| Literature DB >> 26814644 |
Maria Helena Galdino Figueiredo-Carvalho1, Livia de Souza Ramos2, Leonardo Silva Barbedo1, Alessandra Leal da Silva Chaves3, Ilda Akemi Muramoto3, André Luis Souza dos Santos2, Rodrigo Almeida-Paes1, Rosely Maria Zancopé-Oliveira1.
Abstract
This study evaluated the antifungal susceptibility profile and the production of potential virulence attributes in a clinical strain of Candida nivariensis for the first time in Brazil, as identified by sequencing the internal transcribed spacer (ITS)1-5.8S-ITS2 region and D1/D2 domains of the 28S of the rDNA. For comparative purposes, tests were also performed with reference strains. All strains presented low planktonic minimal inhibitory concentrations (PMICs) to amphotericin B (AMB), caspofungin (CAS), and voriconazole. However, our strain showed elevated planktonic MICs to posaconazole (POS) and itraconazole, in addition to fluconazole resistance. Adherence to inert surfaces was conducted onto glass and polystyrene. The biofilm formation and antifungal susceptibility on biofilm-growing cells were evaluated by crystal violet staining and a XTT reduction assay. All fungal strains were able to bind both tested surfaces and form biofilm, with a binding preference to polystyrene (p < 0.001). AMB promoted significant reductions (≈50%) in biofilm production by our C. nivariensis strain using both methodologies. This reduction was also observed for CAS and POS, but only in the XTT assay. All strains were excellent protease producers and moderate phytase producers, but lipases were not detected. This study reinforces the pathogenic potential of C. nivariensis and its possible resistance profile to the azolic drugs generally used for candidiasis management.Entities:
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Year: 2016 PMID: 26814644 PMCID: PMC4727436 DOI: 10.1590/0074-02760150376
Source DB: PubMed Journal: Mem Inst Oswaldo Cruz ISSN: 0074-0276 Impact factor: 2.743

Dendrograms based on analysis of internal transcribed spacer (ITS) (A) and D1/D2 (B) regions of the 893391 strain and sequences from GenBank. The evolutionary histories of both trees were inferred using the UPGMA method. The percentage of replicate trees in with the associated taxon clustered in the bootstrap test (1,000 replicates) is show next to the branches. The evolutionary distances were computed using the maximum composite likelihood method and were in expressed as the number of base substitutions per site. There were 700 ITS and 580 D1/D2 positions in the final dataset.
Candida nivariensis isolates described in the literature
| Reference | Country | Total of isolates (n) | Source of isolates (n) | Clinical details | Susceptibility antifungal profile | ||
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| S/low MIC | SDD/I | R/high MIC | |||||
| Alcoba-Flórez et al. (2005b) | Spain | 3 | Broncho-alveolar lavage (1), blood culture (1), urine (1) | Multiple pulmonary abscesses, pancreatic abscess, lumbar pain | Not stated | ||
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| Japan | 1 | Catheter (1) | Rheumatoid arthritis | - | - | FLC |
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| Indonesia | 1 | Oral rinse (1) | HIV infection | FLC, ITC, VRC and CAS/AMB, 5FC, POS, and ISA | - | - |
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| UK | 16 | Blood (3), oral cavity (3), pelvic abscess (2), ascetic fluid (1), peritoneal fluid (1), lung biopsy (1), not stated (5) | Oral candidosis, neutropaenia, pneumonia, malignancy, peritonitis, and others | - | - | FLC and ITC/5FC and VRC |
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| Australia | 1 | Pleural fluid (1) | Not stated | FLC | - | - |
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| India | 2 | Sputum (1), blood (1) | HIV infection, diabetes | FLC, ITC, VRC and CAS/AMB, 5FC, and POS | - | - |
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| Spain | 2 | Blood (1), catheter (1) | Intestinal fistula associated to a severe malnutrition | Echinocandins, FLC, and VRC/AMB | ITC | - |
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| India | 5 | High vaginal swab (4), bronchoalveolar lavage (1) | Vulvovaginal candidiasis, not stated | VRC, ITC and echinocandins/AMB, POS, and ISA | - | FLC |
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| UK | 1 | Urine (1) | Renal transplant | - | - | FLC |
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| China | 7 | Vaginal swab (7) | Vulvovaginal candidiasis | NYT | FLC, ITC, MCN, and CLT | - |
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| Malaysia | 2 | Blood culture (1), vaginal swab (1) | Not stated, vulvovaginal candidiasis | FLC, VRC, and CAS/AMB and POS | - | CLT |
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| Poland | 13 | Urine (8), lower respiratory tract (3), surgical specimens (1), body fluids (1) | Not stated | Not stated | ||
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| China | 1 | Toenail (1) | Not stated | FLC, VRC, and POS | - | ITC |
| Present paper (2015) | Brazil | 1 | Nasal secretion (1) | Non-Hodgkin lymphoma | VRC and CAS/AMB | ITC | FLC/POS |
AMB: anfotericin B; CAS: caspofungin; CLT: clotrimazole; FLC: fluconazole; HIV: human immunodeficiency virus; I: intermediate; ISA: isaconazole; ITC: itraconazole; MCN: iconazole; MIC: minimal inhibitory concentration; NYT: nistatina; POS: posaconazole; R: resistant; S: susceptible; SDD: susceptible-dose dependent; VRC: voriconazole; 5FC: flucytosine.
