Cryptococcus gattii in AIDS patients, Southern California.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. isolates from AIDS patients in southern California were characterized by molecular analyses. Pheromone pheromone Any chemical compound secreted by an organism in minute amounts to elicit a particular reaction from other organisms of the same species. Pheromones are widespread among insects and vertebrates (except birds) and are present in some fungi, slime molds, and algae. MF[alpha]1 and MF[alpha]1 gene fragments were polymerase chain reaction-amplified with fluorescently labeled primers and analyzed by capillary electrophoresis (CE) on 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. analyzer. CE-fragment-length analyses (CE-FLAs) and CE-single-strand conformation con·for·ma·tion n. One of the spatial arrangements of atoms in a molecule that can come about through free rotation of the atoms about a single chemical bond. polymorphisms (CE-SSCPs) were used to determine Cryptococcus gattii (Cg), C. neoformans (Cn) varieties neoformans (CnVN) and grubii (CnVG), mating types, and hybrids. Corroborative cor·rob·o·rate tr.v. cor·rob·o·rat·ed, cor·rob·o·rat·ing, cor·rob·o·rates To strengthen or support with other evidence; make more certain. See Synonyms at confirm. tests carried out in parallel included growth on specialized media and serotyping with a commercial kit. All 276 clinical strains tested as haploid haploid /hap·loid/ (hap´loid) 1. having half the number of chromosomes characteristically found in the somatic (diploid) cells of an organism; typical of the gametes of a species whose union restores the diploid number. MAT[alpha] by CE-FLA. CE-SSCP analyses of MF[alpha]1 showed 219 (79.3%) CnVG, 23 (8.3%) CnVN, and 34 (12.3%) Cg isolates. CE-FLA and CE-SSCP are promising tools for high-throughput screening of Cryptococcus isolates. The high prevalence of Cg was noteworthy, in view of its sporadic reports from AIDS patients in North America and its recent emergence as a primary pathogen on Vancouver Island, Canada. ********** The encapsulated basidiomycete basidiomycete Any of a large and diverse class of fungi (division Mycota), including jelly and shelf, or bracket, fungi; mushrooms, puffballs, and stinkhorns; and the rusts and smuts. Cryptococcus neoformans was recently divided into 2 species, C. neoformans (Cn) and C. gattii (Cg) (1). Cn consists of 2 varieties, grubii (CnVG) and neoformans (CnVN), which are opportunistic pathogens and predominantly infect 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 (2,3). CnVG is the major causative agent of cryptococcosis cryptococcosis: see fungal infection. worldwide, except in central Europe, where CnVN infection is most prominent. In contrast, Cg is a primary pathogen, which predominantly infects immunocompetent im·mu·no·com·pe·tent adj. Having the normal bodily capacity to develop an immune response following exposure to an antigen. im persons (4). Cg was previously thought to be restricted to tropical and subtropical sub·trop·i·cal adj. Of, relating to, or being the geographic areas adjacent to the Tropics. subtropical Adjective of the region lying between the tropics and temperate lands climates with a special ecologic niche on Eucalyptus trees (5,6). However, the recent outbreak of Cg infection in healthy humans and animals in the temperate climate of Vancouver The climate of Vancouver, British Columbia is a moderate oceanic climate (Koppen climate classification Cfb) tempered by the warm Japan Current. The city is also sheltered by the mountains of Vancouver Island, to the west. Island, British Columbia, Canada, and its isolation from several species of trees other than Eucalyptus have raised the strong possibility that this fungus might have broader geographic distribution (7-9). The mechanisms underlying pathogenic and environmental differences between Cn and Cg are not known. Within Cn species, CnVN infections are more likely to display skin involvement and to afflict older patients, whereas CnVG infections are reported to cause a higher mortality rate (3,10). In contrast, infections caused by Cg result in a lower mortality rate but are frequently complicated by neurologic sequelae sequelae Clinical medicine The consequences of a particular condition or therapeutic intervention and require surgery and prolonged therapy (4,11). Our recent studies with the Cu,Zn SOD (SOD1) and MnSOD (SOD2) knockout mutants of Cg indicated that these antioxidants Antioxidants Substances that reduce the damage of the highly reactive free radicals that are the byproducts of the cells. Mentioned in: Aging, Nutritional Supplements antioxidants, n. are crucial for Cg pathogenesis (12,13). In contrast, the antioxidant antioxidant, substance that prevents or slows the breakdown of another substance by oxygen. Synthetic and natural antioxidants are used to slow the deterioration of gasoline and rubber, and such antioxidants as vitamin C (ascorbic acid), butylated hydroxytoluene function of SOD1 in CnVG is less crucial for pathogenesis (14). These observations are the first