Affiliation:
1. Department of Laboratory Medicine, Divisions of
2. Pulmonology
3. Therapeutics Development Network Resource Center for Microbiology, Children's Hospital and Regional Medical Center, University of Washington, Seattle, Washington
4. Infectious Disease, Department of Pediatrics
Abstract
ABSTRACT
Pseudomonas aeruginosa
and other gram-negative isolates from patients with cystic fibrosis (CF) may be difficult to identify because of their marked phenotypic diversity. We examined 200 gram-negative clinical isolates from CF respiratory tract specimens and compared identification by biochemical testing and real-time PCR with multiple different target sequences using a standardized combination of biochemical testing and molecular identification, including 16S rRNA partial sequencing and
gyrB
PCR and sequencing as a “gold standard.” Of 50 isolates easily identified phenotypically as
P. aeruginosa
, all were positive with PCR primers for
gyrB
or
oprI
, 98% were positive with exotoxin A primers, and 90% were positive with
algD
primers. Of 50
P. aeruginosa
isolates that could be identified by basic biochemical testing, 100% were positive by real-time PCR with
gyrB
or
oprI
primers, 96% were positive with exotoxin A primers, and 92% were positive with
algD
primers. For isolates requiring more-extensive biochemical evaluation, 13 isolates were identified as
P. aeruginosa
; all 13 were positive with
gyrB
primers, 12 of 13 were positive with
oprI
primers, 11 of 13 were positive with exotoxin A primers, and 10 of 13 were positive with
algD
primers. A single false-positive
P. aeruginosa
result was seen with
oprI
primers. The best-performing commercial biochemical testing was in exact agreement with molecular identification only 60% of the time for this most difficult group. Real-time PCR had costs similar to those of commercial biochemical testing but a much shorter turnaround time. Given the diversity of these CF isolates, real-time PCR with a combination of two target sequences appears to be the optimum choice for identification of atypical
P. aeruginosa
and for non-
P. aeruginosa
gram-negative isolates.
Publisher
American Society for Microbiology
Cited by
106 articles.
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