Abstract
Invasive candidiasis (IC), caused by Candida yeasts, particularly Candida albicans, poses a significant threat with high mortality rates. Diagnosis is challenging due to Candida's common presence in human microbiota. To address this, our research group developed an immunofluorescence assay detecting Candida albicans Germ Tube Antibodies (CAGTA) in IC patients. CAGTA, indicative of invasive processes, is associated with a lower mortality rate in ICU patients. Based on this premise, this study aims to provide results regarding the lack of knowledge about the potential activity of CAGTA against invasive infections in humans caused by the fungus Candida albicans. Therefore, in order to characterize the activity of CAGTA produced by patients with IC, we used sera from 29 patients with IC caused by either C. albicans or non-albicans Candida species. Whole serum IgG antibodies were fractionated into anti-blastospores, CAGTA-enriched, and purified CAGTA and the assessments included XTT colorimetric assays for metabolic activity, CFU counts for viability, and microscopy for growth, viability, and morphological analysis. The CAGTA-enriched IgG fraction significantly reduced the metabolic activity and viability of C. albicans compared to anti-blastospores. Purified CAGTA altered germ tube cell wall surfaces, as revealed by electron microscopy, and exhibited fungicidal properties by DiBAC fluorescent staining. In conclusion, antibodies in response to invasive candidiasis have antifungal activity against Candida albicans, influencing metabolic activity, viability, and cell wall structure, leading to cell death. These findings suggest the potential utility of CAGTA as diagnostic markers and support the possibility of developing immunization protocols against Candida infections.
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Introduction
Invasive Candidiasis (IC) is a fungal infection caused by yeasts of the genus Candida, among which Candida albicans is the most frequently isolated, affecting more than 250,000 people worldwide every year and cause more than 50,000 deaths [1]. Some species of Candida are common colonizers of the skin, and of the gastrointestinal, genitourinary and respiratory tract mucous membranes. Nevertheless, under certain circumstances, they can cause both superficial and invasive infections, and the latter are associated with high mortality rates due to the diagnostic difficulties derived from the absence of pathognomonic signs [2].
Despite some improvement in diagnostic methods and the introduction of new drugs for treatment, IC is still a major problem in critically ill patients [3,4,5]. Other risk conditions for an invasive fungal disease (IFD) are immunosuppression, HIV infected patients, recipients of hematopoietic or solid organ transplantation, and long stay in the ICU [6, 7].
Globally, the incidence of C. albicans isolates is decreasing (65.3% to 48.4%), in favor of non-albicans Candida species (NAC) such as Candida glabrata (from 11.3 to 18.2%), Candida parapsilosis (6% to 17.1%) or Candida tropicalis (7.2% to 10. 6%) [8]. In Spain, nowadays, C. albicans is still the major cause of IC (47.7%), followed by C. parapsilosis (22%), C. glabrata (15.8%), C. tropicalis (9.3%) and Candida krusei (2.8%) [9].
Blood culture remains the “gold standard” for diagnosis of IC or, alternatively, histopathological evidence in normally sterile sites, but both techniques have low sensitivity, and a long turnaround time (72–96 h) leading to a delay in specific treatment that results in increased mortality [10]. In this line, a multicenter retrospective study conducted in 23 ICUs of 9 European countries reported an IC incidence of 7.07 episodes per 1000 admissions with a 30-day mortality of 42% [11].
In an attempt to improve the diagnostic resources for IC, our group of research developed an indirect immunofluorescence (IIF) assay detecting antibodies that recognize specific antigens located on the cell wall surface of C. albicans germ tubes; such antibodies are associated to the invasive candidiasis process and were termed CAGTA (Candida albicans Germ Tube Antibodies) [12,13,14,15,16,17,18]. The detection of CAGTA has achieved very interesting results, even in neutropenic patients, and its diagnostic value has been proved successful for monitoring antifungal therapies [19]. A Spanish multicenter study with 53 IC patients admitted to ICU evidenced that those with increased CAGTA titers along with antifungal treatment greatly reduced their associated mortality rate from 61.2 to 22.7% [20]. This aspect is related to an efficient anti-Candida response that requires the cooperation of different mechanisms of the immune system [21,22,23,24]. In this regard, antibodies confer protection against fungal infections by opsonization and phagocytosis, complement activation and antibody-dependent cell toxicity [25, 26]. In addition to direct neutralization of fungi and their antigens, antibodies can inhibit fungal growth, modify gene expression, signaling and lipid metabolism, induce iron starvation, and reduce polysaccharide release and biofilm formation [6, 24].