molecular evidence of a likely divergence in the pathogenic mechanisms used by Cn and Cg. Both Cn and Cg have a single locus, 2-allele mating system comprising MAT[alpha] and MATa strains. The MAT[alpha] strains of Cn and Cg predominate in nature and in clinical settings, and this predominance over MATa strains is linked to high virulence and reproduction by haploid fruiting (3,15). Generally, Cryptococcus strains are haploid, but hybrid strains have also been characterized from both clinical and environmental sources (16-20). Thus, characterizing clinical Cryptococcus isolates to the individual species or varieties and according to mating and hybrid types could be useful for managing cryptococcosis cases and for further understanding the epidemiology of this disease. Several laboratory typing methods have been used in epidemiologic studies of cryptococcosis, including serotyping, electrophoretic karyotyping Karyotyping A laboratory test used to study an individual's chromosome make-up. Chromosomes are separated from cells, stained, and arranged in order from largest to smallest so that their number and structure can be studied under a microscope. , use of mitochondrial DNA probes, use of genomic DNA probes, determination of allelic al·lele n. One member of a pair or series of genes that occupy a specific position on a specific chromosome. [German Allel, short for Allelomorph, allelomorph, from English variations at the URA Ura uracil. 5 locus, multilocus enzyme typing, measurement of creatinine utilization, polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) ), fingerprinting and amplified fragment-length polymorphism (reviewed in [2]). Previously, we described a PCR-restriction fragment length polymorphism (PCR-RFLP PCR-RFLP Polymerase Chain Reaction–Restriction Fragment Length Polymorphism ) typing scheme for Cn and Cg pheromone genes, which could be used for characterizing mating types, hybrids, and variety (21). In the present study, we developed a capillary electrophoresis-fragment length analysis (CE-FLA) test, and a CE-single stranded conformation polymorphism (CE-SSCP) test by using the pheromone genes MF[alpha]1 and MF[alpha]1. These tests were used in parallel with more traditional specialized culture medium and a commercial serotyping kit to characterize Cryptococcus isolates from AIDS patients in southern California. Materials and Methods Cryptococcus Isolates Two hundred seventy-six Cryptococcus isolates originating from patients with HIV/AIDS HIV/AIDS Human Immunodeficiency Virus/Acquired Immune Deficiency Syndrome were obtained from the Infectious Diseases Laboratory, Los Angeles County Hospital, Los Angeles, California. The isolates were suspended in sterile skim milk skim milk n. The milk from which the cream has been removed. skim milk the residue from whole milk after the cream has been skimmed off. In today's usage it is the residue after the butterfat is removed. and stored at -20[degrees]C. The isolates were transferred frozen to the Mycology mycology Study of fungi (see fungus), including mushrooms and yeasts. Many fungi are useful in medicine and industry. Mycological research has led to the development of such antibiotic drugs as penicillin, streptomycin, and tetracycline. Laboratory of the Wadsworth Center in Albany, New York For other uses, see Albany. Albany is the capital of the State of New York and the county seat of Albany County. Albany lies 136 miles (219 km) north of New York City, and slightly to the south of the juncture of the Mohawk and Hudson Rivers. , USA, where they were streaked on Niger seed agar plates (3) to check for purity and reconfirmation of their identity; a typical colony was picked for further analysis. The subcultures were placed in long-term storage in sterile 15% glycerol glycerol, glycerin, glycerine, or 1,2,3-propanetriol (prō`pāntrī'ŏl), CH2OHCHOHCH2OH, colorless, odorless, sweet-tasting, syrupy liquid. at -70[degrees]C. These isolates were further characterized in our laboratory by testing their growth on canavanine-glycine-bromothymol blue (CGB CGB Certified Graduate Builder (professional builder designation) CGB Consumer and Governmental Affairs Bureau CGB Commonwealth Geographical Bureau (UK) CGB Game Boy Color ) agar for differentiation of Cryptococcus species (22) and serotyping with Crypto Check Kit (Iatron Laboratories Inc., Tokyo, Japan). Several investigators gave strains to put together a panel of reference isolates that were either currently being used in molecular pathogenesis studies, represented type strains, or were otherwise unique. The details of these 16 reference isolates are listed in Table 1. Six additional A/D A/D See advance-decline line (A/D). hybrid strains, characterized in our earlier study, were also used (18). Multiplex PCR for Pheromone Genes A previous report from this laboratory described the use of specific primers for amplification of MF[alpha]1 and MFa1 gene fragments, which could be separated as 100-bp and 117-bp fragments on a specialized agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gel (21). The primer sets