Microbiology Professor Sidelsky 2007
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Transcript of Microbiology Professor Sidelsky 2007
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Staining
MicrobiologyProfessor Sidelsky2007
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Part Two - StainingHow to Make a SmearStain with Simple StainStain with Gram StainAcid FastSpecialized Staining( Endospore
and Capsule)Negative Staining
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How to Make a Smear1. Label the frosted side of your
slide with your initials, the name of the organism, and the date.
Turn the slide over and draw an oval on the reverse side with a Sharpie
2. You are going to make the smear on the frosted side
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Broth Directions for making a smear
*****If you are using broth follow these directions Flame your inoculating loop. Use aseptic technique and remove the top of the culture
tube, flame the mouth or the culture tube, and dip the loop into the broth. Make sure that the loop is filled.
Transfer the loopful of broth and bacteria to the slide. Using a circular motion, spread the broth on the slide.
This is now a " smear" Allow the smear to dry When the smear has been allowed to " air dry" , pass the
smear through the flame to " heat fix" - Heat fixation causes the proteins and cell parts to coagulate and stick to the slide.
Let the slide cool.
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How to Make a Smear- Plate or Slant
*****If you are using colonies from a plate( Petri Dish) Place a drop of water on the slide. Using aseptic technique, " pick" a colony from the
Plate in order to study the cells that make up a colony
If you are using a slant Using a circular motion spread move the inoculating
loop in a circular motion in the drop of water. Start in the center of the drop and move in a circular motion to the outside of the drop. The objective is to have fewer cells on the outside of the circle.
Follow the directions from above Don't forget to " air dry" and to " heat fix" before
staining
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Simple StainSimple Stains- Crystal violet and
methylene blue1. Place a drop(s) of stain over the
smear. Make sure it covers the entire area of the smear. Leave the stain on the smear for one minute. Rinse with water from the bottle.
2. Refer to page 64 for cellular morphology.
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The Gram Stain Gram Stain- See Gram Stain Directions on separate page.
Please refer to pages 71-73 in your laboratory manual. All staining work is to be done at the sink Care should be taken to work directly over the sink Place drop(s) of crystal violet stain on the smear ( 1 minute) Rock or roll the slide to cover the area Use the water bottle to drip water down the slide
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Gram Stain ( II) Place drop(s) of iodine on the slide ( 1
minute) Place drops of alcohol on the slide 10
seconds ( KEY – do not leave on longer than 10 seconds or it will decolorize)
Place drop(s) of saffranin on the slide for 1 minute
Rinse with water from the bottle Let the slide air dry
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The Microbe Library – A great Resource
Animation on Gram Stainshttp://www.microbelibrary.org/ASMOnly/details.asp?id=2020&Lang
=
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Gram Stain( step by step)http://medic.med.uth.tmc.edu/path/
grampro.htmhttp://www.lumen.luc.edu/lumen/De
ptWebs/microbio/med/gram/tech.htm
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Typical Gram Stainhttp://www.uphs.upenn.edu/bug
drug/antibiotic_manual/Gram3.htm
http://www.uphs.upenn.edu/bugdrug/antibiotic_manual/Gramstains/small/tocframeset1.htm
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Staphylococcus
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Gram Negative bacteria
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Gram Stain animations and information
http://www.microbiologybytes.com/video/Gram.html
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Bacterial Cell Morphology
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Acid Fast Stains( Mycobacterium)
Acid- Fast Stain Carbol Fuschin Stain is a red stain that is soluble in a lipid
environment. The outer cell wall of the mycobacterium is mycolic acid
The stain can be absorbed by placing the stain over a beaker boiling water. Heat assists the stain inits penetration of the waxy cell wall
Cool and rinse with cool water Add acid- Alcohol drop by drop until the alcohol runs alost
clear. Rinse with water Counterstain by applying methylene blue for at least two
minutes
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Acid Fast Staining A shows cells that
are stained with methylene blue – These re non acid fast
B shows cells that are stained with carbol fuschin which is retained in the lipid cell walls
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Acid Fast
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Differential Staining( Spores) Add Malachite Green to slide and steam over a
beaker of boiling water ( beaker may be placed on a hot plate) If stain starts to evaporate, add additional stain. Stain should remain on for 2-3 minutes
Remove slides from hot plate and cool Rinse with water
Counter stain with Saffranin for a minute. Rinse with water
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Endospore structure
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Endospore
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Capsule stain Crystal violet is applied to the bacterial
smears The decolorizing agent is Copper sulfate(
20%) which washes the primary stain out of the capsule without removing the stain from the cell wall
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Capsule stain( Klebsiella pneumoniae and Streptococcus pneumoniae)
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Negative staining Place a drop of nigrosin on the end of a
slide- Use a plain slide Use the inoculating loop to mix some of
the bacterial culture with the drop of stain Use a clean slide. Hold at a 45o angle
against the drop. The drop will spread along this line
Push the slide away from the previously spread drop
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Negative staining
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Negative staining