Several species belonging to the genus Candida have emerged as important pathogens causing a broad variety of clinical infections. The C. parapsilosis complex (C. parapsilosis sensu stricto, C. orthopsilosis, and C. metapsilosis) are among the most common species of Candida responsible for nosocomial bloodstream infections and are an important cause of onychomycosis, mainly affecting the fingernails1.
Although members of the C. parapsilosis complex are closely related, their clinical prevalence and virulence are different. These virulence factors including the ability to secrete hydrolytic enzymes, adhesion to host epithelial cells, biofilm production capability, and hemolytic activity are considered important to the initiation and maintenance of their infections1,2. In this study, we evaluated the in vitro capacity of C. parapsilosis sensu stricto, C. orthopsilosis, and C. metapsilosis isolates to produce hydrolytic enzymes, to adhere to human buccal epithelial cells, and produce biofilm.
In total, the 87 isolates identified were C. parapsilosis sensu stricto (n = 78), C. orthopsilosis (n = 5), and C. metapsilosis (n = 4), which included 54 candidemia cases and 33 onychomycosis cases obtained from the Laboratory of Mycology, Institute of Tropical Pathology and Public Health, Federal University of Goiás, from 2007 to 2012. These isolates were stored at -70°C in yeast extract peptone dextrose (YEPD) broth (Difco®) with 10% glycerol. Subcultivation was carried out on YEPD agar (Difco®) for 48 h at 37°C. The study was approved by the Bioethics Committee of the Clinical Hospital of the Federal University of Goiás (Protocol no. 065/2008).
Aspartic proteinase (Sap) was assessed using a 10-µL aliquot of yeast suspension (107 cells/mL), which was inoculated on the surface of bovine serum albumin (BSA) agar medium (pH 3.5) and incubated at 37°C for 7 days. For the phospholipase assay, 10 µL of yeast suspension (107 cells/mL) was placed on the surface of agar medium containing egg yolk and incubated at 37°C for 4 days. To determine esterase activity, a 5-µL aliquot of a yeast suspension (107 cells/mL) was placed on the surface of Tween opacity test medium and incubated at 37°C for 10 days2.
Hemolytic enzyme activity was determined by inoculating 5 µL of yeast suspension (108 cells/mL) on the surface of Sabouraud agar medium supplemented with 7% sheep blood and 3% glucose2. The plates were then incubated at 37°C for 48 h, and hemolysis was observed based on the presence of a translucent halo around the colony. A β-hemolytic Staphylococcus aureus strain (ATCC 6538) was used as the positive control.
Measurements and calculations of hydrolytic enzyme activity (Pz) were performed as described by Price et al.3. Pz coefficients of the analyzed Candida strains were grouped into five classes: very strong (Pz < 0.69), strong (Pz = 0.70-0.79), mild (Pz = 0.80-0.89), weak (Pz = 0.90-0.99), and negative (Pz = 1.0).
For biofilm production, C. parapsilosis complex isolates at a final concentration of 1.0 × 106 cells/mL, were suspended in RPMI 1640 broth supplemented with L-glutamine and buffered with MOPS. Aliquots of 100 µL were then inoculated into flat-bottom 96-well microtiter plates and incubated for 48 h at 37°C. After biofilm formation, the wells were washed thrice with PBS to remove non-adhered cells. Semiquantitative measurements of biofilm production were obtained via the XTT reduction assay4. The absorbance of XTT assays was read spectrophotometrically (Tp-Reader-Basic, Thermo Plate) at 492 nm. Biofilm production was measured based on optical density (OD) > 0.2.
For adhesion assay, 500 µL of each yeast suspension (107 yeast/mL) were mixed with 500 μL of human buccal epithelial cell (HBEC) suspension (2 × 105 cells/mL) and incubated at 37°C with agitation for 1 h. The mixture was subsequently filtered through a 20 μm-pore-size membrane filter and transferred to a slide by pressing the filter paper against it. After fixing the cells with methanol, they were subjected to Gram staining, and the number of cells that adhered to 100 HBECs was counted5.
