Protocol detail

Histological Analysis of Mouse Brain

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Mice were perfused transcardially with PBS followed by PBS containing 4% paraformaldehyde (PFA) at day 5 p.i. Brain tissue was collected, post-fixed in 4% PFA overnight, and embedded in paraffin [28 (link)]. Brains were sectioned at 5 μm and stained with hematoxylin and eosin (H&E) to evaluate inflammation or meningitis. The paraffin-embedded slides were first deparaffinized on a hot plate followed by xylene treatment for 10 mins. Sections were then rehydrated gradually through different alcohol grades from 100 to 50%. Sections were then treated with hematoxylin for 1 min and excess stain was washed under running tap water. Subsequently, sections were dehydrated by passing through 50 to 95% ethanol. Sections were then stained with eosin stain for 30 s and washed with 95% ethanol twice. Further dehydration was carried out with 100% ethanol and xylene. Sections were mounted with Refrax mounting medium (Anatech Ltd., MI, USA) and observed under the upright light microscope (Nikon Eclipse 50i) and analyzed with Nikon imaging software (NIS, Nikon Corp. Tokyo, Japan).

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Bose A., Basu R., Maulik M, & Das Sarma J. (2018). Loss of Cx43-Mediated Functional Gap Junction Communication in Meningeal Fibroblasts Following Mouse Hepatitis Virus Infection. Molecular Neurobiology, 55(8), 6558-6571.

Publication 2018

Refrax mounting medium Eclipse 50i

Alcohol Brains Dehydration Embedded paraffin Eosin Ethanol Hematoxylin Inflammation Meningitis Mice Microscope light Paraffin Paraformaldehyde Stain Tissue Xylene

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Variable analysis

independent variables

Day 5 post-infection (p.i.)

dependent variables

Brain inflammation
Meningitis

control variables

Perfusion with PBS
Perfusion with 4% paraformaldehyde (PFA)
Overnight post-fixation in 4% PFA
Paraffin embedding
Sectioning at 5 μm
Hematoxylin and eosin (H&E) staining
Deparaffinization on hot plate and xylene treatment
Rehydration through alcohol grades
Hematoxylin staining for 1 min
Dehydration through alcohol grades
Eosin staining for 30 s
Further dehydration with 100% ethanol and xylene
Mounting with Refrax mounting medium
Observation under upright light microscope
Analysis with Nikon imaging software

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