Your search keyword '"Quindós, G."' showing total 19 results

1. Impact of Aspergillusspp. isolation in the first 24 hours of admission in critically ill patients with severe influenza virus pneumonia

Author

Claverias, L., Daniel, X., Martín-Loeches, I., Vidal-Cortez, P., Gómez-Bertomeu, F., Trefler, S., Zaragoza, R., Borges-Sa, M., Reyes, L.F., Quindós, G., Peman, J., Bodí, M., Díaz, E., Sarvisé, C., Pico, E., Papiol, E., Solé-Violan, J., Marín-Corral, J., Guardiola, J.J., and Rodríguez, A.

Abstract

To determine the incidence and impact of Aspergillusspp. isolation (AI) on ICU mortality in critically ill patients with severe influenza pneumonia during the first 24h of admission.

Published

2022

2. Impact of a multifaceted educational intervention including serious games to improve the management of invasive candidiasis in critically ill patients

Author

Ferrer, R., Zaragoza, R., Llinares, P., Maseda, E., Rodríguez, A., and Quindós, G.

Abstract

Infections caused by Candida species are common in critically ill patients and contribute to significant morbidity and mortality. The EPICO Project (Epico 1 and Epico 2.0 studies) recently used a Delphi approach to elaborate guidelines for the diagnosis and treatment of this condition in critically ill adult patients. We aimed to evaluate the impact of a multifaceted educational intervention based on the Epico 1 and Epico 2.0 recommendations.

Published

2017

3. Multicenter Study of Epidemiological Cutoff Values and Detection of Resistance in Candidaspp. to Anidulafungin, Caspofungin, and Micafungin Using the Sensititre YeastOne Colorimetric Method

Author

Espinel-Ingroff, A., Alvarez-Fernandez, M., Cantón, E., Carver, P. L., Chen, S. C.-A., Eschenauer, G., Getsinger, D. L., Gonzalez, G. M., Govender, N. P., Grancini, A., Hanson, K. E., Kidd, S. E., Klinker, K., Kubin, C. J., Kus, J. V., Lockhart, S. R., Meletiadis, J., Morris, A. J., Pelaez, T., Quindós, G., Rodriguez-Iglesias, M., Sánchez-Reus, F., Shoham, S., Wengenack, N. L., Borrell Solé, N., Echeverria, J., Esperalba, J., Gómez-G. de la Pedrosa, E., García García, I., Linares, M. J., Marco, F., Merino, P., Pemán, J., Pérez del Molino, L., Roselló Mayans, E., Rubio Calvo, C., Ruiz Pérez de Pipaon, M., Yagüe, G., Garcia-Effron, G., Guinea, J., Perlin, D. S., Sanguinetti, M., Shields, R., and Turnidge, J.

Abstract

ABSTRACTNeither breakpoints (BPs) nor epidemiological cutoff values (ECVs) have been established for Candidaspp. with anidulafungin, caspofungin, and micafungin when using the Sensititre YeastOne (SYO) broth dilution colorimetric method. In addition, reference caspofungin MICs have so far proven to be unreliable. Candidaspecies wild-type (WT) MIC distributions (for microorganisms in a species/drug combination with no detectable phenotypic resistance) were established for 6,007 Candida albicans, 186 C. dubliniensis, 3,188 C. glabratacomplex, 119 C. guilliermondii, 493 C. krusei, 205 C. lusitaniae, 3,136 C. parapsilosiscomplex, and 1,016 C. tropicalisisolates. SYO MIC data gathered from 38 laboratories in Australia, Canada, Europe, Mexico, New Zealand, South Africa, and the United States were pooled to statistically define SYO ECVs. ECVs for anidulafungin, caspofungin, and micafungin encompassing ≥97.5% of the statistically modeled population were, respectively, 0.12, 0.25, and 0.06 μg/ml for C. albicans, 0.12, 0.25, and 0.03 μg/ml for C. glabratacomplex, 4, 2, and 4 μg/ml for C. parapsilosiscomplex, 0.5, 0.25, and 0.06 μg/ml for C. tropicalis, 0.25, 1, and 0.25 μg/ml for C. krusei, 0.25, 1, and 0.12 μg/ml for C. lusitaniae, 4, 2, and 2 μg/ml for C. guilliermondii, and 0.25, 0.25, and 0.12 μg/ml for C. dubliniensis. Species-specific SYO ECVs for anidulafungin, caspofungin, and micafungin correctly classified 72 (88.9%), 74 (91.4%), 76 (93.8%), respectively, of 81 Candidaisolates with identified fksmutations. SYO ECVs may aid in detecting non-WT isolates with reduced susceptibility to anidulafungin, micafungin, and especially caspofungin, since testing the susceptibilities of Candidaspp. to caspofungin by reference methodologies is not recommended.