All assays were performed in triplicate for each isolate on different days, and the mean values were determined. Statistical analysis employed Mann-Whitney and Kruskal-Wallis tests when appropriate (non-parametric tests). The significance level was set at 0.05. The data were analyzed using IBM SPSS Statistics version 20.
Most of the 87 isolates of C. parapsilosis presented very strong enzymatic activity (Pz > 0.69) for proteinase (n = 85; 97.7%), esterase (n = 55; 63.2%), and hemolysin (n = 72; 82.8%). However, phospholipase activity was negative in 89.8% (n = 78) of strains (Table 1).
TABLE 1: Enzymatic profiles of C. parapsilosis species complex isolates (n = 87) from blood and nail samples. Goiania-GO, Brazil.
| Enzymatic activity (Pz*) | C. parapsilosis | C. orthopsilosis | C. metapsilosis | Total | ||
|---|---|---|---|---|---|---|
| sensu stricto | blood | blood | nails | n (%) | ||
| blood | nails | (n = 5) | (n = 2) | (n = 2) | (n = 87) | |
| (n = 47) | (n = 31) | |||||
| Proteinase | ||||||
| Very strong | 47 | 31 | 5 | 2 | – | 85 (97.7) |
| Negative | – | – | – | – | 2 | 2 (2.3) |
| Phospholipase | ||||||
| Very strong | – | 5 | – | 2 | – | 7 (8.0) |
| Strong | – | 1 | – | – | – | 1 (1.1) |
| Mild | – | 1 | – | – | – | 1 (1.1) |
| Negative | 47 | 24 | 5 | – | 2 | 78 (89.8) |
| Esterase | ||||||
| Very strong | 29 | 19 | 4 | 2 | 1 | 55 (63.2) |
| Strong | 13 | 6 | – | – | – | 19 (21.8) |
| Negative | 5 | 6 | 1 | – | 1 | 13 (15.0) |
| Hemolysin | ||||||
| Very strong | 42 | 23 | 4 | 2 | 1 | 72 (82.8) |
| Strong | 3 | 4 | – | – | 1 | 8 (9.2) |
| Mild | 2 | 4 | – | – | – | 6 (6.9) |
| Weak | – | – | 1 | – | – | 1 (1.1) |
*Pz = Value obtained by dividing the diameter of the colony (mm) by the total diameter of the colony including the precipitation zone (mm). Pz ≤ 0.69: very strong; Pz = 0.70-0.79: strong; Pz = 0.80-0.89: mild; Pz = 0.90-0.99: weak; Pz = 1: negative.
C. parapsilosis sensu stricto isolates produced mean Pz of esterase activity higher than the others (p = 0.015), especially in blood samples (p = 0.025) (Table 2).
TABLE 2: Values of enzymatic activity (Pz mean) by C. parapsilosis species complex isolates, according to enzyme and anatomical site (blood and nails). Goiânia-GO, Brazil.
| Enzymes | Candida parapsilosis complex | p-value*** | ||
|---|---|---|---|---|
| C. parapsilosis sensu stricto | C. orthopsilosis | C. metapsilosis | ||
| Pz* mean ± SD** | Pz mean ± SD | Pz mean ± SD | ||
| Total (n = 87) | n = 78 | n = 5 | n = 4 | |
| Proteinase | 0.304 ± 0.084 | 0.316 ± 0.096 | 0.385 ± 0.078 | 0.251 |
| Phospholipase | 0.664 ± 0.075 | – | 0.630 ± 0.042 | 0.551 |
| Esterase | 0.559 ± 0.130 | 0.466 ± 0.303 | 0.383 ± 0.076 | 0.015**** |
| Hemolysin | 0.592 ± 0.100 | 0.572 ± 0.147 | 0.552 ± 0.147 | 0.599 |
| Blood (n = 54) | n = 47 | n = 5 | n = 2 | |
| Proteinase | 0.328 ± 0.096 | 0.316 ± 0.096 | 0.385 ± 0.078 | 0.590 |
| Phospholipase | – | – | 0.630 ± 0.042 | – |
| Esterase | 0.562 ± 0.132 | 0.466 ± 0.303 | 0.350 ± 0.070 | 0.025**** |
| Hemolysin | 0.580 ± 0.087 | 0.572 ± 0.147 | 0.450 ± 0.070 | 0.122 |
| Nails (n = 33) | n = 31 | n = 0 | n = 2 | |
| Proteinase | 0.263 ± 0.039 | – | – | – |
| Phospholipase | 0.664 ± 0.075 | – | – | – |
| Esterase | 0.554 ± 0.128 | – | 0.450 ± 0 | 0.345 |
| Hemolysin | 0.609 ± 0.117 | – | 0.655 ± 0.134 | 0.650 |
*Pz = Value obtained by dividing the diameter of the colony (mm) by the total diameter of the colony including the precipitation zone (mm). **SD: Standard deviation. ***Kruskal-Wallis test. ****Bold p-values indicate statistically significant differences (p < 0.05).
