stage 

1.Wash slide with soap
2. Label slide (circle in center of slide/place your name+ bacterial species) Flip slide over
3. Place drop of DW in circle if bacterial species is dry

4. Aseptic technique (sterilize loop 5 seconds till red hot, cool loop 30 seconds, aseptically open bacterial culture (open culture Using clam shell + gather bacteria on loop and transfer to slide) sterilize loop by heating loop in incinerator for 5 second and place on side of incinerator to cool)

5. Let slide dry of slide warmer 

6. Heat fix slide 

describes unevenly dispersed growth containing suspended aggregates and clumps

starch--amylase-->glucose + glucose

MR tests for presence of acid (methyl red)
VP tests for presence of acetoin (VP-A & VP-B)

have one hand on arm and one on base with microscope close to chest securely 

Aseptically prepare smear, air dry slide on slide warmer &heat fix

1. Flood smear with Crystal violet 

2. Rinse with DW above smear until clear

3. Flood swear with Gram's iodine 

4. Rinse with DW

5. Decolorize with Gram's alcohol holding slide at angle. Use dropper and place decolorizer to run through smear till clear

6. Rinse with DW

7. Counterstain with safranin 

8.Rinse with DW

9. Air dry (slide warmer)

Displays the microbe is susceptible to antibiotic making the antibiotic effective against microbes.

Deaminase

(+) = fuchsia/ hot pink
(-) = not fuchsia

False 

1. Begin w/ drop Congo red stain at end of clean slide
2. Sterilize loop& aseptically remove small amount of bacteria culture mixing it with the Congo red and resterilize loop
3. Use 2nd clean slide to draw drop across to other end
4. Air-dry (do NOT heat-fix)
5. Flood w/ Maneval's stain
6. Gently rise with DW
7. Allow to air dry

-On Aerobic Petri plate: Little growth
-On Anaerobic Petri plate: Little/No growth
-On thioglycolate broth: Growth on the top

2H2O2 --> 2H2O + O2

nitrate was reduced to nitrogen gas