Published

2015

4. In Vitro Activities of Voriconazole and Five Licensed Antifungal Agents Against Candida dubliniensis: Comparison of CLSI M27-A2, Sensititre YeastOne, Disk Diffusion, and Etest Methods

Author

Salgado-Parreño, F.J., Alcoba-Flórez, J., Arias, A., Moragues, M.D., Quindós, G., Pontón, J., and Arévalo, M.P.

Abstract

We compared the in vitro activity of six antifungal agents against 62 isolates of Candida dubliniensis by the Clinical Laboratory Standards Institute (CLSI [formerly National Committee for the Clinical Laboratory Standards]) M27-A2, Sensititre YeastOne, disk diffusion, and Etest methods and we studied the effect of the time of reading. For the azoles, voriconazole was the most potent in vitro followed by fluconazole, ketoconazole, and itraconazole. All the isolates were susceptible to amphotericin B and flucytosine. The highest rate of resistance was obtained against itraconazole with a high number of isolates defined as susceptible dose-dependent. At 24 hr, 100% of the isolates were susceptible to ketoconazole, amphotericin B, and flucytosine, 98% susceptible to voriconazole and fluconazole, and 95% for itraconazole. At 48 hr, 100% of the isolates remained susceptible for flucytosine and amphotericin B, 95% for voriconazole, 93% for fluconazole, 90% for ketoconazole, and 82% for itraconazole. The agreement between the CLSI and the other methods was better at 24 than 48 hr.

Published

2006

5. Candida dubliniensis, a new fungal pathogen

Author

Gutiérrez, J., Morales, P., González, M. A., and Quindós, G.

Abstract

There is a high interest in Candida species other than Candida albicans because of the rise and the epidemiological shifts in candidiasis. These emerging Candida species are favored by the increase of immunocompromised patients and the use of new medical practices, and m. Most oropharyngeal candidiasis can be foundare observed in those HIV-infected patients infected with human immunodeficiency virus (HIV). Candida dubliniensis is a recently described opportunistic pathogen that is closely related to C. albicans but differs from it with respect to epidemiology, certain virulence characteristics, and the ability to develop fluconazole resistance in vitro. C. dubliniensis has been linked to oral candidiasis in AIDS patients, although it has recently been associated to invasive disease. C. dubliniensis shares diagnostic characteristics with C. albicans, as germ tube- and chlamydospore-production, and it is generally misclassified as C. albicans by standard diagnostic procedures. Several recent studies have attempted to elucidate useful phenotypic and genotypic characteristics for separating both species. A large variety of methods have been developed with the aim of facilitating rapid and, accurate identification of this species. These have included differential chromogenic isolation platesculture media, direct immunological tests, and enhanced manual and automated biochemical and enzymatic panels. Chromogenic isolation media, as CHROMagar Candida, demonstrate better detection rates than traditional media, and allow the presumptive identification of C. dubliniensis by means of colony color (dark-green colonies). API 20 C AUX system is considered a reference method, but ID 32 C strip, the VITEK Yeast Biochemical Card and the VITEK 2 ID-YST system correctly identify most C. dubliniensis isolates, being VITEK 2 ID-YSTthe latter the most accurate. Spectroscopic methods, such as Fourier transformed-infrared spectroscopy, offer potential advantages. However, many authors consider that standard methods for differentiation of Candida species are time-consuming, often insensitive and can fail to distinguish C. dubliniensis. To overcome these low sensitivity, poor specificity and intolerable delay,drawbacks, molecular tools have been developed to discriminate C. dubliniensis, and particularly those based on the polymerase chain reaction. But, molecular tools prove difficult and too complex for routine use in the clinical laboratory setting and new developments are necessary. Moreover, an increased resistance to antifungal drugs has been described. Although preliminary studies indicate that most strains of C. dubliniensis are susceptible to establishedantifungal agents, fluconazole-resistant strains have been detected. Furthermore, fluconazole-resistant strains are easily derived in vitro, showing an increased expression of multidrug resistance transporters, as MDR1.

