Environmental source of Candida dubliniensis.We isolated Candida dubliniensis from a nonhuman source, namely, tick samples from an Irish seabird colony. The species was unambiguously identified by phenotypic and genotypic means. Analysis of the 5.8S rRNA gene showed that the environmental isolates belong to C. dubliniensis genotype 1. ********** The ever-increasing number of immunosuppressed Immunosuppressed A state in which the immune system is suppressed by medications during the treatment of other disorders, like cancer, or following an organ transplantation. Mentioned in: Fifth Disease humans has led to a marked rise in opportunistic infections, particularly those caused by fungi (1). Candida albicans is the yeast species most commonly associated with oropharyngeal oropharyngeal /oro·pha·ryn·ge·al/ (-fah-rin´je-al) 1. pertaining to the mouth and pharynx. 2. pertaining to the oropharynx. and systemic candidiasis candidiasis (kăn'dĭdī`əsĭs), infection of the mucous membranes caused by the fungus Candida albicans. Other terms for candidiasis are yeast infection, moniliasis (after a former name of the fungal genus), and thrush, the in immunocompromised immunocompromised /im·mu·no·com·pro·mised/ (-kom´pro-mizd) having the immune response attenuated by administration of immunosuppressive drugs, by irradiation, by malnutrition, or by certain disease processes (e.g., cancer). persons. However, the last 2 decades have seen an increase in infections by other Candida species, including C. dubliniensis, which was first recognized as distinct from C. albicans in 1995 in Ireland (2,3). C. dubliniensis has been recovered mainly from the oral cavities of HIV-infected persons (4) but also from lungs, vaginas, blood, and feces; occasionally this organism causes fatal systemic infections (5). Isolates are assigned to 4 genotypes, defined by the sequence of the internal transcribed spacer ITS (for internal transcribed spacer) refers to a piece of non-functional RNA situated between structural ribosomal RNAs (rRNA) on a common precursor transcript. Read from 5' to 3', this polycistronic rRNA precursor transcript contains the 5' external transcribed sequence (5' ETS), regions of the rRNA gene (6). C. dubliniensis is globally distributed. In HIV-infected patients, the oral prevalence is 1.5%-32% (5). In healthy persons not infected with HIV HIV (Human Immunodeficiency Virus), either of two closely related retroviruses that invade T-helper lymphocytes and are responsible for AIDS. There are two types of HIV: HIV-1 and HIV-2. HIV-1 is responsible for the vast majority of AIDS in the United States. , C. dubliniensis is absent or rare, but 14% of healthy Caucasians had oral C. dubliniensis in a South African study (7). Like C. albicans, C. dubliniensis may be a member of the normal oral microbial flora of humans, and oral candidosis candidosis see candidiasis. candidiasis, candidosis infection by fungi of the genus Candida, generally C. albicans. Three specific syndromes are recorded as being caused by C. may result from overgrowth of resident strains. In contrast to other Candida species, some of which are associated with birds (8,9), C. dubliniensis has not been found to date in nonhuman environmental sources. This has led to speculation that the species may be restricted to humans, possibly occupying sites deep within the oropharynx oropharynx /oro·phar·ynx/ (-far´inks) the part of the pharynx between the soft palate and the upper edge of the epiglottis. o·ro·phar·ynx n. or upper respiratory tract (5). The Study Fungal strains were obtained from Ixodes uriae ticks (as part of a National Environment Research Council--funded study of a tickborne virus) at a seabird breeding colony on Great Saltee Island, Ireland (52[degrees] 07'N, 6[degrees]36'W). The ticks were taken from cracks in cliffs used by common guillemots (Uria aalge). Tissue cultures of tick homogenates undertaken for virus isolation were occasionally contaminated with yeastlike fungi. To investigate this, individual adult ticks were homogenized ho·mog·e·nize v. ho·mog·e·nized, ho·mog·e·niz·ing, ho·mog·e·niz·es v.tr. 1. To make homogeneous. 