Measurement of autophagy flux in the nervous system in vivo
Author
dc.contributor.author
Castillo, K.
Author
dc.contributor.author
Valenzuela, V.
es_CL
Author
dc.contributor.author
Matus, S.
es_CL
Author
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Nassif, M.
es_CL
Author
dc.contributor.author
Oñate, M.
es_CL
Author
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Fuentealba Escobar, Yerko
es_CL
Author
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Encina, G.
es_CL
Author
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Irrazabal, T.
es_CL
Author
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Parsons, G.
es_CL
Author
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Court, F. A.
es_CL
Author
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Schneider, B. L.
es_CL
Author
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Armentano, D.
es_CL
Author
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Hetz, G.
es_CL
Admission date
dc.date.accessioned
2014-01-09T18:11:50Z
Available date
dc.date.available
2014-01-09T18:11:50Z
Publication date
dc.date.issued
2013
Cita de ítem
dc.identifier.citation
Cell Death and Disease (2013) 4, e917
en_US
Identifier
dc.identifier.other
doi:10.1038/cddis.2013.421
Identifier
dc.identifier.uri
https://repositorio.uchile.cl/handle/2250/129121
General note
dc.description
Artículo de publicación ISI
en_US
Abstract
dc.description.abstract
Accurate methods to measure autophagic activity in vivo in neurons are not available, and most of the studies are based on
correlative and static measurements of autophagy markers, leading to conflicting interpretations. Autophagy is an essential
homeostatic process involved in the degradation of diverse cellular components including organelles and protein aggregates.
Autophagy impairment is emerging as a relevant factor driving neurodegeneration in many diseases. Moreover, strategies to
modulate autophagy have been shown to provide protection against neurodegeneration. Here we describe a novel and simple
strategy to express an autophagy flux reporter in the nervous system of adult animals by the intraventricular delivery of adenoassociated
viruses (AAV) into newborn mice. Using this approach we efficiently expressed a monomeric tandem mCherry-
GFP-LC3 construct in neurons of the peripheral and central nervous system, allowing the measurement of autophagy activity in
pharmacological and disease settings.