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Article

Preliminary Investigation about Aspergillus spp. Spread in Umbrian Avian Farms

by
Deborah Cruciani
1,*,
Silvia Crotti
1,
Carmen Maresca
1,
Ivan Pecorelli
1,
Emanuela Verdini
1,
Marinella Rodolfi
2,
Eleonora Scoccia
1,
Sara Spina
1,
Andrea Valentini
1 and
Francesco Agnetti
1
1
Istituto Zooprofilattico Sperimentale dell’Umbria e delle Marche “Togo Rosati” (IZSUM), 06126 Perugia, Italy
2
Department of Earth and Environmental Sciences, University of Pavia (UNIPV), 27100 Pavia, Italy
*
Author to whom correspondence should be addressed.
J. Fungi 2022, 8(11), 1213; https://doi.org/10.3390/jof8111213
Submission received: 25 October 2022 / Revised: 10 November 2022 / Accepted: 15 November 2022 / Published: 16 November 2022
(This article belongs to the Special Issue Fungal Diseases in Animals)
Browse Figures
Review Reports Versions Notes

Abstract

:
Among the fungi responsible for deep mycosis, the genus Aspergillus plays a predominant role both in human and veterinary medicine. From a “One Health” perspective, infections by Aspergillus spp. often represent a public health problem linked to specific occupational categories that could have a greater risk of inhaling spores and developing any respiratory disease. This preliminary investigation allowed to acquire information about the spread of Aspergillus spp. in avian livestock of the Umbria region (Central Italy), their sensitivity to antifungals, and the presence of mycotoxins in the considered farms. Environmental, feed, animal, and human samples were collected for mycological investigations; chemical analyses were also performed in feed samples. Moreover, prevalence estimated of the fungal isolates were provided for each individual farm sampled. Direct fungal identification was possible in 298 out of the 559 total samples; 162 of the samples were positive for Aspergillus spp. Mycotoxins were detected in 5 out of the 21 feed samples collected. All the aspergilli tested for antifungal susceptibility were resistant to fluconazole. The results obtained show how much the genus Aspergillus is widespread in the investigated farms; therefore, the poultry livestock represents a favorable environment for the maintenance and spread of fungal spores and their potential transmission to animals and humans.

1. Introduction

In the last decades, mycoses have acquired a considerable clinical importance. Nowadays, human mortality due to invasive fungal infections is comparable to that induced by tuberculosis or malaria worldwide [1,2,3]. The global increase in fungal diseases is mainly related to the better ability to diagnose them, the greater number of immunocompromised patients, the increasingly frequent use of invasive medical procedures, as well as prolonged antibiotic or corticosteroid therapies. Concerning animals, different groups such as pet, livestock, and wild species are widely affected by fungal agents too.
Deep and systemic mycoses play a more worrying role in public health, given their incidence, their clinical evolution, and their often difficult therapeutic management [4]. Furthermore, many fungal organisms often implicated in deep mycosis are intrinsically resistant to common antifungals [5].
The genus Aspergillus plays a preponderant role among the fungi responsible for deep mycosis; in particular, A. fumigatus can be responsible of bronchopulmonary allergic forms, especially in humans, worsening the clinical signs in patients with asthma, cystic fibrosis, or Chronic Pulmonary Aspergillosis (CPA). Allergic Bronchopulmonary Aspergillosis (ABPA) is still underestimated from a diagnostic point of view; its clinical or radiological features are confused with pulmonary tuberculosis, especially in developing countries. In industrialized countries, the estimated incidence of the disease is very high (e.g., in Europe about one million patients). From a pathogenesis perspective, recurrent exposure to high concentrations of A. fumigatus spores is the most cited risk factor in the development of ABPA, even if not the only one [6,7]. Also in veterinary medicine, A. fumigatus is associated with deep fungal respiratory infections, almost exclusively in birds [8]: exposure to high concentrations of environmental spores is the determining predisposing factor for the onset of the disease, even in this case. Hot-humid farm environments, often overcrowded and lacking in ventilation and hygiene, could contribute to the proliferation of these fungi and increase the exposure of animals to the infection, as well as poorly stored foodstuffs. The immune status of birds, prolonged therapies with antibiotics or corticosteroids, vaccinations, and metabolic disorders also represent further predisposing factors [9]. Aspergillus spp. is also mentioned in cases of dog rhinitis, mycosis of the guttural pockets in horses, bovine abortions and pneumonia in dolphins; however, these clinical conditions are uncommon [10,11]. The greater susceptibility of birds compared with mammals could be explained by differences between the innate and the acquired immunity against fungi, as well as the anatomical features of birds, such as a lack of epiglottis and a diaphragm or limited distribution of pseudo stratified columnar ciliated cells in the respiratory tract which could facilitate fungal engraftment [8]. Therefore, from a “One Health” perspective, deep infections by Aspergillus spp. can have an impact to public health. In particular, they represent a problem linked to specific occupational fields because some workers (e.g., veterinarians, breeders, poultry farms or feed mills operators) could have a greater risk of inhaling spores and developing any respiratory conditions [12].
Particularly, thanks to a multidisciplinary approach, this investigation provided information relating to: (i) Aspergillus spp. spread in some avian farms of the Umbria region (Central Italy); (ii) their sensitivity to common antifungals; (iii) the presence and spread of mycotoxins in feed samples. The data obtained have been useful to understand the potential risk of spreading and transmitting fungal spores and air-borne mycotoxins to workers operating in the poultry sector.

