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      Improved Sample Selection and Preparation Methods for Sampling Plans Used to Facilitate Rapid and Reliable Estimation of Aflatoxin in Chicken Feed

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          Abstract

          Aflatoxin B1 (AFB1), a toxic fungal metabolite associated with human and animal diseases, is a natural contaminant encountered in agricultural commodities, food and feed. Heterogeneity of AFB1 makes risk estimation a challenge. To overcome this, novel sample selection, preparation and extraction steps were designed for representative sampling of chicken feed. Accuracy, precision, limits of detection and quantification, linearity, robustness and ruggedness were used as performance criteria to validate this modification and Horwitz function for evaluating precision. A modified sampling protocol that ensured representativeness is documented, including sample selection, sampling tools, random procedures, minimum size of field-collected aggregate samples (primary sampling), procedures for mass reduction to 2 kg laboratory (secondary sampling), 25 g test portion (tertiary sampling) and 1.3 g analytical samples (quaternary sampling). The improved coning and quartering procedure described herein (for secondary and tertiary sampling) has acceptable precision, with a Horwitz ratio (HorRat = 0.3) suitable for splitting of 25 g feed aliquots from laboratory samples (tertiary sampling). The water slurring innovation (quaternary sampling) increased aflatoxin extraction efficiency to 95.1% through reduction of both bias (−4.95) and variability of recovery (1.2–1.4) and improved both intra-laboratory precision (HorRat = 1.2–1.5) and within-laboratory reproducibility (HorRat = 0.9–1.3). Optimal extraction conditions are documented. The improved procedure showed satisfactory performance, good field applicability and reduced sample analysis turnaround time.

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          Occurrence, Toxicity, and Analysis of Major Mycotoxins in Food

          Mycotoxins are toxic secondary metabolites produced by certain filamentous fungi (molds). These low molecular weight compounds (usually less than 1000 Daltons) are naturally occurring and practically unavoidable. They can enter our food chain either directly from plant-based food components contaminated with mycotoxins or by indirect contamination from the growth of toxigenic fungi on food. Mycotoxins can accumulate in maturing corn, cereals, soybeans, sorghum, peanuts, and other food and feed crops in the field and in grain during transportation. Consumption of mycotoxin-contaminated food or feed can cause acute or chronic toxicity in human and animals. In addition to concerns over adverse effects from direct consumption of mycotoxin-contaminated foods and feeds, there is also public health concern over the potential ingestion of animal-derived food products, such as meat, milk, or eggs, containing residues or metabolites of mycotoxins. Members of three fungal genera, Aspergillus, Fusarium, and Penicillium, are the major mycotoxin producers. While over 300 mycotoxins have been identified, six (aflatoxins, trichothecenes, zearalenone, fumonisins, ochratoxins, and patulin) are regularly found in food, posing unpredictable and ongoing food safety problems worldwide. This review summarizes the toxicity of the six mycotoxins, foods commonly contaminated by one or more of them, and the current methods for detection and analysis of these mycotoxins.
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            Human aflatoxicosis in developing countries: a review of toxicology, exposure, potential health consequences, and interventions.

            Aflatoxins are well recognized as a cause of liver cancer, but they have additional important toxic effects. In farm and laboratory animals, chronic exposure to aflatoxins compromises immunity and interferes with protein metabolism and multiple micronutrients that are critical to health. These effects have not been widely studied in humans, but the available information indicates that at least some of the effects observed in animals also occur in humans. The prevalence and level of human exposure to aflatoxins on a global scale have been reviewed, and the resulting conclusion was that approximately 4.5 billion persons living in developing countries are chronically exposed to largely uncontrolled amounts of the toxin. A limited amount of information shows that, at least in those locations where it has been studied, the existing aflatoxin exposure results in changes in nutrition and immunity. The aflatoxin exposure and the toxic affects of aflatoxins on immunity and nutrition combine to negatively affect health factors (including HIV infection) that account for >40% of the burden of disease in developing countries where a short lifespan is prevalent. Food systems and economics render developed-country approaches to the management of aflatoxins impractical in developing-country settings, but the strategy of using food additives to protect farm animals from the toxin may also provide effective and economical new approaches to protecting human populations.
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              Harmonized guidelines for single-laboratory validation of methods of analysis (IUPAC Technical Report)

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                Author and article information

                Journal
                Toxins (Basel)
                Toxins (Basel)
                toxins
                Toxins
                MDPI
                2072-6651
                16 March 2021
                March 2021
                : 13
                : 3
                : 216
                Affiliations
                [1 ]Biotechnology Research Institute, Kenya Agricultural and Livestock Research Organization, P.O. Box 362, Kikuyu 00902, Kenya; rayelliemdachi@ 123456gmail.com
                [2 ]Department of Biochemistry, Microbiology and Biotechnology, School of Pure and Applied Sciences, Kenyatta University, P.O. Box 43844, Nairobi 00100, Kenya; nmburu01@ 123456gmail.com
                [3 ]Department of Animal Science, School of Agriculture and Enterprise Development, Kenyatta University, P.O. Box 43844, Nairobi 00100, Kenya; munga.leonard@ 123456ku.ac.ke
                [4 ]Department of Biological and Agricultural Engineering, North Carolina State University, Box 7625, Raleigh, NC 27695-7625, USA; whitaker@ 123456ncsu.edu
                [5 ]Hygiena LLC, Santa Ana, CA 92704-6804, USA; thuynh@ 123456hygiena.com
                [6 ]Department of Biosciences, International Livestock Research Institute, P.O. Box 30709, Nairobi 00100, Kenya; D.Randolph@ 123456cgiar.org (D.G.); J.Lindahl@ 123456cgiar.org (J.F.L.)
                [7 ]Department of Clinical Sciences, Swedish University of Agricultural Sciences, 75007 Uppsala, Sweden
                [8 ]Department of Medical Biochemistry and Microbiology, Uppsala University, 75123 Uppsala, Sweden
                Author notes
                [* ]Correspondence: jkkibugu1@ 123456yahoo.com
                Author information
                https://orcid.org/0000-0003-2724-4868
                https://orcid.org/0000-0002-0102-6291
                https://orcid.org/0000-0002-1175-0398
                Article
                toxins-13-00216
                10.3390/toxins13030216
                8002447
                fcefd0d9-7184-4966-8f85-c80b1023e551
                © 2021 by the authors.

                Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license ( http://creativecommons.org/licenses/by/4.0/).

                History
                : 15 January 2021
                : 10 March 2021
                Categories
                Article

                Molecular medicine
                aflatoxin,chicken feed,representative sampling,improved aflatoxin test procedure,validation

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