![]() Place a blotting paper on the slide (covering the smear) and saturate with carbolfuchsin to steam (for about 5 minutes).Allow the slide to dry (air dry) and then heat fix.Therefore, vegetative cells appear colorless, endospores stain red, and the background is black. Since the counterstain nigrosin is negatively charged, bacterial cells don’t easily take up the counterstain. When decolorized with acid alcohol, color washes off the vegetative cells, making them colorless. ![]() Principle of Dorner’s method for staining endosporesĬarbol fuchsin, when applied to a heat-fixed slide and heated, softens the structure of the bacterial spores and the basic fuchsin gets into the spores. It employed a lengthy heating step but resulted in differential staining of endospores and vegetative cells in the same sample. This method utilizes carbol fuchsin as primary stain, acid alcohol as decolorizer, and nigrosin as counterstain. Dorner’s Methodĭorner’s method is an alternative method for staining the endospores published by Dorner in 1922. ![]() Observe the bacteria under 1000X (oil immersion) total magnification. When viewed under 1000X of a light microscope, vegetative cells appear pink/red, and spores appear green. Rinse both sides of the slide to remove the secondary stain and blot the slide/ air dry.Stain the smear with safranin for 2 minutes.Rinse the slide thoroughly with tap water (to wash the malachite green from both sides of the microscope slide).Remove the blotting paper and allow the slide to cool to room temperature for 2 minutes.After 5 minutes, remove the slide from the rack using a clothespin.As the paper begins to dry, add a drop or two of malachite green to keep it moist, but don’t add so much at once that the temperature is appreciably reduced.Alternatively, the slide may be steamed over a container of boiling water. Saturate the blotting paper with malachite green stain solution and steam for 5 minutes, keeping the paper moist and adding more dye as required.Place a small piece of blotting paper (absorbent paper) over the smear and place the slide (smear side up) on a wire gauze on a ring stand.Prepare smears of organisms to be tested for the presence of endospores on a clean microscope slide and air dry it.Mature, free endospores should not be associated with vegetative bacteria and should be seen as green ellipses.the vegetative cells containing endospores should stain pink, while the spores should be seen as green ellipses.the vegetative cells should appear pink/red (i.e., the color of counterstain),.When visualized under microscopy, the cells should have three characteristics: When counter-stained with safranin, the vegetative cells take the color of safranin and appear red or pink, in contrast to the endospores that appear green. Once the endospore has absorbed the stain, it is resistant to decolorization, but the vegetative cells are easily decolorized with water (leaving the vegetative cells colorless). In this technique, heating acts as a mordant. When a heat-fixed smear is flooded with aqueous malachite green solution (the primary stain) and steamed, the heat assists the stain in penetrating through the spore. The method utilizes malachite green as the primary stain and safranin as a counterstain. Schaeffer and MacDonald Fulton in the 1930s. The technique was first described by Alice B. It is the most widely used technique for endospore staining. They appear as large refractile oval or spherical bodies within the mother cell. Endospores can also be demonstrated in unstained wet films under a phase-contrast microscope. Spores can generally be recognized on Gram’s stains (endospores do not stain and appear as refractile, nonstaining bodies). There are different methods for endospore staining. Other techniques of endospore staining Methods for endospore staining.Principle of Dorner’s method for staining endospores.
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