2. Materials and Methods

Through the involvement of the territorial Veterinary Services, eight poultry farms located in the Umbria region were selected for the investigations as follows: four intensive farms in the province of Perugia, three intensive farms, and one rural farm in the province of Terni. All farms were constantly monitored for the main infectious diseases, such as Influenza, West Nile Disease, and salmonellosis.
In the intensive farms, broilers (Gallus gallus) were raised indoors, in sheds ranging from 400 to 800 m2 (Figure S1), with controlled ventilation and temperature; animal density was about 20 subjects per m2; the litter was changed every two months, at the end of the production cycle; the feed was commercial and stored in special silos adjacent to the sheds; two operators worked six days a week in each farm.
In the rural farm, broilers, guinea fowl (Numida meleagris), and ducks (Anas platyrhynchos) were bred in stables with a surface of about 40 m2 and the possibility of access to outdoor parks (Figure S2); there was not monitoring of the ventilation or temperature inside the stables; the litter was changed approximately every two months; the feed was self-produced and stored in a closed room adjacent to the stables; there was only one operator responsible for the farm.

2.1. Sampling

For the isolation and the identification of Aspergillus spp. strains, the following specimens were collected: environmental samples, represented by air; surface swabs (from the walls of the sheds), litter, and soil; feed samples, directly collected from the silos and the feeders inside the sheds; animal samples, represented by respiratory mucosal swabs and pools of trachea, lungs, and air bags of birds found dead in the investigated farms; and human samples, represented by nasal swabs from farm workers.
The collection was planned on a monthly basis, in two periods of the year, one colder and one warmer: January–April and June–September. All the samples were stored in sterile containers until their transfer to the laboratory.
For mycotoxins analysis, to ensure representativeness of the entire feed lot, sampling was conducted according to EU Commission Regulation (EC) n. 152/2009.

2.2. Isolation of Aspergillus spp.

2.2.1. Environmental Samples: Air and Surface Swabs

A quantitative mycological analysis was carried out at the IZSUM for the air monitoring and for the surface swabs. Czapek agar (CZA) stimulating the growth of xerophilic species deeply colonizers of substrates was used as a selective reference medium for Aspergillus spp. and Penicillium spp. For air and swabs samples, the gravity sedimentation method settling plates exposed for 20 min, and plating by dilution were the techniques used. For air samples, plates were incubated at 25 ± 1 °C in aerobiosis, whereas for swabs the incubation was performed at 37 ± 1 °C in aerobiosis, according to the laboratory standards provided for fungi. The observation of the colonies was performed within 72–96 h.

