Staining Flashcards

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1
Q

What is gram staining?

A
  • invented by Hans Christian gram in 1884
  • it allows identification of a bacterial cell from gram positive and gram negative
  • gram positive bacteria have a thicker peptidoglycan cell wall and trap more of a crystal video stain and will appear purple under the microscope
  • gram negative bacteria have thinner peptidoglycan cell walls and cannot trap crystal violet stain, a counter stain called safranin can confirm their identity and show as pink/red
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2
Q

Why is gram staining important in medicine?

A
  • Penicillin is more effective at stopping the growth of the thick cell wall of gram positive bacteria
  • penicillin is effective in killing gram positive bacteria but penicillin is less effective at killing gram negative bacteria as they have a thinner cell wall
  • makes it possible to determine whether to treat a bacterial infection with penicillin or a different antibiotic
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3
Q

What is the procedure of gram staining?

A
  • Heat a sample of bacteria on a slide with a Bunsen burner so the bacteria cannot be washed away
  • apply Crystal Violet stain (floods slide) to make them appear purple
  • apply iodine to the sample, iodine binds to the crystal video stain
  • apply ethanol to wash away excess crystal violet stain and decolourise the rest of the slide
  • apply safranin to the sample, this is taken up by the bacteria cells, the gram negative bacteria show up pink/red, in gram positive this is hidden by the Crystal violet
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4
Q

Prepare slides - dry mount

A

-specimens cut into thin slices, they are either whole or cut (sectioned)
- specimen placed in centre of slide and coverslip

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5
Q

Prepare slides - wet mount

A

-Specimens suspended in a liquid (water or oil)
- coverslip placed at an angle

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6
Q

Prepare slides - squash slides

A

-Wet mount is first prepared, lens tissue is used to press down cover slip
- squash the sample between two slides to ensure there is no damage to the cover slip
- good for soft samples

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7
Q

Prepare slide - smear slides

A
  • Edge of slide used to smear sample
  • thin even coating
  • cover slip placed over sample
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8
Q

Staining - crystal violet/ methylene blue

A

-Positive charged dyes attracted to negative charged materials in cytoplasm
-stains cell components

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9
Q

Staining - Congo red/ nigrosin

A

-Negative charged dyes, repelled by negative charged cytosol
-cells left unstained stand out against stained background

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10
Q

Staining - gram stain technique

A
  • Separates bacteria into gram positive and negative, crystal violet and iodine put on slides, wash with ethanol
    -Gram positive will appear purpose and gram negative will lose stain due to thinner cell wall and will be stained with safranin (counterstain)
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11
Q

Staining - acid fast technique

A

-Differentiates species of mycobacterium from other bacteria
-Lipid solvent carries carbolfuchsin dye into cells
-Cells washed with acid solution, Mycobacterium is not affected and retain carbolfuchsin stain which is red, other bacteria lose the stain and are exposed to methylene blue

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12
Q

Stages involved in making pre prepared slides

A

FIXING - chemicals preserve specimens in as near natural state as possible
SECTIONING- specimens dehydrated with alcohol, placed in mould with wax to form hard block
STAINING - Specimens treated with multiple stains to show structues
MOUNTING - specimens are secured to a slide and cover slips placed on top

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13
Q

Risk management for slides

A

-Stains could be toxic
-CLEAPSS support for practical work in schools, provide student safety sheets that identify risks in schools, more slides are pre prepared in schools due to the danger of stains

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14
Q

Why is staining used?

A

All stains increase the contrast between cell structures and back-ground

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