Your search keyword '"Hagler WM Jr"' showing total 61 results

1. Dietary exposure of broiler breeders to aflatoxin results in immune dysfunction in progeny chicks

Author

Qureshi, MA, Brake, J, Hamilton, PB, Hagler, WM, Jr, and Nesheim, S

Published

1998

2. T-2 tetraol is cytotoxic to a chicken macrophage cell line

Author

Kidd, MT, Qureshi, MA, Hagler, WM, Jr, and Ali, R

Published

1997

3. Predicting aflatoxin and fumonisin in shelled corn lots using poor-quality grade components.

Author

Johansson AS, Whitaker TB, Hagler WM Jr, Bowman DT, Slate AB, and Payne G

Subjects

Algorithms, Quality Control, Aflatoxins analysis, Fumonisins analysis, Mycotoxins analysis, Zea mays chemistry

Abstract

A study was conducted to determine if aflatoxin and fumonisin are concentrated in the poor-quality grade components of shelled corn. Four 1.0 kg test samples were each taken from 23 lots of shelled corn marketed in North Carolina. Inspectors from the Federal Grain Inspection Service divided each test sample into 3 grade components: (1) damaged kernels (DM), (2) broken corn and foreign material (BCFM), and )3) whole kernels (WH). The aflatoxin and fumonisin concentration was measured in each component and a mass balance equation was used to calculate the total concentration of each mycotoxin in each test sample. Averaged across all test samples, the aflatoxin concentrations in the DM, BCFM, and WH components were 1300.3, 455.2, and 37.3 ppb, respectively. Averaged across all test samples, the fumonisin concentrations in the DM, BCFM, and WH components were 148.3, 51.3, and 1.8 ppm, respectively. The DM and BCFM components combined accounted for only 5.0% of the test sample mass, but accounted for 59.8 and 77.5% of the total aflatoxin and fumonisin mass in the test sample, respectively. Both aflatoxin mass (ng) and aflatoxin concentration (ng/g) in the combined DM and BCFM components had high correlations with aflatoxin concentration in the lot. The highest correlation occurred when aflatoxin mass (ng) in the combined DM and BCFM components was related to aflatoxin concentration in the lot (0.964). Similar results were obtained for fumonisin. This study indicated that measuring either aflatoxin or fumonisin in the combined DM and BCFM grade components could be used as a screening method to predict either aflatoxin or fumonisin in a bulk lot of shelled corn.

Published

2006

4. Aflatoxin binders II: reduction of aflatoxin M1 in milk by sequestering agents of cows consuming aflatoxin in feed.

Author

Diaz DE, Hagler WM Jr, Blackwelder JT, Eve JA, Hopkins BA, Anderson KL, Jones FT, and Whitlow LW

Subjects

Aflatoxin B1 metabolism, Animals, Cattle, Dairying, Lactation, Zea mays chemistry, Aflatoxin M1 metabolism, Animal Feed, Bentonite metabolism, Food Contamination, Milk chemistry

Abstract

Sequestering agents bind dietary aflatoxin B1 (AFB1) and reduce absorption from an animal's gastrointestinal tract. As a result, they protect an animal from the toxic effects of AFB1 and reduce transfer of the metabolite, aflatoxin M1 (AFM1), into milk. Three experiments, using late-lactation Holstein cows fed AFB1-contaminated feed, were conducted to evaluate several potential sequestering agents for their abilities to prevent or reduce the transmission of AFM1 into milk. Six agents previously tested in our laboratory for AFB1 binding in vitro were evaluated in these experiments. These were: SA-20, an activated carbon (AC-A); Astra-Ben-20, a sodium bentonite (AB-20); MTB-100, an esterified glucomannan (MTB-100); Red Crown, a calcium bentonite (RC); Flow Guard, a sodium bentonite (FG); and Mycrosorb, a sodium bentonite (MS). Five of the six sequestering agents significantly (P < 0.01) reduced AFM1 contamination of milk (AB-20, 61%; FG, 65%; MS, 50%; MTB-100, 59%; and RC, 31%); whereas, AC-A, activated carbon, had no effect on AFM1 transmission at 0.25% of feed. By the first milking (1 day after cows consumed contaminated feed), AFM1 appeared in milk, then reached maximum levels after three days, and was absent from milk within four days after AFB1 was removed from the feed. Sodium bentonites at 1.2% of feed showed good potential as AFB1 binders; MTB-100, a yeast cell wall product, was equally effective at 0.05% in feed. Potential AFB1 binding agents should be evaluated experimentally to demonstrate efficacy. Our data show that sequestering agents can reduce AFM1 in milk of cows fed AFB1-contaminated feed.

Published

2004

5. Effect of fermentation on Sweetpotato (Ipomoea batatas) toxicity in mice.

Author

Thibodeau MS, Poore MH, Hagler WM Jr, and Rogers GM

Subjects

Animals, Chemical and Drug Induced Liver Injury, Fusarium, Kidney Diseases chemically induced, Kidney Diseases pathology, Liver Diseases pathology, Lung Diseases chemically induced, Lung Diseases pathology, Male, Mice, Plant Extracts administration & dosage, Plant Extracts chemistry, Sesquiterpenes, Terpenes administration & dosage, Terpenes toxicity, Phytoalexins, Fermentation, Ipomoea batatas chemistry, Plant Extracts toxicity

Abstract

Unfortunate bovine fatalities occurring after ingestion of mold-damaged sweetpotatoes preclude the use of the culled tubers in livestock feed. In cattle, mold-damaged sweetpotatoes induce an acute respiratory distress syndrome resulting in asphyxiation. Because of this potential toxicity and the general abundance of culled sweetpotatoes, the detoxification efficacy of ensiling was explored since it is an easy and economically viable technique often applied to preserve livestock feed. Sweetpotato slices with or without mold damage were stored either frozen (to represent unfermented samples) or fermented for 6 weeks at room temperature. Following fermentation, organic extracts were generated for administration to mice. Thirty hours following administration of the extracts, mice were evaluated for gross and microscopic lesions affecting the lungs, liver, and kidneys. Fermentation of 6 weeks duration was observed to inadequately eliminate the lung, liver, and kidney toxicity caused by mold-damaged sweetpotatoes. In fact, fermentation exacerbated the hepatotoxicity of mold-damaged sweetpotatoes. This is also the first demonstration that sweetpotato regions lacking visible mold damage can induce lung and kidney injury, which, however, is preventable by fermentation.

Published

2004

6. Aflatoxin binders I: in vitro binding assay for aflatoxin B1 by several potential sequestering agents.

Author

Diaz DE, Hagler WM Jr, Hopkins BA, and Whitlow LW

Subjects

Hydrogen-Ion Concentration, Solutions, Aflatoxin B1 chemistry, Bentonite chemistry, Charcoal chemistry, Mannans chemistry

Abstract

Nine potential proprietary sequestering agents consisting of 4 activated charcoals, 3 sodium bentonites, a calcium bentonite, and an esterified glucomannan were compared in a novel in vitro assay for aflatoxin B1 (AFB1) binding. Agents were evaluated in 10% methanol prepared as 1% stirred suspensions at pH 3, 7, 10 and pH-unadjusted, with or without AFB1 at 5 microg/ml. All nine agents bound more than 95% of the 5 microg of AFB1 in solution, regardless of pH. The sodium bentonites bound 98, 95, and 98% of the AFB1. The four activated charcoals bound over 99%, the calcium bentonite bound 98%, and the esterified glucomannan bound 97% of the AFB1 in solution. The results suggested that the sequestering agents tested here had sufficient potential to bind AFB1 at pH values commonly found in the gastrointestinal tracts of ruminants and other animals.

Published

2002

7. Sampling wheat for deoxynivalenol.

Author

Whitaker TB, Hagler WM Jr, Giesbrecht FG, and Johansson AS

Subjects

Algorithms, Analysis of Variance, Calibration, Quality Control, Reproducibility of Results, Trichothecenes analysis, Triticum chemistry

Abstract

The variability associated with testing wheat for deoxynivalenol (DON) was measured using a 0.454 kg sample, a Romer mill, 25 g of comminuted subsample and the Romer Fluoroquant analytical method. The total variability was partitioned into sampling, sample preparation, and analytical variability components. Each variance component was found to be a function of the DON concentration and equations were developed to predict each variance component using regression techniques. The effects of sample size, subsample size, and number of aliquots on reducing the variability of the DON test procedure were also determined. Using the test procedure described above, the coefficient of variation (CV) associated with testing wheat at 5 ppm DON was found to be 13.4%. The CVs associated with sampling, sample preparation, and analysis were 6.3, 10.0, and 6.3%, respectively. The sample variations associated with testing wheat are relatively small when compared to CVs associated with testing other commodities for other mycotoxins such as aflatoxin in peanuts. Even with the use of a small sample size (0.454 kg), the sampling variation was not the largest source of error as found in other mycotoxin test procedures.

Published

2002

8. Distribution among sample test results when testing shelled corn lots for fumonisin.

Author

Whitaker TB, Hagler WM Jr, Johansson AS, Giesbrecht FG, and Trucksess MW

Subjects

Chromatography, Liquid, Regression Analysis, Statistics as Topic, Carboxylic Acids analysis, Food Contamination statistics & numerical data, Fumonisins, Mycotoxins analysis, Zea mays chemistry

Abstract

The statistical distribution known as the compound gamma function was studied for suitability in describing the distribution of sample test results associated with testing lots of shelled corn for fumonisin. Thirty-two 1.1 kg test samples were taken from each of 16 contaminated lots of shelled corn. An observed distribution consisted of 32 sample fumonisin test results for each lot. The mean fumonisin concentration, c, and the variance, s2, among the 32 sample fumonisin test results along with the parameters for the compound gamma function were determined for each of the 16 observed distributions. The 16 observed distributions of sample fumonisin test results were compared with the compound gamma function using the Power Divergence test. The null hypothesis that the observed distribution could have resulted from sampling a family of compound gamma distributions was not rejected at the 5% significance level for 15 of the 16 lots studied. Parameters of the compound gamma distribution were calculated from the 32-fumonisin sample test results using the method of moments. Using regression analysis, equations were developed that related the parameters of the compound gamma distribution to fumonisin concentration and the variance associated with a fumonisin test procedure. An operating characteristic curve was developed for a fumonisin sampling plan to demonstrate the use of the compound gamma function.

