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. 2014 Jul 8;2014:968215. doi: 10.1155/2014/968215

Mycotoxins and Mycotoxigenic Fungi in Poultry Feed for Food-Producing Animals

Mariana Vanesa Greco 1,2,*, María Luisa Franchi 3, Silvia Laura Rico Golba 4, Alejandro Guillermo Pardo 1,2, Graciela Noemí Pose 1,2,3
PMCID: PMC4121149  PMID: 25126610

Abstract

Moulds are capable of reducing the nutritional value of feedstuff as well as elaborating several mycotoxins. Mycotoxin-contaminated feed has adverse effects on animal health and productivity. Also, mycotoxins may be carried over into meat and eggs when poultry are fed with contaminated feed. In a point prevalence study feedstuff used for poultry nutrition in Argentina was analyzed for fungal flora, natural incidence of selected mycotoxins, and nutritional quality. Ten mould genera were recovered, six of them known to be mycotoxigenic. More than 28 species were determined. Fumonisins were detected in all the samples (median 1,750 ppb). Forty-four out of 49 samples (90%) were contaminated with DON (median 222 ppb) and OTA (median 5 ppb). Also, 44 out of 49 samples were contaminated with aflatoxins (median 2.685 ppb), 42 samples (86%) with ZEA (median 50 ppb), and 38 samples (78%) with T2-toxin (median 50 ppb). Ninety percent of the samples had at least one type of nutritional deficiency. This study indicates the need for continuous assessment of the mycological status of animal feed production, in order to feed animals for optimal performance ensuring food safety.

1. Introduction

The rapid growth in the meat sector has been underpinned by the rising demand of poultry meat, which has consistently increased about threefold the rate of population growth over each of the past five decades [1].

The presence of microscopic fungi affects the quality of feeds, their organoleptic attributes, and nutritional quality [2]. Moulds like other microorganisms will assimilate and utilize the most readily available nutrients in the materials they grow upon and spoilage may result in the loss of 5 to 100% of the nutrients in the feed [3]. Regarding nutritional quality, lipids, proteins, and minerals are of essential importance for the proper development and growth of farm animals. The quantity and the nutritional requirements of feed depend on the weight and age of the poultry as well as the season. Healthy poultry require sufficient amounts of carbohydrates, lipids, and proteins, along with the necessary vitamins and dietary minerals [4, 5].

In addition to their negative impact on nutritional and organoleptic properties, moulds can synthesize different mycotoxins [6]. It is well known that contamination of animal feed with mycotoxins may induce sanitary disturbances and mortality among animals and secondary contamination of human consumers via eggs, meat, or milk [7]. Consumption of a mycotoxin-contaminated diet may induce acute and long-term chronic toxic effects [8, 9]. With respect to humans and animals, in general terms, mycotoxins exhibit toxic actions and are characterized by carcinogenic, mutagenic, teratogenic, and estrogenic properties [2].

Most toxic species belong to the genera Aspergillus, Penicillium, Fusarium, and Alternaria [10]. According to several authors mycotoxins such as aflatoxins, zearalenone, T2-toxin, deoxynivalenol, ochratoxin A, fumonisins, and patulin can be considered the most common mycotoxins found in feed and food [1113].

Most mycotoxicoses of poultry are caused by an intake of low concentration of contaminants over a long whit the typical chronic symptoms of poor growth, poor feed efficiency, and suboptimal production. Ingestion of higher concentration however leads to acute clinical symptoms associated with specific vital organs, the immune system, and other aspects of avian physiology as well as mortality [2, 14].

For quality control the identification of the contaminating mycobiota is essential because it provides data on the potential production of its mycotoxins and is a helpful indicator to determine feed hygienic quality [15].

In the European Union the limits for several mycotoxins are regulated. The maximum content of aflatoxin B1 in poultry feed has been set in 0.02–0.05 ppm. Moreover, based on studies about feed to food mycotoxin transfer limits for ochratoxin A, deoxynivalenol, zearalenone, and fumonisins B1 and B2 in feed have been recommended [1618].

In Argentina there is information on the fungal status including mycobiota and mycotoxins in poultry feed, but this is limited to the central region of the country, particularly Córdoba province and more recently to Entre Ríos province [1925]. In Argentina three geographical regions can be clearly distinguished: the northern-central with grasslands, the southern (Patagonia) with tablelands, and the western with mountains.

The aim of the present study was to determine the hygienic and nutritional quality and the occurrence of selected groups of fungi and mycotoxins in poultry feeds in other important producing regions of Argentina, not previously studied. Samples were collected from the central region, particularly from Buenos Aires (the largest producing area of Argentina) and La Pampa provinces, and from Río Negro province (an increasing producing area belonging to the Patagonia region). The study includes enumeration and identification of mould genera and species, natural levels of mycotoxins such as aflatoxin, ochratoxin A (OTA), T2-toxin, fumonisin, deoxinivalenol (DON), and zearalenone (ZEA), and the evaluation of some variables related to nutritional quality (crude proteins, fats, humidity, and total ashes).

2. Materials and Methods

2.1. Samples

A total of 49 representative samples (1-2 kg per sample) of nine commercially prepared and farm mixed poultry feeds were collected from Buenos Aires, La Pampa, and Río Negro provinces during 2010 (details about samples are shown in Table 1). All samples were homogenized and divided to obtain a 1 kg of working sample for analysis. Each sample was ground in a laboratory mill.

Table 1.