V290/V291, which was earlier designed to amplify MFa1 gene from CnVN, did not amplify similar genes from MATa strains of either CnVG or Cg. Multiple alignment of MFa1 indicated that this gene is highly polymorphic among CnVG, CnVN, and Cg (Figure 1). Therefore, 2 new sets of primers were designed to obtain MFa1 amplicons from CnVG and Cg. These primers are listed in Table 2. A multiplex PCR for simultaneous amplification of MF[alph]1 and MFa1 in a 50-[micro]L reaction volume was performed with 5 [micro]L of 10x PCR buffer with 15 mmol/L Mg[Cl.sub.2], 2.5 [micro]L of each of 8 primers (10 [micro]mol/L stock), 3.0 [micro]L dNTP mix (10 [micro]mol/L each), and 2.0 U Taq DNA polymerase DNA polymerase /DNA po·lym·er·ase/ (pah-lim´er-as) any of various enzymes catalyzing the template-directed incorporation of deoxyribonucleotides into a DNA chain, particularly one using a DNA template. (Perkin Elmer, Foster City, CA, USA). The template DNA was 5.0 [micro]L of either a boiled cell suspension or 50 ng genomic DNA. Initial denaturation denaturation, term used to describe the loss of native, higher-order structure of protein molecules in solution. Most globular proteins exhibit complicated three-dimensional folding described as secondary, tertiary, and quarternary structures. was conducted at 95[degrees]C for 3 min, followed by 30 cycles of denaturation at 94[degrees]C for 1 min, annealing annealing (ənēl`ĭng), process in which glass, metals, and other materials are treated to render them less brittle and more workable. at 57.5[degrees]C for 1 min, amplification at 72[degrees]C for 1 min, and final extension at 72[degrees]C for 7 min, in a GeneAmp PCR System 9600 (Perkin Elmer). In preliminary experiments, PCR products (10-[micro]L aliquots) were resolved by electrophoresis on 3.5% MetaPhor agarose (FMC See fixed mobile convergence. Bio-Products, Rockland, ME, USA) gels in Tris-borate-EDTA (TBE) buffer, and were detected by ethidium bromide staining. The PCR experiments were repeated twice, and identical results were obtained. Gene Scan Analysis The MF[alpha]1 sense primer (V190) was labeled with FAM FAM 5-FU, adriamycin/doxorubicin, mitomycin C Oncology A chemotherapeutic regimen used with varying degrees of failure for advanced gastric CA. See Stomach cancer. (6-carboxyfluorescein) at the 5' end, the antisense antisense, DNA or RNA manipulated in a laboratory so that its components (nucleotides) form a complementary copy of normal, or "sense," messenger RNA (mRNA; see nucleic acid). primer (V191) was labeled with tetrachloro-fluorescein (TET) at the 3' end, and Mfa1 sense primers (V290, V1311, V1313) were labeled with 6-carboxy-2', 4', 4', 5', 7', 7'-hexachlorofluorescein (HEX) at the 5' end. The fluorescent dye-labeled primers were custom ordered (Operon Technologies, Inc., Alameda, CA, USA). FLA FLA Florida (old style) FLA Macromedia Flash (file extension) FLA Flash Files (file extension) FLA Fair Labor Association FLA Front Line Assembly and SSCP (1) (System Services Control Point) A controlling program in an SNA domain. It resides in the host and is a component within VTAM. See also SCCP. of the MF[alpha]1 and MFa1 PCR amplicons were determined by CE with an 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. PRISM 310 Genetic Analyzer, and the electronic images were analyzed by using GeneScan analysis software (Applied Biosystems Inc., Foster City, CA, USA). The sample preparation for CE consisted of 1 [micro]L MF[alpha]1 and Mfa1 PCR amplicons, 12 [micro]L highly deionized de·i·on·ize tr.v. de·i·on·ized, de·i·on·iz·ing, de·i·on·iz·es To remove ions from (a solution) using an ion-exchange process. de·i formamide, and 0.5 [micro]L GeneScan-500 (TAMRA TAMRA Technical And Miscellaneous Revenue Act of 1988 TAMRA Tetramethyl-6-Carboxyrhodamine (dye) ) size standard (Applied Biosystems). The sample mixture was denatured de·na·ture tr.v. de·na·tured, de·na·tur·ing, de·na·tures 1. To change the nature or natural qualities of. 2. for 5 min at 95[degrees]C and was then rapidly cooled on ice before loading on the instrument. For CE-FLA, the samples were analyzed under denaturing conditions (POP-4 polymer [Applied Biosystems] in buffer supplied by manufacturer) at 60[degrees]C, and for CESSCP, the samples were analyzed under nondenaturing conditions (3% GeneScan polymer in 1x TBE buffer with 10% glycerol) at 30[degrees]C. A capillary (47 cm x 50 [micro]m inside diameter) was installed, and POP-4 or 3% polymer was filled according to manufacturer's instructions. The electrophoresis conditions for CE-FLA were 5-s injection time, 15-kV injection voltage, 15-kV electrophoresis voltage, 150-s syringe pump time, 120-s preinjection electrophoresis, and 20-min collection time for each sample, and the run was performed at 60[degrees]C. The electrophoresis conditions for CE-SSCP were 5-s injection time, 15-kV injection voltage, 13-kV electrophoresis voltage, 30-s syringe pump time with no preinjection time, and 20-min collection time for each sample, and the run was performed at 30[degrees]C. CE-FLA and CE-SSCP standardization experiments were carried