Published

2001

9. Cytosol is required for the modulation by dietary casein of the hepatic microsomal activation of aflatoxin B1 to mutagenic metabolites detectable in Salmonella.

Author

Woodall GM Jr, Dauterman WC, Hagler WM Jr, and DeMarini DM

Subjects

Animals, Biotransformation drug effects, Caseins administration & dosage, Chromatography, High Pressure Liquid, Cytochrome P-450 Enzyme Inhibitors, Cytosol metabolism, Enzyme Inhibitors pharmacology, Glutathione pharmacology, Liver drug effects, Liver enzymology, Liver metabolism, Male, Microsomes, Liver enzymology, Microsomes, Liver metabolism, Mutagenicity Tests, Rats, Rats, Inbred F344, Serum Albumin, Bovine pharmacology, Spectrometry, Fluorescence, Aflatoxin B1 pharmacokinetics, Caseins metabolism, Cytosol drug effects, Microsomes, Liver drug effects, Mutagens pharmacokinetics, Salmonella metabolism

Abstract

We have shown previously that dietary protein (casein) levels can affect the ability of rat liver S9 to metabolize aflatoxin B1 (AFB) as well as other promutagens detectable in Salmonella strain TA98 [Mutat. Res. (1997), 360, 115-126 and 127-143]. The mutagenic potency of AFB was greatest when metabolized by the Aroclor 1254-induced hepatic S9 prepared from F344 male rats that consumed an isocaloric, semisynthetic diet for 6 weeks that contained an adequate (12%) level of methionine-supplemented casein as the sole protein source, compared with S9s from rats fed diets that contained nominally deficient (8%) or high (22%) levels of casein. Here we have extended this observation by performing (i) mutagenicity studies with microsomes, cytosols and reconstituted S9s (recombinations of microsomes and cytosols across dietary groups), and (ii) in vitro incubations followed by analysis of metabolites by fluorescence high-pressure liquid chromatography. Microsomes, but not cytosols, activated AFB; however, activation to the level observed with S9 occurred only when microsomes from the rats fed 12% casein were combined with cytosols from any dietary group. Consistent with the mutagenicity results, the greatest metabolism of the AFB parent compound and the highest level of the glutathione conjugate of the presumptively identified AFB-exo-8,9-epoxide (the ultimate mutagenic form of AFB) were produced by S9s from the rats fed the 12% casein diet. The levels of these metabolites and the mutagenicity of AFB changed in parallel with changes in dietary casein levels. In summary, cytosolic elements, which are not affected by dietary casein levels, interact with microsomal enzymes, which are modulated by dietary casein levels, to influence the ability of hepatic S9 to activate AFB to a mutagen.

Published

1999

10. Performance of sampling plans to determine aflatoxin in farmers' stock peanut lots by measuring aflatoxin in high-risk-grade components.

Author

Whitaker TB, Hagler WM Jr, and Giesbrecht FG

Subjects

Agriculture, Chromatography, High Pressure Liquid, Food Contamination, Regression Analysis, Aflatoxins analysis, Arachis chemistry, Quality Control

Abstract

Five 2 kg test samples were taken from each of 120 farmers' stock peanut lots contaminated with aflatoxin. Kernels from each 2 kg sample were divided into the following U.S. Department of Agriculture grade components: sound mature kernels plus sound splits (SMKSS), other kernels (OK), loose shelled kernels (LSK), and damaged kernels (DAM). The kernel mass (g), aflatoxin mass (ng), and aflatoxin concentration (ng of aflatoxin/g of peanuts) were measured for each of the 2400 component samples. The variabilities associated with measuring aflatoxin mass (ng) in OK + LSK + DAM, or A(OLD)ng, and in LSK + DAM, or A(LD)ng, and aflatoxin concentration (ng/g) in OK + LSK + DAM, or A(OLD)ng/g, and in LSK + DAM, or A(LD)ng/g, were determined. The variance associated with measuring aflatoxin in each of the 4 combinations of components increased with aflatoxin, and functional relationships were developed from regression analysis. The variability associated with estimating the lot concentration from each of the 4 combinations of components was also determined. The coefficients of variation (CV) associated with estimating the aflatoxin for a lot with aflatoxin at 100 ng/g were 90, 86, 94 and 96% for aflatoxin masses A(OLD)ng and A(LD)ng and aflatoxin concentrations A(OLD)ng/g and A(LD)ng/g, respectively. The performance of aflatoxin sampling plans using the combination of aflatoxin masses in OK + LD + DAM and LD + DAM components was evaluated with a 2 kg test sample and a 50 ng/g accept/reject limit.

Published

1999

11. Variability associated with testing shelled corn for fumonisin.

Author

Whitaker TB, Trucksess MW, Johansson AS, Giesbrecht FG, Hagler WM Jr, and Bowman DT

Subjects

Food Analysis statistics & numerical data, Regression Analysis, Reproducibility of Results, Carboxylic Acids analysis, Food Analysis methods, Fumonisins, Zea mays chemistry

Abstract

Variances associated with sampling, sample preparation, and analytical steps of a test procedure that measures fumonisin in shelled corn were estimated. The variance associated with each step of the test procedure increases with fumonisin concentration. Functional relationships between variance and fumonisin concentration were estimated by regression analysis. For each variance component, functional relationships were independent of fumonisin type (total, B1, B2, and B3 fumonisins). At 2 ppm, coefficients of variation associated with sampling (1.1 kg sample), sample preparation (Romer mill and 25 g subsample), and analysis are 16.6, 9.1, and 9.7%, respectively. The coefficient of variation associated with the total fumonisin test procedure was 45% and is about the same order of magnitude as that for measuring aflatoxin in shelled corn with a similar test procedure.

Published

1998

12. Estimating aflatoxin in farmers' stock peanut lots by measuring aflatoxin in various peanut-grade components.

Author

Whitaker TB, Hagler WM Jr, Giesbrecht FG, Dorner JW, Dowell FE, and Cole RJ

Subjects

Product Surveillance, Postmarketing, Regression Analysis, Aflatoxins analysis, Arachis chemistry, Drug Residues analysis

Abstract

Five, 2 kg test samples were taken from each of 120 farmers' stock peanut lots contaminated with aflatoxin. Kernels from each 2 kg sample were divided into the following grade components: sound mature kernels plus sound splits (SMKSS), other kernels (OK), loose shelled kernels (LSK), and damaged kernels (DAM). Kernel mass, aflatoxin mass, and aflatoxin concentration were measured for each of the 2400 component samples. For 120 lots tested, average aflatoxin concentrations in SMKSS, OK, LSK, and DAM components were 235, 2543, 11,775, and 69,775 ng/g, respectively. Aflatoxins in SMKSS, OK, LSK, and DAM components represented 6.9, 7.9, 33.3, and 51.9% of the total aflatoxin mass, respectively. Cumulatively, 3 aflatoxin risk components--OK, LSK, and DAM--accounted for 93.1% of total aflatoxin, but only 18.4% percent of test sample mass. Correlation analysis suggests that the most accurate predictor of aflatoxin concentration in the lot is the cumulative aflatoxin mass in the high 3 risk components OK + LSK + DAM (correlation coefficient, r = 0.996). If the aflatoxin in the combined OK + LSK + DAM components is expressed in concentration units, r decreases to 0.939. Linear regression equations relating aflatoxin in OK + LSK + DAM to aflatoxin concentration in the lot were developed. The cumulative aflatoxin in the OK + LSK + DAM components was not an accurate predictor (r = 0.539) of aflatoxin in the SMKSS component. Statistical analyses of 3 other data sets published previously yielded similar results.

Published

1998

13. Degradation of aflatoxin by poultry litter.

Author

Jones FT, Wineland MJ, Parsons JT, and Hagler WM Jr

Subjects

Aflatoxins analysis, Animals, Biodegradation, Environmental, Temperature, Water, Aflatoxins metabolism, Chickens, Manure, Turkeys, Zea mays chemistry

Abstract

Two trials were conducted to determine whether deep stacking of contaminated corn with poultry litter destroys aflatoxin. Contaminated corn was ground and mixed with litter to carbon:nitrogen ratios of 30:1. Moistures were adjusted by adding tap water just prior to incubation or stacking. The initial laboratory trial included only broiler litter at 40% moisture, whereas the subsequent field trial involved a 2 x 2 factorial design with litter type (turkey or broiler) and moisture (20 or 40%) as main effects. Aflatoxin assays were reduced in the laboratory trial from 433 and 402 to 54 and 8 ppb in Containers 1 and 2, respectively, after 35 d of incubation at 28 C. In the field trial, aflatoxin disappeared from broiler and turkey litter mixtures with projected moistures of 20% after 10 and 6 wk of storage, respectively, whereas disappearance in mixtures containing projected moistures of 40% required 5 and 3 wk, respectively. Differences in moisture appear to account for differences in the ability of turkey and broiler litter to detoxify aflatoxin. Hence, turkey and broiler litter would appear equal with respect to the ability to detoxify aflatoxin-contaminated corn. Disappearance of aflatoxin during storage with litter could have occurred as a result of ammonia release during storage or microbial detoxification mechanisms. However, nitrogen values suggest that microbial action was responsible for much of the detoxification, as aflatoxin disappeared from mixtures with little apparent ammonia release.