2.2.2. Environmental Samples: Litter, Soil, and Feed Samples

A qualitative mycological examination was performed at UNIPV for litter, soil, and feed samples. The method used was direct-plating onto CZA. Plates were incubated at 25 ± 1 °C in aerobiosis, prolonging the incubation until 14 days in order to detect the slower growing strains too, and Petri plates replicates were constantly observed at low magnification (4×).

2.2.3. Animal and Human Samples

A qualitative mycological examination was carried out at IZSUM from collected animal organs or human nasal swabs, as previously described. Samples were direct-plated onto CZA and incubated at 25 ± 1 °C and 37 ± 1 °C in aerobiosis. Colonies were daily observed within 72–96 h.

2.3. Identification of Aspergillus spp. and Evaluation of the Antifungal Resistance

In accordance with the specific monographs, the morphological identification of the isolated aspergilli was carried out through the evaluation of their macroscopic and microscopic features such as growth rate, shape, texture, colour, pigments or exudates of the colonies, micro-morphology of the conidiophores and the conidia, and any other fruiting organs and cellular organelles.
They were morphologically analysed according to Klich M. A. [13], and also referring to the most recent classification of Houbraken J. et al. [14].
A total of 12 strains were subjected to DNA extraction for molecular typing using QIAamp DNA mini kit (QIAGEN®, Valencia, CA, USA) following the initial analysis step with Lysozyme Buffer (File S1). Amplification of the β-tubulin gene, specific for non-dermatophytic molds belonging to the genus Aspergillus, was subsequently carried out [15]. The amplification product was then sequenced through the automated Sanger method to reach species identification. To further confirm the results, a Neighbor-Joining phylogenetic tree has been constructed using the Maximum Composite Likelihood method (MEGA11 Sofware). These strains were also tested for the sensitivity to the most common antifungals with semi-automatic method of micro-dilution in broth using SensititreTM YeastOne YO10 (Thermo Fisher Scientific, Waltham, MA, USA): the evaluation of the M.I.C. (Minimal Inhibitory Concentration) ensure compliance with CLSI recommendation [16,17]. The antifungal molecules tested were: anidulafungin, micafungin, caspofungin, 5-fluorocytosine, posaconazole, voriconazole, itraconazole, fluconazole, and amphotericin B.

2.4. Evaluation of the Presence of Mycotoxins in the Feed

The presence of mycotoxins in 21 poultry feed samples collected from the investigated farms was evaluated by IZSUM using an ISO 17025 [18] accredited method for the simultaneous determination of Aflatoxin B1, Ochratoxin A, and Zearalenone in feeds for zootechnical use and raw materials. Limits of quantification (LOQs) were set at 0.0020, 0.025, and 0.050 mg/kg for Aflatoxin B1, Ochratoxin A, and Zearalenone, respectively. After shredding in slurry form, the samples were extracted by MeOH/H2O (80/20 v:v) and purified with Immunoaffinity columns (IAC), which ensured maximum specificity and allowed concentrations to be reached well below the levels set by current EU regulations: Directive 2002/32/EC of the European Parliament and Commission Recommendation (EU) 2016/1319. The instrumental determination was carried out by Ultra High Performance Liquid Chromatography couplet with fluorescence detector (UHPLC-FLUO).

2.5. Statistical Data Processing

A descriptive analysis of the obtained information was carried out considering the farms and the types of samples. In addition, the prevalence and the relative 95% confidence interval (95% CI) for each tested farm were calculated.
The antifungal susceptibility of the isolated aspergilli from the animals and the environment as well as the possible presence of mycotoxins in the feed samples examined were evaluated (in particular A. fumigatus ones).