out on [greater than or equal to] 4 independent occasions, and unknown sample analyses were repeated at least once. Results Multiplex PCR The 4 sets of primers (MF[alpha]a1/MFa1) produced reproducible results for control CnVG, CnVN, Cg haploids (Figure 2A), and A/D hybrid strains (Figure 2B). These results validated the robustness of the primers, which had been designed from well within the open reading frames of 2 pheromone genes, to prevent amplification of any non-target DNA. The latter objective also informed the decision to anchor the 3' ends of all PCR primers within the characteristic Cys-Val-Ile-Ala (CVIA CVIA Computer Virus Industry Association ) motifs; this eliminated any possible amplification of other pheromone genes since this is the only sequence shared among fungal pheromones pheromones, any of a variety of substances, secreted by many animal species, that alter the behavior of individuals of the same species. Sex attractant pheromones, secreted by a male or female to attract the opposite sex, are widespread among insects. (18). Even though multiple copies of MF[alpha] and MFa genes have been reported in C. gattii and C. neoformans by Southern hybridization hybridization /hy·brid·iza·tion/ (hi?brid-i-za´shun) 1. crossbreeding; the act or process of producing hybrids. 2. molecular hybridization 3. and whole genome-sequencing, PCR primers only amplify single amplicons because these genes have identical nucleotide sequences (18,23,24). Although this multiplex method was well suited for identifying mating types and hybrids, further delineation of species and varieties would require restriction digestion with several unique enzymes as we stated previously (21). Therefore, we decided to use CE-FLA and CESSCP to further characterize pheromone gene amplicons. These techniques have been successfully used to delineate fragment length as well gene mutations for characterizing various fungal and bacterial isolates (25-27). The SSCP analysis displays migration of the amplified DNA fragment as a function of that fragment's structural conformation. Given that the tertiary structure of a fragment is sensitive to single nucleotide substitutions, this method was shown to be suitable for detecting single nucleotide changes when 100-bp to 300-bp DNA fragments were analyzed (28). Since amplified pheromone fragments yield [approximately equal to] 100- to 120-bp products, they were an ideal substrate for this method of mutant detection. [FIGURE 2 OMITTED] CE-FLA The 16 reference strains of known Cryptococcus species, varieties, mating types, and hybrids were used to establish a robust CE-FLA protocol with denaturing POP4 polymer at 60[degrees]C. The electrophoretic runs with POP-4 polymer produced a 112-bp DNA fragment for Mfa1 and 97-bp fragment for MF[alpha]1, which were easily distinguished with the GeneScan software by the characteristic peak sizes (Figure 3). CE-FLA allowed Cryptococcus mating types and hybrids to be identified, but not CnVG, CnVN, and Cg. [FIGURE 3 OMITTED] CE-SSCP CE-SSCP test under nondenaturing conditions with 3% GeneScan polymer at 30[degrees]C allowed characteristic peak patterns to be detected in MF[alpha]1 and MFa1 genes because of the individual differences within the nueleotide sequences. Distinct patterns obtained for CnVG, CnVN, and Cg by using MF[alpha]1 gene are shown in Figure 4. The sense strand (labeled blue) yielded 1 characteristic peak pattern, while the antisense strand antisense strand one of the two strands in a DNA molecule that is not transcribed. (labeled green) yielded 2-3 characteristic peak patterns. We subsequently decided to label only the sense strand to reduce the cost of the PCR primers as well the complexity of the peak patterns observed with antisense strand. For determining an unknown sample, the instrument analyses needed to yield highly reproducible results. Therefore, a sample of each of the Cryptococcus strains was injected on 4 separate occasions into the same capillary, and the precision of the sizing was calculated. The low standard deviations associated with each mean peak value indicated that the assignment of variety or species for an unknown sample, based on pattern sizing information alone, would be highly reliable (Table 3). [FIGURE 4 OMITTED] Based on our success with MF[alpha]1 sense primer in the detection of characteristic peaks for CnVG, CnVN, and Cg, we labeled Mfa1 sense strands and analyzed MATa strains. In this case, we had to use individual sets of Mfa1 primers because of the substantial polymorphism observed at the 5' and 3' end of this gene between Cg and Cn, and within Cn varieties (Figure 1). Again, the Mfa1 peak pattern was unique to each Cn variety and Cg (Table 3). Overall, our results indicated that either MF[alpha]1 or Mfa1 gene products yielded unique SSCP patterns and could be used for identifying Cn varieties and Cg strains. California Isolates We used standardized CE-FLA and CE-SSCP techniques to analyze 276 isolates of Cryptococcus that were obtained from AIDS patients and that were stored at the Infectious Diseases Laboratory, Los