Abstract

Organophosphorus induced delayed neurotoxicity (OPIDN) has occurred in factory workers exposed in production of organophosphorus chemicals, which are used as plasticizers, lubricants, fire-retardants, or pesticides. Certain animal species (i.e., cats, dogs, cows, and chickens) are also susceptible, while others (rodents and some primates) are not. Although the chicken is the animal of choice to study this effect, it has many drawbacks. Our previous studies suggest the cat may be a better animal model to study the mechanisms of OPIDN. Although the mechanisms of OPIDN are not known, it is generally believed that the initial event is the phosphorylation of a protein (e.g. neurotoxic esterase, NTE) at the neurotoxicity target. We have postulated that subsequent changes in cellular Ca++ content leads to either enhanced phosphorylation of tubulin or a dissolution of neurofilaments. Both consequences lead to a disruption of axoplasmic transport and larger accumulations of Ca++ resulting in focal internodal swelling and Ca++ dependent proteolysis. Our preliminary studies have shown that in the cat brain, proteins relevant to OPIDN are concentrated in the synaptosomal fraction. Also, phosphorylation of brain synaptosomal protein with Gamma 32p-ATP was altered in cats as a result of TOCP treatment. We propose to study the effect of the neurotoxic organophosphorus esters (OP), TOCP, EPN, and DFP in comparison with the non-neurotoxic parathion on the normal phosphorylating mechanisms of neuronal proteins and on Ca++ concentrations of the axoplasm of neuronal organelles, as well as the isolation and characterization of tubulin and neurofilaments. In the beginning, we will examine the [Gamma 32p]ATP phosphorylatable proteins in brain and spinal cord synaptosomal cytosol and membrane fractions of normal cats. Optimum phosphorylating conditions will be established including the effect of calcium ions and calmodulin. The effect of in vivo protein phosphorylation will be determined. The effect of TOCP, EPN, DFP and parathion on slow and fast axoplasmic transport of radiolabeled proteins as well as NTE will be investigated. The characterization of tubulin and neurofilaments using electron microscopy as well as SDS-PAGE in TOCP treated cats will be studied. Electron microscopy will also be used to study cellular Ca++ levels in various organelles using x-ray energy spectrometry for the demonstration of calcium ions in swollen and degenerating axons. Finally, cats administered glucocorticoids in combination with OP's will be used to examine the reported benefit of glucocorticoid therapy in relation to the postulated mechanisms.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute for Occupational Safety and Health (NIOSH)
Type
Research Project (R01)
Project #
5R01OH002003-02
Application #
3420206
Study Section
Safety and Occupational Health Study Section (SOH)
Project Start
1985-05-01
Project End
1988-04-30
Budget Start
1986-05-01
Budget End
1987-04-30
Support Year
2
Fiscal Year
1986
Total Cost
Indirect Cost

  Institution

Name
Duke University
Department
Type
Schools of Medicine
DUNS #
071723621
City
Durham
State
NC
Country
United States
Zip Code
27705

  Publications

Violanti, John M; Fekedulegn, Desta; Gu, Ja Kook et al. (2018) Effort-reward imbalance in police work: associations with the cortisol awakening response. Int Arch Occup Environ Health 91:513-522
Suwita, E; Abou-Donia, M B (1990) Pharmacokinetics and metabolism of a single subneurotoxic oral dose of tri-o-cresyl phosphate in hens. Arch Toxicol 64:237-41
Carrington, C D; Lapadula, D M; Abou-Donia, M B (1989) Acceleration of anterograde axonal transport in cat sciatic nerve by diisopropyl phosphorofluoridate. Brain Res 476:179-82
Abou-Donia, M B; Lapadula, D M; Suwita, E (1988) Cytoskeletal proteins as targets for organophosphorus compound and aliphatic hexacarbon-induced neurotoxicity. Toxicology 49:469-77
Suwita, E; Lapadula, D M; Abou-Donia, M B (1986) Calcium and calmodulin stimulated in vitro phosphorylation of rooster brain tubulin and MAP-2 following a single oral dose of tri-o-cresyl phosphate. Brain Res 374:199-203
Nomeir, A A; Abou-Donia, M B (1986) Studies on the metabolism of the neurotoxic tri-o-cresyl phosphate. Synthesis and identification by infrared, proton nuclear magnetic resonance and mass spectrometry of five of its metabolites. Toxicology 38:1-13
Patton, S E; Lapadula, D M; Abou-Donia, M B (1986) Relationship of tri-O-cresyl phosphate-induced delayed neurotoxicity to enhancement of in vitro phosphorylation of hen brain and spinal cord proteins. J Pharmacol Exp Ther 239:597-605
Nomeir, A A; Abou-Donia, M B (1986) Studies on the metabolism of the neurotoxic tri-o-cresyl phosphate. Distribution, excretion, and metabolism in male cats after a single, dermal application. Toxicology 38:15-33
Suwita, E; Lapadula, D M; Abou-Donia, M B (1986) Calcium and calmodulin-enhanced in vitro phosphorylation of hen brain cold-stable microtubules and spinal cord neurofilament triplet proteins after a single oral dose of tri-o-cresyl phosphate. Proc Natl Acad Sci U S A 83:6174-8
Carrington, C D; Abou-Donia, M B (1985) Paraoxon reversibly inhibits neurotoxic esterase. Toxicol Appl Pharmacol 79:175-8

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