Characteristics of the samples analyzed.

Province Type of feed Number of samples Sample characteristics
Bs. As. Broiler Chicken Starter 1 Commercial Pelleted
Broiler Chicken Starter 1 Noncommercial, private use Milled
Pullet Starter 4 Commercial Pelleted
Pullet Finisher 4 Commercial Pelleted
Laying Hen Finisher 3 Commercial Pelleted
Choique 5 Commercial Pelleted

La Pampa Pullet Starter 4 Commercial Pelleted
Pullet Finisher 4 Commercial Pelleted
Laying Hen Finisher 2 Commercial Pelleted

Río Negro Broiler Chicken Pre Starter 1 Commercial Milled
Broiler Chicken Starter 2 Commercial Milled
Broiler Chicken Starter 3 Noncommercial, private use Milled
Broiler Chicken Finisher 1 Commercial Pelleted
Broiler Chicken Finisher 3 Noncommercial, private use Milled
Pullet Starter 1 Commercial Pelleted
Pullet Finisher 1 Commercial Pelleted
Laying Hen Starter 1 Commercial Pelleted
Laying Hen Starter 1 Noncommercial, private use Milled
Laying Hen Finisher 1 Commercial Milled
Laying Hen Finisher 3 Noncommercial, private use Milled

The main component of samples was corn followed by deactivated soybean, soybean pellet, wheat bran, sorghum, animal proteins, and grain mill products.

For mycological examination feed samples were immediately analyzed upon arrival or they were stored for 2-3 days in paper bags at room temperature (about 25°C). Feed samples intended for mycotoxin analysis were stored at −20°C.

2.2. Mycobiota Determination

The dilute plate technique was used for enumeration and isolation of fungi [10]. Ten grams of each milled feed sample was mixed with 90 mL of 0.1% peptone and shaken on a horizontal shaker for 20 minutes. Then, 0.1 mL of this dilution was inoculated on each of three different media: Dichloran Rose Bengal Chloramphenicol Agar (DRBC) to enumerate total culturable fungi, Dichloran 18% Glycerol Agar (DG18) to enumerate xerophilic fungi, and Dichloran Chloramphenicol Peptone Agar (DCPA) for selective isolation of Alternaria and Fusarium species. Plates were incubated at 25°C for 7 days. The DCPA plates were incubated under 12 hours of light: 12 hours of darkness photoperiod. For counting, plates containing 10–100 colonies were used and the results were expressed as colony-forming units per gram of sample (CFU/g) [10]. Individual CFU/g counts for each colony type, considered to be different, were recorded. Representative colonies of each type were transferred for subculturing onto plates with Malt Extract Agar (MEA) or Water Agar (WA), for moulds suspected to belong to Alternaria or Fusarium genera. Filamentous fungi were identified at genus level according to macro- and microscopic criteria in accordance with Samson et al. [26]. Fungal isolates were identified at species level: Penicillium and Aspergillus spp. according to Pitt and Hocking [10], Fusarium spp. according to Nelson et al. [27], Alternaria spp. according to Simmons [28], and other fungi according to Pitt and Hocking [10]. The isolation frequency (Fr) and relative density (RD) of genus/species were calculated according to Gonzalez et al. [29], Pacin et al. [30], and Saleemi et al. [31] as follows:

Fr(%)=number  of  samples  with  a  genus  or  speciestotal  number  of  samples×100,RD(%)=number  of  isolates  of  a  genus  or  speciestotal  number  of  fungi  isolated×100. (1)

Aspergillus and Penicillium isolates were preserved on agar slants of MEA and Alternaria and Fusarium isolates on Potato Dextrose Agar (PDA) at 4°C and cryopreserved in 18% glycerol at −20°C.

2.3. Mycotoxin Analysis

To evaluate mycotoxin occurrence, feed samples were subjected to quantitative analysis using ELISA-based analytical test kits for aflatoxin, ochratoxin A, T2-toxin, fumonisin, deoxynivalenol, and zearalenone (RIDASCREEN FAST, R-BiopharmAG). The extraction procedures were according to manufacturer's protocol. In brief, 5 g of ground sample was extracted with 25 mL of 70% methanol for aflatoxins, T2-toxin, ZEA, and fumonisins. For OTA and DON, samples were extracted with 12.5 mL of 70% methanol or 100 mL of distilled water, respectively. Afterwards, samples were shaken vigorously for 3 minutes and the extracts filtered through Whatman N°1 paper. Then, aflatoxins, OTA, T2-toxin, and ZEA filtrates were diluted with distilled water in the ratio 1 : 1 and fumonisin filtrates in the ratio 1 : 14. Fifty μL of the diluted filtrate per well was used for testing [32].

2.4. Nutritional Analysis

Feed samples were subjected to proximate analysis in accordance with standard methods described by the AOAC [33]. In terms of nutritional composition crude proteins (Kjeldahl) (Method 984.13), fats (Soxhlet) (Method 945.16), humidity (Method 934.01), and total ashes (to constant weight) (Method 942.05) were determined. Prior to analysis feed samples supplied as pellets were ground with a blade grinder or laboratory mill. All analyses were done in duplicate.

To obtain the moisture content the oven-drying method was used. Samples were dried overnight in an oven at 100°C, cooled in a desiccator to room temperature, and weighed. This procedure was performed as many times as necessary until constant weight. The result was obtained by weight difference with the sample at the beginning of the procedure.

All other analyses were performed on dry matter.