Angeles County Hospital, Los Angeles, California. The investigations were fully compliant with Los Angeles County Hospital-University of Southern California (USC An abbreviation for U.S. Code. ) Institutional Review Board guidelines (proposal #924008). CE-FLA showed that all 276 isolates were MATa strains, and no MATa or hybrid strains were found in our samples. CESSCP found that among the total 276 clinical isolates, 219 (79.3%) were CnVG, 23 (8.3%) were CnVN, and 34 (12.3%) were Cg. For corroborations, all of these isolates were also tested by growth on CGB agar, and by serotyping with the Crypto Check Kit, both of which yielded results in agreement with those obtained with pheromone typing. Discussion The relatively high prevalence of Cg in this survey is noteworthy for several reasons (Table 4). First, we believe it is the first instance in which a large number of Cg clinical isolates from AIDS patients have been identified in the United States. Second, Cg has never been considered a substantial cause of cryptococcosis among US AIDS patients, including those in the southern California. Third, the presence of Cg in HIV-AIDS patient samples in the USC collection is similar to the prevalence recently reported from some countries in Central and South America (29), and it contrasts with the rare occurrence of Cg in immunocompromised patient populations in Australia, Southeast Asia, and Africa (30-32). The prevalence of CnVN (8%) in our samples closely matches its recently reported prevalence in New York City New York City: see New York, city. New York City City (pop., 2000: 8,008,278), southeastern New York, at the mouth of the Hudson River. The largest city in the U.S. (33). Thus, cryptococcosis due to CnVN in AIDS patients is not a rare clinical entity in the United States, and its pattern of distribution on the East and West Coasts does not differ. The absence of MATa strains in our samples is not surprising, in view of the rare occurrence of this mating type among clinical and environmental specimens (34). This finding is consistent with the results of other recent clinical and environmental surveys in the United States, Europe, and Australia. The Cg outbreak on Vancouver Island also yielded only MAT[alpha] isolates (8,35). Overall, our inferences are based on limited data, since most published studies on cryptococcosis do not include detailed characterization of Cryptococcus strains. Future epidemiologic studies will likely yield a more complete picture of the causative varieties or species of Cryptococcus across the United States. As previously noted, CnVG infections are predominant in AIDS patients around the world, except in Europe, where CnVN is seen in sizable numbers. One explanation for this phenomenon is that CnVG is best adapted for the colonization of soil and pigeon droppings. However, CnVN may dominate the same ecologic niche in parts of Europe for undetermined causes (10). The lower incidence of Cg infection in AIDS patients could be due to the paucity of regions around the world in which Cg is endemic and the reported association of Cg disease with the flowering of Eucalyptus camaldulensis trees in certain areas (6). The unprecedented outbreak of Cg infection in Vancouver Island already comprises 66 human and 50 animal cases of cryptococcosis. Ongoing investigation in Vancouver Island indicate that the numbers of human and animal cases are increasing (130 human cases and >200 animal cases), which led to the recent change in the definition of Cg outbreak to Cg endemicity in this region (7). Additionally, Cg was isolated from swab samples from the bark of trees of many species (alder, arbutus arbutus Any of about 14 species (genus Arbutus) of broad-leaved evergreen shrubs or trees, in the heath family. Native to southern Europe and western North America, they are characterized by loosely clustered white or pink flowers and red or orange berries. A. , bitter cherry, cedar, fir, garry oak, maple, spruce), as well as from soil and air samples near these trees (7). These investigations have added a new dimension to our understanding of Cg ecology and suggest that this pathogen is neither restricted in its geographic distribution nor to its presumed natural host, Eucalyptus trees. Our results indicated that both CE-FLA and CE-SSCP of pheromone genes are amenable to semi-automation and large-scale analyses of pathogenic Cryptococcus species, varieties, mating types, and hybrids. Each step of this analysis, namely, PCR, heat denaturation with formamide, and subsequent loading of samples, can be carried out in 48- or 96-well trays, which allow the use of multichannel or automated pipettors. Both CE-FLA and CE-SSCP individual runs are completed in [less than or equal to] 20 min, and the instrument can be programmed for multiple runs, thereby giving a high throughput. Thus, analyzing hundreds to thousands of strains is a good possibility, especially in reference laboratories. Moreover, the electrophoretic runs are saved as electronic files for easy portability over the Internet and to facilitate interlaboratory