2. a. To reduce to particles and disperse throughout a fluid. b. in 1 mL minimum essential medium (MEM). After centrifugation (30 s, 10,000x g), 0.2 mL of supernatant was added to 4 mL MEM, 5% fetal bovine serum Fetal bovine serum ( or foetal bovine serum) is serum taken from the fetuses of cows. Fetal Bovine Serum (or FBS) is the most widely used serum in the culturing of cells. In some papers the expression foetal calf serum is used. , and 100 [micro]g/mL penicillin-streptomycin. Cultures incubated at 37[degrees]C were examined microscopically daily for up to 6 days. Positive cultures were plated twice on Sabouraud dextrose dextrose: see glucose. agar (SAB) with chloramphenicol chloramphenicol (klōr'ămfĕn`əkŏl'), antibiotic effective against a wide range of gram-negative and gram-positive bacteria (see Gram's stain). It was originally isolated from a species of Streptomyces bacteria. (bioMerieux, Marcy l'Etoile, France) before phenotypic testing. Isolates were identified by using API identification kits (bioMerieux) and by conventional methods (10). Antifungal drug susceptibility was tested according to the Clinical Laboratory Standards Institute guidelines (11). The control strains were C. albicans ATCC ATCC American Type Culture Collection, see there 90028, C. glabrata ATCC 90030, C. krusei ATCC 6258, and C. dubliniensis NCPF NCPF Northern Counties Photographic Federation NCPF National Collection of Pathogenic Fungi NCPF National Cancer Prevention Fund NCPF National Certificate in Professional Floristry (UK) NCPF Nature Crusaders of the Philippines Foundation 3949. Internal transcribed spacer 1 and 2 regions (ITS1/ ITS2) and the 5.8S rRNA gene were amplified with primers ITS1 and ITS4, described by White et al. (12). Template DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. was prepared by boiling single SAB-grown colonies in 50 [micro]L ultrapure water for 10 min. After centrifugation (5 min 10,000x g), 15 [micro]L supernatant was added to 50 [micro]L PCRs containing 1x reaction buffer, 1 [micro]mol/L ITS primers, 1.5 mmol/L Mg[Cl.sub.2], 400 [micro]mol/L deoxynucleoside triphosphates, and 2.5 U Immolase (BiolineLtd, London, England, UK). Cycling parameters were 7 min at 95[degrees]C, 30 cycles of 1 min at 95[degrees]C, 1 min at 58[degrees]C, 1 min at 72[degrees]C, and a final extension of 5 min at 72[degrees]C. Products were purified (QiaQuick kit, QIAGEN Ltd., West Sussex, England, UK) and sequenced (BigDye kit and ABI Abi (ā`bī) [short for Abijah], in the Bible, King Hezekiah's mother. (Application Binary Interface) A specification for a specific hardware platform combined with the operating system. 377 sequencer; Applied Biosystems, Foster City, CA, USA) by using the ITS primers. Sequences were assembled by using Lasergene 6, Seqman version II, and aligned by using BioEdit software (13). Fungal isolation was undertaken on 2 separate days with samples from 2 distinct sites on the island (Table 1). On both days, Happy Hole West (HHW HHW Household Hazardous Waste (recycling and resource conservation) HHW Heating Hot Water HHW Haarlemse Honkbal Week (Netherlands) HHW High High Water (same as HW springs) ) ticks were processed immediately after Labour in Vain (LIV) ticks in the same class II microbiologic cabinet. No fungi were detected in HHW ticks, whereas 16.7%-27.6% of ticks sampled from 2 locations within LIV gave positive cultures (Table 1). Twenty-two isolates were obtained (Table 1); SL370-429 were from LIV-1 and SL495-531 from LIV-2 (SL = Saltee). On SAB the colonies from positive cultures were a creamy white color with a glabrous glabrous /gla·brous/ (gla´brus) smooth and bare. gla·brous adj. Having no hairs or projections, especially on body parts that normally have hair; smooth. appearance similar to C. albicans. SL375 had a mixed phenotype (large and small colonies, designated