Determination of total ashes (mineral content) was performed by ignition of samples in a muffle oven set at 600°C until complete calcination of organic components. This is achieved when ashes obtained are white or light gray and the weight is constant. Samples were cooled in a desiccator at room temperature and weighed. At the beginning of this procedure samples were heated until obtention carbonaceous residue.

A Soxhlet extractor was used to determine free lipid content. Dried samples were weighed into an extraction thimble. The extraction was performed using petroleum ether of 60–80 boiling range for approximately 2 hours (occurring at least 7 cycles of filling and siphoning of the extraction tube). Then the flask with the solvent-free lipid extract was dried in an oven, cooled in a desiccator, and weighed. Results are expressed as percentage of lipids.

Determination of total nitrogen (crude protein) was conducted using the Kjeldahl method. The percentage of crude protein was calculated by multiplying the total nitrogen by a correction factor of 6.25.

2.5. Statistical Analysis

Fungal counts and toxins content were analyzed with the Kruskal-Wallis test. Multiple Range Test for variables was employed to compare means of fungal counts and toxins content of samples from different provinces. Differences were considered significant when P < 0.05. Statgraphics Centurion XVI version 16.1.18 was used for all analyses.

3. Results and Discussion

Fungal contamination of animal feed, with the consequent mycotoxin production, is one of the major threats to human and animal health [34]. In our study, all the samples analyzed were contaminated with fungi and mycotoxins.

Fungal counts (CFU/g) were obtained from different poultry feed samples on the three culture media and the mycological quality was determined according to Gimeno [35]: samples can be qualified as good (count range < 3.104 UFC/g), regular (count range 3.104–7.104 UFC/g), and bad (>7.104 UFC/g). On both media, DRBC and DCPA, fungal count range was 10–106 CFU/g. According to the mycological quality criterion 56% (26/46) samples could be qualified as good, 7% (3/46) as regular, and 37% (17/46) as bad (on DRBC). In Argentina there is information about the mycobiota and natural occurrence of mycotoxins in feedstuff [1924, 32, 36, 37]. However these reports on poultry feed refer mostly to Córdoba and Entre Rios provinces (central area of the country). With respect to the hygienic quality of poultry feed the last report from Córdoba province [24] was informed that 79% of finisher poultry feed samples exceeded the maximum allowed total fungal count to ensure hygienic quality. In Entre Rios province, 120 pelleted poultry feed samples were analyzed and total fungal count was below the established value (1 × 104 UFC/g) [25]. Significant differences among fungal contamination levels in feed from Río Negro province were observed (P < 0.05) while nonsignificant differences were found between feed samples from each province. These results indicate the need for continuous assessment of the mycological status of animal feed production.

Xerophilic fungal counts were in the range 1 × 102–1.45 × 106 CFU/g. Spoilage of feedstuff can be due to xerophilic fungi, which are capable of rapid growth above about 0.77 water activity (a w) and of slow growth at 0.75 a w and below-down to about 0.68 a w [10]. Although a w of poultry feed is low (average 0.537) it should be kept in a dry and fresh place. If by carelessness or negligence feed is not kept under proper conditions, as the humidity increases fungal growth and proliferation of xerophilic fungi can occur. Fungal counts average and median were similar between all culture media tested (105 CFU/g and 103 CFU/g, resp., data not shown).

The mycobiota and natural incidence of aflatoxin B1, ZEA, and DON were investigated by Dalcero and colleagues [19, 20]. In the first study Penicillium (98%), Fusarium (87%), and Aspergillus (52%) were the most prevalent genera determined whereas in the second study Aspergillus (85%) and Fusarium (70%) were the dominant genera. The predominant species of the genera abovementioned were particularly studied [21, 22]. The predominant species of Aspergillus were A. flavus and A. parasiticus. For Penicillium they were P. brevicompactum, P. purpurogenum, and P. oxalicum. With regard to Fusarium genus the predominant species were F. moniliforme and F. nygamai. Aflatoxin B1 was the most prevalent mycotoxin. The last study [24] indicates that A. flavus was the only species belonging to section Flavi which was isolated while Fusarium verticillioides was the prevalent species. In Entre Rios province A. flavus and A. parasiticus were the aflatoxigenic species isolated.

In our study ten mould genera were recovered, four of them known to be mycotoxigenic [10]. The frequency (Fr) and relative density (RD) are showed in Table 2. While the predominant genera are coincident with the abovementioned results, the most frequent mycotoxigenic fungi were those from the genus Fusarium (69.6), followed by Eurotium (52.2%), Penicillium (45.65%), and Aspergillus (43.5%), although the presence of Eurotium spp. was not previously reported. The occurrence of Aspergillus spp. and Fusarium spp. is widespread in tropical countries, also, in corn in Argentina [38]. Corn is the main component of poultry feed in the samples analyzed.

Table 2.

Fungal genus present in poultry feed samples.

Genus Number of isolates Fr (%)∗ RD (%)∗∗
Aspergillus 20 43.5 10.5
Cladosporium 22 47.8 11.5
Eurotium 24 52.2 12.5
Fusarium 32 69.6 16.7
Mucor 18 39.1 9.4
Penicillium 21 45.6 10.9
Paecilomyces 1 2.2 0.5
Scopulariopsis 2 4.3 1.0
Others 16 34.8 8.4
Yeast 36 78.3 18.8

*Isolation frequency.

∗∗Isolation relative density.