Published

2002

6. In-vitro antifungal activity of liposomal nystatin in comparison with nystatin, amphotericin B cholesteryl sulphate, liposomal amphotericin B, amphotericin B lipid complex, amphotericin B desoxycholate, fluconazole and itraconazole.

Author

Carrillo-Muñoz, A J, Quindós, G, Tur, C, Ruesga, M T, Miranda, Y, del Valle, O, Cossum, P A, and Wallace, T L

Abstract

The in-vitro susceptibilities of 120 clinical isolates of yeasts to liposomal nystatin were compared with those to amphotericin B lipid complex (ABLC), liposomal amphotericin B (LAB), amphotericin B cholesteryl sulphate (ABCD), amphotericin B desoxycholate, nystatin, fluconazole and itraconazole. Yeast isolates examined included strains of Candida albicans, Candida parapsilosis, Candida glabrata, Candida krusei, Candida guilliermondii, Candida tropicalis, Candida kefyr, Candida viswanathii, Candida famata, Candida rugosa, Rhodotorula rubra, Trichosporon spp., Cryptococcus laurentii and Cryptococcus neoformans. The mean MICs for all strains examined were: liposomal nystatin 0.96 mg/L; nystatin 0.54 mg/L; ABLC 0.65 mg/L; LAB 1.07 mg/L; ABCD 0.75 mg/L; amphotericin B 0.43 mg/L; fluconazole 5.53 mg/L; and itraconazole 0.33 mg/L. No significant differences were seen between the activity of liposomal nystatin and the polyene drugs or itraconazole, but liposomal nystatin was more active than fluconazole. MICs were lower than the reported blood concentrations following therapeutic doses of this drug, indicating the potential for a therapeutic use of liposomal nystatin in humans. These results indicate good activity in vitro against medically important yeasts, which compares favourably with the activities of other currently available antifungal drugs. Liposomal nystatin may have a role in the treatment of disseminated and systemic mycoses.

Published

1999

7. In-vitro activity of voriconazole (UK-109,496), LY303366 and other antifungal agents against oral Candida spp. isolates from HIV-infected patients.

Author

Chávez, M, Bernal, S, Valverde, A, Gutierrez, M J, Quindós, G, and Mazuelos, E M

Abstract

In this report we compare the activity of two new antifungal agents, voriconazole (UK-109,496) and LY303366 with the activities of other antifungals including fluconazole, itraconazole, 5-fluorocytosine (5FC) and amphotericin B against 219 oral Candida spp. isolates from HIV-infected patients. We used the broth microdilution method following the guidelines of the NCCLS. The in-vitro activity of voriconazole (UK-109,496) (MIC(90) 0.12 mg/L) and LY303366 (CMI(90) 0.25 mg/L) against clinical isolates of Candida spp. was excellent and comparable with that of amphotericin B (MIC(90) 0.5 mg/L), and better than those of fluconazole (MIC(90) > or = 64 mg/L), itraconazole (MIC(90) 4 mg/L) and 5FC (MIC(90) 1 mg/L).

Published

1999

8. A comparative evaluation of Etest and broth microdilution methods for fluconazole and itraconazole susceptibility testing of Candida spp.