Proteinase activity was higher in isolates from blood than in isolates from nails (p < 0.001) (Figure 1A).
All C. parapsilosis complex isolates could produce biofilms. Although the biofilms formed by C. metapsilosis isolates from blood had a higher mean OD than nail isolates, no statistically significant difference was detected (p = 1.000) (Figure 1B).
The C. parapsilosis complex isolates exhibited high adherence to HBEC, with no statistically significant differences between isolates or anatomical sites (Figure 1C). The greatest number of adhered yeasts was observed in case of C. parapsilosis sensu stricto (100.2 ± 88.7), followed by C. metapsilosis (90.8 ± 28.9), and C. orthopsilosis (38.0 ± 19.3).
FIGURE 1: Differences in the mean enzymatic activities of phospholipase, proteinase, esterase, and hemolytic factors, the metabolic activity of biofilms, and the mean number of yeasts that adhered to 100 HBECs between different sources and species of the C. parapsilosis complex. (A) Values of enzymatic activity (Pz mean), according to enzyme and anatomical site (blood and nails). (B) Optical density (OD) mean of the biofilms formed, according to anatomical site (blood and nails). (C) Mean number of yeast cells adhered/100 human buccal epithelial cells, according to anatomical site (blood and nails). *Mann-Whitney test (p < 0.05).
Very strong in vitro proteinase activity was detected in all isolates of C. parapsilosis sensu stricto and C. orthopsilosis, whereas only two isolates of C. metapsilosis showed positive enzymatic activity. Treviño-Rangel et al.2 also observed proteinase activity in three species of the complex. Several studies have shown that Candida parapsilosis complex species express different proteinase activities. Silva et al.6 found positive protease activity in 37.7% isolates of C. parapsilosis sensu stricto; however, only 7.8% of the isolates revealed high enzymatic activity. Furthermore, none of the C. metapsilosis and C. orthopsilosis isolates exhibited protease activity in that study.
Some studies on the virulence of Candida species verified that few isolates of the C. parapsilosis complex have proteinase activity, regardless of whether the isolation site was nail or blood1,7. Our research identified significantly higher enzymatic activity of proteinase in isolates from blood than from nails (Figure 1A). This difference in proteinase activity between nail and blood isolates suggests that this enzyme may be associated with increased adhesion and invasion capacity in the bloodstream.
Few isolates in our study produced phospholipase (10.3%), which was also found by Dagdeviren et al.5 and Silva et al.6, who verified phospholipase activity in 15.1% and 8.7% of C. parapsilosis isolates, respectively. However, some isolates of the C. parapsilosis complex may show high production of phospholipase. Among these C. orthopsilosis has the highest phospholipase activity, with up to 69% of isolates exhibiting very high enzymatic activity2.
