Affiliation:
1. Associated Regional and University Pathologists Institute for Clinical and Experimental Pathology1 and
2. the University of Utah Department of Pathology,2 Salt Lake City, Utah
Abstract
ABSTRACT
Legionella
spp. are a common cause of community-acquired respiratory tract infections and an occasional cause of nosocomial pneumonia. A PCR method for the detection of legionellae in respiratory samples was evaluated and was compared to culture. The procedure can be performed in 6 to 8 h with a commercially available DNA extraction kit (Qiagen, Valencia, Calif.) and by PCR with gel detection. PCR is performed with primers previously determined to amplify a 386-bp product within the 16S rRNA gene of
Legionella pneumophila
. We can specifically detect the clinically significant
Legionella
species including
L. pneumophila
,
L. micdadei
,
L. longbeachae
,
L. bozemanii
,
L. feeleii
, and
L. dumoffii
. The assay detects 10 fg (approximately two organisms) of legionella DNA in each PCR. Of 212 clinical specimens examined by culture, 100% of the culture-positive samples (31 of 31) were positive by this assay. By gel detection of amplification products, 12 of 181 culture-negative samples were positive for
Legionella
species by PCR, resulting in 93% specificity. Four of the 12 samples with discrepant results (culture negative, PCR positive) were confirmed to be positive for
Legionella
species by sequencing of the amplicons. The legionella-specific PCR assay that is described demonstrates high sensitivity and high specificity for routine detection of legionellae in respiratory samples.
Publisher
American Society for Microbiology
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