3. Results

3.1. Isolation and Identification of Aspergillus spp. and Evaluation of The Antifungal Resistance

In the eight selected farms, a total of 559 samples were collected and represented as follows: 394 environmental samples (121 air, 124 surface swabs, 112 litter, and 37 soil), 38 animal samples, 46 feed samples, and 81 human samples (Table 1).
Fungal growth was recorded in 298 out of the 559 total samples (53%, Table 2). As specifically regards the air and the surface swabs samples, the mycological positivity was expressed as colony-forming units, according to the current legislation [19,20]. Table 2 also shows a total of 162 strains (29%) with macroscopic and microscopic features referable to Aspergillus spp.: in particular, 26 (5%), 5 (0.9%), and 3 (0.5%) of them were identified as members of A. fumigatus complex, A. flavus complex, and black aspergilli (A. niger complex), respectively.
Macroscopically, colonies referable to A. fumigatus complex grown velvety onto CZA appeared green to blue to greyish in colour and edged in white, with a cream-colored reverse (Figure 1a,b). Microscopically, the characteristics observed perfectly agreed with those reported by monographs: hyphae hyaline and septate, conidiophores with smooth wall, vesicles dome or claviform with phialides originating directly on the upper half or 2/3 of the vesicle, conidia with small spikes covering their surface and produced in basipetal column chains (Figure 1c).
A. flavus complex colonies appeared yellow to yellow-green in colour, with a cream-colored reverse; the surface was grainy, often with radial grooves and edged in white (Figure 2a,b). Microscopically, hyphae hyaline and septate, conidiophores with rough wall, vesicles dome or claviform with phialides originating, both directly and from metulae; on the entire vesicle surface, spherical and echinulated conidia were noticed (Figure 2c).
Young sterile colonies referable to black aspergilli appeared white-yellow in colour at maturity, covered by a layer of black conidial heads with a cream-colored reverse; the surface was grainy and edged in white (Figure 3a,b). Microscopically, hyphae hyaline and septate, smooth conidiophores with a tick wall, spherical vesicles with phialides originating from metulae on the entire vesicle surface, spherical/oval rough conidia were observed (Figure 3c).
In Table 3 the distribution of positive samples for Aspergillus spp. in the investigated farms is showed.
The three aspergilli species isolated through mycological examination were confirmed by PCR and Sanger sequencing. In particular, the molecular investigation was performed on 4 A. fumigatus complex strains (one for each sample category), 5 A. flavus complex strains, and 3 A. niger complex strains. The consensus sequences obtained showed significant similarity with those registered in the Westerdijk Fungal Biodiversity Institute database for A. fumigatus, A. flavus, and A. niger (Table 4); these results were also supported by the phylogenetic analysis (Figure 4).
The results of the antifungal susceptibility testing are shown in Table 5: Aspergillus spp. strains showed resistance to all the antimycotic drugs, particularly to fluconazole (n = 12, 100%), 5-fluorocytosine (n = 8, 67%), and anidulafungin, micafungin, and caspofungin (n = 6, 50%).

3.2. Evaluation of the Presence of Mycotoxins in Feed

The investigation on mycotoxins (Aflatoxin B1, Ochratoxin A and Zearalenone) was carried out on 21 out of 46 feed samples, and 5 of them, all collected at the rural farm using self-produced feed, presented mycotoxins at concentrations above LOQs. In four of them Aflatoxin B1 was detected while in the other one both Aflatoxin B1 and Zearalenone were found. Although, the concentrations of the mycotoxins (0.0040 mg/kg, 0.0103 mg/kg, 0.0028 mg/kg and 0.0091 mg/kg for Aflatoxin B1; 0.054 mg/kg for Zearalenone) were below the limits established by current EU legislation the presence of these molecules (100% of the samples collected at the rural farm) is of high concern.

