Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase

Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase

<p>Abstract</p> <p>Background</p> <p>Both (-) and (+)-naloxone attenuate inflammation-mediated neurodegeneration by inhibition of microglial activation through superoxide reduction in an opioid receptor-independent manner. Multiple lines of evidence have documented a pi...

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Main Authors: Wang Qingshan, Zhou Hui, Gao Huiming, Chen Shih-Heng, Chu Chun-Hsien, Wilson Belinda, Hong Jau-Shyong
Format: Article
Language:English
Published: BMC 2012-02-01
Series:Journal of Neuroinflammation
Subjects:
Neuroinflammation
Microglia
NADPH oxidase
Opioid receptor
Binding
Online Access:http://www.jneuroinflammation.com/content/9/1/32
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spelling doaj-fd9816884cce4044a2937603e9e58e202020-11-24T22:16:23ZengBMCJournal of Neuroinflammation1742-20942012-02-01913210.1186/1742-2094-9-32Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidaseWang QingshanZhou HuiGao HuimingChen Shih-HengChu Chun-HsienWilson BelindaHong Jau-Shyong<p>Abstract</p> <p>Background</p> <p>Both (-) and (+)-naloxone attenuate inflammation-mediated neurodegeneration by inhibition of microglial activation through superoxide reduction in an opioid receptor-independent manner. Multiple lines of evidence have documented a pivotal role of overactivated NADPH oxidase (NOX2) in inflammation-mediated neurodegeneration. We hypothesized that NOX2 might be a novel action site of naloxone to mediate its anti-inflammatory actions.</p> <p>Methods</p> <p>Inhibition of NOX-2-derived superoxide by (-) and (+)-naloxone was measured in lipopolysaccharide (LPS)-treated midbrain neuron-glia cultures and phorbol myristate acetate (PMA)-stimulated neutrophil membranes by measuring the superoxide dismutase (SOD)-inhibitable reduction of tetrazolium salt (WST-1) or ferricytochrome c. Further, various ligand (<sup>3</sup>H-naloxone) binding assays were performed in wild type and gp91<it><sup>phox-/- </sup></it>neutrophils and transfected COS-7 and HEK293 cells. The translocation of cytosolic subunit p47<it><sup>phox </sup></it>to plasma membrane was assessed by western blot.</p> <p>Results</p> <p>Both (-) and (+)-naloxone equally inhibited LPS- and PMA-induced superoxide production with an IC50 of 1.96 and 2.52 μM, respectively. Competitive binding of <sup>3</sup>H-naloxone with cold (-) and (+)-naloxone in microglia showed equal potency with an IC50 of 2.73 and 1.57 μM, respectively. <sup>3</sup>H-Naloxone binding was elevated in COS-7 and HEK293 cells transfected with gp91<sup><it>phox</it></sup>; in contrast, reduced <sup>3</sup>H-naloxone binding was found in neutrophils deficient in gp91<sup><it>phox </it></sup>or in the presence of a NOX2 inhibitor. The specificity and an increase in binding capacity of <sup>3</sup>H-naloxone were further demonstrated by 1) an immunoprecipitation study using gp91<sup><it>phox </it></sup>antibody, and 2) activation of NOX2 by PMA. Finally, western blot studies showed that naloxone suppressed translocation of the cytosolic subunit p47<sup><it>phox </it></sup>to the membrane, leading to NOX2 inactivation.</p> <p>Conclusions</p> <p>Strong evidence is provided indicating that NOX2 is a non-opioid novel binding site for naloxone, which is critical in mediating its inhibitory effect on microglia overactivation and superoxide production.</p> http://www.jneuroinflammation.com/content/9/1/32NeuroinflammationMicrogliaNADPH oxidaseOpioid receptorBinding
collection DOAJ
language English
format Article
sources DOAJ
author Wang Qingshan
Zhou Hui
Gao Huiming
Chen Shih-Heng
Chu Chun-Hsien
Wilson Belinda
Hong Jau-Shyong
spellingShingle Wang Qingshan
Zhou Hui
Gao Huiming
Chen Shih-Heng
Chu Chun-Hsien
Wilson Belinda
Hong Jau-Shyong
Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase
Journal of Neuroinflammation
Neuroinflammation
Microglia
NADPH oxidase
Opioid receptor
Binding
author_facet Wang Qingshan
Zhou Hui
Gao Huiming
Chen Shih-Heng
Chu Chun-Hsien
Wilson Belinda
Hong Jau-Shyong
author_sort Wang Qingshan
title Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase
title_short Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase
title_full Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase
title_fullStr Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase
title_full_unstemmed Naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of NADPH oxidase
title_sort naloxone inhibits immune cell function by suppressing superoxide production through a direct interaction with gp91<sup><it>phox </it></sup>subunit of nadph oxidase
publisher BMC
series Journal of Neuroinflammation
issn 1742-2094
publishDate 2012-02-01
description <p>Abstract</p> <p>Background</p> <p>Both (-) and (+)-naloxone attenuate inflammation-mediated neurodegeneration by inhibition of microglial activation through superoxide reduction in an opioid receptor-independent manner. Multiple lines of evidence have documented a pivotal role of overactivated NADPH oxidase (NOX2) in inflammation-mediated neurodegeneration. We hypothesized that NOX2 might be a novel action site of naloxone to mediate its anti-inflammatory actions.</p> <p>Methods</p> <p>Inhibition of NOX-2-derived superoxide by (-) and (+)-naloxone was measured in lipopolysaccharide (LPS)-treated midbrain neuron-glia cultures and phorbol myristate acetate (PMA)-stimulated neutrophil membranes by measuring the superoxide dismutase (SOD)-inhibitable reduction of tetrazolium salt (WST-1) or ferricytochrome c. Further, various ligand (<sup>3</sup>H-naloxone) binding assays were performed in wild type and gp91<it><sup>phox-/- </sup></it>neutrophils and transfected COS-7 and HEK293 cells. The translocation of cytosolic subunit p47<it><sup>phox </sup></it>to plasma membrane was assessed by western blot.</p> <p>Results</p> <p>Both (-) and (+)-naloxone equally inhibited LPS- and PMA-induced superoxide production with an IC50 of 1.96 and 2.52 μM, respectively. Competitive binding of <sup>3</sup>H-naloxone with cold (-) and (+)-naloxone in microglia showed equal potency with an IC50 of 2.73 and 1.57 μM, respectively. <sup>3</sup>H-Naloxone binding was elevated in COS-7 and HEK293 cells transfected with gp91<sup><it>phox</it></sup>; in contrast, reduced <sup>3</sup>H-naloxone binding was found in neutrophils deficient in gp91<sup><it>phox </it></sup>or in the presence of a NOX2 inhibitor. The specificity and an increase in binding capacity of <sup>3</sup>H-naloxone were further demonstrated by 1) an immunoprecipitation study using gp91<sup><it>phox </it></sup>antibody, and 2) activation of NOX2 by PMA. Finally, western blot studies showed that naloxone suppressed translocation of the cytosolic subunit p47<sup><it>phox </it></sup>to the membrane, leading to NOX2 inactivation.</p> <p>Conclusions</p> <p>Strong evidence is provided indicating that NOX2 is a non-opioid novel binding site for naloxone, which is critical in mediating its inhibitory effect on microglia overactivation and superoxide production.</p>
topic Neuroinflammation
Microglia
NADPH oxidase
Opioid receptor
Binding
url http://www.jneuroinflammation.com/content/9/1/32
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