SL375 1 and SL375-2). Like C. albicans, all SL isolates were germ-tube positive and produced chlamydospores at 37[degrees]C on Corn Meal Tween 80 agar (Oxoid Ltd, Basingstoke, England, UK) and Czapek Dox (1%) Tween 80 agar (Oxoid) (Figure 1A). None of the SL isolates grew at 43[degrees]C on SAB (Figure 1B), which suggested that they might be C. dubliniensis (14). This was confirmed by carbohydrate assimilation tests (Table 2) and by sequencing the 5.8S rRNA gene (Figure 2). With the API 20C AUX kit, all SL isolates yielded the same profile at 48 h, interpreted as 99.9% C. dubliniensis (Table 2). Eleven isolates from LIV-1 and the C. dubliniensis (NCPF 3949) reference strain were also tested with API 32C. All had an identical profile (7143100015), interpreted as 81.9% C. dubliniensis and 16.9% C. albicans. [FIGURES 1-2 OMITTED] ITS sequences of isolates SL375, SL397, SL407, SL410, SL411, SL417, and SL422 were identical to that of C. dubliniensis CD33 genotype 1 (Figure 2). Nevertheless, phenotypic variation among the SL isolate was evident. In addition to variation in trehalose tre·ha·lose n. A sweet-tasting, crystalline disaccharide, C12H22O11, found in trehala and in many fungi. assimilation rates, 3-4 distinct types were apparent in the germ tube test. Three independent inoculations ([10.sup.5] CFU/mL, mid log growth phase) of each isolate gave consistent morphologic differences. One group produced very long germ tubes (SL375-1, SL422, SL417 SL387, SL397, and SL413); another, medium size (SL411, SL407); a third, mainly long germ tubes with cells that aggregate like C. parapsilosis (SL375-2 and SL410); and the last, elongated e·lon·gate tr. & intr.v. e·lon·gat·ed, e·lon·gat·ing, e·lon·gates To make or grow longer. adj. or elongated 1. Made longer; extended. 2. Having more length than width; slender. cigarlike cells that clamped together with few germ tubes (SL370 and SL371). To determine whether C. dubliniensis was present on their outer surface LIV-2 and HHW-2 ticks (n = 102) were individually washed in 1 mL MEM before homogenization homogenization (həmŏj'ənəzā`shən), process in which a mixture is made uniform throughout. Generally this procedure involves reducing the size of the particles of one component of the mixture and dispersing them evenly . C. dubliniensis was cultured from the wash supernatants of 8 of 9 ticks that proved positive after homogenization but not from any of the negative ticks. These findings strongly suggest that the fungus is present in particles adhering to the ticks. The SL isolates (n = 11) were extremely sensitive to antifungals. MIC90s ([micro]g/mL) were as follows: amphotericin B 0.031 (Sigma-Aldrich, Saint Louis, MO, USA), flucytosine 0.031 (Valeant Pharmaceuticals International Valeant Pharmaceuticals International is a pharmaceutical company with activities spanning the drug discovery pipeline from target identification through clinical trials and commercialization. , Aliso Viejo, CA, USA), fluconazole fluconazole /flu·con·a·zole/ (floo-kon´ah-zol) a triazoleantifungal used in the systemic treatment of candidiasis and cryptococcal meningitis. flu·con·a·zole n. 0.125 (Pfizer Inc., Sandwhich, Kent, England, UK), itraconazole itraconazole /it·ra·co·na·zole/ (it?rah-kon´ah-zol) a triazoleantifungal used in a variety of infections. it·ra·con·a·zole n. 0.007 (Ortho Biotech, Bridgewater, NJ, USA), voriconazole 0.007 (Pfizer), posaeonazole 0.007 (Schering-Plough, Kenilworth, N J, USA), ketoconazole ketoconazole /ke·to·co·na·zole/ (ke?to-kon´ah-zol) a derivative of imidazole used as an antifungal agent. ke·to·co·na·zole n. <0.007 (Ortho Biotech), and caspofungin <0.007 (Merck & Co., Inc., Rahway, NJ, USA). Conclusions Our serendipitous isolation of C. dubliniensis from the environment ends speculation (5) that the species might be confined to humans. Because ticks were collected from cracks filled with guillemot guillemot (gĭl`əmŏt'), northern sea bird, genus Cephas, of the auk family. The black guillemot, or