Author

Martín-Mazuelos, E, Gutiérrez, M J, Aller, A I, Bernal, S, Martínez, M A, Montero, O, and Quindós, G

Abstract

The Etest strip is a promising tool of broad application in clinical microbiology. The method provides MIC readings and is easier to perform than broth microdilution. We carried out a study to compare the MICs of fluconazole and itraconazole obtained by the Etest with those obtained by broth microdilution, performed according to the guidelines of the NCCLS document M27-A, with 402 clinical isolates (360 Candida albicans, 17 Candida tropicalis, nine Candida krusei, nine Candida glabrata and seven Candida parapsilosis) and seven control isolates. The agreement between MICs by the two methods (at +/- 2 dilutions) was 74.5% for fluconazole and 61.4% for itraconazole. These results suggest that further development is necessary to standardize the medium and incubation conditions before introduction of the Etest as a routine method in the clinical microbiology laboratory for fluconazole and itraconazole susceptibility testing.

Published

1999

9. Value of detection of antibodies toCandida albicans germ tube in the diagnosis of systemic candidosis

Author

Quindós, G., Pontón, J., Cisterna, R., and Mackenzie, D. W. R.

Abstract

To test the value of detection of anti-Candida albicans germ tube antibodies by indirect immunofluorescence assay in the diagnosis of systemic candidosis, a retrospective study was done using 126 sera from 27 patients with presumptive systemic candidosis (13 immunocompromised), 165 sera from 45 patients with aspergillosis (29 immunocompromised), 35 sera from eight patients with cryptococcosis (6 immunocompromised), and 101 sera from 101 blood donors. While 21 of 27 patients with systemic candidosis (77.8%) had anti-germ tube antibodies, these antibodies were absent in all patients with cryptococcosis and in all blood donors. They were however detected in 5 of 45 patients with aspergillosis (11.1%). Ten of 13 (76.9%) immunocompromised patients with candidosis had anti-germ tube antibodies; similar results were obtained in immunocompetent patients with candidosis (78.6%). The specificity was 96.8%, indicating a high degree of discrimination was possible between systemic candidosis and other invasive mycoses in the patients studied. Anti-germ tube responses did not appear to be significantly reduced in immunocompromised patients.

Published

1990

10. Detection of antibodies to Candida albicans germ tubes for diagnosis and therapeutic monitoring of invasive candidiasis in patients with hematologic malignancies

Author

García-Ruiz, J C, del Carmen Arilla, M, Regúlez, P, Quindós, G, Alvarez, A, and Pontón, J

Abstract

We prospectively investigated the ability of detection of antibodies to Candida albicans germ tubes (CAGT) to diagnose invasive candidiasis in 95 consecutive admissions of 73 patients with hematologic disorders undergoing intensive chemotherapy. The episodes were divided into three groups according to clinical and microbiological diagnosis. Group 1 comprised eight admissions of eight patients with invasive candidiasis. Group 2 comprised 42 admissions of 34 patients without evidence of invasive candidiasis. Group 3 comprised the remaining 45 admissions of 37 patients with febrile episodes which were not diagnosed by microbiological culture. Antibodies to CAGT were detected in 87.5% of group 1 patients. Detection of antibodies to CAGT in patients with Candida fungemia was delayed somewhat relative to the time the blood culture was positive, but antibodies to CAGT were detected earlier than a diagnosis was made in patients with deep-tissue candidiasis. Sera from 2 admissions in group 2 and 12 admissions in group 3 revealed antibodies to CAGT. At a titer of > or = 1:20, detection of antibodies to CAGT had a sensitivity of 87.5%, specificity of 95.2%, positive predictive value of 77.8%, and negative predictive value of 97.6%. Antibodies to CAGT were usually detected before beginning of empiric antifungal therapy. Titers of antibodies to CAGT were maintained in most patients who died but declined and eventually disappeared in the patients who survived. Since antibodies to CAGT were detected in all patients with tissue-proven invasive candidiasis but negative by blood culture, detection of antibodies to CAGT complemented blood cultures for diagnosis and therapeutic monitoring of patients with hematologic malignancies and invasive candidiasis.