Furthermore, the identification of specific antigens that are recognized by CAGTA, such as hyphal wall protein 1 (Hwp1), agglutinin-like sequence protein 3 (Als3), and methionine synthase protein 6 (Met6) has served to develop experimental immunoassays to detect antibodies that may help to the diagnosis of IC in patients at risk, even in immunocompromised ones [27]. In this line, since CAGTA have been related to a better prognosis of the infection, members of our group have assayed some epitopes of the antigens recognized by CAGTA as a complex peptide vaccine conjugated to KLH (3P-KLH) for protection in a murine model of hematogenously disseminated candidiasis, with promising results (Diez et al. data not published). In fact, patients who survived systemic infections developed strong antibody responses to certain C. albicans proteins that could help as a prognostic signature for an IC clinical-outcome prediction model [28,29,30].
An alternative approach to the management of IC is the development of prophylactic treatments based on monoclonal or polyclonal antibodies [31].
Therefore, the aim of this study is to assess the efficacy of antibodies raised by patients with Invasive Candidiasis against Candida albicans, with a particular focus on CAGTA. The investigation involves recording the effect of these antibodies in vitro on the metabolic activity and viability of the fungus, as well as on the structure of its cell wall. This research is essential for gaining insights into the immune response to invasive Candidiasis, potentially contributing to the development of therapeutic strategies or vaccines.
Material and Methods
Yeast Strain and Culture Conditions
Candida albicans SC 5314 (Stanford DNA Sequencing and Technology Center, Stanford, USA) was used in all experiments. Yeast cells were grown on Sabouraud Dextrose Agar (SDA; Difco, Sparks, MD, USA) at 37 °C for 48 h. To obtain germ tubes, cells grown in SDA were inoculated into TC199 medium (Sigma-Aldrich, St. Louis, MO, USA) and incubated at 24 °C overnight; blastospores were collected by centrifugation and inoculated into four volumes of TC199 medium (Sigma-Aldrich, St. Louis, MO, USA) preheated at 37 °C. The germ tubes were collected after 4 h of incubation at 37 °C and 120 rpm.
In order to prepare the inoculum for the experiments, yeasts were freshened overnight in SDA at 37 °C. Then, 2–3 colonies were inoculated into Sabouraud Dextrose broth (SDB, Difco, Sparks, MD, USA) and incubated overnight at 24ºC and 200 rpm. Yeast cells were collected by centrifugation at 2500 rpm for 5 min and washed three times with sterile PBS. The concentration of the inoculum was adjusted to 106 cell/ml by using a Bürker chamber (Hirshmann, Germany) [32].
Patients and Sera
Immune sera were obtained from 29 patients with IC from different clinical units (Hospital Severo Ochoa-Leganés-Madrid and University Hospital Cruces-Barakaldo-Bizkaia, Spain) (Table 1). Group I: 15 patients diagnosed with invasive C. albicans infection. Group II: 14 patients infected with NAC species.
CAGTA titer of sera was assessed by indirect immunofluorescence as previously described [13], and based on their antibody titer they were classified as HIGH-titer sera (1/160–1/5120) or LOW-titer sera (0–1/80). The sera are included in an anonymized samples collection (C.0005025) registered by the Instituto de Salud Carlos III-Spain. This study was approved by of the Institutional Committee for Research with Human Beings (CEISH) of the Ethics Commission for Research and Teaching (CEID) of the University of the Basque Country (CEID) with reference number CEISH/216RM/2013/MORAGUES TOSANTOS.
Serum IgG Fractions and Purification of Antibodies
Immune sera were fractionated to run the different assays as described previously [31]. Serum whole IgG class antibodies (w-IgG) were purified with Melon™ Gel IgG Spin Purification Kit (ThermoFisher Scientific, St. Louis, MO, USA). The CAGTA enriched fraction of serum IgG (CAGTA-enr IgG) was obtained after incubating w-IgG with an equal volume of heat-killed C. albicans blastospores (1010 cell/ml of PBS) for 2 h at room temperature, followed by centrifugation at 2500 rpm for 5 min to remove the blastospores. The anti-blastospore antibodies (antiBl-IgG) adsorbed onto the surface of the yeast cells were eluted by gentle shaking in 2.5 M sodium iodide (Sigma-Aldrich, St. Louis, MO, USA) at room temperature for 1 h, and blastospores were spun down. The eluted antiBl-IgG fraction was dialyzed (MWCO 12,000–14,000 Da; Medicell International, London, UK) against PBS and concentrated with polyethylene glycol 20,000 (Merck, Hohenbrunn, Germany).
