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Giemsa s azur eosine methylene blue solution

Manufactured by Merck Group
Sourced in Japan, Germany

Giemsa's azur eosine methylene blue solution is a laboratory staining solution used for the differential staining of blood cells and other cellular structures in microscopy. It is a combination of the dyes azure B, eosin Y, and methylene blue, which selectively stain different cellular components, enabling the visualization and identification of various cell types.

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2 protocols using giemsa s azur eosine methylene blue solution

1

Histopathological Analysis of Airway Inflammation

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All mice were used for pathological examination. The lungs were fixed by 10% neutral phosphate-buffered formalin. After separation of the lobes, 2-mm-thick blocks were taken for paraffin embedding. Embedded blocks were sectioned at a thickness of 3 µm, and then stained with May-Grunwald’s stain solution (Nacalai tesque, Inc, Kyoto, Japan) and Giemsa’s azur eosine methylene blue solution (Merck KGaA, Darmstadt, Germany) to evaluate the degree of infiltration of eosinophils and lymphocytes in the airway from proximal to distal. The sections were stained with periodic acid-Schiff (PAS) to evaluate the degree of proliferation of goblet cells in the bronchial epithelium. A pathological analysis of inflammatory cells and epithelial cells in the airway was performed using a Nikon ECLIPSE light microscope (Nikon Co., Tokyo, Japan). The degree of infiltration of eosinophils and lymphocytes in the airway or proliferation of goblet cells in the bronchial epithelium was graded in a blinded fashion: 0, not present; 1, slight; 2, mild; 3, moderate; 4, moderate to marked; 5, marked. ‘Slight’ was defined as less than 20% of the airway with eosinophilic inflammatory reaction or with goblet cells stained with PAS; ‘mild’ as 21–40%; ‘moderate’ as 41–60%; ‘moderate to marked’ as 61–80%; and marked as more than 80% of the airway [8 (link), 16 (link)].
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2

Cytospin Preparation and Staining

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Fifty thousand cells were subjected to a cytospin (Thermo Shandon, Pittsburgh, PA). The cytospin preparations were fixed with methanol and visualized with May-Gr€ unwald-Giemsa staining using the May-Gr€ unwald staining solution (Wako Pure Chemical Industries) and microscopy Giemsa's azur eosine methylene blue solution (Merck, Darmstadt, Germany) (Figure 4E).
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