Published

1997

11. Detection of antibodies to Candida albicans germ tubes during experimental infections by different Candida species.

Author

Bikandi, J, San Millán, R, Regúlez, P, Moragues, M D, Quindós, G, and Pontón, J

Abstract

Identification and characterization of Candida albicans germ tube-specific antigens may be of relevance for the serodiagnosis of invasive candidiasis since they could be the basis for the development of new diagnostic tests. In this study, we have identified two antigens of 180 and >200 kDa in the cell wall of C. albicans germ tubes which are responsible for the induction of antibodies to C. albicans germ tubes. Antigens of similar molecular masses have been demonstrated in the cell walls of the Candida species C. stellatoidea, C. parapsilosis, C. guilliermondii, C. tropicalis, and C. krusei, but not C. glabrata. The kinetics of the antibody responses to C. albicans germ tubes were studied in rabbits infected with different Candida species. Although these antibodies were detected in rabbits infected with all Candida species except C. glabrata, the kinetics of the antibody responses to C. albicans germ tubes induced by the Candida species studied were different. Both the highest titer and the earliest response of antibodies to C. albicans germ tubes were observed in rabbits infected with either of the two serotypes of C. albicans used. However, the time needed to elicit the antibodies to C. albicans germ tubes can be reduced as the result of an anamnestic antibody response. The results presented in this study show that a test designed to detect antibodies against C. albicans germ tube antigens may be suitable for the diagnosis of infections caused by most of the medically important Candida species.

Published

1998

12. Identification of antigens reacting with anti-Candida albicans germ tube antibodies

Author

Regulez, P., Arilla, M. C., Bikandi, J., Quindós, G., Cisterna, R., and Ponton, J.

Abstract

Anti-Candida albicans germ tube antibodies can be induced in rabbits immunized with different C. albicans extracts. Antigens responsible for the induction of those antibodies have molecular weights of approximately 230–250, 62, 43 and 41 kDa. These antigens are present in the cell wall of both C. albicans morphological forms, although their location seems to be different.

Published

1992

13. Characterization of Scedosporium prolificans clinical isolates by randomly amplified polymorphic DNA analysis

Author

San Millán, R, Quindós, G, Garaizar, J, Salesa, R, Guarro, J, and Pontón, J

Abstract

Fingerprinting by randomly amplified polymorphic DNA (RAPD) analysis was used to differentiate Scedosporium prolificans isolates. A total of 59 arbitrary primers were screened with six unrelated S. prolificans isolates, and a panel of 12 primers was selected. The 12 primers were then used to detect DNA polymorphisms among 17 S. prolificans isolates from 11 patients with systemic S. prolificans infections diagnosed in three hospitals located in geographically different areas of Spain. Eight patients were diagnosed with S. prolificans infection in a single institution over a 6-year period, and two other patients were diagnosed with S. prolificans infection in a different hospital over a 1-year period. No single primer allowed for the discrimination of all the isolates from different patients, but this was possible by combining the RAPD patterns from three primers (UBC 701, AB1.08, and AB1.11 or UBC 701, AB1.08, and UBC 707). However, multiple isolates from the same patient were identical. In this study, we also compared a visual method and a computerized method for the analysis of the RAPD patterns. Both methods were satisfactory and gave few discordances, but given the advantages and disadvantages of each method, both systems should be used together. RAPD analysis provided a fast and economical means of typing S. prolificans isolates, with a high level of discrimination among unrelated isolates. Typing by RAPD analysis confirmed that the S. prolificans infections were epidemiologically unrelated.

