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Fluorescence Staining of Neural Crest Cells Cultured on Hydrogels of Varying Stiffness

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Take adherent neural crest cell cultures grown on coverslips coated with hydrogels of varying stiffness. Wash the cells with buffer.

Add paraformaldehyde to fix the cells and preserve cellular morphology.

Wash the cells with buffer to remove any excess paraformaldehyde.

Next, add a non-ionic detergent to permeabilize the cell membranes.

Wash the cells with buffer to remove excess detergent.

Then, introduce a blocking solution to prevent non-specific binding.

Incubate the cells with a high-affinity filamentous actin probe that binds to actin filaments.

Wash the cells with buffer to remove any unbound probes.

Add a fluorescent nuclear dye to stain the nuclei, then wash with buffer to remove excess dye.

Apply mounting media to the coverslips and examine the stained cells under a fluorescence microscope.

Cells grown on stiffer hydrogels show increased actin filament formation and a more spread-out morphology than those grown on softer hydrogels.

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Fluorescence Staining of Neural Crest Cells Cultured on Hydrogels of Varying Stiffness

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