4. Discussion

This preliminary investigation aimed to evaluate an often underestimated public health problem through a multidisciplinary approach and different technical skills. Nowadays, deep or systemic mycoses play a more worrying role, both in the human and veterinary medicine, given their incidence, their clinical evolution, and their often-difficult therapeutic management. Moreover, fungal infections can be difficult to overcome due to few effective molecules available and the possibility that resistance phenomena arise. Especially in human medicine they can be involved in occupational diseases [21].
Despite the small number of poultry farms participating in the study, some considerations can be made.
Fungal species are widespread in the avian livestock investigated (53%). In particular, the genus Aspergillus was isolated in 162 of the total samples analysed (29%), with a high percentage if compared with the total of fungi observed (54%). This evidence agree with data emerged from other studies carried out in some European countries [12,22]. Combining conventional and molecular diagnostic approaches, 34 strains (21%) were identified as members of three of the major complexes threatening human and animal health. In detail, 4 A. fumigatus, 5 A. flavus, and 3 A. niger has been sequenced from environmental, feed, animal, and human samples with significant similarity to the sequences deposited in the specific database. The importance of these three species was given according to the literature data about respiratory fungal diseases in humans and animals [6,9]. The molecular analyses proposed in this investigation helped to overcome the limitation of conventional methods in the fungal discrimination compared with the most recent introduced taxonomy [23].
In seven investigated farms the prevalence of aspergilli ranging from 19% to 43%; only in the remaining one no aspergilli were isolated, even if this intensive farm was the less sampled (14 samples out of 559, 2.5%). The only rural farm showed a prevalence of 28%, with 20 positive samples for Aspergillus spp. in a total of 72 collected ones. Despite the small amount of the investigated farms, the high prevalence of fungal growth, approximately 50% in the “C” intensive farm, encourages similar studies.
In the present survey, the rural poultry farm used a self-produced feed, stored on the floor of a room adjacent to the stables where the poultry were raised, whereas in the intensive farms the commercial feed was stored in silos. Feed storage in an environment without monitoring in temperature, humidity, ventilation, or the presence of fungal spores can easily allow its contamination by molds, including mycotoxin-producing Aspergilli. Storage in silos can prevent the mycotoxins production as long as biosafety guidelines will be respected. Mycotoxins can spread as free air-borne particles or through spores as vectors, thus becoming inhalable for animals and workers with serious health implications [24]. The mycotoxins values found in this survey fell within the limits established by current European legislation. Nevertheless, they must be considered as “indicators” of the degree of farm environmental mycotic contamination.
In a total of 81 human nasal swabs, 20 (25%) showed fungal growth, 18/20 (90%) has been identified as Aspergillus spp. and 6/18 (33%) as A. fumigatus (n = 4, 67%) and A. flavus (n = 2, 33%). These fungi were found in the upper respiratory tract, but no cases of deep mycoses were reported. Despite this, all the strains subjected to antifungal susceptibility showed high percentages of resistance to common antifungals, especially fluconazole (100%) [25,26]. Periodical mycological investigations could represent a good tool to monitor the degree of the environmental contamination by fungal spores and enhance any corrective or preventive measures to limit ABPA forms or other respiratory mycotic diseases.
Finally, further studies are necessary including more farms with different management (intensive and rural) to improve the monitoring of fungi and correlate the isolated strains with those of human origin, especially considering the resistance to common antifungal molecules.
Many Aspergillus species (particularly belonging to sections Nigri and Flavi) are also highly used for enzyme production, food fermentations, biotechnology, and production of pharmaceuticals [27]. In industry and laboratory contexts, they are clearly harmless, and their contribution is advantageous considering that their use complies with the safety regulations and implies the use of individual and collective protection devices. To support this, data obtained in this preliminary investigation highlight the importance of biosafety also in management farm. Some precautions can be adopted to reduce the fungal spread, especially aspergilli, such as i) a correct feed storage to avoid mycotoxins production, (ii) an appropriate animal density to avoid overcrowding and to reduce the circulation of infective agents; (iii) the use of individual protection devices (filter masks, visors, disposable gloves and coveralls, etc.) to protect the farm workers; (iv) the introduction of periodic monitoring of the operators for a self-control plan.

Supplementary Materials

The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/jof8111213/s1, Figure S1: Broilers raised in an intensive farm; Figure S2: A detail of the rural farm; File S1: Protocols for Bacteria, Isolation of genomic DNA from Gram-positive bacteria modified.

Author Contributions

Conceptualization, D.C., S.C. and F.A.; methodology, D.C., S.C., I.P., M.R. and F.A.; software, C.M. and E.S.; validation, S.C., I.P., M.R. and F.A.; formal analysis, D.C., E.V., E.S., S.S. and A.V.; investigation, D.C., E.V., S.S. and A.V.; resources, F.A.; data curation, D.C., S.C. and F.A.; writing—original draft preparation, D.C., C.M., I.P., M.R. and F.A.; writing—review and editing, D.C., S.C. and F.A.; visualization, D.C. and F.A.; supervision, S.C., C.M., I.P., M.R. and F.A.; project administration, D.C., S.C. and F.A.; funding acquisition, F.A. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by Italian Ministry of Health, current research funds 2018–2020 (Grant Number: IZS UM 011/18 RC).