Antifungal susceptibility of Candida nivariensis andCandida glabrata planktonic and sessile cells
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L-1)/susceptibility profile | CV MBEC (mg L-1)/% reduction of biomass | XTT MBEC (mg L-1)/% reduction of viability | ||||||
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| 893391/INCA | WM 09.150 | ATCC 2001 | 893391/INCA | WM 09.150 | ATCC 2001 | 893391/INCA | WM 09.150 | ATCC 2001 | |
| AMB | 0.25/NA | 0.25/NA | 0.12/NA | ≥ 16/54.2 | ≥ 16/30.7 | ≥ 16/28.4 | ≥ 16/54 | ≥ 16/73.1 | ≥ 16/72.8 |
| CAS | 0.03/S | 0.12/S | 0.12/S | ≥ 8/31.6 | ≥ 8/22.8 | ≥ 8/40.4 | ≥ 8/63.7 | ≥ 8/0 | ≥ 8/79.8 |
| FLC | ≥ 64/R | 8/SDD | 8/SDD | ≥ 64/6.7 | ≥ 64/23.7 | ≥ 64/13.7 | ≥ 64/1.5 | ≥ 64/15 | ≥ 64/0 |
| ITC | 0.25/SDD | 0.06/S | 0.06/S | ≥ 16/19.1 | ≥ 16/31.1 | ≥ 16/1.7 | ≥ 16/16 | ≥ 16/0 | ≥ 16/10.7 |
| VRC | 0.25/S | 0.03/S | 0.03/S | ≥ 16/13.1 | ≥ 16/41.7 | ≥ 16/20.5 | ≥ 16/20 | ≥ 16/7 | ≥ 16/22 |
| POS | 2/NA | 0.06/NA | 0.03/NA | ≥ 16/21.5 | ≥ 16/24.3 | ≥ 16/6.9 | ≥ 16/54.5 | ≥ 16/29.3 | ≥ 16/13.8 |
a: determined according to Clinical and Laboratory Standards Institute (CLSI) M27-S3 (CLSI 2008b); b: the CLSI has not defined interpretative cut-offs for amphotericin B (AMB). In general, isolates with AMB minimal inhibitory concentration (MIC) >1 mg L-1 are likely to be resistant to this drug (CLSI 2008a); c: breakpoints not established by CLSI (CLSI 2008b, 2012); CAS: caspofungin; CLT: clotrimazole; CV: crystal violet; FLC: fluconazole; ITC: itraconazole; MBEC: minimum biofilm eradication concentration; NA: not applicable; PMIC: MIC of the drugs on planktonic cells; POS: posaconazole; R: resistant; S: susceptible; SDD: susceptible-dose dependent; VRC: voriconazole; XTT: 2,3-bis (2-methoxy-4-nitro-5-sulfophenyl)-5-[(phenylamino)carbonyl]-2H-tetrazolium hydroxide.
Production of hydrolytic enzymes, adhesion to abiotic substrates, and biofilm formation detected in Candida nivariensis andCandida glabrata strains
| Species/code | Hydrolytic activities | Adhesion to abiotic substrates (1 h) | Biofilm | |||
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| 893391/INCA | 0.347 ± 0.040 | 0.629 ± 0.025 | 17.0 ± 4.4 | 25.4 ± 4.9 | 0.330 ± 0.045 | 1.173 ± 0.054 |
| WM 09.150 | 0.375 ± 0.000 | 0.634 ± 0.047 | 14.0 ± 3.0 | 23.9 ± 2.4 | 0.440 ± 0.095 | 0.811 ± 0.080 |
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| ATCC 2001 | 0.357 ± 0.034 | 0.714 ± 0.00 | 16.0 ± 3.0 | 24.1 ± 5.3 | 0.858 ± 0.009 | 1.084 ± 0.028 |
a: the protease and phytase activities were measured by the formation of a clear halo around the colony and expressed asPz value as previously described (Price et al. 1982) (thePz value was scored into four categories:Pz of 1.0 indicated no enzymatic activity,Pz between 0.999-0.700 indicated low enzymatic activity, Pz between 0.699-0.400 corresponded to moderate enzymatic activity, and Pz between 0.399-0.100 mean high enzymatic activity); b: the results were expressed as number of fungal cells per microscopic field; c: the biomass and viability of biofilm were measured by crystal violet incorporation at 540 nn and 2,3-bis (2-methoxy-4-nitro-5-sulfophenyl)-5-[(phenylamino)carbonyl]-2H-tetrazolium hydroxide reduction at 492 nm, respectively. All the results were reported as the arithmetic means ± standard deviation.