comparisons. This study reports a logical improvement over our earlier published method on pheromone PCR-RFLP for characterizing Cryptococcus isolates. The use of CE-FLA and CE-SSCP allowed us to dispense with To permit the neglect or omission of, as a form, a ceremony, an oath; to suspend the operation of, as a law; to give up, release, or do without, as services, attention, etc.; to forego; to part with To allow by dispensation; to excuse; to exempt; to grant dispensation to or for. running specialized gels as well as the use of unique restriction digestion schemes (21). Thus, CE-FLA alone leads to visualization of size differences in MF[alpha]1 versus Mfa1 pheromones, which would distinguish mating types and hybrids. The species and varieties could be distinguished by CE-SSCP on the basis of polymorphisms in nucleotide sequences of MF[alpha]1 and Mfa1 in Cg, CnVG, and CnVN. Thus, 1 typing method had the potential to replace multiple tests, such as specialized media and serotyping kits for species/variety determination, crossing with tester strains on mating agar, and flow cytometry flow cytometry (flōˑ sī·t  ˑ·m for hybrid determination. The current
limitations of this approach include the use of 2 polymers and nm
temperatures, which makes it necessary to run CE-FLA and CESSCP as batch
applications on ABI 310 Genetic Analyzer. Since individual
electrophoretic runs are completed in [approximately equal to] 20 min,
[approximately equal to] 16 hours will be necessary to analyze
[approximately equal to] 45 samples (one 48-sample tray) by CE-FLA,
followed by change of polymer and run conditions, and another 16 hours
to complete CE-SSCP analyses. However, these limitations could be easily
overcome in the upgraded model of this instrument (ABI 3130), which has
4-16 capillaries and hands-free, 24-hour operation capabilities for
simultaneous analyses of multiple samples, thereby considerably
decreasing turnaround time (1) In batch processing, the time it takes to receive finished reports after submission of documents or files for processing. In an online environment, turnaround time is the same as response time. .Acknowledgments We thank Birgit Stein and Andrea Doney for technical support and Adriana Verschoor for editorial comments. This study was funded in part with NIH "Not invented here." See digispeak. NIH - The United States National Institutes of Health. grants AI-48462 (S.C.), AI-41968 (S.C.), AI-53732 (V.C.) and an educational award from Pfizer Inc. (V.C.). References (1.) Kwon-Chung KJ, Boekhout T, Fell JW, Daiz M. Proposal to conserve the name Cryptococcus gattii against C. hondurianus and C. bacillisporus (Basidiomycota, Hymenomycetes, Tremellomycetidae). Taxon. 2002;51:804-6. (2.) Casadevall A, Perfect JR. Cryptococcus neoformans, 1st ed. Washington: ASM (1) (Association for Systems Management) An international membership organization based in Cleveland, Ohio. Founded in 1947 and disbanded in 1996, it sponsored conferences in all phases of administrative systems and management. Press; 1998. (3.) Kwon-Chung KJ, Bennett JE. Medical mycology. Philadelphia: Lea & Febiger; 1992. (4.) Speed BR, Dunt n. 1. A blow. D. Clinical and host differences between infections with two varieties of Cryptococcus neoformans. Clin Infect Dis. 1995;21:28-34. (5.) Lazera MS, Cavalcanti MA, Londero AT, Trilles L, Nishikawa MM, Wanke B. Possible primary ecological niche of Cryptococcus neoforroans. Med Mycol. 2000;38:379-83. (6.) Sorrell TC. Cryptococcus neoformans variety gattii. Med Mycol. 2001;39:155-68. (7.) Bartlet K. Canadian Cryptococcus gattii--temporary visa or landed immigrant? Abstr. S13, p 71. In: Abstracts of the 6th International Conference on Cryptococcus and Cryptococcosis, Boston, MA, USA. Boston: Boston University School of Medicine Boston University School of Medicine (BUSM) is one of the graduate schools of Boston University. It is an American medical school located in the South End neighborhood of Boston, Massachusetts. ; 2005. (8.) Kidd SE, Hagen F, Tscharke RL, Huynh M, Bartlett KH, Fyfe M, et al. A rare genotype of Cryptococcus gattii caused the cryptococcosis outbreak on Vancouver Island (British Columbia, Canada). Proc Natl Acad Sci U S A. 2004;101:17258-63. (9.) Stephen C, Lester S, Black W, Fyfe M, Raverty S. Multispecies outbreak of cryptococcosis on southern Vancouver Island, British Columbia. Can Vet J. 2002;43:792-4. (10.) Dromer F, Mathoulin S, Dupont B, Letenneur L, Ronin ronin (rō`nĭn), in Japanese history, masterless samurai. Ronin were retainers who were deprived of their place in the usual loyalty patterns of Japanese feudalism. B. 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Dimorphism dimorphism /di·mor·phism/ (di-mor´fizm) the quality of existing in two distinct forms.dimor´phicdimor´phous sexual dimorphism 1. physical or behavioral differences associated with sex. and haploid fruiting in Cryptococcus neoformans: association with the [alpha]-mating type. Proc Natl Acad Sci U S A. 1996;93:7327-31. (16.) Boekhout T, Theelen B, Diaz M, Fell JW, Hop WC, Abeln EC, et al. Hybrid genotypes in the pathogenic yeast Cryptococcus neoformans. Microbiology. 