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Journal of Clinical Microbiology, March 2006, p. 1202-1203, Vol. 44, No. 3
0095-1137/06/$08.00+0 doi:10.1128/JCM.44.3.1202-1203.2006
Copyright © 2006, American Society for Microbiology. All Rights Reserved.
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We used the same 0.1% sodium taurocholate-enriched cycloserine-cefoxitin-amphotericin B mixture (CCA) (bioMerieux, Marcy L'Etoile, France) (TCCA) broth for recovery of C. difficile strains from hospital environmental swabs and from the palms/fingernails of the medical personnel. One hundred sixty-four environmental swabs were collected from hospital environments of maternity (94 swabs) and surgical (70 swabs) wards (5, 6). Environmental samples from a 76-bed maternity ward were collected from neonates' bedrails, baby sinks, baskets for diapers, surfaces of baby-changing tables, baby scales, and walls behind radiators. From a 60-bed surgical ward, environmental samples were collected from patients' beds, stretchers, push-chairs, sinks, and toilets (Table 1). In both hospital wards, C. difficile strains were at the same time isolated from 17% fecal samples of neonates and 9% fecal samples of surgical patients (4). Out of 164 collected environmental swabs inoculated on TCCA Columbia blood agar and subsequently inoculated in TCCA broth, C. difficile strains were isolated in 8 and 12 (13%) cases, respectively, in the maternity hospital and in 3 and 5 (7.4%) cases, respectively, in the surgical ward. Ribotyping classified the majority of C. difficile strains isolated from the maternity environment (type A) and from the surgical environment (type B) in the same fashion. Moreover, ribotyping classified strains from the maternity ward and neonatal fecal samples and from the surgical ward environment and patients' fecal samples as the same types (data not shown). One hundred fifty swab samples taken from the palms/fingernails of medical personnel were C. difficile negative.
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TABLE 1. Characteristics of environmental strains of Clostridium difficile isolated from maternity and surgical wards
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Because stool samples usually contain a high number of bacterial spores (2), Columbia blood agar with an antibiotic mixture is a good choice when stool samples are cultured within the first 24 to 48 h after collection. When environmental swab samples are cultured for C. difficile, the use of broth enriched with 0.1% sodium taurocholate and an antibiotic mixture is recommended because in the hospital environment, the number of spores is smaller than that in fecal samples. The contamination of the hospital environment may play an important role in transmission, since spores of C. difficile can survive for up to 6 months (3, 8). It is also important from an epidemiological point of view to recognize the source of C. difficile strains and to compare strains isolated from different sources in terms of clonality (7).
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ajczyk. 1995. PCR ribotyping and arbitrarily primed PCR for typing strains of Clostridium difficile from a Polish maternity hospital. J. Clin. Microbiol. 33:2016-2021.[Abstract]
ski, A. Szubert, and F. Meisel-Miko
ajczyk. 1993. C. difficile in a department of surgery. Mater. Med. Pol. 25:145-147.[Medline]|
Gayane Martirosian*
Department of Medical Microbiology, Medical University of Silesia, 18 Medykow Str. Katowice 40-752, Poland
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| * Phone: 48 32 252 6075, Fax: 48 32 252 6075, E-mail: gmartir{at}slam.katowice.pl |
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