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Composting Practices and Pathogen Reduction

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Title: Composting Practices and Pathogen Reduction


1
Composting Practices and Pathogen Reduction
  • Joan Jeffrey, Extension Veterinarian
  • University of California
  • School of Veterinary Medicine
  • VMTRC---TULARE, CA

2
Composting
  • Heat generated by microbial activity
  • Application of heat over time kills mesophilic
    bacteria and favors thermophilic bacterial
    population
  • Bacteria in mature compost compete against and
    inhibit pathogen regrowth

3
Composting methods
  • Passive Aerated Static Piles or Windrows
  • Stacked Pile
  • Aerated Stacked Pile
  • Windrow
  • Enclosed System
  • Containerized Systems (Aerated Static Piles in a
    box)

4
Methods applicable to non-green waste
  • Non-green waste food, dairy products,
    raw/cooked meat, dead animals (cows, poultry,
    fish)

5
Methods applied to poultry carcasses
  • Two stage bin composting
  • Refers to 2 heating cycles
  • Containerized system
  • Reference FS 717 U. of Maryland

6
Methods suitable for blood/feathers
  • Windrow
  • Most common method for green waste/manures
  • gt3000 facilities in USA
  • Rows 8 ft high x 12-16 feet wide
  • Approved by EPA for pathogen destruction if
    windrows are turned 5x in 15 d and temperatures
    stay gt 131 F (55 C)
  • Aerated Static Pile
  • Piles 7 to 9 feet high connected to blowers
  • Approved by EPA for pathogen destruction
  • Requires 131 F (55 C) for 3 days

7
Federal guidelines for pathogen destruction in
compost
  • For windrows15 days, turned no less than 5
    times, temperature of 131 F (55 C)
  • For aerated static piles3 days at temperature
    gt131 F (55 C)
  • Governed by Code of Federal Regulations 40, CFR
    Part 503, 1993

8
Killing of pathogens during composting
  • Temperature (thermal kill)
  • Ammonia (chemical kill)
  • Microbial antagonism

9
Rate of microbial decomposition
  • A function of surface area
  • i.e. whole carcasses would compost at a slower
    rate than tissues like blood or feathers

10
Temperature-Time relationships for pathogen
reduction
  • D-values time required for 1 log reduction in a
    pathogen at a given temperature
  • Can compare hardiness of different organisms
  • Used to establish pathogen elimination criteria

11
Poultry pathogens addressed by specific studies
  • Senne, D. A., et al. (1994) Highly Pathogenic
    Avian Influenza virus and EDS-76 Adenovirus
  • Compost Bin method used with poultry carcasses
  • Two-stage
  • Turned after 10 days
  • Average temperatures 57-58 C
  • 1/20 tissues positive for adenovirus at d 10
  • 0/20 tissues positive for virus at d 20

12
Poultry pathogens addressed by specific studies
  • Conner, D. E. et al. (1991)
  • Fungi and coliform, aerobic, anaerobic,
    thermophilic and thermotolerant bacteria were
    represented
  • S. enteritidis, S. typhimurium, S. seftenberg,
  • L. monocytogenes, E. coli, P. multocida and
    Aspergillus fumigatus
  • Used wheat straw, peanut hulls and other
    materials
  • Pathogens placed into carcasses
  • No bacteria after stage I of composting
  • No fungal spores after stage II of composting

13
Poultry pathogens addressed by specific studies
  • Murphy, D. W. et al. (1990)
  • Newcastle disease virus
  • Infectious Bursal Disease virus
  • Bin compost method for carcasses
  • Two stage composting method

14
Other pathogens addressed by specific studies
  • M. tuberculosis (Morgan McDonald 69)
  • Salmonella, Shigella, poliovirus, enterovirus,
    parasite cysts (Gaby 75)
  • Coliforms, Salmonella, Ascaris ova (Hay 96)
  • Salmonella, bacteriophage (Epstein 76 and
    others)

15
Potential problems
  • Recontamination by equipment, other vectors
  • Regrowth
  • Only possible for bacteriaa
  • Studies cite salmonella and coliforms as most
    likely to regrow
  • These organisms are used as indicators of
    pathogen elimination

16
Use of indicator organisms to ensure pathogen
destruction
  • Sampling for indicator organisms is conducted to
    validate composting processes (temperature/time)
    (USEPA 40)
  • Temperatures are then verified for each compost
    pile or windrow
  • Microbial sampling is generally not required for
    every batch assuming consistent feedstock and
    processing

17
USEPA standards for Class A biosolids
  • Fecal coliform level of lt 1000 MPN per gram of
    dry solids, OR
  • Salmonella spp. level of lt 3 MPN per 4 gram of
    dry solids

18
Conclusions
  • Composting methods for pathogen destruction are
    well documented
  • Monitoring of the composting process is a valid
    substitute for microbiologic testing

19
Conclusions
  • Studies addressing major poultry pathogens have
    been conducted
  • Due to greater surface area, blood, feathers and
    processing waste should compost more rapidly and
    uniformly than carcasses
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