Purified CAGTA (pur-CAGTA) were eluted from C. albicans germ tubes after being incubated with an equal volume of CAGTA-enr IgG fraction for 1 h at room temperature with gentle agitation. Purified CAGTA were eluted, dialyzed and concentrated following the same protocol described for antiBl-IgG. The scheme of the serum fractionation process is depicted in Fig. 1.
The protein concentration of serum IgG fractions was estimated with Pierce™ Coomassie Plus (Bradford) Assay Kit (ThermoFisher Scientific, St. Louis, MO, USA) according to the manufacturer's instructions.
Evaluation of Metabolic Activity of Candida albicans
The effect of the antibodies on C. albicans was evaluated by measuring the cell metabolic activity with the colorimetric XTT assay.
Candida albicans blastospores grown overnight in SDB at 30 °C and 120 rpm, were suspended in fresh medium 106 cell/ml, and distributed in a U-bottom 96-well microplate (Cellstar, Greiner bio-one, USA), 25 μl per well. Each well was supplemented with 25 μl of SDB containing the correspondent IgG fraction to reach different final concentrations (50, 100 or 200 μg/ml). Plates were incubated at 37 °C for 2.5 h with gentle shaking, and then centrifuged at 2500 rpm, The supernatant was discarded, and the metabolic activity of cells was estimated with the 2.3-bis(2-methoxy-4-nitro-5-sulfophenyl)2H-tetrazolium-5-carboxanilide-inner salt (XTT; Sigma-Aldrich, St. Louis, MO, USA), according to the protocol of Henriques et al. [33]. Briefly, cell pellets in each well were supplemented with 90 μl of XTT 0.75 mg/ml in PBS and 10 μl of phenazine methasulfate (PMS; Sigma-Aldrich, St. Louis, MO, USA) 0.32 mg/ml in ultrapure water, both sterile filtered (0.45 µm pore-size filters; Minisart, Sartorius, Spain), and they were incubated at 37 °C for 2 h. Then, each well content was homogenized and the absorbance at 492 nm (Abs 492 nm) was registered using a spectrophotometer (Microplate Autoreader Elx808, Bio-Tek Instruments). Two different controls were included in every experiment, one without antibodies, and a second one with an equivalent concentration of an irrelevant non-specific human IgG (irr-IgG; Sigma-Aldrich, St. Louis, MO, USA).
Evaluation of Cell Viability
After being exposed to different IgG fractions, C. albicans cell viability was estimated by inoculating aliquots of duplicate wells on SDA plates, and counting colony forming units (CFU) grown at 37 °C for 48 h.
Alternatively, viability was assessed by staining with fluorochromes as described by Bowman et al. [34]. 5, (6)carboxyfluorescein Diacetate (CFDA; Molecular Probes, Eugene, OR, USA) dyes live cells while bis(1,3dibutylbarbituric acid) trimethine oxonol (DiBAC; Molecular Probes, Eugene, OR, USA) dyes death cells.
Briefly, Candida albicans blastospores grown overnight in SDB at 30 °C and 120 rpm, were suspended in fresh medium 106 cell/ml, and distributed in a U-bottom 96-well microplate (Cellstar, Greiner bio-one, USA), 25 μl per well. Each well was supplemented with 25 μl of PBS containing pur-CAGTA to reach the final concentrations of 20 μg/ml. Then the cells were incubated for 2.5 h at 37 °C with gentle shaking. Then, the cells were centrifuged at 2500 rpm for 15 min and the pellet was split in parallel in 100 μl of CFDA and DiBAC solutions.
CFDA 50 μg/ml was prepared in MOPS 3 (0.1 M MOPS–50 mM citric acid at pH 3.0) from a stock solution of CFDA 5 mg/ml in dimethyl sulfoxide. Cells were incubated with the dye in the dark at 37 °C for 45 min with gentle shaking and then stored on ice until analysis. DiBAC 2 μg/ml in MOPS 7 (0.1 M MOPS at pH 7.0) was prepared from a 1 mg/ml stock solution in ethanol, and cells were stained at room temperature for 1 h in the dark, washed twice with MOPS 7 and stored on ice until analysis. Parallel phase-contrast and fluorescent images of the same field were taken using AZ100 Multizoom microscope (Nikon, Japan) and analyzed through Image Fiji software (Version 2.0, USA).