trystie, Cephus grylle, is about 13 in. guano guano (gwä`nō), dried excrement of sea birds and bats found principally on the coastal islands of Peru, Africa, Chile, and the West Indies. It contains about 6% phosphorus, 9% nitrogen, 2% potassium, and moisture. and the fungal isolates were associated with the surface of ticks, the most likely source of the fungus is bird excrement. Thus, like C. albicans (8), C. dubliniensis may inhabit the digestive tract of marine birds. Only C. dubliniensis was isolated from the Great Saltee ticks; however, we have detected other Candida spp. from both soil and tick samples (unpub. data) at other seabird colonies, which suggests that marine as well as terrestrial birds (9) carry a variety of yeast species (15). The environmental isolates are members of human C. dubliniensis genotype 1, commonly associated with HIV patients (6). Sequencing of the genotype 1 CD36 isolated from an HIV patient is nearly complete (www.sanger.ac.uk/ sequencing/Candida/dubliniensis). Phylogenetic comparison of variable loci from environmental and human genotype 1 isolates could be used to estimate when they last shared a common ancestor and thus how often C. dubliniensis is transmitted from the environment to humans. Acknowledgments We thank Smart Murray for collecting tick and soil samples from Great Saltee Island and Guido Paesen for reviewing the manuscript. This work was supported by the National Environment Research Council Environmental Genomics and Biodiversity Programs. References (1.) Pfaller MA, Diekema DJ. Rare and emerging opportunistic fungal pathogens: concern for resistance beyond Candida albicans and Aspergillus fumigatus. J Clin Microbiol. 2004;42:4419-31. (2.) Sullivan DJ, Westerneng TJ, Haynes KA, Bennett DA, Coleman DC. Candida dubliniensis sp. nov.: phenotypic and molecular characterization of a novel species associated with oral candidosis in HIV-infected individuals. Microbiology. 1995; 141:1507-21. (3.) Sullivan D, Coleman D. Candida dubliniensis: characteristics and identification. J Clin Microbiol. 1998;36:329-34. (4.) Sullivan D, Haynes K, Bille J, Boerlin P, Rodero L, Lloyd S, et al. Widespread geographic distribution of oral Candida dubliniensis strains in human immunodeficiency virus-infected individuals. J Clin Microbiol. 1997;35:960-4. (5.) Sullivan DJ, Moran GP, Coleman DC. Candida dubliniensis: ten years on. FEMS Microbiol Lett. 2005;253:9-17. (6.) Gee SF, Joly S, Soll DR, Meis JFGM, Verweij PE, Polacheck I, et al. Identification of four distinct genotypes of Candida dubliniensis and detection of microevolution mi·cro·ev·o·lu·tion n. Evolution resulting from a succession of relatively small genetic variations that often cause the formation of new subspecies. in vitro and in vivo. J Clin Microbiol. 2002;40:556-74. (7.) Blignaut E, Pujol C, Joly S, Soll DR. Racial distribution of Candida dubliniensis among South Africans. J Clin Microbiol. 2003;41: 1838-42. (8.) Buck JD. Isolation of Candida albicans and halophilic halophilic pertaining to or characterized by an affinity for salt; requiring a high concentration of salt for optimal growth. Vibrio vibrio Any of a group of aquatic, comma-shaped bacteria in the family Vibrionaceae. Some species cause serious diseases in humans and other animals. They are gram-negative (see spp. from aquatic birds in Connecticut and Florida. Appl Environ Microbiol. 1990;56:826-8. (9.) Cafarchia C, Camarda A, Romito D, Campolo M, Quaglia NC, Tullio D, et al. Occurrence of yeast in cloacae of migratory birds. Mycopathologia. 