More than 28 species were recovered from poultry feed samples. Several species from different genera were determined in each sample. Up to 12 different species were recovered in several samples. The frequency (Fr) and relative density (RD) are showed in Table 3. Different to the studies from Cordoba province, the most prevalent mycotoxigenic Fusarium species determined was F. proliferatum (Fr 69.5%–RD 17.7%). In accordance with previous studies in Córdoba [19, 20] and Entre Rios provinces [25], A. flavus and A. parasiticus (Fr 6.5%) were the aflatoxigenic species isolated. Penicillium chrysogenum and P. nalgiovense (Fr 13.0%) were the most prevalent Penicillium species recovered. Some other studies have shown that most poultry feeds are contaminated with species belonging to Penicillium, Fusarium, and Aspergillus genera [23]. From 120 samples of poultry feed Magnoli et al. [23] reported the presence of 15 genera of filamentous fungi. Fusarium and Penicillium were isolated in 67.5% of the samples and Aspergillus in 57.5% of them [23]. In South America, mycobiota and natural occurrence of aflatoxins, fumonisins, and ZEA in poultry feed were studied in Rio de Janeiro, Brazil [39]. The most frequent genus isolated was Penicillium (41.26%) followed by Aspergillus (33.33%) and Fusarium (20.63%). Penicillium citrinum, A. flavus F. verticillioides, and F. graminearum were the most prevalent species in decreasing order. On the other hand, we found Fusarium and Penicillium species, followed by Aspergillus, as prevalent mycobiota (Tables 2 and 3). Eurotium species such as E. amstelodami, E. repens (Fr 26.1%), E. chevalieri (Fr 19.6%), and E. rubrum (15.2%) were also found.

Table 3.

Fungal species present in poultry feed samples.

Species Number of isolates Fr (%)∗ RD (%)∗∗
Eurotium amstelodami 12 26.1 6.6
E. chevalieri 9 19.6 4.9
E. herbariorum 1 2.2 0.5
E. repens 12 26.1 6.6
E. rubrum 7 15.2 3.9
Eurotium sp. 2 4.3 1.1
Aspergillus candidus 4 8.7 2.2
A. flavus 3 6.5 1.7
A. fumigatus 1 2.2 0.5
A. niger 3 6.5 1.7
A. niveus 1 2.2 0.5
A. parasiticus 3 6.5 1.7
A. terreus 2 4.3 1.1
A. versicolor 1 2.1 0.5
Aspergillus sp. 7 15.2 3.9
Cladosporium cladosporioides 22 47.8 12.1
Penicillium brevicompactum 1 2.2 0.5
P. chrysogenum 6 13.0 3.3
P. citrinum 1 2.2 0.5
P. decumbens 1 2.2 0.5
P. funiculosum 3 6.5 1.7
P. implicatum 3 6.5 1.7
P. nalgiovense 6 13.0 3.3
P. oxalicum 2 4.3 1.1
P. pinophilum 2 4.3 1.1
P. variabile 1 2.2 0.5
Penicillium sp. 6 13.0 3.3
Fusarium proliferatum 32 69.5 17.7
Fusarium sp. 5 10.9 2.8
Paecilomyces variotii 1 2.2 0.5
Scopulariopsis brevicaulis 1 2.2 0.5
S. fusca 1 2.2 0.5
Scopulariopsis sp. 1 2.2 0.5
Mucor sp. 18 39.1 9.9

*Isolation frequency.

∗∗Isolation relative density.

Table 4 shows the distribution concentration of mycotoxins in the poultry feed tested in this study. Fumonisins were detected in all the samples analyzed in a range of 222–6,000 ppb (median 1,750 ppb). Forty-four out of 49 samples (90%) were contaminated with DON (median 222 ppb) and OTA (median 5 ppb). Also, 44 out of 49 samples were contaminated with aflatoxins (median 2.685 ppb), 42 samples (86%) were contaminated with ZEA (median 50 ppb), and 38 samples (78%) were contaminated with T2-toxin (median 50 ppb). Fumonisins and DON showed the highest levels detected (6,000 ppb and 318 ppb, resp.). Significant differences were found for fumonisins in feed from La Pampa, for OTA and T2-toxin in feed from Río Negro, and for ZEA in feed from Buenos Aires. However, no differences were found for aflatoxins (P = 0.0604) and DON (P = 0.1211).

Table 4.

Concentration of different mycotoxins in poultry feed samples (ND: not detected).

Province Parameter Mycotoxins (ppb)
Aflatoxin∗ DON∗ Fumonisin∗ OTA∗ T2-toxin∗ ZEA∗
Bs. As. Number of samples positive/tested 17/18 (94.5%) 18/18 (100%) 18/18 (100%) 17/18 (94.5%) 15/18 (83.4%) 12/18 (66.7%)
Minimum ND 222.00 222.00 ND ND ND
Maximum 11.85 318.00 4980.00 12.31 50.00 50.00
Median 4.32 222.00 890.00 5.00 50.00 50.00

La Pampa Number of samples positive/tested 8/10 (80%) 8/10 (80%) 10/10 (100%) 9/10 (90%) 4/10 (40%) 9/10 (90%)
Minimum ND ND 1160.00 ND ND ND
Maximum 4.24 247.00 6000.00 5.00 50.00 95.58
Median 1.96 222.00 4565.00 5.00 ND 50.00

Río Negro Number of samples positive/tested 17/18 (94.5%) 18/18 (100%) 18/18 (100%) 18/18 (100%) 18/18 (100%) 18/18 (100%)
Minimum ND 222.00 222.00 5.00 ND 50.00
Maximum 37.67 222.00 6000.00 13.20 107.23 75.76
Median 2.47 222.00 708.50 5.00 50.00 50.00

*LOD (ppb): aflatoxin: <1.7; DON: 200; fumonisins: 222; OTA: 5; T2-toxin: <20; ZEA: 17–41.