In contrast to the observations for phospholipase, a high percentage of our isolates could produce esterase. High esterase activity was found by Pakshir et al.8 in 56.5% of the C. parapsilosis isolates studied, but Akyol & Cerikçioğlu9 detected this activity in only 1.88% of the examined isolates. In the present study, esterase activity was similar among members of the C. parapsilosis complex with 85.8% of C. parapsilosis sensu stricto, 80% of C. orthopsilosis, and 75% of C. metapsilosis isolates. Different results were obtained by Treviño-Rangel et al.2, who observed esterase production in 13.3% of C. parapsilosis and 66.6% of C. orthopsilosis isolates studied but not in any C. metapsilosis isolates.
We identified hemolytic activity in 100% of the C. parapsilosis complex isolates (Table 1). Different results were found by Abi-Chacra et al.10, who detected weak hemolytic activity in all the C. parapsilosis complex isolates examined. Similarly, Treviño-Rangel et al.2 detected hemolysis ability among the isolates studied, but did not report high activity (Pz < 0.69), as observed in our isolates.
As noted above, these differences in the enzymatic activity of phospholipase and esterase, and hemolytic capacity among of the C. parapsilosis complex isolates in vitro can be explained by the biological variation between isolates according to the infected anatomic site. Nail isolates had higher Pz mean values than blood isolates, although this difference was not significant. This difference can be due to the evolution of the infection, as most cases of onychomycosis were characterized by chronic evolution, whereby more physiological conditions of the etiological agent were required to maintain its pathogenic capacity. Other hydrolytic enzymes with unknown activities against different relevant substrates specific to human cutaneous infections such as onychomycosis, unlike those used in the present study, could further our understanding of this biological variation in enzymatic secretion between isolates according to the isolation site.
In the present work, C. parapsilosis complex isolates presented a high affinity for human buccal epithelial cells in vitro, with adherence of 96.0 yeasts per 100 epithelial cells. Costa et al.11 verified increased adherence capacity, with an average value of 155.3 yeasts whereas Dagdeviren et al.5 and Lima-Neto et al.12 reported lower numbers of adhered yeasts, at 54.9 and 25.6 on average, respectively. Thus, intraspecies variation in adherence to human buccal epithelial cells is evident among C. parapsilosis isolates, with values up to more than 150 fungal cells per 100 epithelial cells.
Although Németh et al.13 demonstrated that C. metapsilosis is the least virulent species of the psilosis group, our results showed no statistically significant differences in HBEC adherence ability within the C. parapsilosis complex isolates. However, C. metapsilosis isolated from blood had greater ability to adhere than the other strains, which may be because C. parapsilosis interacts with different mammalian nails.
This study confirmed that all the examined C. parapsilosis complex isolates could produce a biofilm. Similarly, Lattif et al.14 reported that all clinical isolates of the C. parapsilosis complex obtained from silicone disks of catheters could form biofilms. Some authors14,15reported contrasting results regarding the ability of these three species of the complex to form biofilms. Song et al.15 found that C. orthopsilosis and C. metapsilosis did not form biofilms, whereas Lattif et al.14 verified that all three species were capable of biofilm production. In terms of our findings, even though C. metapsilosis are considered the less virulent, these isolates had higher adhesion capacity and biofilm formation than C. parapsilosis stricto sensu and C. orthopsilosis.
In the present work, comparison of biofilm-forming abilities among isolates did not reveal any significant differences between the three species of the C. parapsilosis complex. However, according to the anatomical site of isolation, C. parapsilosis stricto sensu isolated from nails showed higher mean values of adhered yeasts and O.D. in biofilm formation than blood isolates.
In conclusion, the proteinase activity of C. parapsilosis isolates was higher, but a statistical evaluation could not be performed due to the small number of species obtained. These results suggest that the high adherence ability of species participates in initial biofilm formation. The association of adherence ability to buccal cells with biofilm formation can be an important parameter to differentiate invasive from non-invasive strains. Screening phospholipase production in biofilm-forming isolates can also an important parameter to distinguish invasive strains from noninvasive colonizers. The data presented in this report reinforce the necessity of assessing the phenotypic differences in the C. parapsilosis complex, including those related to the expression of virulence attributes that play relevant roles in establishing the infectious process.
