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Journal of Clinical Microbiology, May 2001, p. 2015-2016, Vol. 39, No. 5
Department of Oral
Medicine1 and Department of
OCBS,2 Dental School, University of
Maryland, and Department of Pathology, The Johns Hopkins
University,3 Baltimore, Maryland
Received 11 August 2000/Returned for modification 29 November
2000/Accepted 6 March 2001
CHROMagar Candida is a differential culture medium for the
isolation and presumptive identification of clinically important yeasts. Recently the medium was reformulated by Becton Dickinson. This
study was designed to evaluate the performance of the new formula of
CHROMagar against the original CHROMagar Candida for recovery, growth,
and colony color with stock cultures and with direct plating of
clinical specimens. A total of 90 stock yeast isolates representing
nine yeast species, including Candida dubliniensis, as well
as 522 clinical specimens were included in this study. No major
differences were noted in growth rate or colony size between the two
media for most of the species. However, all 10 Candida
albicans isolates evaluated consistently gave a lighter shade of
green on the new CHROMagar formulation. In contrast, all 26 C. dubliniensis isolates gave the same typical dark green color on
both media. A total of 173 of the 522 clinical specimens were positive
for yeast, with eight yeast species recovered. The recovery rates for
each species were equivalent on both media, with no consistent
species-associated differences in colony size or color. Although both
media were comparable in performance, the lighter green colonies of
C. albicans isolates on the new CHROMagar made it easier to
differentiate between C. albicans and C. dubliniensis isolates. In conclusion, the newly formulated Becton
Dickinson CHROMagar Candida medium is as equally suited as a
differential medium for the presumptive identification of yeast species
and for the detection of multiple yeast species in clinical specimens
as the original CHROMagar Candida medium.
CHROMagar Candida (CR-O)
(CHROMagar, Paris, France) is a differential culture medium for
the isolation and presumptive identification of clinically important
yeasts within 24 to 48 h on the basis of strongly contrasting
colony colors (1, 6, 7). The identification of pathogenic
yeasts in the laboratory is very important in this era of increasing
opportunistic infections and resistant yeasts (2, 5, 8).
However, a definitive identification may take several additional days
after pure culture. Another advantage of CR-O is that multiple yeast
species can be detected in a clinical specimen more easily than on
normal mycologic media. Recently, the medium was reformulated by Becton
Dickinson (CR-B) (BBL, Cockeysville, Md.) to remove medium components
originating from countries with an incidence of bovine spongiform
encephalopathy or transmissible spongiform encephalopathy.
This study was designed to evaluate the performance of the new formula
of CHROMagar by Becton Dickinson against the original CR-O for
recovery, growth, and colony color with stock cultures and with direct
plating of clinical specimens. Special emphasis was placed on
determining the ability of CR-B to differentiate between Candida
albicans and the newly characterized species Candida dubliniensis (2-5, 8). Both formulations of the
CHROMagar Candida medium (CR-B and CR-O) were donated by Becton
Dickinson in dehydrated form and were prepared according to the
manufacturer's instructions.
A total of 90 yeast isolates from stock cultures representing nine
different species and previously identified by the clinical microbiology laboratories at the University of Maryland Hospital were
used in this study. Isolates were subcultured twice on Sabouraud dextrose agar medium prior to inoculation of chromogenic media. A
single yeast colony was streaked for isolation on both CR-O and CR-B
plates and incubated at 37°C without CO2. Plates were checked for growth after 24 h of incubation and read for
visual colony color independently by three investigators after 48 h of incubation. Colony color and morphology were recorded for each isolate in a side-by-side comparison of the two media. Presumptive identifications were made at 48 h.
All 90 yeast isolates tested grew well on both agars after 24 h of
incubation at 37°C in ambient air. No major differences were noted in
growth rate or colony size between the two media. However, subtle
variations in the intensity of colony color were noted between the two
media for some of the species.
All 10 C. albicans isolates evaluated gave the
characteristic light green color with a whitish sheen to the colonies;
however, all isolates consistently gave a lighter, yellowish shade of
green on CR-B. In contrast, all 26 C. dubliniensis isolates,
including the type strain CD36 (2), gave the typical dark
green color on both media. When different yeast species were mixed in a
single broth suspension and simultaneously plated out on CR-B and CR-O, the distinctions in colors and forms were equally easy to recognize on
both media (data not shown).
For evaluation of clinical specimens, a total of 522 surveillance stool
and respiratory cultures were collected. These included stool and
respiratory specimens from oncology patients as well as vaginal and
oral specimens from human immunodeficiency virus-positive women. All
specimens were directly inoculated onto both media. Plates were
incubated at 37°C. All plates were read daily for 10 days and were
evaluated for yeast quantity, color, size, and bacterial contamination.
All yeast isolates were identified by using germ tube production,
microfermentation, microscopic morphology, cornmeal agar, and API 20C
strips (if needed).
A total of 173 specimens were positive for yeast; 158 (91.3%) were
positive on CR-B and 157 (90.8%) were positive on CR-O (Table
1). Thirty specimens were positive for
multiple species, 25 on both media. Eight species of yeast were
recovered, including C. albicans, Candida glabrata, Candida
tropicalis, Candida parapsilosis, Saccharomyces cerevisiae, Candida
krusei, Candida lusitaniae, and Candida lambica. The
recovery rates for each species were equivalent on both media, and
bacterial contamination was not a problem on either medium. All germ
tube-positive isolates were screened at 45°C, but C. dubliniensis was not detected. Color readings were recorded after
48 h of incubation at 37°C as specified in the manufacturer's
instructions, and colony colors for all of the clinical yeast species
tested were comparable on both media.
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.5.2015-2016.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Evaluation of a Reformulated CHROMagar
Candida
ABSTRACT
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TABLE 1.
Performance of the reformulated CHROMagar (CR-B) compared
to the original CHROMagar (CR-O) with plating of direct clinical
specimens
The difference in colony color between C. albicans and C. dubliniensis isolates was, in general, slightly more enhanced on CR-B. Although colony colors were clear and distinguishable after 48 h on both media, colors generally deepened after 72 h of incubation at room temperature. With C. dubliniensis especially, the dark green color was found to be more pronounced if plates were incubated for longer than 48 h (e.g., up to 72 h), similar to what has been reported by other investigators regarding the original CHROMagar (6, 8).
With the clinical specimens, colonies on CR-B and CR-O were equal in size at 24 h of incubation. However, color development was inadequate on either medium, and therefore presumptive identification was made after 48 h. At 48 h there was an overall noticeable difference in colony size and enhanced color development. CR-O colony size was generally smaller, and colony color was slightly less developed than that observed on CR-B.
In conclusion, the newly formulated Becton Dickinson CHROMagar Candida medium is as equally suited as a differential medium for the presumptive identification of yeast species and for the detection of multiple yeast species in clinical specimens as the original CHROMagar Candida medium. The subtle variations in color shades observed between the two media when comparing yeast species colony color were insignificant and did not interfere with species identification. The lighter green colonies of C. albicans isolates seen with CR-B, however, made it easier to differentiate between C. albicans and C. dubliniensis isolates on CR-B.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Oral Medicine, Dental School, UMAB, 666 W. Baltimore St., Baltimore, MD 21201. Phone: (410) 708-7628. Fax: (410) 706-0519. E-mail: mrizk{at}umaryland.edu.
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Journal of Clinical Microbiology, May 2001, p. 2015-2016, Vol. 39, No. 5
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.5.2015-2016.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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