Estimation of Growth and Cell Morphology by Optical Microscopy
Cell growth and morphology of C. albicans treated with CAGTA-enr IgG 6.25–200 µg/ml for 2.5 h at 37 °C were assessed by optical microscopy. Growth conditions of planktonic cells were the same as indicated for XTT and CFU assays. Two controls were run in every experiment, one without antibodies, and a second one with an equivalent concentration of a human irr-IgG. Images were obtained with an inverted microscope Olympus Fluoview FV500 (Olympus, Japan) and analyzed through Image Fiji software (Version 2.0, USA).
Electron Microscopy
Candida albicans blastospores grown overnight in SDB at 30 °C and 120 rpm, were suspended in fresh medium 106 cell/ml, and 50 μl per well were distributed in a U-bottom 24-well microplate (Iwaki®, Cell Biology, USA), previously filled with a nitrocellulose membrane (pore size 0,2 µm, Protran®, GE Healthcare, UK), fitting the well surface. Then, each well was supplemented with 50 μl of SDB containing pur-CAGTA fraction to reach the final concentrations of 20 μg/ml. Cells were grown for 2.5 h at 37 °C. Negative controls were run without CAGTA. Then, cells were gently washed by aspiration in Sorenson’s buffer [0.133 M Na2HPO4, 0.133 M KH2PO4 (4:1, v/v), pH 7.2], treated with fixing solution (2% glutaraldehyde in Sorenson’s buffer) at room temperature for 1 h, and washed three times with 6% sucrose in Sorenson’s buffer. Cells were dehydrated using graded ethanol solutions (50%, 70% and 100%) for 5 min each. Then membranes were washed twice for 5 min each with 5 ml hexamethyldisilazane (Electron Microscopy Sciences, Hatfield, PA, USA), that was removed by vacuum filtration. Membranes were left to dry in the air and processed for electron microscopy at the Service of Analytic and High Resolution Microscopy in Biomedicine (SGIker, University of the Basque Country UPV/EHU). Images were assembled through Image Fiji Software (Version 2.0, USA).
Statistical Analysis
All assays were performed in duplicate and repeated three times. Statistical analysis was performed using GraphPad Prism Software (Version 6.00, Boston, Massachusetts, USA) for Windows. Significant differences were assesed using Kruskal–Wallis test. P values < 0.05 were considered statistically significant.
Results
Effect of Serum IgG Fractions from Patients with Invasive Candidiasis on Candida albicans Metabolic Activity and Viability
Whole-IgG (w-IgG) from patients infected with C. albicans (group I) reduced the metabolic activity of C. albicans blastospores, as evaluated by the XTT assay, and the effect was concentration dependent; of note, the required amount of w-IgG that significantly reduced C. albicans metabolic activity was ≥ 50 µg/ml for immunoglobulins isolated from patients with high CAGTA titers (1/160–1/5120), whereas it was 200 µg/ml for low CAGTA titers (< 1/160) patients (Fig. 2a). Although the irrelevant commercial IgG (irr-IgG) showed a trend in reducing C. albicans metabolic activity compared to the control group, differences were not statistically significant.
The separate assay with CAGTA-enriched (CAGTA-enr IgG) and anti-blastospores IgG (antiBl-IgG) fractions revealed that the latter, up to 200 µg/ml, did not reduce the metabolic activity of C. albicans, relying the registered w-IgG inhibitory activity on the CAGTA-enr IgG fraction (Fig. 2b).
In addition, we also studied the effect of CAGTA-enr IgG fraction of sera from patients infected with non-albicans Candida spp. (NAC; group II). Candida parapsilosis, C. glabrata or C. tropicalis caused infections in 14 patients whose serum CAGTA titers were ≤ 1/320, except 1/2560 for one of the patients infected with C. glabrata (Table 1). As shown in Fig. 2c, the CAGTA-enr IgG fraction of NAC patients reduced C. albicans metabolic activity to a diverse extent, but their mean values were concentration dependent and resembled those of low-titer CAGTA patients infected with C. albicans (Fig. 2b).
CAGTA-enr IgG treatment of patients showing the highest effect on metabolic activity of C. albicans blastospores resulted in a significant reduction of CFU counts compared to untreated and irr-IgG treated control cells (Fig. 2d).