Published

1996

14. Endocrine and metabolic response to muscarinic stimulation and inhibition in the ruminant: effects of slaframine.

Author

Chapa AM, Fernandez JM, Thompson DL Jr, Tempelman RJ, Berrio LF, Croom WJ Jr, and Hagler WM Jr

Subjects

Alkaloids administration & dosage, Animals, Blood Glucose analysis, Endocrine Glands drug effects, Fatty Acids, Nonesterified blood, Female, Goat Diseases blood, Goat Diseases chemically induced, Goats blood, Growth Hormone blood, Hyperglycemia blood, Hyperglycemia chemically induced, Hyperglycemia veterinary, Hyperinsulinism blood, Hyperinsulinism chemically induced, Hyperinsulinism veterinary, Injections, Intravenous veterinary, Insulin blood, Male, Muscarinic Agonists administration & dosage, Muscarinic Antagonists administration & dosage, Parasympathomimetics administration & dosage, Parasympathomimetics pharmacology, Piperidines administration & dosage, Receptors, Muscarinic drug effects, Thyroxine blood, Triiodothyronine blood, Alkaloids pharmacology, Endocrine Glands physiology, Goats physiology, Muscarinic Agonists pharmacology, Muscarinic Antagonists pharmacology, Piperidines pharmacology, Receptors, Muscarinic physiology

Abstract

The influence of slaframine (SF), a parasympathomimetic compound isolated from the fungus Rizoctonia leguminicola, on circulating metabolic hormone concentrations was investigated in goats. In Exp. 1, SF was administered i.v. at 0 (CONT), 50 (LSF), 100 (MSF), or 150 (HSF) microgram/kg.75 BW in four mature Spanish-cross does (average BW 36 +/- 7 kg) fitted with indwelling jugular vein catheters in a 4 x 4 Latin square design. Plasma glucose peaked (P < .06) at 120 min with LSF and at 180 min with HSF and was higher (P <.06) than the CONT at these times. Glucose exhibited a quadratic response (P < .03) to SF. Area under the response curve for glucose differed (P < .02) in HSF from CONT and MSF. Insulin peaked (P < .01) at 240 min with MSF and at 180 min with HSF. Plasma triiodothyronine was maintained at a higher level (P < .03) with HSF. Thyroxine peaked (P < .06) at 120 min with MSF and 300 min with HSF. Plasma NEFA and somatotropin concentrations were not affected (P > .10) by SF. In Exp. 2, four mature Spanish-cross wethers (average BW 27 +/- 2 kg) fitted with jugular vein catheters were administered SF (0 and 114 micrograms/kg.75 BW) and 4-diphenylacetoxy-N-methylpiperidine methiodide (4DAMP; 0 and 258 micrograms/kg.75 BW), a M3-muscarinic receptor antagonist, i.v. in a 4 x 4 Latin square design with a 2 x 2 factorial arrangement of treatments. With SF, glucose peaked (P < .06) at 60 min and insulin peaked (P < .05) at 180 min. Plasma triiodothyronine levels were maintained (P < .05) with SF but declined with other treatments. Plasma NEFA and thyroxine concentrations remained unchanged regardless of treatment. Slaframine administration induced hyperglycemia and hyperinsulinemia in goats; however, these changes were blocked by preadministration of isomolar quantities of the M3-muscarinic receptor antagonist, 4DAMP.

Published

1995

15. Fusarium proliferatum culture material alters several production and immune performance parameters in White Leghorn chickens.

Author

Qureshi MA, Garlich JD, Hagler WM Jr, and Weinstock D

Subjects

Animals, Antibody Formation drug effects, Body Weight drug effects, Chickens, Cyclobutanes toxicity, Female, Macrophages drug effects, Macrophages physiology, Male, Organ Size drug effects, Sheep, Fumonisins, Fusarium pathogenicity, Immunity drug effects, Mycotoxins toxicity

Abstract

White Leghorn Cornell K-strain chicks (3 replicates of 16 per pen) were started at Day 7 on feed amended with Fusarium proliferatum culture material containing fumonisin B1, fumonisin B2, and moniliformin at 61, 10.5, and 42.7 ppm, respectively. Observed effects on performance of treated birds included reduced feed conversion at 2 wk, and reduced body weight of males and females up to 6 wk (P < or = .05). Splenic, thymic, and liver weights, normalized for body weight, were reduced (P < or = .05) with no change in bursa of Fabricius. No significant changes were observed histologically in the spleen, bursa, kidney, heart, liver, cecal tonsils, colon, or tibia. Significant suppression in total Ig and IgG levels occurred. Macrophages from treated chicks exhibited a 34% reduction in phagocytic activity. Natural killer cell activity was not affected. These findings, which showed that Fusarium toxins alter performance and immune end points in chickens, imply that chickens exposed to mycotoxins may be more susceptible to infectious diseases.

Published

1995

16. Influence of duodenal slaframine infusion on site of nutrient disappearance from the digestive tract of steers fed a high-concentrate diet.

Author

Streeter MN, Froetschel MA, Croom WJ Jr, and Hagler WM Jr

Subjects

Alkaloids administration & dosage, Ammonia analysis, Animals, Catheterization methods, Catheterization veterinary, Cattle metabolism, Diet standards, Digestion physiology, Duodenum physiology, Fermentation, Hydrogen-Ion Concentration, Ileum physiology, Male, Nitrogen analysis, Parasympathomimetics administration & dosage, Random Allocation, Rumen chemistry, Rumen physiology, Starch metabolism, Alkaloids pharmacology, Cattle physiology, Diet veterinary, Digestion drug effects, Parasympathomimetics pharmacology

Abstract

The effect of duodenal slaframine (SF) infusion on site and extent of digestion was determined using four steers equipped with ruminal, duodenal, and ileal cannulas in a 4 x 4 Latin square. A 77% dry-rolled corn diet was provided in 12 equal portions daily at a DMI of 2.26% BW. Slaframine in a .9% saline excipient was infused into the duodenum every 12 h with total daily dose of 0, 30, 60, or 90 micrograms /kg of BW. Slaframine infusion had no effect on ruminal pH, ruminal NH3 N, or solids and liquids passage rate. Slaframine increased (linear, P < .10) total tract OM and starch disappearance and digestibility and tended to increase (linear, P = .14) total tract N digestibility. Ruminal starch disappearance tended to be decreased (quadratic, P = .16) by SF. Small intestinal OM digestibility was increased (linear, P < .10) but starch digestibility in the small intestine was not affected by SF. Increased total tract starch digestibility was caused by increased (quadratic, P < .10) starch fermentation in the large intestine. Ruminal feed N digestibility decreased at the intermediate doses of SF (quadratic, P < .10). Total N digestibility in the small intestine tended to be increased (cubic, P = .13) with 30 and 90 micrograms of SF/kg of BW. Decreased ruminal feed N digestion was compensated for by increased (quadratic, P < .10) small intestinal feed N disappearance for steers treated with intermediate doses of SF. The potential of SF to increase starch digestion in the rumen and small intestine seems to be limited.

Published

1995

17. Trichothecene mycotoxins depress the mononuclear-phagocytic system of young turkeys.

Author

Kidd MT, Hagler WM Jr, and Qureshi MA

Subjects

Animals, Cells, Cultured, T-2 Toxin analogs & derivatives, T-2 Toxin toxicity, Turkeys, Leukocytes, Mononuclear drug effects, Phagocytosis drug effects, Trichothecenes toxicity

Abstract

Macrophage cells isolated from the abdominal cavity of 21-day-old turkeys after a single injection of Sephadex suspension were used to quantitate the effects of direct in vitro exposure to deoxynivalenol (DON), 3-acetyldeoxynivalenol (3ac-DON), scirpentriol (STO), or 15-acetylscirpenol (15-MAS). Macrophage monolayers were established on glass surfaces and cells were exposed to graded levels of individual mycotoxins for 1 hour: DON, 20-640 micrograms/microliters of culture; 3ac-DON, STO, 15-MAS, 20-1280 micrograms/microliters of culture. All four mycotoxins caused dose-related effects. A concentration of 50 micrograms/microliter DON caused a significant decrease in macrophage adherence, phagocytosis of opsonized SRBC, and number of opsonized SRBC per macrophage; at 200 micrograms/microliter, phagocytosis of unopsonized SRBC was decreased. There were also increasing percentages of damaged macrophages with increasing DON doses as indicated by morphological alterations. Linear decreases in macrophage viability on exposure to 3-acDON and STO were observed. Moreover, STO and 15-MAS decreased macrophage adherence to glass and 3-acDON, STO, and 15-MAS induced macrophage morphological alterations. This study suggests that trichothecene mycotoxins may be immunosuppressive by affecting viability, adherence and phagocytic potential of mononuclear phagocytic cells of young turkeys.

Published

1995

18. The involvement of slaframine and swainsonine in slobbers syndrome: a review.

Author

Croom WJ Jr, Hagler WM Jr, Froetschel MA, and Johnson AD

Subjects

Alkaloids chemistry, Animals, Cattle, Cattle Diseases physiopathology, Central Nervous System physiology, Mycotoxicosis etiology, Mycotoxicosis physiopathology, Parasympathomimetics chemistry, Poaceae microbiology, Rhizoctonia isolation & purification, Salivation physiology, Sialorrhea etiology, Sialorrhea physiopathology, Swainsonine chemistry, Syndrome, Alkaloids pharmacology, Cattle Diseases etiology, Mycotoxicosis veterinary, Parasympathomimetics pharmacology, Sialorrhea veterinary, Swainsonine pharmacology

Abstract

The history of "slobbers syndrome," a mycotoxicosis associated with Rhizoctonia leguminicola infestation of pastures and stored forages, is discussed. The chemistry and physiological effects of the two known biologically active alkaloids of R. leguminicola, slaframine and swainsonine, are described. Slaframine administration is generally associated with increased exocrine function, especially salivation. Ingestion of swainsonine may be linked to serious and potentially lethal central nervous system defects similar to that described for locoism. However, the singular effects of these alkaloids do not completely account for the total clinical picture noted in the field during the occurrence of slobbers syndrome. It is possible that this phenomenon is the result of an interaction between both known and unidentified biologically active metabolites of R. leguminicola.

