We have previously shown that subjects exposed to acute hypobaric hypoxia display an erythrocyte membrane protein band 3 with an increased susceptibility to proteolytic degradation. We suggested it was due to an oxidative damage of band 3. We now report that exposure to hypobaric hypoxia followed by reoxygenation affects protein band 3 functions such as anion transport and binding of glyceraldehyde-3P-dehydrogenase. Transport capacity was assessed with the fluorescent probe 2-[N-(7-nitrobenz-2-oxa-1,3-diazol-4-yl)amino] ethanesulfonate (NBD-taurine). Binding capacity was evaluated from the activity of the membrane-associated enzyme. Healthy young men were exposed for 20 min to hypobaric hypoxia, simulating an altitude of 4,500 m above sea level and after recompression band 3 function was assessed. An inhibition of band 3 anion transport function and a decrease in the binding of glyceraldehyde-3P-dehydrogenase to band 3 were observed. Evidence is given supporting the hypothesis that functional alteration of band 3 is due to its oxidative modification originated as a consequence of the exposure to hypobaric hypoxia and further reoxygenation.
Arsenic has been associated with multiple harmful effects at the cellular level. Indirectly these defects could be related to impairment
of the integrity of the immune system, in particular in lymphoid population. To characterize the effect of Arsenic on redox status on this
population, copper smelter workers and arsenic unexposed donors were recruited for this study. We analyzed urine samples
and lymphocyte enriched fractions from donors to determinate arsenic levels and lymphocyte proliferation. Moreover, we studied the
presence of oxidative markers MDA, vitamin E and SOD activity in donor plasma. Here we demonstrated that in human beings
exposed to high arsenic concentrations, lymphocyte MDA and arsenic urinary levels showed a positive correlation with SOD activity,
and a negative correlation with vitamin E serum levels. Strikingly, lymphocytes from the arsenic exposed population respond to
a polyclonal stimulator, phytohemaglutinin, with higher rates of thymidine incorporation than lymphocytes of a control population.
As well, similar in vitro responses to arsenic were observed using a T cell line. Our results suggest that chronic
human exposure to arsenic induces oxidative damage in lymphocytes and could be considered more relevant than evaluation of T cell
surveillance.
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