Abstract
BackgroundApically located tight junctions in airway epithelium perform a fundamental role in controlling macromolecule migration through paracellular spaces. Alterations in their expression may lead to disruptions in barrier integrity, which subsequently facilitates entry of potential bacterial and other pathogens into the host. Furthermore, there is emerging evidence that the barrier integrity of the airway in certain airway inflammatory diseases may be altered. However, there is little consensus on the way this is assessed and measured and the type of cells used to achieve this.MethodsHere, we assessed four fixation methods including; (i) 4% (v/v) paraformaldehyde; (ii) 100% methanol; (iii) acetone or; (iv) 1:1 methanol: acetone. Pre-extraction with Triton X-100 was also performed and assessed on cells prior to fixation with either methanol or paraformaldehyde. Cells were also permeabilized with 0.1% (v/v) Saponin in 1× TBS following fixation and subsequently stained for tight junction proteins. Confocal microscopy was then used to visualise, compare and evaluate staining intensity of the tight junctional complexes in order to determine a standardised workflow of reproducible staining.ResultsPositive staining was observed following methanol fixation for claudin-1 and ZO-1 tight junction proteins but no staining was detected for occludin in 16HBE14o- cells. Combinatorial fixation with methanol and acetone also produced consistent positive staining for both occludin and ZO-1 tight junction proteins in these cells. When assessed using primary cells cultured at air-liquid interface, similar positive staining for claudin-1 and ZO-1 was observed following methanol fixation, while similar positive staining for occludin and ZO-1 was observed following the same combinatorial fixation with methanol and acetone.ConclusionsThe present study demonstrates the importance of a personalised approach to optimise staining for the visualisation of different tight junction proteins. Of significance, the workflow, once optimised, can readily be translated into primary airway epithelial cell air-liquid interface cultures where it can be used to assess barrier integrity in chronic lung diseases.
Highlights
Located tight junctions in airway epithelium perform a fundamental role in controlling macromolecule migration through paracellular spaces
Data generated showed that use of saponin slightly increased junctional staining post paraformaldehyde fixation for zona occludens-1 (ZO-1), but positive staining was highly variable within samples
In the current study, we found that fixation of 16HBE14o- cells for the tight junction proteins ZO-1, claudin-1 and occludin require different fixation protocols for reliable staining patterns
Summary
Located tight junctions in airway epithelium perform a fundamental role in controlling macromolecule migration through paracellular spaces. Alterations in their expression may lead to disruptions in barrier integrity, which subsequently facilitates entry of potential bacterial and other pathogens into the host. The airway epithelial layer remains the frontline of defence against pathogens, aeroallergens and noxious gases by establishing and maintaining a physical barrier The integrity of this layer is typically maintained by the presence of a range of junctional complexes including: tight junctions; adherens junctions; and desmosomes [1,2,3,4]. In association with the transmembrane tight junction proteins is the intracellular protein zona occludens-1 (ZO-1) [10] which act by anchoring the tight junction proteins to the cytoskeleton [13]
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