Published

1995

19. The effect of slaframine on salivary output and subacute and acute acidosis in growing beef steers.

Author

Hibbard B, Peters JP, Chester ST, Robinson JA, Kotarski SF, Croom WJ Jr, and Hagler WM Jr

Subjects

Acidosis drug therapy, Acidosis physiopathology, Acute Disease, Alkaloids therapeutic use, Animals, Cattle physiology, Cattle Diseases drug therapy, Dose-Response Relationship, Drug, Hydrogen-Ion Concentration, Lactates analysis, Male, Parasympathomimetics therapeutic use, Random Allocation, Rumen chemistry, Rumen physiology, Salivary Glands drug effects, Salivary Glands physiology, Salivation physiology, Acidosis veterinary, Alkaloids pharmacology, Cattle growth & development, Cattle Diseases physiopathology, Parasympathomimetics pharmacology, Salivation drug effects

Abstract

Experiments were conducted to determine 1) the effect of injecting slaframine (SF) on salivary output in growing beef steers and 2) whether increased salivary output after SF injection would inhibit the decrease in ruminal pH that occurs after experimentally induced subacute and acute ruminal acidosis. In Exp. 1 and 2, we measured ruminal pH and salivary output in ruminally and esophageally cannulated beef steers fed an 88% concentrate diet. Injections of 66 or 100 micrograms of SF/kg BW increased salivary flow approximately 50% compared with controls. Those doses were tested in subacute and acute acidosis models using ruminally cannulated beef steers in Exp. 3 and 4, respectively. In these experiments, salivation was assessed indirectly using a visual scoring system. In the subacute acidosis model, SF reduced (P < .10) the decrease in ruminal pH (1.1, .7, and .6 pH units for control, 66, and 100 micrograms of SF/kg BW doses, respectively), and excessive salivation was observed in all SF-injected steers. In the acute acidosis model, there were no differences (P > .10) in ruminal pH at 12 h after injection between control and SF-treated steers. Mean ruminal lactate concentrations for all treatment groups were between 87 and 112 mM. Although treatment with 66 micrograms of SF/kg BW reduced (P < .10) ruminal lactate concentrations, all ruminal lactate concentrations were indicative of acute acidosis. These results indicate that SF will reduce the decrease in ruminal pH associated with subacute acidosis in growing beef steers, but SF does not attenuate acute ruminal acidosis.

Published

1995

20. Fusaric acid in Fusarium moniliforme cultures, corn, and feeds toxic to livestock and the neurochemical effects in the brain and pineal gland of rats.

Author

Porter JK, Bacon CW, Wray EM, and Hagler WM Jr

Subjects

Animal Feed analysis, Animal Feed toxicity, Animals, Brain metabolism, Chromatography, High Pressure Liquid, Culture Media, Dopamine metabolism, Dopamine beta-Hydroxylase antagonists & inhibitors, Food Microbiology, Fusaric Acid administration & dosage, Fusaric Acid analysis, Gas Chromatography-Mass Spectrometry, Hydroxyindoleacetic Acid metabolism, Hydroxytryptophol metabolism, Injections, Intraperitoneal, Male, Mycotoxins administration & dosage, Mycotoxins analysis, Norepinephrine metabolism, Pineal Gland metabolism, Poultry, Rats, Rats, Sprague-Dawley, Serotonin analogs & derivatives, Serotonin metabolism, Tyrosine metabolism, Zea mays metabolism, Zea mays microbiology, Brain drug effects, Fusaric Acid toxicity, Fusarium metabolism, Mycotoxins toxicity, Pineal Gland drug effects

Abstract

Fusaric acid is produced by several species of Fusarium, which commonly infect corn and other agricultural commodities. Since this mycotoxin may augment the effects of other Fusarium toxins, a gas chromatography/mass spectrometry method of analysis in feeds was developed. Fusaric acid was analyzed as the trimethylsilyl-ester from F. moniliforme-cultures, -contaminated corn screenings, and feeds toxic to livestock. The mycotoxin was found in all samples and ranged from 0.43 to 12.39 micrograms/g sample. Also, fusaric acid was tested for its neurochemical effects in the brain and pineal gland of rats. Animals were dosed intraperitoneally (100 mg/kg body weight) 30 min prior to the onset of the dark phase (lights out) and the effects were studied at 1.5, 3.5, and 5.5 h after treatment. Brain serotonin (5HT), 5-hydroxyindoleacetic acid (5HIAA), tyrosine (TYRO), and dopamine (DA) were increased (P < 0.05) by fusaric acid, and norepinephrine (NEpi) was decreased (P < 0.05). Analogously, DA in the pineal gland increased and NEpi decreased (P < 0.05). Pineal N-acetylserotonin (NAc5HT) was increased (P < 0.05), whereas pineal 5HT and its two major metabolites 5HIAA and 5-hydroxytryptophol (5HTOL) decreased (P < 0.05). Elevated brain TYRO and brain and pineal DA, with decreased NEpi, may be consistent with fusaric acid's partial inhibitory effect on tyrosine-hydroxylase and its inhibitory effect on dopamine-beta-hydroxylase, respectively. Elevated pineal Nac5HT is consistent with decreased pineal 5HT and the increased pineal DA, and support the dopaminergic stimulatory activity of the enzyme responsible for the conversion of 5HT to NAc5HT. This is the first report of fusaric acid's in vivo effect on pineal DA, NEpi, 5HT, and NAc5HT in rats, and a relation for the effects on TYRO, 5HT, and 5HIAA in brain tissue. The results indicate fusaric acid alters brain and pineal neurotransmitters and may contribute to the toxic effects of Fusarium-contaminated feeds.

Published

1995

21. Predicting the distribution of aflatoxin test results from farmers' stock peanuts.

Author

Whitaker TB, Giesbrecht FG, Wu J, Hagler WM Jr, and Dowell FE

Subjects

Agriculture, Mathematics, Regression Analysis, Aflatoxins analysis, Arachis chemistry, Food Contamination

Abstract

Suitability of the negative binomial function for use in estimating the distribution of sample aflatoxin test results associated with testing farmers' stock peanuts for aflatoxin was studied. A 900 kg portion of peanut pods was removed from each of 40 contaminated farmers' stock lots. The lots averaged about 4100 kg. Each 900 kg portion was divided into fifty 2.26 kg samples, fifty 4.21 kg samples, and fifty 6.91 kg samples. The aflatoxin in each sample was quantified by liquid chromatography. An observed distribution of sample aflatoxin test results consisted of 50 aflatoxin test results for each lot and each sample size. The mean aflatoxin concentration, m; the variance, S2 mean among the 50 sample aflatoxin test results; and the shape parameter, k, for the negative binomial function were determined for each of the 120 observed distributions (40 lots times 3 sample sizes). Regression analysis indicated the functional relationship between k and m to be k = 0.000006425m0.8047. The 120 observed distributions of sample aflatoxin test results were compared to the negative binomial function by using the Kolmogorov-Smirnov (KS) test. The null hypothesis that the true unknown distribution function was negative binomial was not rejected at the 5% significance level for 114 of the 120 distributions. The negative binomial function failed the KS test at a sample concentration of 0 ng/g in all 6 of the distributions where the negative binomial function was rejected. The negative binomial function always predicted a smaller percentage of samples testing 0 ng/g than was actually observed.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1994

22. Effects of slaframine and 4-diphenylacetoxy-N-methylpiperidine methiodide (4DAMP) on pancreatic exocrine secretion in the bovine.

Author

Walker JA, Krehbiel CR, Harmon DL, St Jean G, Croom WJ Jr, and Hagler WM Jr

Subjects

Animals, Cattle, Chymotrypsin metabolism, Hydrogen-Ion Concentration, Male, Pancreas drug effects, Pancreas enzymology, Pancreatic Juice metabolism, Proteins metabolism, alpha-Amylases metabolism, Alkaloids pharmacology, Muscarinic Antagonists, Pancreas metabolism, Parasympatholytics pharmacology, Parasympathomimetics pharmacology, Piperidines pharmacology

Abstract

Three Holstein steers (345 +/- 22 kg) surgically fitted with a pancreatic cannula were used in two 3 x 3 Latin square design experiments to examine the effects of slaframine (SF), a muscarinic agonist, or 4-diphenylacetoxy-N-methylpiperidine methiodide (4DAMP), an M3 muscarinic glandular receptor antagonist, on pancreatic exocrine secretion. Pancreatic exocrine secretion was collected for 8 h postdosing at 30-min intervals beginning 1 h postfeeding. In experiment 1, steers were dosed with 0, 25, or 50 micrograms.kg-1 body weight (BW) of SF. Secretion of pancreatic juice and the pH of the secreted juice increased linearly (p < 0.05) with SF; however, secretion rate showed a time by treatment interaction (p < 0.05), as treatments converged 7 h postdosing. Trypsin secretion tended (p < 0.10) to show a quadratic response to SF administration, with the 25 micrograms SF.kg-1 BW dose having the lowest value. In experiment 2, steers received 50 micrograms.kg-1 BW of SF (positive control), 113 micrograms.kg-1 BW of 4DAMP (isosmolar with SF), or both. SF caused a greater pancreatic fluid secretion (p < 0.10) than 4DAMP, with SF plus 4DAMP intermediate. A time by treatment interaction (p < 0.04) was found, since treatments converged 8 h postdosing. Trypsin secretion was higher (p < 0.05) for SF than the other treatments. Chymotrypsin, alpha-amylase, and protein secretion were not affected. SF and 4DAMP alter pancreatic fluid secretion in the steer but have minimal effects on enzyme secretions.

Published

1994

23. Tropical pasture hay utilization with slaframine and cottonseed meal: ruminal characteristics and digesta passage in wethers.