Published

1997

14. Colony morphotype on Sabouraud-triphenyltetrazolium agar: a simple and inexpensive method for Candida subspecies discrimination

Author

Quindós, G, Fernández-Rodríguez, M, Burgos, A, Tellaetxe, M, Cisterna, R, and Pontón, J

Abstract

A new method of Candida subspecies discrimination on Sabouraud-triphenyltetrazolium agar is reported. Five hundred sixty-two strains of Candida and Torulopsis glabrata, previously identified by conventional mycological methods, were studied. Each strain received a three-letter code and a number based on its colonial morphology. Sixteen morphotypes were found for Candida albicans, 6 were found for Candida parapsilosis, 4 were found for both Candida guilliermondii and Candida krusei, and 12 were found for Candida tropicalis. None of the 56 T. glabrata strains studied grew on this agar. A reproducibility of 95% was found for C. albicans. The simplicity and low cost could make this method useful for typing Candida spp.

Published

1992

15. Evaluation of a commercial medium for identification ofCandida species

Author

San-Millán, R., Ribacoba, L., Pontón, J., and Quindós, G.

Abstract

CHROMagar Candida (CHROMagar, France) was evaluated as a medium for the presumptive identification and isolation of yeasts using 1,537 isolates of medically important yeasts, including 970Candida albicans, 165Candida parapsilosis, 131Candida glabrata, 62Candida guilliermondii, 35Candida krusei, 32Candida tropicalis, 31Rhodotorula rubra, 23Trichosporon spp. (17Trichosporon beigelii), 17Candida famata, 16Candida pelliculosa, 10Pichia etchelsii, 10Saccharomyces cerevisiae, 8Candida lusitaniae, 7 Cryptococcus spp., and 20 isolates of otherCandida spp. After 48 h of incubation at 37°C, the sensitivity and specificity were, respectively, 99% and 100% forCandida albicans, 93.8% and 99.1 % forCandida tropicalis, and 100% and 100% forCandida krusei. In addition to colony color, other colony characteristics were important for identification of some species, such as rough colonies inCandida krusei isolates or the halo around the colonies ofCandida tropicalis. A great variety of colors was observed among species other thanCandida albicans, Candida tropicalis, andCandida krusei. For identification purposes, CHROMagar Candida medium has an accuracy similar to that of germ-tube tests and chlamydospore development tests forCandida albicans and to that of the ATB ID32C kit (API, bioMérieux, France) forCandida tropicalis andCandida krusei.

Published

1996

16. In vitro susceptibility ofAeromonas caviae, Aeromonas hydrophila andAeromonas sobria to fifteen antibacterial agents

Author

Burgos, A., Quindós, G., Martínez, R., Rojo, P., and Cisterna, R.

Abstract

In vitro testing of the activity of 15 antibacterial agents against 522 clinical isolates ofAeromonas species demonstrated some species-associated trends. Amoxicillin plus clavulanic acid was effective against approximately 45% ofAeromonas caviae andAeromonas hydrophila, but allAeromonas sobria isolates were resistant. Aztreonam, piperacillin and mezlocillin were highly active against all the strains ofAeromonas tested. Ticarcillin was equally effective againstAeromonas caviae andAeromonas hydrophila, but more than 50% ofAeromonas sobria isolates were resistant. The latter species was more susceptible to cephalosporins thanAeromonas hydrophila andAeromonas caviae. Chloramphenicol, tetracycline and trimethoprim-sulfamethoxazole were extremely active against all threeAeromonas species, likewise ofloxacin and ciprofloxacin. Aztreonam, third-generation cephalosporins, chloramphenicol and the quinolones can thus be considered for therapy of infections whenAeromonas is implicated.

Published

1990

17. Detection of antibodies toCandida albicans germ tube in the diagnosis of systemic candidiasis

Author

Quindós, G., Pontón, J., and Cisterna, R.

