M3: Staining Flashcards
Gram Staining overview
- discovered in 1884 by Hans Christian Gram
- differential stain that divides bacteria into 2 categories (Gram-positive and Gram-negative) based on their interactions with crystal violet & iodine dyes
- process: add crystal violet and iodine die, then wash with alcohol, re-dye with Safranin (pink)
Gram-positive bacteria
- has thick cell wall with overlapping peptidoglycan layers
- peptidoglycan traps crystal violet & iodine inside cell, doesn’t let it leave when washed with alcohol, keeping it from absorbing Safranin dye
- -> stained cell appears purple
Gram-negative bacteria
- thin peptidoglycan layer in cell wall, surrounded by outer membrane of lipopolysaccharides
- thin peptidoglycan layer / membrane doesn’t retain crystal violet & iodine once washed with alcohol, absorbs pink Safranin dye afterwards
- -> stained cell appears pink
dyes used for Gram-staining (3)
- crystal violet
- iodine
- safranin
disadvantage of Gram-staining
cells must be attached tightly to glass slide so they are not lost during washing –> process of attaching them kills the cells, so can’t examine cell’s motility as part of Gram-stain
decolorization wash
final step of Gram-staining: wash sample with alcohol, which removes crystal violet & iodine from gram-negative cells
heat fixation
- method of attaching cells to slide
- process: place sample on slide, then pass slide through flame until all liquid evaporates
chemical fixation
uses paraformaldehyde, ethanol, or methanol to attach cells to slide
differential stain
technique separating specimens into subgroups
wet mount
- method of preparing live samples for viewing
- process: prepare small liquid culture containing microorganism, put one drop on slide, cover slide with glass coverslip (protects objective and keeps sample in place)
simple staining
- used to quickly observe size/shape/arrangement of cells
- process: use positively charged dye (e.g. methylene blue, crystal violet, safranin, fuchsin) to bind and stain the negatively charged membrane of microorganism
negative staining
- stain everything except micro-organism
- process: use negatively charged dye (nigrosin aka india ink) –> repelled by cell membrane
- mildly invasive, may kill micro-org or not
- contraindicated for pathogenic samples
acid-fast staining
- aka Ziehl-Neelsen stain
- differential stain, used on bacterial strains with high degree of resistance to decolorization (most commonly mycobacterium tuberculosis)
- process: stain cells red with carbolfuchsin dye, then counterstain with methylene blue –> acid-fast bacteria (what looking for) stay red, others go blue
giemsa
- differential stain, often used clinically
- combined with wrights stain to test for bacteria w/in blood smears
- human blood cells = purple, bacterial cells (e.g. malaria) = pink
pathogen causing TB
mycobacterium tuberculosis