Magnoli et al. [23] also found that fumonisins had the highest incidence and were found in 97% of the analyzed samples followed by aflatoxin B1 (46%), ZEA (18%), and DON (6%). Jaramillo [40] found that fumonisin B1 and ZEA occurred in most of the samples, whereas aflatoxin B1 occurred in lower proportion. Aflatoxin B1 values ranged between 1.2 and 17.5 ppb. Fumonisin B1 levels ranged between 1,500 and 5,500 ppb. Zearalenone levels ranged between 100 and 7,000 ppb. In both reports, the simultaneous occurrence of two carcinogenic mycotoxins, aflatoxin B1 and fumonisin B1, was determined in feed intended for poultry consumption. In Córdoba province several mycotoxins were monitored in feeds. One hundred percent of poultry samples were contaminated with fumonisins B1, but aflatoxin B1 and T2- toxin, in between other selected mycotoxins, were not detected in any poultry feed [24]. On the other hand, cooccurrence of fumonisin B1, T2-toxin, and HT-2 was detected in 100% of the samples of poultry feed analyzed in Entre Rios province, with mean levels from 4502 to 5813, 19.6 to 30.3, and 6.7 to 21.6 ppb, respectively. Also, samples were cocontaminated with aflatoxin B1 [25].

In this work cooccurrence of mycotoxins was determined in all of the samples analyzed. Cooccurrence of at least three out of six mycotoxins was determined in all of the samples analyzed. Cooccurrence of six mycotoxins was determined in 57% (28/49) of the samples. The combined action of mycotoxins can generate an interactive effect such as additivity, synergism, or antagonism. The synergistic interaction causes the most toxic effects in the case of aflatoxins and OTA, or aflatoxins and toxin T2. An additive effect of aflatoxins and DON in fattening poultry has been demonstrated. This effect was obvious in proventriculus weight, blood glucose level, and lactate dehidrogenase activity. Synergistic effects in fattening poultry were observed in the case of aflatoxins and OTA. This interaction provoked reduction of body weight and increased mortality. Moreover, synergistic effects were observed for aflatoxins and toxin T2. A reduction in body weight, increased relative weight of kidneys, gizzard and hearth, and reduction of the mean corpuscular volume and potassium levels in blood were observed [41]. In our study cooccurrence of aflatoxins and OTA was observed in 42 out of 49 samples. The cooccurrence of aflatoxins and T2-toxin was observed in 37 samples. Synergism between aflatoxins and toxin T2 is extremely important in poultry due to the prevalence and severity of both mycotoxins [40]. Simultaneous occurrence of two carcinogenic mycotoxins, aflatoxins and fumonisins, was recorded in 44/49 (90%) of the samples.

Around the world other researchers have studied the mycobiota and mycotoxins in poultry feed during the last years. Okoli et al. [3] analyzed the mycobiota of commercial poultry feed in Nigeria. The common moulds isolated were Aspergillus spp., Penicillium spp., Mucor spp., Rhizopus spp., Epicoccum spp., Gymnoascus spp., Cladosporium spp., Mortierella spp., yeast, and bacteria. In Pakistan, Saleemi et al. [31] found Aspergillus species as most predominant fungi, followed by Penicillium, Fusarium, and Alternaria. Among the Aspergillus isolates, A. niger (37.74%) was the most frequently isolated species followed by A. flavus (22.64), A. ochraceous (16.98%), A. parasiticus (13.21%), A. carbonarius (3.77%), A. fumigatus (3.77%), and A. oryzae (1.89%). The proportion of toxigenic fungi among Aspergillus isolates was 73.58%. Shareef [6] recovered fourteen mould genera from Iraq poultry feed. The most frequent fungi were Aspergillus followed by Penicillium, Mucor, Rhizopus, Scopulariopsis, Alternaria, and Eurotium. They also study the presence of 4 mycotoxins; aflatoxins and ochratoxins were determined in 91.1% of the samples, fumonisins were determined in 51.1%, and T2-toxin was determined in 2.2% of the samples [3, 6, 31].

The toxicogenic fungal contamination of the raw materials occurs during the preharvest and/or the postharvest periods, and the finished feeds are exposed during production, processing, transportation, and storage [24]. It has been observed that moulds and mycotoxins presence varies depending on the geographical location and the year. Temperature and humidity play important roles not only in the development of fungi but also in mycotoxin production [24].

With respect to nutritional aspects, poor health can be caused by an imbalance of nutrients either by deficiency or by excess. Also, malnutrition if prolonged eventually leads to animal death. We found that 90% of the analyzed samples presented some kind of nutritional deficiency. The results are showed in Table 5. Forty-one out of 42 samples contained adequate moisture. However, 90% of them had at least one type of nutritional deficiency. Nineteen out of 38 samples did not reach the minimum of protein content required, 31 out of 40 did not contain the minimum requirements of lipids, and 9 out of 38 exceeded the ash content.

Table 5.

Nutritional composition of poultry feed samples analyzed and recommendations (NA: not analyzed).