2001;147:891 907. (17.) Brandt MS, Bragg SL, Pinner RW. Multilocus enzyme typing of Cryptococcus neoformans. J Clin Microbiol. 1993;31:2819-23. (18.) Chaturvedi V, Fan J, Stein B, Behr MJ, Samsonoff WA, Wickes BL, et al. Molecular genetic analyses of mating pheromones reveals inter-variety mating/hybridization in Cryptococcus neoformans. Infect Immun. 2002;70:5225-35. (19.) Lengeler KB, Cox GM, Heitman J. Serotype AD strains of Cryptococcus neoformans are diploid diploid /dip·loid/ (dip´loid) 1. having two sets of chromosomes, as normally found in the somatic cells; in humans, the diploid number is 46. 2. an individual or cell having two full sets of homologous chromosomes. or aneuploid an·eu·ploid n. A cell or an organism characterized by aneuploidy. Aneuploid An abnormal number of chromosomes in a cell. and are heterozygous het·er·o·zy·gous adj. 1. Having different alleles at one or more corresponding chromosomal loci. 2. Of or relating to a heterozygote. at the mating-type locus. Infect Immun. 2001;69:115-22. (20.) Tanaka R, Nishimura K, Miyaji M. Ploidy ploidy Number of sets of chromosomes in the nucleus of a cell. In normal human body cells, chromosomes exist in pairs, a condition called diploidy. During meiosis the cell produces sex cells (gametes), each containing half the normal number of chromosomes, a condition called of serotype AD strains of Cryptococcus neoformans. J Med Mycol. 1999;40:31-4. (21.) Chaturvedi S, Rodeghier B, Fan J, McClelland CM, Wickes BL, Chaturvedi V. Direct PCR of Cryptococcus neoformans MAT[alpha] and MATa pheromones to determine mating types, ploidy, and variety: a tool for epidemiological and molecular pathogenesis studies. J Clin Microbiol. 2000;38:2007-9. (22.) Kwon-Chung KJ, Polacheck I, Bennett JE. Improved diagnostic medium for separation of Cryptococcus neoformans var. neoformans (serotype A and D) and Cryptococcus neoformans var. gattii (serotype B and C). J Clin Microbiol. 1982;15:535-7. (23.) Davidson RC, Moore TD, Odom AR, Heitman J. Characterization of the MF[alpha] pheromone of the human fungal pathogen Cryptococcus neoformans. Mol Microbiol. 2000;38:1017-26. (24.) McClelland CM, Fu J, Woodlee GL, Seymour TS, Wickes BL. Isolation and characterization of the Cryptococcus neoformans MATa pheromone gene. Genetics. 2002;160:935-47. (25.) Baere TD, Claeys G, Swinne D, Massonet C, Verschraegen G, Muylaert A, et al. Identification of cultured isolates of clinically important yeast species using fluorescent fragment length analysis of the amplified internally transcribed rRNA spacer 2 region. BMC (BMC Software, Inc., Houston, TX, www.bmc.com) A leading supplier of software that supports and improves the availability, performance, and recovery of applications in complex computing environments. Microbiol. 2002;2:21-8. (26.) Ghozzi R, Morand P, Ferroni A, Bereti JL, Bingen E, Segond C, et al. Capillary electrophoresis-single strand confirmation polymorphism analysis for rapid identification of Pseudomonas aeruginosa Pseudomonas aeruginosa A normal soil inhabitant and human saprophyte that may contaminate various solutions in a hospital, causing opportunistic infection in weakened Pts Clinical Infective endocarditis in IVDAs, RTIs, UTIs, bacteremia, meningitis, 'malignant' and other gram-negative nonfermenting bacilli bacilli /ba·cil·li/ (bah-sil´i) plural of bacillus. bacilli see bacillus. recovered from patients with cystic fibrosis. J Clin Microbiol. 1999;37:3374-9. (27.) Montiel D, Dickinson MJ, Lee HA, Dyer PS, Jeenes DJ, Roberts 1N, et al. Genetic differentiation of the Aspergillus Aspergillus Any fungus of the genus Aspergillus of the Fungi Imperfecti (form-class Deuteromycetes). Species for which the sexual phase is known are placed in the order Eurotiales. A. niger causes black mold on some foods; A. niger, A. flavus, and A. section Flavi complex using AFLP fingerprints. Mycol Res. 2003; 107:143427-13. (28.) Sheffield VC, Beck JS, Kwitek AE, Sandstrom DW, Stone EM. The sensitivity of single-strand conformation polymorphism analysis for the detection of single base substitutions. Genomics. 1993;16: 325-32. (29.) Castanon-Olivares LR, Arreguin-Espinosa R, Ruiz-Palacios y Santos G, Lopez-Martinez R. Frequency of Cryptococcus species and varieties in Mexico and their comparison with some Latin American countries. Rev Latinoam Microbiol. 2000;42:35-40. (30.) Chen SC. Cryptococcosis in Australasia and the treatment of cryptococcal and other fungal infections with liposomal amphotericin B. J Antimicrob Chemother. 2002;49(Suppl 1):57-61. (31.) Karstaedt AS, Crewe-Brown HH, Dromer F. Cryptococcal meningitis caused by Cryptococcus neoformans var. gattii, serotype C, in AIDS patients in Soweto, South Africa. Med Mycol. 2002;40:7-11. (32.) Poonwan N, Mikami Y, Poosuwan S, Boon-Long J, Mekha N, Kusum M, et al. Serotyping of Cryptococcus neoformans strains isolated from clinical specimens in Thailand and their susceptibility to various antifungal agents. Eur J Epidemiol. 