Three-year experience with sonicated vascular catheter cultures in a clinical microbiology laboratory.

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J Clin Microbiol. 1990 January; 28(1): 76-82

Three-year experience with sonicated vascular catheter cultures in a clinical microbiology laboratory.

R J Sherertz, I I Raad, A Belani, L C Koo, K H Rand, D L Pickett, S A Straub and L L Fauerbach

Department of Medicine, University of Florida School of Medicine, Gainesville.

ABSTRACT

Using a quantitative sonication method, we cultured 1,681 consecutivevascular catheters submitted to a clinical microbiology laboratoryin a 36-month period. A total of 46% of the cultures were positive;the most common organisms isolated were coagulase-negative staphylococci(36.4%), Pseudomonas aeruginosa (13.9%), enterococci (10.0%),yeasts (9.2%), Staphylococcus aureus (5.8%), and Enterobacterspecies (4.4%). The frequencies of positive blood cultures within48 h prior to a positive catheter culture result were as follows:Candida albicans (68.4%), S. aureus (60%), Enterobacter cloacae(42.9%), Staphylococcus epidermidis (32.1%), P. aeruginosa (27.7%),and enterococci (23.3%). The sonication method allowed quantificationof the number of CFU removed from a catheter for between 10(2)and 10(7) CFU. For catheter cultures in which greater than orequal to 10(2) CFU grew, a linear regression equation couldbe calculated: (risk of positive blood culture for the sameorganism) = 14 [log10 (number of organisms removed from thecatheter)] -21 (r = 0.93). For catheter cultures in which lessthan 10(2) CFU grew, positive blood cultures for the same organismwere strongly associated with a proven infection at a site distantfrom the catheter (P = 0.001) or probable contamination (S.epidermidis). Our findings indicate that this technique hasconsiderable potential for use in clinical microbiology laboratoriesto aid in the diagnosis of vascular catheter infections andfor clinical investigations into the pathogenesis of these infections.

J Clin Microbiol. 1990 January; 28(1): 76-82

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