Background/aims: The colonic H, K ATPase (HKA2) is a heterodimeric membrane protein that exchanges luminal K for intracellular H and is involved in maintaining potassium homeostasis. Under homeostatic conditions, the colonic HKA2 remains inactive, since most of the potassium is absorbed by the small intestine. In diarrheal states, potassium is secreted and compensatory potassium absorption becomes necessary. This study proposes a novel mechanism whereby the addition of penicillin G sodium salt (penG) to colonic crypts stimulates potassium uptake in the presence of intracellular nitric oxide (NO), under sodium-free (0-Na) conditions.

Methods: Sprague Dawley rat colonic crypts were isolated and pHi changes were monitored through the ammonium prepulse technique. Increased proton extrusion in 0-Na conditions reflected heightened H, K ATPase activity. Colonic crypts were exposed to penG, L-arginine (a NO precursor), and N-nitro l-arginine methyl ester (L-NAME, a NO synthase inhibitor).

Results: Isolated administration of penG significantly increased H, K ATPase activity from baseline, p 0.0067. Co-administration of arginine and penG in 0-Na conditions further upregulated H, K ATPase activity, p <0.0001. Crypt perfusion with L-NAME and penG demonstrated a significant reduction in H, K ATPase activity, p 0.0058.

Conclusion: Overall, acute exposure of colonic crypts to penG activates the H, K ATPase in the presence of NO. This study provides new insights into colonic potassium homeostasis.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8095381PMC
http://dx.doi.org/10.33594/000000305DOI Listing

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