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Glucose transporter 1 and monocarboxylate transporters 1, 2, and 4 localization within the glial cells of shark blood-brain-barriers
Indexado
WoS WOS:000302999600038
Scopus SCOPUS_ID:84857516757
DOI 10.1371/JOURNAL.PONE.0032409
Año 2012
Tipo artículo de investigación

Citas Totales

Autores Afiliación Chile

Instituciones Chile

% Participación
Internacional

Autores
Afiliación Extranjera

Instituciones
Extranjeras


Abstract



Although previous studies showed that glucose is used to support the metabolic activity of the cartilaginous fish brain, the distribution and expression levels of glucose transporter (GLUT) isoforms remained undetermined. Optic/ultrastructural immunohistochemistry approaches were used to determine the expression of GLUT1 in the glial blood-brain barrier (gBBB). GLUT1 was observed solely in glial cells; it was primarily located in end-feet processes of the gBBB. Western blot analysis showed a protein with a molecular mass of 50 kDa, and partial sequencing confirmed GLUT1 identity. Similar approaches were used to demonstrate increased GLUT1 polarization to both apical and basolateral membranes in choroid plexus epithelial cells. To explore monocarboxylate transporter (MCT) involvement in shark brain metabolism, the expression of MCTs was analyzed. MCT1, 2 and 4 were expressed in endothelial cells; however, only MCT1 and MCT4 were present in glial cells. In neurons, MCT2 was localized at the cell membrane whereas MCT1 was detected within mitochondria. Previous studies demonstrated that hypoxia modified GLUT and MCT expression in mammalian brain cells, which was mediated by the transcription factor, hypoxia inducible factor-1. Similarly, we observed that hypoxia modified MCT1 cellular distribution and MCT4 expression in shark telencephalic area and brain stem, confirming the role of these transporters in hypoxia adaptation. Finally, using three-dimensional ultrastructural microscopy, the interaction between glial end-feet and leaky blood vessels of shark brain was assessed in the present study. These data suggested that the brains of shark may take up glucose from blood using a different mechanism than that used by mammalian brains, which may induce astrocyte-neuron lactate shuttling and metabolic coupling as observed in mammalian brain. Our data suggested that the structural conditions and expression patterns of GLUT1, MCT1, MCT2 and MCT4 in shark brain may establish the molecular foundation of metabolic coupling between glia and neurons.

Revista



Revista ISSN
P Lo S One 1932-6203

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Disciplinas de Investigación



WOS
Biology
Multidisciplinary Sciences
Scopus
Sin Disciplinas
SciELO
Sin Disciplinas

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Publicaciones WoS (Ediciones: ISSHP, ISTP, AHCI, SSCI, SCI), Scopus, SciELO Chile.

Colaboración Institucional



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Autores - Afiliación



Ord. Autor Género Institución - País
1 Balmaceda-Aguilera, Carolina Mujer Universidad de Concepción - Chile
2 CAMPOS-ACEVEDO, CRISTIAN ANDRES Hombre Universidad de Concepción - Chile
3 CIFUENTES-DELGADO, MANUEL Hombre Univ Malaga - España
Universidad de Málaga - España
4 Peruzzo, Bruno Hombre Universidad Austral de Chile - Chile
5 Mack, Lauren Mujer Universidad de Concepción - Chile
6 TAPIA-AMARO, JUAN CARLOS Hombre Columbia Univ - Estados Unidos
Columbia University in the City of New York - Estados Unidos
Columbia University - Estados Unidos
7 OYARCE-MERICO, KARINA ALEJANDRA Mujer Universidad de Concepción - Chile
8 de los Angeles Garcia-Robles, Maria Mujer Universidad de Concepción - Chile
8 García, María Angeles Mujer Universidad de Concepción - Chile
9 NUALART-SANTANDER, FRANCISCO JAVIER Hombre Universidad de Concepción - Chile

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Financiamiento



Fuente
National Institute of General Medical Sciences
Fondo de Ciencia y Tecnologia (FONDECYT)
Ring of Research (PBCT)

Muestra la fuente de financiamiento declarada en la publicación.

Agradecimientos



Agradecimiento
The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. This work was supported by grants from Fondo de Ciencia y Tecnologia (FONDECYT 1100396 and 1100705) to FN and MAG, Ring of Research (PBCT ACT-02) to FN and MAG.

Muestra la fuente de financiamiento declarada en la publicación.