Author

Bird AR, Croom WJ Jr, Bailey JV, O'Sullivan BM, Hagler WM Jr, Gordon GL, and Martin PR

Subjects

Alkaloids administration & dosage, Ammonia analysis, Animal Feed, Animals, Bacteria drug effects, Bacteria growth & development, Cottonseed Oil administration & dosage, Dietary Fiber metabolism, Eating, Fatty Acids, Volatile analysis, Food, Fortified, Gastrointestinal Transit drug effects, Hydrogen-Ion Concentration, Injections, Intramuscular veterinary, Male, Mycotoxins administration & dosage, Mycotoxins pharmacology, Parasympathomimetics administration & dosage, Poaceae, Rumen chemistry, Rumen microbiology, Salivation drug effects, Alkaloids pharmacology, Digestion drug effects, Parasympathomimetics pharmacology, Rumen drug effects, Sheep physiology

Abstract

Sixteen mature, ruminally cannulated wethers (average BW = 41 +/- 1 kg) were fed a low-quality hay diet with or without a cottonseed meal (CSM) supplement and the parasympathomimetic agonist slaframine (SF). Treatments were basal diet (Mitchell grass hay, 4.8% CP, 46.8% ADF) available on an ad libitum basis, basal diet plus SF (8 micrograms/kg BW, 2 x daily i.m. injection), basal diet plus CSM (41.0% CP; 100 g/d), or basal diet plus SF and CSM. Treatments were arranged as a 2 x 2 factorial within a replicated 4 x 4 Latin square with 20-d periods followed by a 10-d adjustment during which only the basal diet was fed. All measurements were performed within the final 10 d of each period. Slaframine increased salivary flow by 10 to 35% (P < .07), ruminal fluid dilution rate by 8 to 11% (P < .10), and pH by 3 to 4% (P < .001). A twofold increase (P < .05) in ruminal cellulolytic bacteria numbers occurred in SF-treated wethers. Despite these SF-induced changes in the ruminal environment, whole-tract apparent nutrient digestibility, N and mineral balance, and ruminal VFA concentrations were not changed. Cottonseed meal increased forage intake by 34 to 54% (P < .001) and DM digestibility by 30% (P < .001). Cottonseed meal supplementation of a Mitchell grass hay diet improved nutritional status and attenuated live weight loss.

Published

1993

24. Pancreatic splenic lobe organ culture system: viability and amylase release.

Author

Johnson AD, Croom WJ Jr, Hagler WM Jr, Ort JF, and Henrikson CK

Subjects

Aging metabolism, Animals, Culture Media, L-Lactate Dehydrogenase metabolism, Male, Organ Culture Techniques, Pancreas anatomy & histology, Amylases metabolism, Chickens metabolism, Pancreas enzymology

Abstract

An organ explant culture system for the intact chick pancreatic splenic lobe (SL) was characterized for exocrine function. Organ cultures were prepared using the pancreatic splenic lobe from 9- and 15-day-old male broiler chicks (Arbor Acres x Arbor Acres) to characterize amylase release as well as tissue integrity during 2, 4, 8, and 12 h of incubation. Light microscopy studies indicated necrosis of the exocrine pancreatic acini after 4 h of incubation. Changes in islets of Langerhans were noted 4 h after incubation, but islet structural integrity remained intact for up to 12 h of incubation. Lactate dehydrogenase (LD) levels measured in the culture medium did not increase significantly from 2 to 4 h of incubation. After 4 h of incubation, total LD levels increased (P < .05) for the 9-day-old SL cultures, and LD levels increased (P < .01) per unit weight of SL for the 15-day-old cultures. Medium amylase activity did not increase after 2 h of incubation. Large increases occurred for total amylase activity and amylase activity per unit weight of SL between 4 and 12 h of incubation for both 9- and 15-day-old cultures. Histological examination as well as increases in LD and amylase activities for total and per unit weight of SL in the incubation medium suggest that the viability of the 9- and 15-day-old SL organ incubation system decreases after 4 h.

Published

1993

25. Effect of fumonisin-B1 exposure on chicken macrophage functions in vitro.

Author

Qureshi MA and Hagler WM Jr

Subjects

Animals, Cell Death drug effects, Cell Line, Cells, Cultured, Female, Macrophages immunology, Macrophages physiology, Peritoneal Cavity cytology, Phagocytosis drug effects, Carcinogens, Environmental toxicity, Chickens immunology, Fumonisins, Macrophages drug effects, Mycotoxins toxicity

Abstract

Fumonisin-B1 (FB1) is one of the recently discovered metabolites of Fusarium moniliforme (Sheldon) occurring naturally in infected corn. It is hepatocarcinogenic and causes death in several animal species including rats, horses, swine, and ducklings. In the present study, chicken peritoneal macrophages (PM) and a chicken macrophage cell line, MQ-NCSU, were exposed in vitro to various doses of FB1. Exposure to .5, 5, and 10 micrograms FB1/mL caused significant cytotoxicity in PM after 2 and 4 h of exposure. Morphological alterations induced by FB1 in PM included cytoplasmic blebing or nuclear disintegration or both, which were maximal in cultures treated with 20 micrograms FB1/mL. Significant depression in the phagocytic potential of PM occurred after 4 h treatment with 20, 40, and 100 micrograms FB1. However, exposure to FB1 alone, as well as after stimulation with lipopolysaccharide, induced secretion of a cytolytic factor by MQ-NCSU cells. These findings, which showed that FB1 exposure induced morphological and functional alterations in chicken macrophages, imply that FB1 exposure may result in increased susceptibility of chickens to bacterial infection.

Published

1992

26. Cholinergic manipulation of digestive function in ruminants and other domestic livestock: a review.

Author

Croom WJ Jr, Froetschel MA, and Hagler WM Jr

Subjects

Animals, Digestive System drug effects, Exocrine Glands innervation, Exocrine Glands metabolism, Parasympathomimetics pharmacology, Receptors, Muscarinic physiology, Animals, Domestic metabolism, Digestion physiology, Digestive System innervation, Parasympathetic Nervous System physiology, Ruminants physiology

Abstract

Exocrine secretions in the digestive tract of domestic livestock are controlled by a combination of neural and endocrine inputs. The parasympathetic domain of the autonomic nervous system is responsible for efferent signals that regulate most exocrine secretory processes. Exocrine tissues possess cholinergic muscarinic receptor subtypes that are different from those found in brain, heart and muscle tissues. Cholinergic stimulation of specific muscarinic receptor subtypes has enhanced secretions of the salivary glands and pancreas. These changes in output of exocrine glands can alter digestive function that may benefit production of cattle and swine.

Published

1990

27. Effect of feeding diets containing corn treated with a commercial mold inhibitor (Myco Curb) on broiler-breeder performance.

Author

Brake J, Hagler WM Jr, and Jones FT

Subjects

Animals, Chickens growth & development, Female, Fertility, Food Handling, Fungi isolation & purification, Male, Mycotoxins analysis, Oviposition, Zea mays, Animal Feed analysis, Antifungal Agents pharmacology, Chickens physiology, Food Contamination analysis, Food Microbiology

Abstract

Corn purchased from commercial sources was split at delivery and was left untreated or treated with a commercial mold inhibitor. Feed was prepared from these two lots of corn from within 1 wk to as much as 20 wk after delivery over the course of two experiments. There was evidence of reduced mold growth due to the mold inhibitor, particularly in the second experiment where initial mold populations were higher. Mycotoxins were evident in feed samples, regardless of the corn treatment. There was no significant effect from the treatment of corn on growth, livability, egg production, feed conversion, egg weight, or the eggshell quality of broiler breeders. Treatment of corn with a mold inhibitor significantly increased hatchability of fertile eggs in both experiments. Fertility was also significantly improved in the second experiment. These data suggest that using corn treated with a mold inhibitor results in significantly better hatchability in broiler breeders than untreated corn, although there were no observed differences in the incidence of mycotoxins in the samples taken.

Published

1990

28. Liquid chromatographic determination of aflatoxin M1 in milk.

Author

Tyczkowska K, Hutchins JE, and Hagler WM Jr

Subjects

Aflatoxin M1, Animals, Cattle, Chromatography, Liquid methods, Chromatography, Thin Layer methods, Densitometry methods, Food Contamination analysis, Spectrometry, Fluorescence methods, Swine, Aflatoxins analysis, Milk analysis

Abstract

The official AOAC method for aflatoxin M1 in milk was modified by replacing cellulose column chromatography with cartridge chromatographic cleanup and replacing thin layer chromatographic (TLC) determination with liquid chromatographic (LC) quantitation to yield a new method for bovine and porcine milk. An acetone extract of milk is treated with lead acetate and defatted with hexane, and M1 is partitioned into chloroform as in the AOAC method. Chloroform is removed by evaporation under a stream of nitrogen at 50 degrees C. The residue is dissolved in chloroform, the vessel is rinsed with hexane, and the 2 solutions are applied in sequence to a hexane-activated silica Sep-Pak cartridge. Less polar impurities are removed with hexane-ethyl ether, and M1 is eluted with chloroform-methanol, and determined by C18 reverse phase LC using fluorescence detection. Recoveries of M1 added to bovine milk at 0.25, 0.50, and 1.0 ng/mL were 90.8, 93.4, and 94.1%, respectively. The limit of detection was less than 0.1 ng M1/mL for both bovine and porcine milk.

Published

1984

29. Destruction of Aflatoxin in Corn with Sodium Bisulfite 1, 2, 3 .

Author

Hagler WM Jr, Hutchins JE, and Hamilton PB

Abstract

The ability of sodium bisulfite to destroy aflatoxins B 1 and B 2 in naturally contaminated corn containing about 2350 ppb of B 1 and 450 ppb of B 2 was investigated. Under certain conditions, complete destruction of aflatoxin B 1 was achieved. Aflatoxin B 2 , on the other hand, was resistant to sodium bisulfite and never over about 50% was destroyed. Moisture, sodium bisulfite level, time, as well as temperature had significant effects on aflatoxin degradation. Moisture levels of over 50% (wet weight basis) had a strongly adverse effect on the aflatoxin-bisulfite reaction. The most effective treatment involved soaking whole-kernel corn in a 10% sodium bisulfite solution for 72 h, removing the solution and incubating the corn in sealed plastic bags at 50°C. Complete destruction of aflatoxin B 1 was achieved by 21 d. Sodium bisulfite exhibited antimicrobial activity in corn comparable to that of propionic acid, indicating possible utility as an effective mold inhibitor in stored corn at up to 40% moisture. Feed consumption by young chickens was unaffected until feed containing over 20 g of sodium bisulfite/kg was presented.

