Aerobic Plate Count, Gram Stain, and Isolation

1. Aerobic Plate Count, Gram Stain, and Isolation Food Microbiology Laboratory

2. Aerobic Plate Count • Provides general estimate of live, aerobic, bacteria • Excludes • Obligate Anaerobes • Microaerophiles

3. Plate Counts • Assumption • Each colonies arises from a single bacterial cell • Bacteria like to “clump” together so some colonies may arise from more than one cell • Report as • Colony Forming Unit (CFU)/gram or ml • NOT at total bacteria

4. APC Results • Evaluate Sanitation of Product • Predict Shelf-life • “Safety” Indicator • Monitor Environment

5. Limitations of APC • Only aerobic organisms are counted • Bacteria Type not known • Media may not support growth of certain bacteria • Eye strain/Human Error • Hard to Distinguish Between food particles and bacteria • Don’t Use on Fermented Foods • Colonies may be too small to see

6. Types of Samples • Liquid • Non-viscous Liquids can be measured with pipet • Viscous liquids should be weighed • Solid • Aseptically weigh Sample • Sponge/Swab Collect sample by swabbing a defined area • Environmental and Container • Rinse inside of Containers • Open Plate to Collect Air Samples • RODAC Plates

7. Protocol for Plate Counts • Prepare a Sample Homogenate • 1:10 dilution • 1 part sample to 10 parts total volume • Blend in Blender or Stomacher for 2 min. 90 ml of diluent 10 g/ml sample 1:10 Dilution – 10-1

8. Formula • 10 ml/g sample, want 1:100 dilution • 100 – 10 = 90 ml of diluent needed • Start with Different Sample Sizes • 50 g sample • Must have 500 g total volume for 1:10 • 500 – 50 = 450 ml diluent needed • 95 ml sample • Must have 950 total volume for 1:10 • 950 – 95 = 855 ml of diluent

9. Plate Count Protocol • Prepare Serial Dilutions • Dilute to a level where you will get countable colonies on plates • Use a NEW STERILE PIPET between each dilution • Place pipet tip down in pipet tanks • Shake each dilution bottle 25 times in a 90 degree arc within 7 seconds. • Phosphate Buffer or Peptone Buffer to Dilute

10. Dilutions Dilution Blanks Containing 90 ml Diluent Sample Homogenate 10 ml 10 ml 10 ml 10 ml 10-2 10-3 10-4 10-5 10-1 (1:100) (1:1000) (1:100000) (1:10) (1:10000)

11. Plating Put 1 ml of Each Dilution into Empty Petri-Dish 10-4 10-5 10-2 10-3 10-1 1 ml 1 ml 1 ml 1 ml 1 ml 1 ml 1 ml 1 ml 1 ml 1 ml

12. APC – Protocol • Add 18-20 ml of tempered (45-50 F), molten plate count agar to the petri dish. • Agar MUST be tempered or the bacteria will be killed by heat • Standard Methods or Plate Count Agar • Swirl 10 times in each direction • Allow to Solidify • Incubate inverted at 35-37 C for 48 hours

13. Sterilization • Equipment and Media MUST be Sterile • Hot Air Sterilization • 170 C for 1 hour • Equipment Temperature • Put in oven for 2 hours • Wrap in paper, foil, etc. • Steam Sterilization • 121 C for 15 min. MUST have 15 psi pressure • Liquid Media or Equipment • Don’t Put Lids on tightly

14. Gram Stain • Gram Positive or Gram Negative • Based on Cell wall Structure • Gram + • Very Thick Cell Wall due to Peptidoglycan Layer • N-acetylglucosamine • N-acetylmuramic acid • Two amino sugars linked by beta 1,4, bonds • Gram – • Thin Cell Wall with a Lipopolysaccharide layer

15. Obtaining Isolated Colonies • Goal is to get Isolated Colonies from Food and/or Cultures • Colonies can be Identified and Further Evaluated • Collect loopful of culture • Streak in each area starting • with area 1 • Flame Loop in between • areas 2 1 3 4

16. Counting Plates • Only count plates with 25-250 colonies • More than 250 • Too Numerous To Count – TNTC • Less than 25 • Too Few to Count - TFTC

17. Counting Plates 1 Too Numerous to Count 2 Too Few to Count • Average two countable plates and Multiply by Dilution Factor • Count is 175 x 104 • Must Convert to TWO Significant Digits • 1.8 x 106 cfu/ml or g

18. Counting - Examples Use ALL FOUR even though 300 is outside range. If ONE PLATE is in RANGE, use BOTH for Average. 250 x 102 – 2.5 x 104 125 x 103 – 1.3 x 105 AVERAGE – 7.8 x 104 cfu/g or ml

19. Counting Examples All Dilutions are outside Range so we MUST use counts Outside range 350 x 104 – 3.5 x 106 cfu/ml or g* Use an “*” when using dilutions outside countable ranges This means it is an ESTIMATED count

20. Counting Examples If Both Dilutions are outside Range, use the Higher Dilution (LOWER COUNTS) 7.5 x 103 cfu/ml or g*

21. Overloaded Plates • Use Highest Dilution and Use Grid on Colony Counter • 1 Grid = 1 cm2 • A standard Plastic Plate has 56 cm2 surface area • If <10 colonies/cm2, count 12 squares (6 consecutive horizontally and 6 consecutive vertically) • Total and Divide by 12 (average). Multiply by 56 to get total colonies on plate. Report as Estimate • If >10 colonies/cm2 • Count 4 squares, average and multiply by 56

22. APC Variations • Psychrotrophic • Incubate at 5-7 C for 10 days • Use Pre-poured Plates • Thermoduric • Hold 5 ml liquid sample or 1:10 diluent of solid sample in 60-80 C water bath for 30 min • Cool on ice for 10 min • Plate and incubate

23. Dilution Variations 99 ml Dilution Blanks 1 ml 1 ml 1 ml 10-7 10-3 10-5 10-1 1 ml 1 ml 0.1 ml 0.1 ml 1 ml 1 ml 0.1 ml 0.1 ml -5 -7 -1 -3 -6 -8 -2 -4 CAN NOT use with petri-film