Animal/type of animal feed Sample Nutritional analysis
Moisture Proteins Lipids Ashes
Broiler Chicken Prestarter P33 10,29 21,34 3,65 5,89

Recommendations: Protein (min) = 22%
Lipids (min) = 5–5,5%
Ashes (max) = 6–8%
Moisture (max) = 12%

Broiler Chicken Starter P1 12,88 NA NA NA
P18 11,75 NA NA NA
P32 8,98 22,99 1,78 6,62
P34 9,08 24,12 2,48 6,99
P35 12,04 19,85 2,49 5,26
P42 Error 23,66 5,31 5,44
P45 10,73 21,13 4,55 6,15

Recommendations: Protein (min) = 20–22%
Lipids (min) = 3–5%
Ashes (max) = 4.9–8%
Moisture (max) = 12-13%

Pullet Starter P12 10,21 22,21 2,89 6,32
P8 10,20 10,58 1,92 9,67
P13 9,48 19,56 4,39 11,45
P16 9,10 10,46 1,79 10,63
P19 Error 21,11 4,97 5,46
P21 NA NA NA NA
P24 11,00 NA 2,38 7,97
P28 10,35 21,48 2,68 5,80
P39 9,99 18,82 4,94 5,01

Recommendations: Protein (min) = 20%
Lipids (min) = 6%
Ashes (max) = —
Moisture (max) = 12.5%

Broiler Chicken Finisher P29 11,54 NA NA NA
P36 12,75 17,88 2,08 4,78
P38 9,47 19,22 2,66 6,29
P43 11,63 16,93 4,30 5,38

Recommendations: Protein (min) = 18–18.5%
Lipids (min) = 4-5%
Ashes (max) = 7.5–8%
Moisture (max) = 12%

Pullet Finisher P9 7,61 11,60 4,26 NA
P10 7,58 18,54 8,08 8,64
P15 9,64 19,46 8,90 5,66
P17 7,44 10,78 3,61 10,20
P20 10,61 20,81 4,99 6,41
P22 10,18 18,35 6,16 8,50
P27 7,37 20,26 8,59 6,53
P25 10,77 NA 2,70 NA
P40 9,44 19,03 5,27 4,74

Recommendations: Protein (min) = 19.5%
Lipids (min) = 5%
Ashes (max) = —
Moisture (max) = 12.5%

Laying Hen Starter P31 8,94 19,06 3,25 17,28
P46 11,85 20,72 4,69 9,03

Recommendations: Protein (min.) = 20%
Lipids (min) = 6%
Ashes (max) = 5%
Moisture (max) = 12%

Laying Hen Finisher P7 8,63 14,10 3,25 11,29
P11 8,08 13,36 3,21 15,89
P14 8,86 18,86 3,25 12,42
P23 10,01 13,38 3,89 14,00
P26 NA NA NA NA
P30 10,18 NA NA NA
P37 11,34 18,82 2,33 10,37
P41 11,34 18,82 2,33 10,37
P44 8,83 12,21 3,91 9,51

Recommendations: Protein (min) = 16%
Lipids (min) = 6%
Ashes (max) = 5%
Moisture (max) = 12%

Choique (Pterocnemia pennata) P2 9,60 22,01 3,22 10,07
P3 9,85 21,69 3,60 10,45
P4 9,20 21,94 3,29 10,02
P5 8,97 21,97 3,25 10,04
P6 9,75 21,97 3,25 10,04

Recommendations: Protein (min) = 20%
Lipids (min) = 5%
Ashes (max) = 11%
Moisture (max) = 12%

Recommendations values were obtained from producers.

This information is quite important considering poultry health, and hence productivity requires proper supply of these nutrients. The nutritional quality of chicken meat lies in their protein, iron, zinc, phosphorus, niacin, folic acid, and vitamins A, B6, and B12 content. The nutritional quality of the chicken thus depends on their feeding conditions.

Moulds are capable of reducing the nutritional values of feedstuff. When conditions are optimal for moulds to colonize grains in the field or in storage, their first effect is utilization of nutrients for their metabolism and propagation. This results in decreased nutritional value of feeds. Energy, crude protein, and crude fat values of mouldy corn were decreased by 5, 7, and 63%, respectively [41].

4. Conclusions

In this work, although the amounts of the mycotoxins detected on poultry feed were lower than the regulation limits established, the cooccurrence of several mycotoxins was demonstrated. The scientific literature offers a broad spectrum of information on the effects of individual mycotoxins in various animal species but concurrent exposure to multiple mycotoxins is more likely in feedstuff [8]. While mycotoxins have attracted worldwide attention due to their direct impact on human health, due to food contamination, it is also relevant to consider to what extent mycotoxins can be carried over into edible tissues like meat and eggs when poultry are fed with contaminated feed.

We suggest that periodic monitoring and the application of the Hazard Analysis and Critical Control Points (HACCP) on the prevention and control of mycotoxins in the animal feed industry are needed in order to guarantee the hygienic and nutritional quality of feed to ensure health and productivity of poultry as well as prevent human foodborne diseases.

Acknowledgments

This work was supported by UNQ, UNRN, CONICET, and Agencia Nacional de Promoción Científica y Tecnológica (ANPCyT).

Conflict of Interests

The authors declare that there is no conflict of interests regarding the publication of this paper.

