Labs 5-8 Flashcards

1
Q

Goals in Preparing a Good Smear

A
  • Causes the cells to adhere to the microscope slide
  • Ensures shrinkage of cells does not occur
  • Prepare thick smears so that individual cells are visible
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2
Q

Steps for Preparing a Smear

A
  • Wash slide(s)
  • Label slide(s) and make a target circle
  • Flame wire loop and then use it to transfer specimen to slide
  • Flame rim of test tube (if used) and wire loop
  • If using slant culture, add two small drops of water to the specimen
  • Spread organism over target circle
  • Allow slide(s) to dry by normal evaporation
  • After completely dry, pass slide over the flame of a Bunsen Burner several times, but avoid prolonged heating
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3
Q

Reasons for Heating a Smear

A
  • Causes bacteria to stick to the slide (denatures protein)

- Kills bacteria so they are no longer hazardous

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4
Q

Simple Staining

A

The use of single stain to color a bacterial cell; creates a contrast between a cell and its background

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5
Q

Simple Staining Procedure

A
  • Use positively charged (cationic) dyes (methylene blue, basic fuchsin, crystal violet), which have color-bearing ions or chromophores
  • Bacteria are negatively charged so dye is attracted and sticks to them
  • Time ranges from 30 seconds to 2 minutes depending on the type of dye used
  • After required time, smear is washed off, blotted dry, and examined under oil immersion
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6
Q

Obtainable Information from a Simple Stain

A
  • Shape and sometimes size (shrinkage possible)
  • Surface structures are sometimes visible
  • Arrangement of cells: can help identify type
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7
Q

Differential Staining

A

Takes advantage of the fact that cells or structures within cells display dissimilar staining reactions that can be distinguished by the use of different dyes

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8
Q

Gram Stain

A

Helps identify cell wall:

  • Gram positive: thick, peptidoglycan cell wall; stains purple
  • Gram negative: thin, peptidoglycan cell wall; stains pink
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9
Q

Gram Staining Procedure

A
  • Primary (initial) Stain: crystal violent for 20 seconds
  • Wash slide with water
  • Mordant: helps stain stick better to gram positive cells; Gram’s iodine for 1 minute
  • Decolorization: washes stain, removing any color from gram negative cells; Ethyl alcohol until colorless (20-30 seconds)
  • Wash slide briefly with water
  • Counterstain: stains gram negative cells without changing gram positive stain; Safranin for 1 minute
  • Wash off slide with water and allow slide to dry
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10
Q

Acid Fast Stain (Ziehl Neelsen Method)

A

A differential stain used for identifying mycolic acid containing mycoplasms - Mycobacterium and some Nocardia

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11
Q

Mycolic Acid

A

Waxy cell wall material; complex lipid composed of fatty acids and fatty alcohols that have hydrocarbon chains up to 80 carbons in length; significantly affects the staining properties of mycoplasms and prevents them from being stained by many routinely used stains

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12
Q

Aced Fast Staining Procedure

A
  • Primary Stain: Carbolfuchsin (mixed with phenol, necessary for dye to penetrate waxy cell wall) heated for 5 minutes
  • Heat acts as a mordant (makes stain complex more permeable to the mycolic acid)
  • Wash with water
  • Decolorization: Acid-alcohol for 1 minute; does not remove the entrapped stain (acid-fast cells); cells not containing mycolic acid are easily decolorized (non-acid-fast)
  • Rinse breifly with water
  • Counterstain: methylene blue for 30 seconds; makes non-acid-fast cells visible
  • Wash briefly with water then allow to dry
  • acid fast appear deep red; non-acid-fast appear blue
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13
Q

Gram Stain Results

A
  • B. subtilis: rod-shaped gram positive
  • S. epidermidis: round gram positive; staphylococcus
  • S. marcesens: rod-shaped gram negative
  • S. aureus: gram-positive staphylococcus
  • E. coli: gram-negative bacillus
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14
Q

Acid Fast Results

A
  • S. epidermidis: acid-fast negative staphylococcus
  • S. aureus: acid-fast negative staphylococcus
  • M. smegmatis: acid-fast positive bacillus
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