Alan A. Brimfield scite author profile

Two mouse immunoglobulin GI monoclonal antibodies that bind to the trichothecene mycotoxin T-2 were prepared. These antibodies, designated 12C12 and 15H6, had affinities for T-2 of 3.5 x 106 and 5.8 x 107 liters/mol, respectively. A competitive inhibition enzyme immunoassay that employed these antibodies had a sensitivity for T-2 of 50 ng per assay. Both antibodies bound to the metabolite HT-2 but not to the related trichothecenes monoacetoxyscirpenol, diacetoxyscirpenol, deoxynivalenol, and deoxyverrucarol. Evidence is presented that T-2-protein conjugates inhibit protein synthesis in lymphoid cells and that this apparent immunotoxicity may be due to the release of T-2 from the protein carrier.

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Free radical production from the interaction of 2-chloroethyl vesicants (mustard gas) with pyridine nucleotide-driven flavoprotein electron transport systems

Brimfield

Mancebo

Mason

et al. 2009

Toxicology and Applied Pharmacology

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The biochemical sequelae to chloroethyl mustard exposure correspond very well to toxic processes initiated by free radicals. Additionally, mustard solutions contain spontaneously formed cyclic onium ions which produce carbon free radicals when reduced electrochemically. Therefore, we hypothesized that the onium ions of sulfur or nitrogen mustards might produce carbon free radicals upon being reduced enzymatically, and that these radicals might constitute a metabolic activation. We set out to document radical production using an in vitro metabolic system and electron paramagnetic resonance (EPR). Our system consisted of NADPH, one of several pyridine nucleotidedriven flavoprotein reductases, cytochrome c as a terminal electron acceptor, various sulfur or nitrogen mustards and the spin trap α-[4-pyridyl-1-oxide]-N-tert-butylnitrone in buffer. Reactions were started by adding the reductase to the other materials, vortexing and immediately transferring the mixture to a 10 mm EPR flat cell. Repeated scans on a Bruker ESP 300E EPR spectrometer produced a triplet of doublets with hyperfine splitting constants of a N = 15.483 G and a H = 2.512 G. The outcome supported our hypothesis that carbon-centered free radicals are produced when mustard-related onium ions are enzymatically reduced. The EPR results varied little with the chloroethyl compound used or with porcine or human cytochrome P450 reductase, the reductase domain of rat brain neuronal nitric oxide synthase or rat liver thioredoxin reductase. Our results offer new insight into the basis for mustard-induced vesication and the outcome of exposure to different mustards. The free radical model provides an explanation for similarities in the lesions arising from mustard exposure and energy-based lesions such as those from heat, ultraviolet and nuclear radiation as well as damage across tissue types such as skin, eyes or airway epithelium.

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Identification of products arising from the metabolism of cis- and trans-chlordane in rat liver microsomes in vitro: Outline of a possible metabolic pathway

Brimfield

Street

Chatfield

1978

Pesticide Biochemistry and Physiology

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Development of a monoclonal antibody based enzyme immunoassay method for analysis of maleic hydrazide

Harrison¹,

Brimfield²,

Nelson³

1989

J. Agric. Food Chem.

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Alan A. Brimfield

In Vitro Human Metabolism and Interactions of RepellentN,N-Diethyl-m-Toluamide

Preparation and characterization of monoclonal antibodies to the trichothecene mycotoxin T-2

Free radical production from the interaction of 2-chloroethyl vesicants (mustard gas) with pyridine nucleotide-driven flavoprotein electron transport systems

Identification of products arising from the metabolism of cis- and trans-chlordane in rat liver microsomes in vitro: Outline of a possible metabolic pathway

Development of a monoclonal antibody based enzyme immunoassay method for analysis of maleic hydrazide

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