terrigena, and Raoultella electrica, all species are inhabitants of soil and plants. Recently, R. planticola and R. ornithinolytica have been associated with human infections and resistance to different antibiotics including carbapenems5. In this report, we describe an infection caused by blaOXA-48 producing R. ornithinolytica. A 64-year-old male patient was admitted into a 700-bed hospital in Quito, in order to restore intestinal transit after ileocecal resection. Two days after admission the patient presented sepsis characterized by hypotension, fever, and leukocytosis. The patient was directed to intensive care unit where he was treated with Ampicillin/sulbactam for 10 days, subsequent blood cultures were negative however Escherichia coli was recovered from tracheal aspirate. The patient was submitted to the surgical department to continue treatment and 10 days late he presented a surgical site infection, R. planticola (resistant to imipenem and piperacillin/tazobactam but susceptible to third generation cephalosporins and ciprofloxacin) was isolated and detected using a Vitek® compact 2 system (Biomeriux, France), CARD AST 272 (Table 1). The patient was treated with ciprofloxacin 500mg i.v. q12h and recov-ered satisfactorily.
Isolate analysis using DNA sequences of rpoB and 16S rRNA genes and MALDI-TOF Vitek MS system, (bioMérieux) indicated that the isolate was R. ornithinolytica (99.9% identificaron score). The RAPIDEC CARBA NP® (bioMérieux) assay was positiveand polymerase chain reaction (PCR) amplifying the blaOXA-48 associated with Tn 1999 was performed3. The amplicon was cleaned, using Wizard® SV gel, and sequenced in Macrogen (South Korea); nucleotide sequences showed the presence of blaOXA-48 gene (accession no.: MH507508) and Tn1999 (accession no.: MK359485). The amplicon showed 99% nucleotide identity to a Tn 1999 harboring blaOXA-48 previously described in Klebsiella pneumoniae (accession no.: JN626286). We were unable to determine the plas-mid incompatibility group (conjugation using E. coli J53 as the recipient was unsuccessful), nor could we establish whether the patient was colonized by R. ornithinolytica before the surgery. To the best of our knowledge, this is the first description of a clinical isolate of R. ornithinolytica harboring blaOXA-48 in Ecuador and possibly in South America. Nevertheless, blaOXA-48 genes in Enterobacteriaceae have been described in Latin American and Caribbean countries2. In Ecuador, a blaOXA-48-like gene was found previously in K. pneumoniae (accession number KY609322.1). The blaOXA-48-like gene has been found associated with 5 isoforms of Tn 1999 in Enterobacteriaceae4; interestingly, an R. ornithinolytica strain containing blaOXA-48 associated with Tn1999.2 was detected in Lebanon1. The genetic closeness of Raoultella spp. and Klebsiella spp., may lead to misidentification using biochemical tests e.g., Vitek 2 system, the introduction of rpoB and 16S rRNA genes analysis and the new technology based in MALDI-TOF MS allowed us a correct Identification to species level of Raoultella spp. Thus, our results underline the accuracy of MALDI-TOF MS in R. ornithinolytica identification. This report was approved by the institutional human ethics committee Cod: 02-01-2018-003.
Ethical approval
This study was approved by Ethics Committee in Humans of Carlos Andrade Marín hospital Cod: 02-01-2018-003.
Funding
This study was funding by Instituto Nacional de Investigación en Salud Pública ''Dr. Leopoldo Izquieta Pérez’’, Quito -Ecuador and Instituto de microbiología, Universidad San Francisco de Quito.
Contributions JR and GT: conception, design of the study and drafting the article. EV, FV, EP, NC, ME: acquisition of data, anal-ysis and interpretation. BN and GT revising critically for important intellectual content of article. GT: final approval of the version to be submitted.
Conflict of interest
The authors declare that they have no conflict of interest.
Acknowledgements
The authors thank the technical staff of microbiology laboratory of the Hospital Carlos Andrade Marín-Quito. Also we appreciate the collaboration of Dr. Luis Solorzano in the Hospital Luis Vernaza for making the MALDITOFMS available.