1997;13:335-40. (33.) Steenbergen JN, Casadevall A. Prevalence of Cryptococcus neoformans vat. neoformans (Serotype D) and Cryptococcus neoformans var. grubii (Serotype A) isolates in New York City. J Clin Microbiol. 2000;38:1974-6. (34.) Kwon-Chung KJ, Bennett JE. Distribution of cr and a mating types of Cryptococcus neoformans among natural and clinical isolates. Am J Epidemiol. 1978;108:337-40. (35.) Fraser JA, Subaran RL, Nichols CB, Heitman J. Recapitulation recapitulation, theory, stated as the biogenetic law by E. H. Haeckel, that the embryological development of the individual repeats the stages in the evolutionary development of the species. of the sexual cycle of the primary fungal pathogen Cryptococcus neoformans var. gattii: implications for an outbreak on Vancouver Island, Canada. Eukaryot Cell. 2003;2:1036-45. Sudha Chaturvedi,* ([dagger]) Madhu Dyavaiah, * Robert A. Larsen, ([double dagger]) ([section]) and Vishnu Chaturvedi * ([dagger]) * Wadsworth Center, Albany, New York, USA; ([dagger]) State University of New York (body) State University of New York - (SUNY) The public university system of New York State, USA, with campuses throughout the state. , Albany, Albany, New York, USA; ([double dagger]) University of Southern California The U.S. News & World Report ranked USC 27th among all universities in the United States in its 2008 ranking of "America's Best Colleges", also designating it as one of the "most selective universities" for admitting 8,634 of the almost 34,000 who applied for freshman admission , Los Angeles, California, USA; and ([section]) Los Angeles County Hospital, Los Angeles, California, USA Dr Sudha Chaturvedi is a research scientist in the Mycology Laboratory of the Wadsworth Center (New York State Department of Health) and an assistant professor of biomedical sciences, School of Public Health, State University of New York, Albany. Her research interests include fungal and parasite pathogenesis, protein transport and secretion mechanisms, and molecular epidemiology. Address for correspondence: Vishnu Chaturvedi, Mycology Laboratory, Wadsworth Center, 120 New Scotland Ave, Albany, NY 12208-2002, USA; fax: 518-486-7811; email: vishnu@wadsworth.org
Table 1. Cryptococcus neoformans (Cn) and Cryptococcus gattii (Cg)
strains used in this study for standardization of reagents *
Strain identity Variety/species Mating type
H99 (NYSD 1649) CnVG [alpha]
KN99[alpha] CnVG [alpha]
KN99a CnVG a
IUM96-2828 CnVG a
NIH12 (ATCC 28959) CnVN [alpha]
JEC21 CnVN [alpha]
JEC20 CnVN a
NIH430 (ATCC 28958) CnVN a
NIH433 (ATCC 34875) CnVN a
NIH444 (ATCC 32609) Cg [alpha]
NIH191 (ATCC 32608) Cg a
NIH198 Cg a
WM0135 Cg a
WM-138 Cg a
UM2 Hybrid (A/D) [alpha]/a
UM8 Hybrid (A/D) [alpha]/a
Strain identity Source
H99 (NYSD 1649) New York State Herbarium, Albany, NY
KN99[alpha] J. Heitman, Duke University, Durham, NC
KN99a J. Heitman, Duke University, Durham, NC
IUM96-2828 B.L. Wickes, University of Texas Health
Sciences Center, San Antonio, TX
NIH12 (ATCC 28959) ATCC, Manassas, VA
JEC21 J.C. Edman, University of California
San Francisco (UCSF), San Francisco, CA
JEC20 J.C. Edman, UCSF, San Francisco, CA
NIH430 (ATCC 28958) ATCC, Manassas, VA
NIH433 (ATCC 34875) ATCC, Manassas, VA
NIH444 (ATCC 32609) ATCC, Manassas, VA
NIH191 (ATCC 32608) ATCC, Manassas, VA
NIH198 K.J. Kwon-Chung, National Institutes of Health,
Bethesda, MD
WM0135 W. Meyer, University of Sydney, Sydney,
Australia
WM-138 W. Meyer, University of Sydney, Sydney,
Australia
UM2 F. Dromer, Institute Pasteur, Paris, France
UM8 F. Dromer, Instotite Pasteur, Paris, France
* ATCC, American Type Culture Collection; VG, var. grubiii; VN, var.
neoformans.
Table 2. Primers used in this study *
Primer name Sequence Target
V190-5' 5'-CTTCACTGCCATCTTCACCA-3' MF[alpha]1-Cg, CnVN,
and CnVG
V191-3 5'-GACACAAAGGGTCATGCCA-3'
V290-5" 5'-CGCCTTCACTGCTACCTTCT-3' MFa1-CnVN
V291-3 5'-AACGCAAGAGTAAGTCGGGC-3'
V1311-5' 5'-TGCCTTCACTGCTATCTTCT-3' MFa1-CnVG
V1312-3' 5'-AACGCAAGAGTAGGTAGGAC-3'
V1313-5' 5'-CGCCTTCACTGCTATCTTTTC-3' MFa1-Cg
V1314-3' 5'-CACACAAGAGTAAGTGATGC-3'
Primer name Source/reference
V190-5' (21)
V191-3
V290-5" (21)
V291-3
V1311-5' This study
V1312-3'
V1313-5' This study
V1314-3'
* Cn, Cryptococcus neoformans; Cg, Cryptococcus gattii; VN, var.
neoformans; VG, var. grubii.
Table 3. Calibration of SSCP peak positions for CnVG, CnVN,
and Cg *
Cn strains Sense strand peak ([dagger])
CnVG (KN99[alpha]; MAT[alpha]) 3230.57 [+ or -] 0.37
CnVG (KN99a; MATa) 4501.35 [+ or -] 1.29
CnVN (NIH12; MAT [alpha]) 3252.77 [+ or -] 1.29
CnVN (NIH340; MATa) 4643.75 [+ or -] 1.12
Cg (NIH 444, MAT[alpha]) 3161.54 [+ or -] 0.95
Cg (NIH 198, MATa) 4593.35 [+ or -] 1.2
* SSCP, single-strand conformation polymorphisms; Cn, Cryptococcus
neoformans; Cg, Cryptococcus gattii; VN, var. neoformans, VG, var.
grubii.
([dagger]) Mean [+ or -] SD of 4 independent experiments.
Table 4. Relative distribution of CnVG, CnVN, and Cg in HIV-AIDS
patients from southern California
Isolates * n (%) (N = 276)
CnVG 219 (79.3)
CnVN 23 (8.3)
Cg 34 (12.3)
* Cn, Cryptococcus neoformans; Cg, Cryptococcus gattii; VN, var.
neoformans; VG, var. grubii.
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