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Nitric oxide from inflammatory origin impairs neural stem cell proliferation by inhibiting epidermal growth factor receptor signaling

Author: Alvarez-Buylla
Alvaro
Ana I. Santos
Ana S. LourenÃ§o
AntÃ³nio F. AmbrÃ³sio
Arvidsson
Bal-Price
Batchelor
Beckman
Beltran
Ben-Hur
Benraiss
Bergsland
Boje
Bruno P. Carreira
Buck
Butovsky
Cacci
Caetana M. Carvalho
Calabrese
Calabrese
Cappella
Carreira
Carreira
Chao
Chehrehasa
Covacu
Curtis
Davalos
Dawson
Dawson
Doetsch
Ekdahl
Ekdahl
Eriksson
Estrada
Gage
Galea
Giulian
Green
Guix
Hanafy
Ignarro
InÃªs M. AraÃºjo
Iosif
Ischiropoulos
Keefer
Kempermann
Kettenmann
Keynes
Lane
Lowenstein
Madhusoodanan
Maria I. Morte
Matarredona
Ming
Misko
Moncada
Monje
Monje
Monteiro
Moreno-Lopez
Murillo-Carretero
Murillo-Carretero
Murphy
Nathan
Nimmerjahn
Ormerod
Packer
Parent
Pryor
Radi
Reynolds
Rock
Salvemini
Saura
Sierra
Szabo
Taupin
Torroglosa
Uc
Vallieres
Walton
Zhang
Zhang
Zhang
Publication venue: 'Frontiers Media SA'
Publication date: 01/01/2014
Field of study

Neuroinflammation is characterized by activation of microglial cells, followed by production of nitric oxide (NO), which may have different outcomes on neurogenesis, favoring or inhibiting this process. In the present study, we investigated how the inflammatory mediator NO can affect proliferation of neural stem cells (NSCs), and explored possible mechanisms underlying this effect. We investigated which mechanisms are involved in the regulation of NSC proliferation following treatment with an inflammatory stimulus (lipopolysaccharide plus IFN-gamma), using a culture system of subventricular zone (SVZ)-derived NSCs mixed with microglia cells obtained from wild-type mice (iNOS(+/+)) or from iNOS knockout mice (iNOS(-/-)). We found an impairment of NSC cell proliferation in iNOS(+/+) mixed cultures, which was not observed in iNOS(-/-) mixed cultures. Furthermore, the increased release of NO by activated iNOS(+/+) microglial cells decreased the activation of the ERK/MAPK signaling pathway, which was concomitant with an enhanced nitration of the EGF receptor. Preventing nitrogen reactive species formation with MnTBAP, a scavenger of peroxynitrite (ONOO-), or using the ONOO- degradation catalyst FeTMPyP cell proliferation and ERK signaling were restored to basal levels in iNOS(+/+) mixed cultures. Moreover, exposure to the NO donor NOC-18 (100 mu M), for 48 h, inhibited SVZ-derived NSC proliferation. Regarding the antiproliferative effect of NO, we found that NOC-18 caused the impairment of signaling through the ERK/MAPK pathway, which may be related to increased nitration of the EGF receptor in NSC. Using MnTBAP nitration was prevented, maintaining ERK signaling, rescuing NSC proliferation. We show that NO from inflammatory origin leads to a decreased function of the EGF receptor, which compromised proliferation of NSC. We also demonstrated that NO-mediated nitration of the EGF receptor caused a decrease in its phosphorylation, thus preventing regular proliferation signaling through the ERK/MAPK pathway.Foundation for Science and Technology, (FCT, Portugal); COMPETE; FEDER [PEst-C/SAU/LA0001/2013-2014, PEst-OE/EQB/LA0023/2013-2014, PTDC/SAU-NEU/102612/2008, PTDC/NEU-OSD/0473/2012]; FCT, Portugal [SERH/BPD/78901/2011, SERH/BD/38127/2007, SFRH/BD/77903/2011, SFRH/BD/79308/2011]info:eu-repo/semantics/publishedVersio

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