References

  • 1.Food and Agriculture Organization of the United Nations (FAO) Statistic Division (FAOSTAT), Trends in the livestock sector, part 3, 2013, http://www.fao.org/docrep/015/i2490e/i2490e03c.pdf.
  • 2.Cegielska-Radziejewska R, Stuper K, Szablewski T. Microflora and mycotoxin contamination in poultry feed mixtures from western Poland. Annals of Agricultural and Environmental Medicine. 2013;20(1):30–35. [PubMed] [Google Scholar]
  • 3.Okoli IC, Nweke CU, Okoli CG, Opara MN. Assessment of the mycoflora of commercial poultry feeds sold in the humid tropical environment of Imo State, Nigeria. International Journal of Environmental Science and Technology. 2006;3(1):9–14. [Google Scholar]
  • 4.Gillespie JR, Flanders FB. Modern Livestock and Poultry Production. 8th edition. Ontario, Canada: Cengage Learning; 2009. [Google Scholar]
  • 5.Damerow G. The Chicken Encyclopedia: An Illustrated Reference. North Adams, Mass, USA: Storey; 2012. [Google Scholar]
  • 6.Shareef AM. Molds and mycotoxins in poultry feeds from farms of potential mycotoxicosis. Iraqi Journal of Veterinary Sciences. 2010;24(1):17–25. [Google Scholar]
  • 7.Nyamongo J, Okioma M. The aflatoxin outbreaks in Kenya in 2004 and 2005: a case study. Proceedings of the Conference on Reducing Impact of Mycotoxins in Tropical Agriculture with Emphasis on Health and Trade in Africa; 2005; Accra, Ghana. p. p. 3. [Google Scholar]
  • 8.Binder EM, Tan LM, Chin LJ, Handl J, Richard J. Worldwide occurrence of mycotoxins in commodities, feeds and feed ingredients. Animal Feed Science and Technology. 2007;137(3-4):265–282. [Google Scholar]
  • 9.Venancio A, Paterson R. The challenge of mycotoxins. In: McElhatton A, Marshall RJ, editors. Food Safety—A Practical and Case Study Approach. Berlin, Germany: Springer; 2007. pp. 24–47. [Google Scholar]
  • 10.Pitt J, Hocking A. Fungi and Food Spoilage. 3rd edition. Berlin, Germany: Springer; 2009. [Google Scholar]
  • 11.Hussein HS, Brasel JM. Toxicity, metabolism, and impact of mycotoxins on humans and animals. Toxicology. 2001;167(2):101–134. doi: 10.1016/s0300-483x(01)00471-1. [DOI] [PubMed] [Google Scholar]
  • 12.Orellano JL. Métodos de determinación, identificación y control de micotoxinas en ingredientes para la nutrición animal. Engormix. 2007 [Google Scholar]
  • 13.Gimeno A, Martins ML. Micotoxinas y Micotoxicosis en Animales y Humanos. 1st edition. Miami, Fla , USA: Special Nutrients; 2007. [Google Scholar]
  • 14.Mabbett T. Keep feeds free from fungi. African Farming. 2004:15–16. [Google Scholar]
  • 15.Khosravi AR, Dakhili M, Shokri H. A mycological survey on feed ingredients and mixed animal feeds in Ghom province, Iran. Pakistan Journal of Nutrition. 2008;7(1):31–34. [Google Scholar]
  • 16.Directive 2002/32/EC of the European Parliament and of the Council of 7 May 2002 on undesirable substances in animal feed. Official Journal of the European Communities. 2002;(L 140/10) [Google Scholar]
  • 17.Commission Regulation (EU) Amending Annex I to Directive 2002/32/EC of the European Parliament and of the Council as regards maximum levels for nitrite, melamine, Ambrosia spp. and carry-over of certain coccidiostats and histomonostats and consolidating Annexes I and II thereto. Official Journal of the European Union. 2011;L159/7 [Google Scholar]
  • 18.Commission recommendation of 17 August 2006 on the presence of deoxynivalenol, zearalenone, ochratoxin A, T-2 and HT-2 and fumonisins in products intended for animal feeding. Official Journal of the European Union. 2006;(L229/7) [Google Scholar]
  • 19.Dalcero AM, Magnoli CE, Chiacchiera SM, Palacios G, Reynoso M. Mycoflora and incidence of aflatoxin B1, zearalenone and deoxynivalenol in poultry feeds in Argentina. Mycopathologia. 1997;137(3):179–184. doi: 10.1023/a:1006890717758. [DOI] [PubMed] [Google Scholar]
  • 20.Dalcero AM, Magnoli CE, Luna M, et al. Mycoflora and naturally occurring mycotoxins in poultry feeds in Argentina. Mycopathologia. 1998;141(1):37–43. doi: 10.1023/a:1006868002985. [DOI] [PubMed] [Google Scholar]
  • 21.Magnoli CE, Dalcero AM, Chiacchiera SM, Miazzo R, Sáenz MA. Enumeration and identification of Aspergillus group and Penicillium species in poultry feeds from Argentina. Mycopathologia. 1998;142(1):27–32. doi: 10.1023/a:1006981523027. [DOI] [PubMed] [Google Scholar]
  • 22.Magnoli CE, Sáenz MA, Chiacchiera SM, Dalcero AM. Natural occurrence of Fusarium species and fumonisin-production by toxigenic strains isolated from poultry feeds in Argentina. Mycopathologia. 1999;145(1):35–41. doi: 10.1023/a:1007053617961. [DOI] [PubMed] [Google Scholar]
