Affiliation:
1. Division of Bacterial and Mycotic Diseases, National Center for Infectious Diseases, Centers for Disease Control and Prevention, Atlanta, Georgia
Abstract
ABSTRACT
Rapid identification of
Candida
species has become more important because of an increase in infections caused by species other than
Candida albicans
, including species innately resistant to azole antifungal drugs. We previously developed a PCR assay with an enzyme immunoassay (EIA) format to detect amplicons from the five most common
Candida
species by using universal fungal primers and species-specific probes directed to the ITS2 region of the gene for rRNA. We designed probes to detect seven additional
Candida
species (
C. guilliermondii
,
C. kefyr
,
C. lambica
,
C. lusitaniae
,
C. pelliculosa
,
C. rugosa
, and
C. zeylanoides
) included in the API 20C sugar assimilation panel, five probes for species not identified by API 20C (
C. haemulonii
,
C. norvegica
,
C. norvegensis
,
C. utilis
, and
C. viswanathii
), and a probe for the newly described species
C. dubliniensis
, creating a panel of 18
Candida
species probes. The PCR-EIA correctly identified multiple strains of each species tested, including five identified as
C. albicans
by the currently available API 20C database but determined to be
C. dubliniensis
by genotypic and nonroutine phenotypic characteristics. Species identification time was reduced from a mean of 3.5 days by conventional identification methods to 7 h by the PCR-EIA. This method is simple, rapid, and feasible for identifying
Candida
species in clinical laboratories that utilize molecular identification techniques and provides a novel method to differentiate the new species,
C. dubliniensis
, from
C. albicans
.
Publisher
American Society for Microbiology
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American Society for Microbiology
Washington D.C
5. Epidemiology of nosocomial fungal infections
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