Published

1982

30. Method for detecting production of zearalenone, zearalenol, T-2 toxin, and deoxynivalenol by Fusarium isolates.

Author

Richardson KE, Hagler WM Jr, and Hamilton PB

Subjects

Culture Media, Species Specificity, Trichothecenes isolation & purification, Zearalenone isolation & purification, Zeranol analogs & derivatives, Zeranol isolation & purification, Fusarium growth & development, Resorcinols biosynthesis, Sesquiterpenes biosynthesis, Trichothecenes biosynthesis, Zearalenone biosynthesis, Zeranol biosynthesis

Abstract

Three methods for detecting toxigenic fusaria in culture were compared by using known producers of zearalenone, zearalenol, T-2 toxin, and deoxynivalenol. Moist, autoclaved rice cultures of known toxigenic isolates grown in 20-ml tubes yielded oily extracts containing compounds which interfered with qualitative and quantitative analysis for the mycotoxins. Vermiculite moistened with nutrient broth in 20-ml tubes yielded a much cleaner extract. Growing the fungi on a liquid medium required a shorter incubation period, but yields of T-2 toxin and deoxynivalenol were low and variable, and the method required greater space in the incubator. Screening of the extracts by thin-layer chromatography with colorimetric spray reagents to detect the presence of these toxins permitted reduction in the number of extracts quantified by the more lengthy gas-liquid chromatographic method. Culturing in nutrient broth on vermiculite in tubes coupled to a qualitative screen before quantitation proved to be a convenient, inexpensive, and relatively rapid method that enabled reliable screening of a large number of Fusarium isolates for toxin production as compared with prior methods.

Published

1984

31. Histologic lesions in broiler chicks given cyclopiazonic acid orally.

Author

Cullen JM, Wilson M, Hagler WM Jr, Ort JF, and Cole RJ

Subjects

Administration, Oral, Animals, Female, Indoles administration & dosage, Liver pathology, Male, Muscles pathology, Mycotoxins administration & dosage, Pancreas drug effects, Pancreas pathology, Proventriculus pathology, Spleen drug effects, Spleen pathology, Chickens anatomy & histology, Indoles toxicity, Liver drug effects, Muscles drug effects, Mycotoxins toxicity, Proventriculus drug effects

Abstract

Cyclopiazonic acid dissolved in corn oil was administered by gavage to broiler chicks (n = 80) daily, from the day of hatching for 23 days. Chicks were assigned to 3 groups (1, 2, or 4 mg of cyclopiazonic acid/kg of body weight); a control group was given corn oil. Each group was composed of 10 male and 10 female chicks. Surviving chicks were euthanatized and necropsied on day 24. Histologic examination revealed that the most common lesions consisted of necrosis and hemorrhage or hyperplasia of the mucosa of the proventriculus and hepatocellular vacuolation. Skeletal muscle degeneration, characterized by myofiber swelling or fragmentation accompanied by an infiltrate of macrophages and heterophils, was detected in the group given 4 mg/kg. This degeneration was associated with an increase of plasma creatine kinase activity. Focal hepatocellular and splenic necrosis also developed in the groups given 4 mg/kg.

Published

1988

32. Feed refusal during ochratoxicosis in turkeys.

Author

Burditt SJ, Hagler WM Jr, and Hamilton PB

Subjects

Animals, Body Weight, Male, Species Specificity, Chickens, Feeding Behavior, Ochratoxins poisoning, Poultry Diseases physiopathology, Turkeys

Abstract

Previous observations of feed refusal associated with apparent field outbreaks of ochratoxicosis in turkeys but not in chickens suggested that these species differed in response to ochratoxin or that different factors were involved in the field outbreaks. The recent development of laboratory models for the study of feed refusal syndromes in poultry permitted an evaluation of the problem. Pure ochratoxin A reduced the consumption of feed by young turkeys. Refusal of graded concentrations of ochratoxin A in feed was not detected in young chickens. These results, which suggested that feed refusal is a symptom of ochratoxicosis in turkeys but not in chickens, provide additional evidence that the aforementioned outbreaks were caused by ochratoxin and that ochratoxicosis is an emerging problem in the poultry industry.

Published

1984

33. Evaluation of silica cartridge purification and hemiacetal formation for liquid chromatographic determination of aflatoxins in corn.

Author

Hutchins JE, Lee YJ, Tyczkowska K, and Hagler WM Jr

Subjects

Chemical Phenomena, Chemistry, Food Contamination analysis, Aflatoxins analysis, Chromatography, High Pressure Liquid instrumentation, Zea mays analysis

Abstract

Rapid silica cartridge cleanup, acid-catalyzed conversion of aflatoxins B1 and G1 to hemiacetals, and reverse-phase liquid chromatography with fluorescence detection were evaluated for effectiveness in determining aflatoxins B1, B2, G1, and G2 in corn at concentrations ranging from 2 ng/g to 100 micrograms/g. In testing the method, aflatoxins applied to silica cartridges were recovered at greater than 97.1% overall. Conversion of aflatoxins B1 and G1 to their hemiacetals was shown to be complete (150 micrograms of toxin per extract). Application of these techniques to spiked corn extracts yielded data indicating excellent repeatability of derivatization relative to paired standards; coefficients of variation ranged from 1.08% to 5.81%. The repeatability of the method with naturally contaminated corn was also excellent; coefficients of variation ranged from 1.15% to 3.97%. Liquid chromatographic determination of aflatoxins in corn using fluorescence detection was sensitive, accurate, and precise resulting in applicability from less than 1 ng/g of aflatoxin B1 to greater than 100,000 ng/g.

Published

1989

34. An epidemiological investigation associating aflatoxin M1 with milk production in dairy cattle.

Author

Corbett WT, Brownie CF, Hagler SB, and Hagler WM Jr

Subjects

Aflatoxin M1, Animal Feed analysis, Animals, Cattle, Epidemiologic Methods, Female, Risk Factors, Aflatoxins analysis, Milk analysis

Abstract

An attempt was made to utilize the analysis for aflatoxin M2 in milk, instead of aflatoxin B1 in feed for a pilot epidemiological study addressing the association of M1 levels and various production parameters. Four dairy farms, representing above average to below average management practices, were identified with 10 animals being randomly selected from each farm for this study. Milk samples and production data were evaluated from these animals in order to gain insight into the possible effects of low level mycotoxin ingestion on production and to test whether or not this approach offered potential for future epidemiological studies. Feed samples were basically negative for the presence of aflatoxin B1, yet milk analysis revealed the presence of M1 in a large percentage of the animals. Further, the M1 levels appeared to be associated with a decrease in daily milk production. This study indicates that employing M1 analysis in milk for epidemiological investigations of low level mycotoxin ingestion effects, instead of B1 feed analysis, is feasible and offers a potential for more definitive studies in this area.

Published

1988

35. Simultaneous occurrence of deoxynivalenol, zearalenone, and aflatoxin in 1982 scabby wheat from the midwestern United States.

Author

Hagler WM Jr, Tyczkowska K, and Hamilton PB

Subjects

Kansas, Nebraska, Aflatoxins analysis, Food Analysis, Food Contamination, Resorcinols analysis, Sesquiterpenes analysis, Trichothecenes analysis, Triticum analysis, Zearalenone analysis

Abstract

Thirty-three samples of wheat of the 1982 crop year from Kansas and Nebraska were analyzed for deoxynivalenol, T-2 toxin, zearalenone, and aflatoxin. Deoxynivalenol was identified in 31 of 33 samples, zearalenone was identified in 3 of 33 samples, and aflatoxin B1 was identified in 23 of 31 samples. One 1982 wheat sample from Illinois and one from Texas were also contaminated with deoxynivalenol at 1,200 and 600 ng/g, respectively. None of the samples contained detectable T-2 toxin. The mean concentration of deoxynivalenol was 1,782 +/- 262 ng/g, and the concentrations of aflatoxin B1 ranged from 0.8 to 17.0 ng/g, with a mean of 3.37 +/- 0.7. Zearalenone concentrations of the three positive samples were 35, 90, and 115 ng/g. However, density segregation of two other samples which tested negative yielded light fractions, comprising less than 2% of the samples, contaminated at 230 and 254 ng of zearalenone per g; calculated zearalenone concentrations for these two samples were below the limit of detection of the method. The high frequency of aflatoxin B1 and deoxynivalenol in wheat from the 1982 crop is unprecedented, as is the simultaneous contamination of some samples with deoxynivalenol, zearalenone, and aflatoxin B1.

Published

1984

36. Density Segregation of Corn and Wheat Naturally Contaminated with Aflatoxin, Deoxynivalenol and Zearalenone.

Author

Huff WE and Hagler WM Jr

Abstract

Density segregation was used to reduce mycotoxin levels of corn samples naturally contaminated with aflatoxin or deoxynivalenol, and wheat samples naturally contaminated with deoxynivalenol or zearalenone. Corn kernels which were buoyant in saturated sodium chloride represented 3% of the total sample, yet contained 74% of the aflatoxin. Corn buoyant in water contained 51 and 14% of the total deoxynivalenol present in two naturally contaminated corn samples. Subsequent segregation of corn non-buoyant in water with 30% sucrose removed additional deoxynivalenol-contaminated kernels, resulting in the combined removal of 59 and 79% of the deoxynivalenol. Removal of deoxynivalenol-contaminated corn kernels with both water and 30% sucrose reduced the concentration of deoxynivalenol by 53 and 77%. Removing wheat buoyant in water and 30% sucrose decreased the deoxynivalenol present by 96 and 68%, and reduced the deoxynivalenol concentration by 96 and 67%. Removing wheat naturally contaminated with zearalenone buoyant in water and 30% sucrose combined resulted in no detectable zearalenone remaining in the non-buoyant fraction of the samples.

