A Phospholipase A2-Related Snake Venom (from Crotalus durissus terrificus) Stimulates Neuroendocrine and Immune Functions: Determination of Different Sites of Action*

Author:

Chisari Andrea12,Spinedi Eduardo1,Voirol Marie-Jeanne3,Giovambattista Andrés12,Gaillard Rolf C.3

Affiliation:

1. Neuroendocrine Unit (A.C., E.S., A.G.), UNLP, 1900 La Plata, Argentina

2. Multidisciplinary Institute on Cell Biology, 1900 La Plata, Argentina; School of Exact Sciences (A.C., A.G.), UNLP, 1900 La Plata, Argentina

3. Division of Endocrinology and Metabolism (M.-J.V., R.C.G.), University Hospital, CH 1011 Lausanne, Switzerland

Abstract

Abstract Immune neuroendocrine interactions are vital for the individual’s survival in certain physiopathological conditions, such as sepsis and tissular injury. It is known that several animal venoms, such as those from different snakes, are potent neurotoxic compounds and that their main component is a specific phospholipase A type 2 (PLA2). It has been described recently that the venom from Crotalus durissus terrificus [snake venom (SV), in the present study] possesses some cytotoxic effect in different in vitro and in vivo animal models. In the present study, we investigated whether SV and its main component, PLA2 (obtained from the same source), are able to stimulate both immune and neuroendocrine functions in mice, thus characterizing this type of neurotoxic shock. For this purpose, several in vivo and in vitro designs were used to further determine the sites of action of SV-PLA2 on the hypothalamo-pituitary-adrenal (HPA) axis function and on the release of the pathognomonic cytokine, tumor necrosis factor α (TNFα), of different types of inflammatory stress. Our results indicate that SV (25 μg/animal) and PLA2 (5 μg/animal), from the same origin, stimulate the HPA and immune axes when administered (ip) to adult mice; both preparations were able to enhance plasma glucose, ACTH, corticosterone (B), and TNFα plasma levels in a time-related fashion. SV was found to activate CRH- and arginine vasopressin-ergic functions in vivo and, in vitro, SV and PLA2 induced a concentration-related (0.05–10 μg/ml) effect on the release of both neuropeptides. SV also was effective in changing anterior pituitary ACTH and adrenal B contents, also in a time-dependent fashion. Direct effects of SV and PLA2 on anterior pituitary ACTH secretion also were found to function in a concentration-related fashion (0.001–1 μg/ml), and the direct corticotropin-releasing activity of PLA2 was additive to those of CRH and arginine vasopressin; the corticotropin-releasing activity of both SV and PLA2 were partially reversed by the specific PLA2 inhibitor, manoalide. On the other hand, neither preparation was able to directly modify spontaneous and ACTH-stimulated adrenal B output. The stimulatory effect of SV and PLA2 on in vivo TNFα release was confirmed by in vitro experiments on peripheral mononuclear cells; in fact, both PLA2 (0.001–1 μg/ml) and SV (0.1–10 μg/ml), as well as concavalin A (1–100 μg/ml), were able to stimulate TNFα output in the incubation medium. Our results clearly indicate that PLA2-dependent mechanisms are responsible for several symptoms of inflammatory stress induced during neurotoxemia. In fact, we found that this particular PLA2-related SV is able to stimulate both HPA axis and immune functions during the acute phase response of the inflammatory processes.

Publisher

The Endocrine Society

Subject

Endocrinology

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