  • 23.Magnoli CE, Chiacchiera SM, Miazzo R, et al. The mycoflora and toxicity of feedstuffs from a production plant in Córdoba, Argentina. Mycotoxin Research. 2002;18:7–22. doi: 10.1007/BF02946135. [DOI] [PubMed] [Google Scholar]
  • 24.del Pilar Monge M, Magnoli CE, Chiacchiera SM. Survey of Aspergillus and Fusarium species and their mycotoxins in raw materials and poultry feeds from Córdoba, Argentina. Mycotoxin Research. 2012;28(2):111–122. doi: 10.1007/s12550-011-0121-8. [DOI] [PubMed] [Google Scholar]
  • 25.Monge MP, Dalcero AM, Magnoli CE, Chiacchiera SM. Natural co-occurrence of fungi and mycotoxins in poultry feeds from Entre Ríos. Food Additives and Contaminants B. 2013;6:168–174. doi: 10.1080/19393210.2013.777946. [DOI] [PubMed] [Google Scholar]
  • 26.Samson RA, Hoekstra ES, Frisvad JC. Introduction to Food and Airborne Fungi. 7th edition. Utrech, The Netherlands: Centraalbureau voor Schimmelcultures; 2004. [Google Scholar]
  • 27.Nelson P, Toussoun T, Marasas W. Fusarium Species: An Illustrated Manual for Identification. University Park, Pa, USA: Pennsylvania State University Press; 1983. [Google Scholar]
  • 28.Simmons E. Alternaria: An Identification Manual. 1st edition. Washington, DC, USA: American Society of Microbiology; 2009. [Google Scholar]
  • 29.Gonzalez HH, Resnik SL, Boca RT, Marasas WF. Mycoflora of Argentinian corn harvested in the main production area in 1990. Mycopathologia. 1995;130(1):29–36. doi: 10.1007/BF01104346. [DOI] [PubMed] [Google Scholar]
  • 30.Pacin AM, González HHL, Etcheverry M, Resnik SL, Vivas L, Espin S. Fungi associated with food and feed commodities from Ecuador. Mycopathologia. 2003;156(2):87–92. doi: 10.1023/a:1022941304447. [DOI] [PubMed] [Google Scholar]
  • 31.Saleemi MK, Khan MZ, Khan A, Javed I. Mycoflora of poultry feeds and mycotoxins producing potential of Aspergillus species. Pakistan Journal of Botany. 2010;42(1):427–434. [Google Scholar]
  • 32.Greco MV, Pardo AG, Ludemann V, Martino PE, Pose GN. Mycoflora and natural incidence of selected mycotoxins in rabbit and chinchilla feeds. The Scientific World Journal. 2012;2012:6 pages. doi: 10.1100/2012/956056.956056 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 33.AOAC. Official Methods of Analysis. 16th edition. Gaithersburg, Md, USA: Association of Official Analytical Chemists; 1997. [Google Scholar]
  • 34.Castillo MD, González HHL, Martínez EJ, Pacin AM, Resnik SL. Mycoflora and potential for mycotoxin production of freshly harvested black bean from the Argentinean main production area. Mycopathologia. 2004;158(1):107–112. doi: 10.1023/b:myco.0000038426.05215.89. [DOI] [PubMed] [Google Scholar]
  • 35.Gimeno A. Los Hongos y las Micotoxinas en la Alimentación Animal; Conceptos, Problemas, Control y Recomendaciones. 2002, http://www.engormix.com/MA-micotoxinas/articulos/criterios-calidad-micologica-t353/p0.htm.
  • 36.Pereyra MLG, Alonso VA, Sager R, et al. Fungi and selected mycotoxins from pre- and postfermented corn silage. Journal of Applied Microbiology. 2008;104(4):1034–1041. doi: 10.1111/j.1365-2672.2007.03634.x. [DOI] [PubMed] [Google Scholar]
  • 37.González Pereyra ML, Pereyra CM, Ramírez ML, Rosa CAR, Dalcero AM, Cavaglieri LR. Determination of mycobiota and mycotoxins in pig feed in central Argentina. Letters in Applied Microbiology. 2008;46(5):555–561. doi: 10.1111/j.1472-765X.2008.02347.x. [DOI] [PubMed] [Google Scholar]
  • 38.Pose GN. Estudio de la biodiversidad de especies de Fusarium contaminantes de trigo y maíz en la provincia de Santa Fe [Ph.D. thesis] Universidad Nacional del Litoral; 2002. [Google Scholar]
  • 39.Oliveira GR, Ribeiro JM, Fraga ME, et al. Mycobiota in poultry feeds and natural occurrence of aflatoxins, fumonisins and zearalenone in the Rio de Janeiro State, Brazil. Mycopathologia. 2006;162(5):355–362. doi: 10.1007/s11046-006-0070-5. [DOI] [PubMed] [Google Scholar]
  • 40.Jaramillo M. Aditividad , Sinergismo y Antagonismo entre Micotoxinas y sus Efectos en Pollos de Engorde. 2006. http://www.engormix.com/MA-avicultura/sanidad/articulos/aditividad-sinergismo-antagonismo-entre-t972/p0.htm. [Google Scholar]
  • 41.Di Constanzo A, Murphy M. St rategies for Feeding Mycotoxin and Mold Contaminated Grains to Cattle. 2012, http://www.extension.umn.edu/agriculture/beef/components/docs/strategies_for_feeding_mycotoxin_and_mold_contaminated_grain.pdf.

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