Effect of Serum IgG Fractions from Patients with Invasive Candidiasis on Candida albicans Growth, Morphology and Viability
The optical microscopy images of C. albicans planktonic cells incubated with increasing concentrations of CAGTA-enr IgG fractions corroborated the above-mentioned findings (Fig. 3). While irr-IgG slightly reduced the growth of Candida, CAGTA-enr IgG reduced the visible yeast growth in a concentration dependent manner, though at the highest concentrations, we still could see some short and narrow germ tubes together with cell debris (Fig. 3).
Consistent with optical microscopy findings, electron microscope images of pur-CAGTA IgG 20 µg/ml-treated C. albicans from patient #1—in group I (CAGTA titer 1/2560) revealed hyphae with altered morphology and surface fissures and protrusions (Fig. 4f, h, j), and surrounded by an altered matrix. On the contrary, the surface of untreated control yeast (Fig. 4a, c) and hyphae (Fig. 4e, g, i) as well as that of pur-CAGTA treated blastospores (Fig. 4: b and d) appeared regular and smooth. In addition, fluorescent DiBAC and CFDA staining of pur-CAGTA 20 µg/ml –treated C. albicans cells of the same patient #1, revealed a fungicidal effect for these antibodies (Fig. 5).
Discussion
Invasive Candidiasis (IC) is a fungal infection caused by yeasts of the genus Candida, among which Candida albicans is the most frequently isolated. The opportunistic pathogen C. albicans has the ability to cause invasive infections, primarily attributed to its capacity to grow as hyphae. Various virulence factors associated with the cell wall are known to engage with host epithelial cells, initiating and fostering an immune response. Therefore, an effective anti-Candida response necessitates the collaboration of various mechanisms within the immune system, including the production of specific antibodies [21, 25, 26].
In addition to that, the development of the indirect immunofluorescence technique that detect CAGTA, conducted in our laboratory, has facilitated not only the diagnosis of IC in patients at risk, since it differentiates colonization from invasion [12, 13], but also, is reflects the importance of those antibodies in a better prognosis for patients with IC admitted at the ICU [20].
Therefore, in order to elucidate the importance of those antibodies, the present study was designed to investigate the antifungal activity of CAGTA against C. albicans.
Whole IgG antibodies from immune serum of patients infected with C. albicans reduced the metabolic activity and viability of Candida planktonic cells in vitro. These effects on the metabolic activity and/or viability of C. albicans have already been reported for antibodies developed in different animal models of invasive candidiasis, such as chickens [35], rabbits [31, 36], and Balb/C mice [37]. Furthermore, the monoclonal antibody C7 (mAb C7) derived from Balb/C mice immunized with C. albicans, exerted metabolic inhibition and fungicidal effect on this yeast [38] and, more recently, mAb Ca37 also inhibited the growth of C. albicans in vitro [39].
Interestingly, in human serum, the antiBl-IgG serum fraction showed slight effect on C. albicans planktonic cells and therefore, the CAGTA-enr fraction appeared as the main responsible for the observed inhibitory effect. Concomitantly, the microscopy images illustrated that CAGTA-enr IgG reduced the growth and filamentation of C. albicans yeast cells in a concentration dependent manner. Similarly, Uppuluri et al. demonstrated that anti-Als3 antibodies have the potential to disrupt various properties of C. albicans like adherence, filamentation, and biofilm formation [40]. Moreover, an Als3-specific monoclonal antibody (3D9.3) was observed to significantly decrease the adhesion of C. albicans germ tubes to human epithelial and vascular endothelial cells [41].
Electron microscopy images of C. albicans germ tubes exposed to CAGTA-enr human IgG revealed an altered cell wall surface with protrusions, whereas the blastospores retained their original smooth surface, and this effect on cell wall structure was consistent with that reported for this same serum fraction in an experimental model of disseminated candidiasis in rabbits [31]. Other authors have reported that C. albicans exposed to a peptide from chilli pepper seeds caused severe alterations in bud formation, the cell wall and the cytoplasmic membrane of the yeast [42] and the antifungal ceragenins CSA-131 induced Candida auris cells to buckle in upon themselves, some of them appearing as merged [43]. Changes in cell wall structure are relevant for viability since they may disturb the traffic of nutrients and the osmotic stability of fungi; in this line, the mAb C7 affected the surface of C. albicans blastospores and altered the iron uptake pathway [38, 44]. In the present work we verified that the CAGTA-enr IgG serum fraction of IC patients reduced the metabolic activity of C. albicans and induced cell wall modifications, and purified CAGTA eventually killed cells, as evidenced by DiBAC staining.