2006; 161:229-34. (10.) Warren NG, Hazen KC. Candida, Cryptococcus Cryptococcus /Cryp·to·coc·cus/ (-kok´us) a genus of yeastlike fungi, including C. neofor´mans, the cause of cryptococcosis in humans.cryptococ´cal Cryp·to·coc·cus n. and other yeasts of medical importance. In: Murray PR, Baron EJ, Pfaller MA, Tenover FC, Volken RH, editors. Manual of clinical microbiology, 7th ed. Washington: ASM Press; 1999. p. 1184-99. (11.) National Committee for Clinical Laboratory Standards. Reference method for broth dilution antifungal susceptibility testing of yeast, approved standard M27-A. Wayne (PA): The Committee, 1997. (12.) White TJ, Bruns TD, Lee SB, Taylor JW. Amplification and direct sequencing of fungal ribosomal RNA genes for phylogenetics phy·lo·ge·net·ics n. The study of phylogeny. . In: Innis MA, Gelfand DH, Sininsky JJ, White TJ, editors. PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) protocols: a guide to methods and applications. San Diego (CA): Academic Press Inc.; 1990. p. 315-22. (13.) Hall TA. BioEdit: a user-friendly biological sequence alignment editor and analysis program for Windows 95/98/NT. Nucl Acids Symp Ser. 1999;41:95-8. (14.) Gales AC, Pfaller MA, Houston AK, Joly S, Sullivan DJ, Coleman DC, et al. Identification of Candida dubliniensis based on temperature and utilization of xylose Xylose A pentose sugar, referred to in the early literature as l -xylose. It is present in many woody materials. and alpha-methyl-D-glucosidase as determined by API 20C AUX and Vitek YBC systems. J Clin Microbiol. 1999;37:3804-8. (15.) Buck JD. A note on the experimental uptake and clearance of Candida albicans in a young captive gull (Larus sp.). Mycopathologia. 1986;94:59-61. Dr Nunn heads the Tick and Tick-Borne Pathogen Research Group at the Centre for Ecology and Hydrology The Centre for Ecology and Hydrology is a publicly-funded body of the United Kingdom specialising in interdisciplinary scientific research on terrestrial and freshwater environments. in Oxford. His research interests focus on the evolution and transmission of tick-borne pathogens and functional characterization of tick immuno-modulators. Address for correspondence: Miles A. Nunn, National Environment Research Council Centre for Ecology and Hydrology, Mansfield Rd, Oxford OXI 3SR, UK; email: amn@ceh.ac.uk All material published in Emerging Infectious Diseases is in the public domain and may be used and reprinted without special permission; proper citation, however, is required. Miles A. Nunn, * Stefanie M. Schafer, * Michael A. Petrou, ([dagger]) and Jillian R.M. Brown * * National Environment Research Council Centre for Ecology and Hydrology, Oxford, United Kingdom; and ([dagger]) Hammersmith Hospital National Health Service Trust, London, United Kingdom
Table 1. Male and female ticks positive for fungi in culture *
No. positive/no. examined
Site Male Female Both sexes
Happy Hole West (HHW)-1 0/26 0/25 0/51
HHW-2 0/17 0/23 0/40
Labour in Vain (LIV)-1 5/30 8/29 13/59 ([dagger])
LIV-2 5/23 4/20 9/43 ([double dagger])
* Adult Ixodes uriae ticks were collected from within 2 guillemot-
breeding colonies on Great Saltee on August 25, 2004. The ticks were
stored frozen and processed by M.A.N on November 11, 2005. (HHW-1
and LIV-1) and 20. 07.06 (HHW-2 and LIV-2).
([dagger]) Isolates SL370, SL371, SL375, SL387, SL397, SL407, SL410,
SL411, SL413, SL414, SL417, SL422, and SL429.
([double dagger]) Isolates SL495, SL497, SL500, SL501, SL509, SL510,
SL522, SL529, and SL531.
Table 2. Substrate assimilation by Great Saltee fungi and
Candida albicans
API 20C AUX assimilation
profile code *
C. albicans
Substrate SL407 (ATCC90028)
Pentoses
L-arabinose - -
D-xylose - +
Hexoses
D-glucose + +
D-galactose + +
[alpha]-methyl-D-glucoside - +
Disaccharides
D-cellobiose - -
D-lactose - -
D-maltose + +
D-saccharose + +
D-trehalose ([dagger]) - +
Trisaccharides
D-melezitose - -
D-raffinose - -
Alcohols
Glycerol + -
Adonitol + +
Xylitol + +
Inositol - -
D-sorbitol + +
Organic acids
2-keto-gluconate + +
Amino acids
N-acetylglucosamine + +
Identification C. dubliniensis C. albicans
API 20C AUX profile code 6172134 2566174
Predictive value 99.9%, excellent 99.2%,
very good
* Results for 48 hours are shown. All 22 Great Saltee isolates
gave similar profiles.
([dagger]) By 72 hours all Saltee isolates showed some assimilation
of trehalose; the degree of assimilation varied between isolates.
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