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Gram Stain HD Animation

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    The Gram Stain is the most
    widely employed staining method
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    in microbiology.
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    It is a differential stain because
    it divides bacteria into 2 classes:
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    gram positive and gram negative.
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    In the first step of the gram stain
    procedure,
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    cells from a fresh culture
    are transferred to a clean slide
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    and allowed to dry.
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    If the cells are on an augur plate,
    they should first be transferred
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    to a liquid medium for dilution.
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    The cells should form a thin,
    barely visible film.
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    This can be achieved
    by smearing cells
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    obtained from the surface
    of an augur medium
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    or from a liquid culture.
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    Fresh cultures must be used
    because as cells age,
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    they lose their ability
    to retain the stain.
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    The cells are then fixed to the slide
    by passing slightly
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    above the flame of a Bunsen burner.
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    After passing above the flame,
    the slide should feel warm
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    when touched to the back of the hand;
    but should not be too hot.
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    The fixed cells are then stained
    with the basic dye, crystal violet,
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    for 30 to 40 seconds.
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    The slide is then rinsed with water
    to remove excess stain.
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    At this point, all cells appear purple
    under the microscope.
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    Next, a solution of Grams iodine
    is added and retained on the slide
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    for about 1 minute.
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    The iodine combines
    with the crystal violet
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    to form a dye-iodine complex,
    thereby decreasing its solubility
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    within the cell.
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    At this point,
    the cells still appear purple.
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    The cells are then de-colorized
    by washing with ethanol or acetone.
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    This is the differential step.
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    Gram positive bacteria retain
    the crystal violet,
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    whereas gram negative bacteria do not.
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    The ethanol or acetone
    should be added dropwise
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    with the slide tilted at an angle
    until the drop coming off
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    the edge of the slide
    just starts to become colorless.
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    Even gram positive cells can lose
    the crystal violet iodine complex
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    during prolonged excessive
    de-coloration.
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    Excess ethanol is then
    washed off with water.
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    When viewed under the microscope,
    gram positive cells appear purple
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    and gram negative cells are colorless.
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    Finally, the rinsed cells are covered
    with the counter stain safranin
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    for 20 to 30 seconds.
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    This stains the gram negative bacteria
    pink.
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    After rinsing with water,
    the slide is dried with filter paper.
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    When viewed microscopically,
    the gram positive bacteria are purple
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    and the gram negative bacteria are pink.
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    Generally, the gram stain correlates
    with the cell wall structure
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    among the bacteria.
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    The ethanol is thought to shrink
    the thick peptidoglycan
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    in gram positive cells,
    thus retaining the dye.
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    The thick dehydrated
    peptidoglycan layer
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    of gram positive bacteria
    appears to be a permeability barrier
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    preventing the loss
    of the crystal violet iodine complex.
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    In contrast, the peptidoglycan
    in gram negative bacteria is very thin,
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    and has large pores.
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    Ethanol may extract lipids
    and increase the porosity
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    thus removing the crystal violet
    iodine complex.
Title:
Gram Stain HD Animation
Video Language:
English
Duration:
03:23
CaptioningWorkspace edited English subtitles for Gram Stain HD Animation
CaptioningWorkspace edited English subtitles for Gram Stain HD Animation
CaptioningWorkspace edited English subtitles for Gram Stain HD Animation
CaptioningWorkspace edited English subtitles for Gram Stain HD Animation

English subtitles

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