With reference to the antifungal effect of sera from patients infected by NAC species, on average they reduced the metabolic activity or viability of C. albicans cells to a lesser extent, comparable to that produced by serum from C. albicans-infected patients who presented a low CAGTA titer. The fact that sera from patients with NAC infections may have CAGTA titers, and thus exert some activity against C. albicans, could be explained by cross-reactivity, a phenomenon previously described by other authors [13, 27, 39, 45, 46]. In this line, sera from patients infected with C. parapsilosis, C. tropicalis, C. glabrata or C. dubliniensis reacted with a recombinant amino terminal section of hyphal wall protein (Hwp1N), a well-characterized cell surface protein expressed only in C. albicans hyphae [13, 47]. Similarly, sera from patients infected with C. tropicalis, C. parapsilosis, C. glabrata or C. guilliermondii also reacted with a recombinant C. albicans enolase-1 (Eno1) [46, 48]. Eno1 is currently considered a moonlighting protein, a glycolysis and gluconeogenesis enzyme that can be secreted to the cell wall of Candida spp.[49] and is well known for promoting a strong humoral immune response in patients with invasive candidiasis [50]. Antibodies reacting with methionine synthase protein 6 (Met6), an essential protein for methionine biosynthesis located in the outer layers of C. albicans germ tubes cell wall [51] were also found in patients infected not only by C. albicans but by NAC species as well [27, 52]. Interestingly, antibodies reacting with Hwp1 and Met6, both proteins targets of CAGTA, resulted good biomarkers of IC in immunocompromised patients, either alone or in combination with beta-D-glucan detection results [27].
Another point to consider with reference to invasive candidiasis is the development of vaccines, and immunization trials in animal models have been conducted with encouraging success rates using various C. albicans components such as heat shock protein 90 (Hsp90) [53], Hwp1-N, Eno1[54] and Met6 among others [55, 56]. Some of these proteins react with CAGTAs, and the identification of new targets would provide us with new candidates as possible immunogenic protective agents against invasive candidiasis. Currently, our research group is searching for additional antigens recognized by CAGTA (data not published). So far, only the NDV-3A vaccine (NovaDigm Therapeutics, Inc.) based on Als3p (agglutinin-like sequence protein) is available, and is in phase 3 clinical trial; however, given that this vaccine is intended only for protection against Recurrent Vulvovaginal Candidiasis, the discovery of a vaccine for Invasive Candidiasis remains elusive and requires further investigation.
In conclusion, based on the proposed objective, our study demonstrated that IgG serum fraction from patients with C. albicans IC reduces the growth and metabolic activity of planktonic C. albicans cells in vitro; in addition, purified CAGTAs modify the surface of hyphal cell walls and, eventually, lead to cell death. Moreover, patients infected with non-albicans Candida species also produce antibodies that can cross-react with C. albicans, and reduce its metabolic activity and viability, although with lower intensity. The findings suggest that CAGTAs and related antibodies could be valuable as diagnostic and prognostic markers for invasive candidiasis, and their target antigens may have potential in the development of immunization protocols against Candida infections. Additional investigation is required to validate these discoveries, delve into their clinical implications, and assess the antibodies' capacity to effectively combat the infection.
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Acknowledgements
The authors are very grateful to Dr Juan Carlos García Ruiz and Dr María Soledad Cuétara for supplying sera from selected patients with Invasive Candidiasis. Technical and human support provided by SGIker (UPV/EHU) is also gratefully acknowledged.
Funding
Open Access funding provided thanks to the CRUE-CSIC agreement with Springer Nature. Funding for this work was provided by the University of the Basque Country UPV/EHU (GIU21/017) project. G. C. was supported by a Department of Education, Universities and Research of the Basque Country fellowship (PRE_2013_562). M. B. was supported by a University of Basque Country fellowship (PIF19/316).
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Conceptualization: [MDM]; Methodology: [GC] and [AD], Formal analysis and investigation: [GC] and [MB-V], Writing—original draft preparation: [GC]; Writing—review and editing: [IA-A], [MDM], Funding acquisition: [MDM]; Resources: [MDM]; Supervision: [IFL].
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Carrano, G., Arrieta-Aguirre, I., Díez, A. et al. Anti-Candida Antibodies of Patients with Invasive Candidiasis Inhibit Growth, Alter Cell Wall Structure, and Kill Candida albicans In Vitro. Mycopathologia 189, 16 (2024). https://doi.org/10.1007/s11046-023-00819-w
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DOI: https://doi.org/10.1007/s11046-023-00819-w