Published

1985

37. Fungal degradation of anaerobically digested sewage sludge.

Author

Hagler WM Jr, Davis ND, and Diener UL

Subjects

Anaerobiosis, Biodegradation, Environmental, Fungi growth & development, Mucorales growth & development, Mucorales metabolism, Species Specificity, Temperature, Fungi metabolism, Sewage, Water Microbiology

Abstract

Fifty isolates of fungi were screened for their ability to grow on and degrade sludge. Cunninghamella elegans was selected for further study of degradation as affected by moisture, nutrients, time and temperature. Maximal sludge degradation (total dry weight basis) was 5.8% by Rhizopus oligosporus, 5.4% by C. elegans and 5.3% by Myrothecium verrucaria, representing approximately 11% degradation of the organic matter present. Added nutrients had little or no effect on sludge degradation. Maximal sludge degradation by C. elegans occurred in three weeks at 30-35 C or four weeks at 25 and 40 C.

Published

1976

38. Mycoflora of activated sewage sludge.

Author

Diener UL, Morgan-Jones G, Hagler WM Jr, and Davis ND

Subjects

Alabama, Aspergillus isolation & purification, Penicillium isolation & purification, Species Specificity, Fungi isolation & purification, Sewage, Water Microbiology

Abstract

Thirty-eight species of fungi were identified in pure culture after isolation from activated sewage sludge by serial dilution. Nine species and genera were identified that had not been previously reported. In 1963, Cooke (1) published an excellent laboratory guide on the identification of fungi from polluted water, sewage, and sewage treatment systems; of approximately 30 papers cited only one (2) dealt with fungi from activated sewage sludge. Later (1970), Cooke & Pipes (3) enumerated 47 fungi consisting of 4 genera of yeasts and 33 genera of filamentous fungi that had been isolated from activated sludge. This paper reports the mycoflora of anaerobically digested sludge from a residential area in Auburn, Alabama.

Published

1976

39. Liquid chromatographic determination of aflatoxicol in porcine liver.

Author

Tyczkowska K, Hutchins JE, and Hagler WM Jr

Subjects

Animals, Chromatography, Liquid, Indicators and Reagents, Solvents, Spectrometry, Fluorescence, Swine, Aflatoxins analysis, Liver analysis

Abstract

A liquid chromatographic (LC) method for determination of aflatoxicol in porcine liver was developed. Liver sample is homogenized with water, diluted with saturated Na2SO4 solution, and extracted with acetone. After filtration, less polar interferences are removed by partition with isooctane. Aflatoxicol in the aqueous fraction is partitioned into CHCl3. The extract is dried over anhydrous Na2SO4 and evaporated nearly to dryness at 35 degrees C under a gentle flow of dry filtered air or nitrogen. Residue is dissolved in CHCl3-hexane and applied to a hexane-activated silica cartridge. The cartridge is washed with hexane-CHCl3, then aflatoxicol is eluted with CHCl3-acetone. Purified extract is evaporated to dryness, dissolved in methanol, and analyzed by C18 reverse phase liquid chromatography using a water-CH3CN-acetic acid mobile phase and fluorescence detection. Recovery of aflatoxicol from spiked liver samples at levels ranging from 0.25 to 4.0 ng aflatoxicol/g wet tissue averaged 92% with a limit of detection of about 0.1 ng aflatoxicol/g liver.

Published

1987

40. Rapid liquid chromatographic determination of aflatoxins in heavily contaminated corn.

Author

Hutchins JE and Hagler WM Jr

Subjects

Zea mays, Aflatoxins analysis, Animal Feed analysis, Food Contamination analysis

Abstract

A procedure is described for rapid, quantitative determination of aflatoxins B1, B2, G1, and G2 in heavily contaminated corn (greater than 500 micrograms B1/kg) from field, greenhouse, and growth chamber experiments employing artificial inoculation of corn with Aspergillus flavus. Whole kernel corn is ground to pass a 1 mm screen and mixed before extraction of a water-wetted (25 mL) 50 g subsample with 250 mL chloroform. The filtered extract is diluted 1:1 with hexane and applied to a hexane-wetted (10 mL) disposable silica cartridge. Interferences are removed with chloroform-hexane (1 + 3), and aflatoxins are quantitatively eluted with hexane-acetone (1 + 1). Aflatoxins B1 and G1 are converted to the more intensely fluorescent hemiacetals, B2a and G2a, by treatment with trifluoroacetic acid-water. Derivatized aflatoxins are separated by reverse phase liquid chromatography (LC) and quantitated fluorometrically. Compared with AOAC method I (CB) for corn, using samples containing approximately 50 and 10 000 micrograms B1/kg, agreement between methods was good at the lower level while the rapid method yielded a considerably larger mean at the higher level. A precision study of 30 replicate samples produced a coefficient of variation of 8.46% at a mean value of 1066 micrograms B1/kg. The cartridge method was developed for LC analysis of samples that contain greater than 500 micrograms aflatoxin B1/kg corn, but it may be used to quantitate as little as 10 micrograms B1/kg with no modification.

Published

1983

41. Effects of a salivary stimulant, slaframine, on ruminal fermentation, bacterial protein synthesis and digestion in frequently fed steers.

Author

Froetschel MA, Amos HE, Evans JJ, Croom WJ Jr, and Hagler WM Jr

Subjects

Abomasum drug effects, Abomasum metabolism, Animal Feed, Animals, Bacterial Proteins biosynthesis, Digestion drug effects, Dose-Response Relationship, Drug, Feces analysis, Fermentation drug effects, Male, Rumen metabolism, Rumen microbiology, Salivation drug effects, Alkaloids pharmacology, Cattle metabolism, Parasympathomimetics pharmacology, Rumen drug effects

Abstract

Slaframine (SF), a parasympathomimetic salivary stimulant, was administered i.m. (10, 15 or 20 micrograms SF/kg BW) to ruminally and abomasally fistulated steers at 12-h intervals for 18-d periods in a latin square-designed experiment. Steers were fed semicontinuously (12 times daily) a 40:60 roughage:concentrate diet at twice their net energy requirement for maintenance. Ruminal digestion coefficients for DM, ADF and starch were 10 to 16% lower and linearly related in an inverse manner to the level of SF administered (P less than .05). Postruminal digestion of DM, ADF and starch increased as much as 46.7, 9.5 and 44.0%, respectively, in a fashion linearly related (P less than .05) to the level of SF administered. Total tract digestion of DM and ADF were not affected by SF; however, total tract starch digestion was increased as much as 5% and was related linearly (P less than .05) to SF treatment. With SF administration, as much as 13% more bacterial protein exited the rumen, resulting in a 16.5% linear improvement (P less than .1) in the efficiency of ruminal bacterial protein production per 100 g of OM fermented. Ruminal concentrations of VFA, ammonia and pH were not affected by SF. These results demonstrate a positive relationship between salivation and ruminal bacterial protein synthesis and suggest that feed utilization by ruminants may be improved by pharmacological stimulation of salivary secretions.

Published

1989

42. Estimating salivary flow and ruminal water balance of intake, diet, feeding pattern, and slaframine.

Author

Jacques K, Harmon DL, Croom WJ Jr, and Hagler WM Jr

Subjects

Animals, Biomarkers, Female, Cattle physiology, Diet, Feeding Behavior physiology, Rumen physiology, Saliva metabolism, Water metabolism

Abstract

Three experiments with ruminally fistulated cattle fed 12 times daily were conducted to study the role of saliva secretion in ruminal water balance when intake, diet, and feeding pattern were altered. Water balance data were determined from continuously infused Co-EDTA and pulse-dosed Cr-EDTA with saliva flow estimated by difference between water intake and ruminal outflow. Any net transruminal water flux would be included in the estimate of salivary flow. When the concentration of bluestem hay in the diet was increased from 50 to 90%, ruminal fluid volume, saliva secretion, water intake, dilution rate, and total ruminal outflow increased. At equal intake, the higher forage diet increased ruminal liquid volume, outflow, and saliva secretion but had no effect on dilution rate. Intake, but not forage concentration, affected ruminal pH when 50 and 90% hay diets were fed. Increasing feeding frequency of forage in a 65% bluestem hay diet from 4 to 12 times daily (the grain portion was fed 12 times daily) increased dilution and ruminal outflow; however, the latter was only significant with data from Cr-EDTA. Ruminal volatile fatty acids were not altered by feeding frequency of forage. Nycterohemeral patterns were seen in water intake, ruminal dilution rate, outflow, and salivary flow in both studies. Slaframine increased saliva flow by 29% and was accompanied by increased ruminal liquid volume, dilution rate, and outflow.

Published

1989

43. Zearalenone and Trichothecene Production in Soybeans by Toxigenic Fusarium.

Author

Richardson KE, Hagler WM Jr, Haney CA, and Hamilton PB

Abstract

Several Fusarium isolates known to produce zearalenone or T-2 toxin were tested for their toxigenic potential on heatsterilized whole and cracked soybeans, on soybean meal, and on rice. Moisture concentration levels and particle sizes of substrate were varied to determine effects on the amount and type of toxin produced. Only one of the three Fusarium isolates known to produce zearalenone, Fusarium roseum 'Graminearum', produced detectable amounts of this mycotoxin on soybeans. Fusarium sporotrichioides NRRL 3299, the T-2 toxin-producing isolate tested, produced T-2 toxin as well as T-2 tetraol, HT-2 toxin and neosolaniol on soybeans. HT-2 toxin production was greatly enhanced on soybean meal in comparison to rice cultures. These findings plus previous field observations suggest that soybean products present a mycotoxic hazard which warrants attention.

