The differentiation medium is replaced by a simpler medium (‘dono

The differentiation medium is replaced by a simpler medium (‘donor buffer’) containing DMEM+25 mM HEPES and 0.1% bovine serum albumin without the differentiating factors for permeability assays. These assays are of short duration

(30 min) and therefore the lack of differentiation factors does not significantly affect the resolution of drug permeation across the PBEC monolayer. In a different PBEC model, Nitz et al. (2003) reported that serum-derived factors destabilised tight junction protein LY2835219 mw strands after tight junctions were established. The present model also avoids using serum after tight junctions are stabilised. Monocultured PBECs in this model are flat cells with a broadly elongate cobblestone-shaped morphology. The more cobblestone morphology could be an effect of hydrocortisone

treatment Selleck Buparlisib as suggested by Förster et al. (2005) or reflect the absence in monoculture of soluble factors released by astrocytes that influence the in vivo morphology of the BBB. Brain capillary endothelial cells in vivo are closely associated with several cell types within the neurovascular unit ( Abbott et al., 2006) including pericytes ( Daneman et al., 2010 and Lai and Kuo, 2005), astrocytes ( Abbott, 2002 and Abbott et al., 2006), perivascular macrophages ( Zenker et al., 2003) and neurons ( Schiera, 2003). Numerous studies have shown that each of these cell types can induce aspects of BBB phenotype when co-cultured with brain endothelial cells, with induction by astrocytes being the most fully documented, and astrocytes the most common cell type used to induce BBB features in co-cultured in vitro BBB models ( Abbott et al., 2006). However, it was not clear which cell type exerts the click here strongest influence in vivo, or how BBB induction occurs during CNS development. Recent studies using a combination of genetically engineered animals and cell culture have provided a clearer developmental sequence, showing initial BBB induction by neural progenitor

cells at the time of vascular ingrowth into the neural tube (angiogenesis), followed by progressive maturation of the BBB phenotype involving influences first from pericytes and later from astrocytes (Armulik et al., 2010, Daneman et al., 2010, Paolinelli et al., 2011 and Thanabalasundaram et al., 2011). Pericytes cause upregulation of key BBB features such as tight junction protein expression and organisation, and expression of nutrient transporters such as Glut-1/SLC2A1, while downregulating ‘default’ features characteristic of peripheral endothelial cells such as leucocyte adhesion molecule expression and vesicle trafficking (Daneman et al., 2010). Astrocytes, which mature later, then refine the BBB phenotype further, especially by upregulation of efflux transporters (Daneman et al., 2010); they also appear able to induce the expression of a greater range of BBB-specific genes than pericytes (Nag, 2011).

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