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Written informed consent was obtained from the farms’ workers for their participation in this study and for the publication of any potentially identifiable images or data included in this article.

Data Availability Statement

Not applicable.

Acknowledgments

Not applicable.

Conflicts of Interest

The authors declare no conflict of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript; or in the decision to publish the results.

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Jof 08 01213 g001 550
Figure 1. Mycological examination of the colonies referable to A. fumigatus complex grown onto CZA. (a) Macroscopic surface of the colonies; (b) Macroscopic reverse of the colonies; (c) Microscopic features of the colonies (methylene blue staining, ×100, bar 10 µm).
Figure 1. Mycological examination of the colonies referable to A. fumigatus complex grown onto CZA. (a) Macroscopic surface of the colonies; (b) Macroscopic reverse of the colonies; (c) Microscopic features of the colonies (methylene blue staining, ×100, bar 10 µm).
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Figure 2. Mycological examination of the colonies referable to A. flavus complex grown onto CZA. (a) Macroscopic surface of the colonies; (b) Macroscopic reverse of the colonies; (c) Microscopic features of the colonies (methylene blue staining, ×40, bar 20 µm).
Figure 2. Mycological examination of the colonies referable to A. flavus complex grown onto CZA. (a) Macroscopic surface of the colonies; (b) Macroscopic reverse of the colonies; (c) Microscopic features of the colonies (methylene blue staining, ×40, bar 20 µm).
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Figure 3. Mycological examination of the colonies referable to black aspergilli grown onto CZA. (a) Macroscopic surface of the colonies; (b) Macroscopic reverse of the colonies; (c) Microscopic features of the colonies (methylene blue staining, ×20, bar 50 µm).
Figure 3. Mycological examination of the colonies referable to black aspergilli grown onto CZA. (a) Macroscopic surface of the colonies; (b) Macroscopic reverse of the colonies; (c) Microscopic features of the colonies (methylene blue staining, ×20, bar 50 µm).
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Figure 4. Neighbor-Joining phylogenetic tree of the sequenced Aspergillus strains. Maximum Composite Likelihood method, 1000 bootstraps (MEGA11 Software).
Figure 4. Neighbor-Joining phylogenetic tree of the sequenced Aspergillus strains. Maximum Composite Likelihood method, 1000 bootstraps (MEGA11 Software).
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Table
Table 1. Sample distribution by farm. Legend: i = intensive; r = rural.
Table 1. Sample distribution by farm. Legend: i = intensive; r = rural.
Farm/TipologyEnvironmental SamplesFeed
Samples		Animal
Samples		Human
Samples		Total
Samples
Air
Samples		Surface SamplesLitter SamplesSoil
Samples
A/i333111214
B/i121212444 1058
C/i666222630
D/i192210353769
E/r1515155751072
F/i121212495862
G/i27272799920128
H/i27272799918126
Total samples12112411237
46
38
81
559
394
Table
Table 2. Results of mycological examination.
Table 2. Results of mycological examination.
Sample
Category		Fungal
Growth 		Aspergillus
spp.		A.
fumigatus
Complex		A.
flavus
Complex		A.
niger
Complex		No Fungal
Growth		Total
Samples
Environmental samples2381111622156394
Feed samples34304011246
Animal samples632103238
Human samples20184206181
Total Aspergillus spp. 162 (29%)26 (5%)5 (0.9%)3 (0.5%)
Total samples298 (53%) 261 (47%)559
Table
Table 3. Aspergillus spp. prevalence distribution by farm. Legend: i = intensive; r = rural.
Table 3. Aspergillus spp. prevalence distribution by farm. Legend: i = intensive; r = rural.
Farm/TipologyAspergillus spp. Positive SamplesTotal
Samples/Farm		Prevalence95% CI
A/i-140%-
B/i115819%10–31%
C/i133043%25–63%
D/i266938%26–50%
E/r207228%18–40%
F/i196231%20–44%
G/i4612836%28–45%
H/i2712621%15–30%
Total samples16255929%2633%
Table
Table 4. Results of aspergilli sequencing.
Table 4. Results of aspergilli sequencing.
Aspergillus
Species		StrainSample
Category		Sample
Type		Accession
Number		OverlapSimilarityProbability
A. fumigatus1EnvironmentAirCNRMA13.34998.07%100.00%0
2FeedFeedCNRMA20.38898.05%100.00%0
3AnimalsLungCNRMA13.34998.25%100.00%0
4HumansNasal swabCNRMA20.14199.37%100.00%0
A. flavus5EnvironmentAirUOA/HCPF 8374A98.25%100.00%0
6EnvironmentAirCBS 120.6298.02%100.00%0
7AnimalsLungCBS 120.6298.02%99.82%0
8HumansNasal swabCBS 11936898.41%100.00%0
9HumansNasal swabCBS 11936898.41%100.00%0
A. niger10EnvironmentSuperficial swabITEM 1144897.91%100.00%0
11EnvironmentAirITEM 1020698.23%100.00%0
12FeedFeedCNRMA13.33098.23%99.64%0
Table
Table 5. Results of antifungal susceptibility test.
Table 5. Results of antifungal susceptibility test.
Antimycotic DrugNumber of Total
Resistant Strains (%)		Number And Type of
Resistant Strains		MIC Value
Anidulafungin6 (50%)3 A. fumigatus
3 A. flavus		8 µg/mL
8 µg/mL
Micafungin6 (50%)3 A. fumigatus
3 A. flavus		8 µg/mL
8 µg/mL
Caspofungin6 (50%)3 A. fumigatus
3 A. flavus		8 µg/mL
8 µg/mL
5-fluorocytosine8 (67%)2 A. fumigatus
4 A. flavus
2 A. niger		32 µg/mL
64 µg/mL
32 µg/mL
Posaconazole1 (8%)1 A. niger4 µg/mL
Voriconazole2 (17%)2 A. niger2 µg/mL
Itraconazole3 (25%)2 A. fumigatus
1 A. flavus		1 µg/mL
2 µg/mL
Fluconazole12 (100%)4 A. fumigatus
5 A. flavus
3 A. niger		128µg/mL
64 µg/mL
64 µg/mL
Amphotericin B1 (8%)1 A. flavus4 µg/mL
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MDPI and ACS Style