Abstract

Sera from 109 subjects were tested for the presence oftantiCandida albicansantibodies by an indirect immunofluorescence assay. Aliquots of the sera were adsorbed with heat-killed blastospores to remove the antibodies against the surface of the yeast-phase cell wall and tested for anti-germ tube cell wall antibodies. Unadsorbed sera stained the entire cell wall of yeast and germ-tubes. Immunoglobulin G (IgG) antibodies were found in all patients with systemic candidiasis and in 81.2% of patients withCandida albicansisolated from skin and mucous membranes. IgA and IgG were found in 67.4 and 57.1 %, respectively, of controls without evidence of candidiasis. After the adsorption only sera from patients with systemic candidiasis showed antibodies, predominantly IgA, against germ tube cell wall. Adsorption of the sera thus increased the specificity, efficiency, and positive and negative predictive values of the test. The test achieved the highest sensitivity in adsorbed sera for the combination of IgA and IgG.

Published

1987

18. Method-Dependent Epidemiological Cutoff Values for Detection of Triazole Resistance in Candidaand AspergillusSpecies for the Sensititre YeastOne Colorimetric Broth and Etest Agar Diffusion Methods

Author

Espinel-Ingroff, A., Turnidge, J., Alastruey-Izquierdo, A., Botterel, F., Canton, E., Castro, C., Chen, Y.-C., Chen, Y., Chryssanthou, E., Dannaoui, E., Garcia-Effron, G., Gonzalez, G. M., Govender, N. P., Guinea, J., Kidd, S., Lackner, M., Lass-Flörl, C., Linares-Sicilia, M. J., López-Soria, L., Magobo, R., Pelaez, T., Quindós, G., Rodriguez-Iglesia, M. A., Ruiz, M. A., Sánchez-Reus, F., Sanguinetti, M., Shields, R., Szweda, P., Tortorano, A., Wengenack, N. L., Bramati, S., Cavanna, C., DeLuca, C., Gelmi, M., Grancini, A., Lombardi, G., Meletiadis, J., Negri, C. E., Passera, M., Peman, J., Prigitano, A., Sala, E., and Tejada, M.

Abstract

Although the Sensititre Yeast-One (SYO) and Etest methods are widely utilized, interpretive criteria are not available for triazole susceptibility testing of Candidaor Aspergillusspecies. We collected fluconazole, itraconazole, posaconazole, and voriconazole SYO and Etest MICs from 39 laboratories representing all continents for (method/agent-dependent) 11,171 Candida albicans, 215 C. dubliniensis, 4,418 C. glabrataspecies complex, 157 C.guilliermondii(Meyerozyma guilliermondii), 676 C. krusei(Pichia kudriavzevii), 298 C.lusitaniae(Clavispora lusitaniae), 911 C.parapsilosissensu stricto, 3,691 C.parapsilosisspecies complex, 36 C.metapsilosis, 110 C.orthopsilosis, 1,854 C.tropicalis, 244 Saccharomyces cerevisiae, 1,409 Aspergillus fumigatus, 389 A.flavus, 130 A.nidulans, 233 A.niger, and 302 A.terreuscomplex isolates.

Published

2018

19. Biotype Diversity of Candida parapsilosis and Its Relationship to the Clinical Source and Experimental Pathogenicity

Author

Cassone, A., Bernardis, F. De, Pontieri, E., Carruba, G., Girmenia, c., Martino, P., Fernández-Rodríguez, M., Quindós, G., and Pontón, J.

Abstract

Environmental, vaginal, and blood isolates of Candida parapsilosis werebiotyped by karyotype analysis in pulsed-fieldgel electrophoresis. Morphotype and resistotype were also determined as was aspartyl proteinase secretion and pathogenicity in a systemic mouse infection model. Overall, the karyotype patterns consisted of 6-9 chromosome bands (>3.0-0.6 Mb) with limited clustering, since most isolates had unique chromosome profiles. Major clusters of C. parapsilosis, differing by source of isolation and in experimental pathogenicity, could be discriminated by morphoresistotyping. The morphotypes of isolates from subjects with candidemia ranged from one that caused elevated mortality in the normal mouse to those that were totally avirulent in the neutropenic animal. Among clinical isolates, secretion of aspartyl proteinase washigher in vaginitis than in candidemia isolates and did not correlate with the experimental pathogenicity. These results emphasize the biotype diversity of C. parapsilosis and have potentially important epidemiologic and pathologic implications.

Published

1995