ABSTRACT
Soybean (Glycine max L. Merrill) is one of eight major allergenic foods with endogenous proteins identified as allergens. To better understand the natural variability of five soybean allergens (Gly m 4, Gly m 5, Gly m 6, Gly m Bd 28k, and Gly m Bd 30k), validated enzyme-linked immunosorbent assays (ELISAs) were developed. These ELISAs measured allergens in 604 soybean samples collected from locations in North and South America over five growing seasons (2009-2013/2014) and including 37 conventional varieties. Levels of these five allergens varied 5-19-fold. Multivariate statistical analyses and pairwise comparisons show that environmental factors have a larger effect on allergen levels than genetic factors. Therefore, from year to year, consumers are exposed to highly variable levels of allergens in soy-based foods, bringing into question whether quantitative comparison of endogenous allergen levels of new genetically modified soybean adds meaningful information to their overall safety risk assessment.
Subject(s)
Allergens/analysis , Glycine max/chemistry , Soybean Proteins/analysis , Antigens, Plant/analysis , Antigens, Plant/immunology , Enzyme-Linked Immunosorbent Assay , Food Hypersensitivity , Genetic Variation , Globulins/analysis , Globulins/immunology , Glycoproteins , Multivariate Analysis , North America , Reproducibility of Results , Seed Storage Proteins/analysis , Seed Storage Proteins/immunology , Seeds/chemistry , South America , Soybean Proteins/genetics , Soybean Proteins/immunology , Glycine max/genetics , Glycine max/immunologyABSTRACT
This study investigated (1) the susceptibility of Bacillus anthracis (Ames strain), Bacillus subtilis (ATCC 19659), and Clostridium sporogenes (ATCC 3584) spores to commercially available peracetic acid (PAA)- and glutaraldehyde (GA)-based disinfectants, (2) the effects that heat-shocking spores after treatment with these disinfectants has on spore recovery, and (3) the timing of heat-shocking after disinfectant treatment that promotes the optimal recovery of spores deposited on carriers. Suspension tests were used to obtain inactivation kinetics for the disinfectants against three spore types. The effects of heat-shocking spores after disinfectant treatment were also determined. Generalized linear mixed models were used to estimate 6-log reduction times for each spore type, disinfectant, and heat treatment combination. Reduction times were compared statistically using the delta method. Carrier tests were performed according to AOAC Official Method 966.04 and a modified version that employed immediate heat-shocking after disinfectant treatment. Carrier test results were analyzed using Fisher's exact test. PAA-based disinfectants had significantly shorter 6-log reduction times than the GA-based disinfectant. Heat-shocking B. anthracis spores after PAA treatment resulted in significantly shorter 6-log reduction times. Conversely, heat-shocking B. subtilis spores after PAA treatment resulted in significantly longer 6-log reduction times. Significant interactions were also observed between spore type, disinfectant, and heat treatment combinations. Immediately heat-shocking spore carriers after disinfectant treatment produced greater spore recovery. Sporicidal activities of disinfectants were not consistent across spore species. The effects of heat-shocking spores after disinfectant treatment were dependent on both disinfectant and spore species. Caution must be used when extrapolating sporicidal data of disinfectants from one spore species to another. Heat-shocking provides a more accurate picture of spore survival for only some disinfectant/spore combinations. Collaborative studies should be conducted to further examine a revision of AOAC Official Method 966.04 relative to heat-shocking.