Cruciani, D.; Crotti, S.; Maresca, C.; Pecorelli, I.; Verdini, E.; Rodolfi, M.; Scoccia, E.; Spina, S.; Valentini, A.; Agnetti, F. Preliminary Investigation about Aspergillus spp. Spread in Umbrian Avian Farms. J. Fungi 2022, 8, 1213. https://doi.org/10.3390/jof8111213

AMA Style

Cruciani D, Crotti S, Maresca C, Pecorelli I, Verdini E, Rodolfi M, Scoccia E, Spina S, Valentini A, Agnetti F. Preliminary Investigation about Aspergillus spp. Spread in Umbrian Avian Farms. Journal of Fungi. 2022; 8(11):1213. https://doi.org/10.3390/jof8111213

Chicago/Turabian Style

Cruciani, Deborah, Silvia Crotti, Carmen Maresca, Ivan Pecorelli, Emanuela Verdini, Marinella Rodolfi, Eleonora Scoccia, Sara Spina, Andrea Valentini, and Francesco Agnetti. 2022. "Preliminary Investigation about Aspergillus spp. Spread in Umbrian Avian Farms" Journal of Fungi 8, no. 11: 1213. https://doi.org/10.3390/jof8111213

APA Style

Cruciani, D., Crotti, S., Maresca, C., Pecorelli, I., Verdini, E., Rodolfi, M., Scoccia, E., Spina, S., Valentini, A., & Agnetti, F. (2022). Preliminary Investigation about Aspergillus spp. Spread in Umbrian Avian Farms. Journal of Fungi, 8(11), 1213. https://doi.org/10.3390/jof8111213

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