Published

1985

44. Influence of dietary protein, fat or amino acids on the response of weanling swine to aflatoxin B1.

Author

Coffey MT, Hagler WM Jr, and Cullen JM

Subjects

Aflatoxin B1, Animal Feed, Animals, Food Contamination, Aflatoxins pharmacology, Amino Acids pharmacology, Dietary Fats pharmacology, Dietary Proteins pharmacology, Swine physiology, Weight Gain drug effects

Abstract

Two experiments were conducted using corn from clean or aflatoxin B1 (AFB1)-contaminated (182 ppb) sources. Weanling pigs (28 d) were fed one of eight dietary treatments arranged in a 2 x 2 x 2 factorial design. In Exp. 1 (192 pigs), treatments varied in corn source (clean or AFB1-contaminated), CP level (18 or 20%) and added fat (0 or 5%). At the end of the 28-d growth trials, plasma samples were obtained. An AFB1 x CP level interaction was detected (P less than .05) for growth rate (ADG), feed intake (FI) and feed/gain ratio (F/G). Feeding AFB1 reduced (P less than .05) ADG (.30 vs .37 kg/d) and FI (.57 vs .66 kg/d) and increased F/G (1.88 vs 1.78) of pigs fed 18% CP diets. Performance of pigs fed 20% CP diets was not altered by AFB1. Adding 5% fat to diets improved (P less than .05) F/G but did not improve ADG of pigs fed AFB1. There was an AFB1 x CP x fat interaction (P less than .05) for plasma cholesterol. Adding fat or increasing the CP level prevented the depression of plasma cholesterol in pigs fed AFB1. In Exp. 2 (96 pigs), all diets contained 18% CP and the treatments varied in corn source (clean or AFB1-contaminated), added L-lysine HCl (0 or .25%) and added DL-methionine (0 or .15%). Feeding AFB1 reduced (P less than .05) ADG of pigs fed the 18% CP diet (.44 vs .50 kg/d) but not of pigs fed diets supplemented with .25% lysine.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1989

45. Effects of slaframine on ruminant digestive function: ruminal motility in sheep and cattle.

Author

Froetschel MA, Croom WJ Jr, Hagler WM Jr, Argenzio R, Liacos J, and Broquist HP

Subjects

Animals, Male, Alkaloids pharmacology, Cattle physiology, Gastrointestinal Motility drug effects, Mycotoxins pharmacology, Parasympathomimetics pharmacology, Rumen drug effects, Sheep physiology

Abstract

Effect of purified slaframine (SF; 1-acetoxy-6-aminooctahydroindolizine), a parasympathomimetic secretagogue isolated from Rhizoctonia leguminicola, on ruminal motility was investigated in cattle and sheep. In trial 1, four ruminal cannulated wethers, fed a pelleted concentrate and hay diet, were injected intramuscularly with 0, 12, 24 and 48 micrograms SF/kg body weight (BW) in a 4 X 4 Latin-square design. Ruminal motility was recorded 1 h before and 1 to 2 h and 3 to 4 h after SF administration by measuring pressure changes exerted upon a fluid-filled, open-tipped catheter inserted into the dorsal sac of the rumen. The frequencies of both primary and secondary ruminal contractions were decreased as much as 20 to 78% with SF (P less than .05) depending upon the dosage level and time after administration. In trial 2, three ruminal-cannulated steers fed a concentrated diet were injected intramuscularly with 0, 12 and 24 micrograms SF/kg BW in a 3 X 3 Latin-square design. A water-filled balloon inserted into the cranial sac of the rumen was used to measure ruminal pressure changes 1 h before and 1 to 2 h, 3 to 4 h and 7 to 8 after SE administration. Frequency of primary and secondary ruminal contractions decreased with SF as much as 27 to 64% depending on the dosage level and time after administration. The frequency of secondary contractions increased 28% (P less than .05) as compared with control during the 7 to 8 h after administration.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1986

46. Effects of chronic administration of slaframine on production and digestive function in broiler chicks.

Author

Froetschel MA, Hagler WM Jr, Croom WJ Jr, Ort J, and Broquist HP

Subjects

Animals, Body Weight drug effects, Digestive System enzymology, Organ Size drug effects, Alkaloids pharmacology, Chickens physiology, Digestion drug effects, Digestive System drug effects

Abstract

Slaframine (SF), 1-acetoxy-6-aminooctahydroindolizine a parasympathomimetic with a high affinity for the gastrointestinal tract, was administered by oral intubation daily to 240 broiler chicks at either 0, 8.9, or 17.8 micrograms/kg body weight.75 (BW.75) in saline for 21 days. Throughout the experimental period weight, feed intake, and fecal output were measured. On Day 21 birds were killed, eviscerated, and wet organ weights were obtained. Pancreas and small intestine digesta were homogenized with saline and frozen for analyses of trypsin, chymotrypsin, amylase, and lipase activity as well as total protein. Weight, feed intake and utilization, pancreatic weight, liver weight, and small intestine digesta weight were not affected by SF treatment. Protein content of the digesta decreased 16.6% with the 17.8 micrograms SF/kg BW.75 treatment. Digesta lipase activity was 13.3% (P greater than .05) and specific activity 24% less (P less than or equal to .02) in 17.8 micrograms/kg BW.75 treated birds in comparison with those of controls, and activities decreased in a linear fashion across treatment levels (P less than or equal to .04). Digesta trypsin-specific activity decreased linearly with SF treatment (P less than or equal to .05), averaging 5.5 to 16.9% lower than control treated birds. Pancreatic chymotrypsin-specific activity was not significantly different among treatments. These results suggest that relatively small dosages of SF may affect digestive function of broiler chicks.

Published

1987

47. Models of feed refusal syndrome in poultry.

Author

Burditt SJ, Hagler WM Jr, Hutchins JE, and Hamilton PB

Subjects

Ammonia pharmacology, Animals, Antineoplastic Agents, Phytogenic pharmacology, Bicarbonates pharmacology, Drinking, Food Additives, Fusarium, Hydrogen-Ion Concentration, Male, Mycotoxins pharmacology, Sodium Bicarbonate, Sodium Chloride pharmacology, Sulfuric Acids pharmacology, Trichothecenes pharmacology, Chickens, Feeding Behavior drug effects, Models, Biological

Abstract

Research on feed refusal syndrome(s), an important problem in the poultry industry, has been hindered by a lack of sensitive and quantitative laboratory models. Suitable models were developed using five groups of 30-week-old male chickens per treatment. Feed or water, depending on which was to be measured, was withdrawn overnight. Then consumption of treated water or feed was measured over a 6-hr period of rehydration or refeeding. In aqueous solutions NaCl, H2SO4, and Na2CO3 reduced liquid consumption in a dose-related manner. Ammonia caused a similar refusal when added to feed. Consumption of feed and water was not influenced by pH over the ranges likely to occur as a result of fungal activity. Consumption of feed on a wet weight, but not dry weight, basis was influenced by the moisture content of feed. A culture filtrate of Fusarium roseum NRRL 1181 containing diacetoxyscirpenol, a trichothecene mycotoxin, reduced consumption of feed by about 77% when added to feed and reduced liquid consumption by about 92% when substituted for drinking water. Thus, the models for consumption of liquids and solids appear to have the attributes necessary for quantitative investigation into the relationships of mycotoxins to feed refusal syndromes.

Published

1983

48. Aflatoxin B 1 S: Revised Structure for the Sodium Sulfonate Formed by Destruction of Aflatoxin B 1 with Sodium Bisulfite 1 , 2 .

Author

Yagen B, Hutchins JE, Cox RH, Hagler WM Jr, and Hamilton PB

Abstract

A promising method for the destruction of aflatoxin B 1 in commodities is treatment with sodium bisulfite to yield a single major product, aflatoxin B 1 S. On the basis of nuclear magnetic resonance, ultraviolet and infrared spectra, elemental analysis, mass spectroscopy, deuterium labeling and stability to highly acidic conditions, the structure of aflatoxin B 1 S was established as the 15 α-sodium sulfonate of aflatoxin B 1 The formation of aflatoxin B 1 products substituted at the 15 position only is unprecedented and implies an unusual mechanism. The formation of a single trans addition product under conditions that seemingly rule out a previously proposed free radical mechanism suggested a newly proposed ionic reaction mechanism. The completeness of the reaction and the water solubility of aflatoxin B 1 S support the promising use of bisulfite to destroy aflatoxin.

Published

1989

49. Survey of molds and mycotoxins for their ability to cause feed refusal in chickens.

Author

Burditt SJ, Hagler WM Jr, and Hamilton PB

Subjects

Aflatoxins pharmacology, Animals, Antineoplastic Agents, Phytogenic pharmacology, Citrinin pharmacology, Depression, Chemical, Drinking drug effects, Eating drug effects, Male, Species Specificity, T-2 Toxin pharmacology, Trichothecenes pharmacology, Chickens physiology, Feeding Behavior drug effects, Food Contamination, Mycotoxins pharmacology

Abstract

The cause of feed refusal by poultry is an important problem that has not been established. T-2 toxin, a culture filtrate of Fusarium roseum NRRL 1181 containing a high concentration of diacetoxyscirpenol, and a filtrate of Penicillium citrinum containing an unknown factor produced refusal activity in week-old chickens. Citrinin stimulated water consumption while aflatoxin did not affect feed consumption. Detection of refusal activity was more sensitive when the refusal factor was presented in the drinking water than in the feed. The experimental model used here was sensitive, and, with appropriate controls, would appear suitable for the isolation and study of new factors capable of causing feed refusal in poultry.

Published

1983

50. Effects of slaframine on circulating concentrations of growth hormone and glucose.

Author

Froetschel MA, Hagler WM Jr, Croom WJ Jr, Ort J, Lauterio TJ, Fernandez JM, Mann DL, Broquist HP, and Scanes CG

Subjects

Animals, Male, Alkaloids pharmacology, Blood Glucose, Chickens blood, Growth Hormone blood, Parasympathomimetics pharmacology

Abstract

The ability of slaframine (SF), a parasympathomimetic, to alter blood growth hormone (GH) and glucose concentrations in broiler chicks was investigated. Eighty male broiler chicks (average weight 225 g) were divided into 10 groups and dosed with either saline (control) or 1 mg SF/kg of body weight by oral intubation. Plasma samples were obtained from separate groups of chicks at 1, 2, 4, 8, and 12 hr after SF administration and analyzed for growth hormone and glucose. One hour after SF administration, glucose increased (P less than .05) 21.4% compared with controls. Growth hormone increased (P less than .05) 449 to 948% from 8 to 12 hr after SF administration. Administration of SF at 1 mg/kg of body weight was associated with increased plasma GH.

Published

1987