Subject(s)
Disinfectants/toxicity , Glutaral/toxicity , Gram-Positive Bacteria/radiation effects , Hot Temperature , Microbial Viability/radiation effects , Peracetic Acid/toxicity , Spores, Bacterial/radiation effects , Colony Count, Microbial , Gram-Positive Bacteria/drug effects , Microbial Viability/drug effects , Spores, Bacterial/drug effectsABSTRACT
This study evaluated the toxicity effects of chlorpyrifos on bobwhite quail (Colinus virginianus) kept in 27 field-exposed large pens arranged over turf in a randomized block design with nine blocks of three pens (16 adult birds per pen). Nine pens were treated with one application of 3.4 kg active ingredient (ai) per hectare followed by a second 3.4 -kg ai/ha application 2 weeks later, nine pens with one 6.7 -kg ai/ha application, and nine pens with formulation blank. In addition, the seed fed to the birds in the two chemically treated pens was also treated with chlorpyrifos. Mean residue in the grass samples from the first 3.4-kg treatment pens ranged from 306+/-95 ppm on day 0 to 18+/-8 ppm on day 14 after treatment. The second 3.4 -kg ai/ha treatment grass residues ranged from 361+/-167 ppm on day 0 to 38+/-24 ppm on day 14 after treatment. Grass residues from the 6.7-kg treatment pens ranged from 903+/-310 ppm on day 0 to 9+/-8 ppm on day 30 after treatment. Half-lives were approximately 2 days and 10 days for grass and seeds, respectively. Whereas the incidence of behavioral deficits was significantly (P = 0.0156) higher in the 6.7-kg pens (five females, one male), two of the females could have been the same bird because they were both seen in the same pen on days 23 and 24 after treatment. There was no significant difference in mortality, brain acetylcholinesterase activity, or any other measured parameter among any of the treatments. We conclude that application of chlorpyrifos to turf at 3.4 and 6.7 kg ai/ha is not expected to have chronic deleterious effects on populations of bobwhite quail grazing on treated grass or seeds, provided there is an abundant supply of seeds for the quail to eat.
Subject(s)
Chlorpyrifos/poisoning , Colinus/physiology , Environmental Exposure , Insecticides/poisoning , Acetylcholinesterase/pharmacology , Animals , Brain/enzymology , Half-Life , Plants, Edible/chemistry , Poaceae , Risk Assessment , SeedsABSTRACT
BACKGROUND: Development of the human craniofacial anatomy involves a number of interrelated, genetically controlled components. The complexity of the interactions between these components suggests that interference with the spaciotemporal interaction of the expanding tongue and elongating Meckel's cartilage correlates with the appearance of cleft palate. Mice homozygous for the semi-dominant Col2a1 mutation Disproportionate micromelia (Dmm), presenting at birth with both cleft palate and micrognathia, provide the opportunity to test the hypothesis that mandibular growth retardation coincides with formation of the secondary palate as predicted from our understanding of the Pierre Robin sequence. The present study was conducted in embryonic day 14 (E14) mice, 1 day before palate closure, to describe the relationship between growth of the lower jaw/tongue complex versus genotype of the embryo. METHODS: Whole heads, isolated from E14.25, E14.5 and E14.75 wild-type and homozygous mutant embryos, were fixed in Bouin's solution, embedded in paraffin, and serially sectioned. Mid-sagittal sections, stained with toluidine blue, were used to estimate growth of both tongue and lower jaw (Meckel's cartilage length) during a 12-hr period preceding palate closure. RESULTS: In control embryos, the largest increase in Meckel's cartilage length occurred between E14.5 and E14.75. Compared to control, the mean Meckel's cartilage length in the mutant was similar at E14.25, but was significantly less at E14.5 and E14.75. Absolute tongue size in control embryos increased linearly during this period of E14.25 to E14.75. Relative to the rapidly growing Meckel's cartilage, however, relative tongue size in control embryos actually decreased over time. Absolute tongue size in the mutant was not significantly different from that of control at any of the embryonic stages examined, however, relative tongue size in the mutant was significantly greater at E14.75 compared to control. CONCLUSION: Mandibular growth retardation, coupled with relative macroglossia in E14 Dmm/Dmm mice, suggests that the concerted development of the palate and lower jaw complex in the mutant is aberrant. Detection of micrognathia and pseudomacroglossia in homozygotes, before the time of palate closure, supports the hypothesis that a relationship exists between growth retardation of Meckel's cartilage and malformation of the secondary palate, as predicted by the Pierre-Robin sequence.
