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Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries

P2X(7) receptor/channels in the retinal microvasculature not only regulate vasomotor activity, but can also trigger cells in the capillaries to die. While it is known that this purinergic vasotoxicity is dependent on the transmembrane pores that form during P2X(7) activation, events linking pore for...

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Autores principales: Shibata, Maho, Ishizaki, Eisuke, Zhang, Ting, Fukumoto, Masanori, Barajas-Espinosa, Alma, Li, Tong, Puro, Donald G.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6166475/
https://www.ncbi.nlm.nih.gov/pubmed/30288454
http://dx.doi.org/10.3390/vision2030025
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author Shibata, Maho
Ishizaki, Eisuke
Zhang, Ting
Fukumoto, Masanori
Barajas-Espinosa, Alma
Li, Tong
Puro, Donald G.
author_facet Shibata, Maho
Ishizaki, Eisuke
Zhang, Ting
Fukumoto, Masanori
Barajas-Espinosa, Alma
Li, Tong
Puro, Donald G.
author_sort Shibata, Maho
collection PubMed
description P2X(7) receptor/channels in the retinal microvasculature not only regulate vasomotor activity, but can also trigger cells in the capillaries to die. While it is known that this purinergic vasotoxicity is dependent on the transmembrane pores that form during P2X(7) activation, events linking pore formation with cell death remain uncertain. To better understand this pathophysiological process, we used YO-PRO-1 uptake, dichlorofluorescein fluorescence, perforated-patch recordings, fura-2 imaging and trypan blue dye exclusion to assess the effects of the P2X(7) agonist, benzoylbenzoyl-ATP (BzATP), on pore formation, oxidant production, ion channel activation, [Ca(2+)](i) and cell viability. Experiments demonstrated that exposure of retinal microvessels to BzATP increases capillary cell oxidants via a mechanism dependent on pore formation and the enzyme, NADPH oxidase. Indicative that oxidation plays a key role in purinergic vasotoxicity, an inhibitor of this enzyme completely prevented BzATP-induced death. We further discovered that vasotoxicity was boosted 4-fold by a pathway involving the oxidation-driven activation of hyperpolarizing K(ATP) channels and the resulting increase in calcium influx. Our findings revealed that the previously unappreciated pore/oxidant/K(ATP) channel/Ca(2+) pathway accounts for 75% of the capillary cell death triggered by sustained activation of P2X(7) receptor/channels. Elucidation of this pathway is of potential therapeutic importance since purinergic vasotoxicity may play a role in sight-threatening disorders such as diabetic retinopathy.
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spelling pubmed-61664752019-09-01 Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries Shibata, Maho Ishizaki, Eisuke Zhang, Ting Fukumoto, Masanori Barajas-Espinosa, Alma Li, Tong Puro, Donald G. Vision (Basel) Article P2X(7) receptor/channels in the retinal microvasculature not only regulate vasomotor activity, but can also trigger cells in the capillaries to die. While it is known that this purinergic vasotoxicity is dependent on the transmembrane pores that form during P2X(7) activation, events linking pore formation with cell death remain uncertain. To better understand this pathophysiological process, we used YO-PRO-1 uptake, dichlorofluorescein fluorescence, perforated-patch recordings, fura-2 imaging and trypan blue dye exclusion to assess the effects of the P2X(7) agonist, benzoylbenzoyl-ATP (BzATP), on pore formation, oxidant production, ion channel activation, [Ca(2+)](i) and cell viability. Experiments demonstrated that exposure of retinal microvessels to BzATP increases capillary cell oxidants via a mechanism dependent on pore formation and the enzyme, NADPH oxidase. Indicative that oxidation plays a key role in purinergic vasotoxicity, an inhibitor of this enzyme completely prevented BzATP-induced death. We further discovered that vasotoxicity was boosted 4-fold by a pathway involving the oxidation-driven activation of hyperpolarizing K(ATP) channels and the resulting increase in calcium influx. Our findings revealed that the previously unappreciated pore/oxidant/K(ATP) channel/Ca(2+) pathway accounts for 75% of the capillary cell death triggered by sustained activation of P2X(7) receptor/channels. Elucidation of this pathway is of potential therapeutic importance since purinergic vasotoxicity may play a role in sight-threatening disorders such as diabetic retinopathy. MDPI 2018-06-25 /pmc/articles/PMC6166475/ /pubmed/30288454 http://dx.doi.org/10.3390/vision2030025 Text en © 2018 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Shibata, Maho
Ishizaki, Eisuke
Zhang, Ting
Fukumoto, Masanori
Barajas-Espinosa, Alma
Li, Tong
Puro, Donald G.
Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries
title Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries
title_full Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries
title_fullStr Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries
title_full_unstemmed Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries
title_short Purinergic Vasotoxicity: Role of the Pore/Oxidant/K(ATP) Channel/Ca(2+) Pathway in P2X(7)-Induced Cell Death in Retinal Capillaries
title_sort purinergic vasotoxicity: role of the pore/oxidant/k(atp) channel/ca(2+) pathway in p2x(7)-induced cell death in retinal capillaries
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6166475/
https://www.ncbi.nlm.nih.gov/pubmed/30288454
http://dx.doi.org/10.3390/vision2030025
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