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Environmental Microbial
Monitoring (EMM)
環境微生物監控
吳淑華
阮綜合醫院迴旋加速器中心
USP Regulations
• <51> Antimicrobial effectiveness testing
• <61> Microbiological examination of nonsterile products:
microbial enumeration tests
• <62> Microbiological examination of nonsterile products:
tests for specified microorganisms
• <71> Sterility tests
• <1113> Microbial characterization identification and strain typing
• <1116> Microbiological control and monitoring of aseptic
processing environments
• <1117> Microbiological Best Laboratory Practices
• <1227> Validation of microbial recovery from
pharmacopeial articles
2017/3/4 2
Purpose of EM
• Critical process within the pharmaceutical industries.
• Determines the microbial and particulate content of
cleanroom air and surfaces.
• Highlights conditions contributing to excessive microbial &
particulate levels due to ineffective cleaning, or
personnel/equipment issues (Trending).
• Alerts to conditions exceeding classifications.
• Proactive tool for Quality Assurance.
2017/3/4 3
Who Does It?
• Quality Control
– Demonstrate product safety
– Environmental Monitoring
– Testing
• Quality Assurance
– Oversight responsibilities – ensure compliance with GMPs
– Review and Approve all Records, Reports, written
procedures, specifications
– Audit methods, results, systems and processes
2017/3/4 4
To be monitored
• Non-viable airborne particulates
• Viable airborn particulates
• Viable surface bound particulates on cleanroom surfaces
and personnel
• Contamination Sources
– People ~75%
– Ventilation ~15%
– Room Structure ~5%
– Equipment ~5%
2017/3/4 5
USP 39 <1116>
• Studies indicate that gowned humans slough particulate and
microbial contamination at a rather consistent rate.
• Where equipment is the primary source of particulate matter,
the resulting particulates are essentially all nonviable.
• It is not possible to clearly distinguish between background
total particulate contamination generated largely by
mechanical operations and the total particulates contributed by
personnel. both a total particulate component and a
microbiological component.
2017/3/4 6
Classifications & Control Level
USP39 <1116>
2017/3/4 7
USP34 <1116> Microbial considerations and Action
levels for Controlled Environment
2017/3/4 8
FDA(2004)
1
10
100
USP39 <1116> Suggested Initial Contamination Recovery
Rates(CRR) in Aseptic Environments
Room Classification Active air Sample
(%)
Settle Plates(9cm)
4hr Exposure(%)
Contact Plates or
Swab(%)
Glove or Garment
(%)
Isolator/Closed
RABS
(ISO 5 or better)
<0.1 <0.1 <0.1 <0.1
ISO 5 <1 <1 <1 <1
ISO 6 <3 <3 <3 <3
ISO 7 <5 <5 <5 <5
ISO 8 <10 <10 <10 <10
2017/3/4 9
EU and FDA recommended limits for microbial contamination
PIC/S Annex 1 PE 009-13(2017) (top) ,FDA Pharmaceutical CGMPs (2004) (bottom)
Grade Air Sample
cfu/m3
Settle Plates
(Ø 90mm), cfu/4hrs
Contact Plates
(Ø 55mm), cfu/plate
Glove Print 5
Fingers, cfu/glove
A <1 <1 <1 <1
B 10 5 5 5
C 100 50 25 -
D 200 100 50 -
Clean Area Classification
(0.5Îźm particles/cfu)
ISO Designation Air Sample
cfu/m3
Settle Plates
(Ø 90mm), cfu/4hrs
100 ISO 5 1 1
1000 ISO 6 7 3
10000 ISO 7 10 5
100000 ISO 8 100 50
2017/3/4 10
Sampling Plain
• Frequency
• Time
• Sites
• Method
2017/3/4 11
Sampling Frequency
• The frequency of sampling depends on the manufacturing
process conducted within an environment.
• Classified environments in which closed manufacturing
operations are conducted, including fermentation, sterile API
processing, and chemical processes, require fewer
monitoring sites and less frequent monitoring because the
risk of microbial contamination from the surrounding
environment is comparatively low.
2017/3/4 12
Sampling Frequency (cont.)
• It is not possible to recommend microbial control levels for
each type of manufacturing environment. depending on
the production activities
• Monitoring should reflect the microbiological control
requirements of manufacturing or processing activities.
• Formal risk assessment techniques can result in a
scientifically valid contamination control program.
2017/3/4 13
USP39 <1116>
ESTABLISHMENT OF SAMPLING PLAN AND SITES
2017/3/4 14
Sampling Time
• Sampling should take place with the facility in the
operational condition (personnel present and normal
operations being carried out).
• Microbial sampling should occur when materials are in the
area, processing activities are ongoing, and a full
complement of personnel is working within the aseptic
processing environment.
• The operational condition for sterile hoods and transfer
devices can be considered to be when an operator is
working in any part of the clean air device.
• Sampling in the static condition should be performed at an
agreed frequency to monitor baseline contamination levels.
2017/3/4 15
Sampling Sites
• Microbial monitoring of manufacturing clean rooms, RABS,
and isolators should include compressed gases, surfaces,
room or enclosure air, and any other materials and
equipment that might produce a risk of contamination.
• The location and movement of personnel within the clean
room correlate with contamination risk to the environment
and to the processes conducted within that environment.
• The location and movement of personnel within the clean
room correlate with contamination risk to the environment
and to the processes conducted within that environment.
2017/3/4 16
Methods of EMM
• Air
- Air sampler(active method): testing of the number of
organisms per volume of air sampled.
-Settling plate(passive method): settling plates can be
used as qualitative, or semi-qualitat
• Surface
-Contact plate: product contact surface, floors, walls,
and equipment should be tested on a
regular basis.
-Swabbing
2017/3/4 17
Air Sampler
(Viable airborne particulates)
Active Air Monitoring
ISO 14644, Fed Std-209E, USP <1116>
• Used to sample a defined volume of air, embedding viable
particulates onto sterile media strips.
• The media strips are incubated to promote the growth of
viable particulates
• The microorganisms are counted and results are reported as
the number of CFU per volume of air sampled.
2017/3/4 18
Settling Plates
(Viable airborne particulates)
Passive Air Monitoring
ISO 14644, Fed Std-209E, USP <1116>
• Settling plates filled with media are used to sample the
microbial fallout over time.
• The plates are incubated to promote growth
• Microorganisms are counted and results are reported as the
number of CFU per time sampled.
• The average size of microbial particle will deposit, by gravity,
onto surfaces at a rate of approximately 1 cm/s.
2017/3/4 19
Sampling Sites for Settling Plates
• Areas where there is little air movement (i.e. "dead spaces")
or where airflows converge or are excessively turbulent.
These conditions are most likely to occur:
– adjacent to doors
– in pass through hatches
– at low level return air grilles
– between HEPA's in clean rooms
– in corners of rooms
• Areas within the clean room where there is personnel
activity or where specific operations are carried out.
2017/3/4 20
RODAC Plates
(Viable, Surface-Bound Particles)
Surface Monitoring
ISO 14644, Fed Std-209E, USP <1116>
• Contact plates (RODAC Plates) filled with media are used to
sample tabletops, walls, benches, floors, garments, and
gowned personnel.
• Measure the number of microorganisms per area sampled.
• Plates are incubated to promote growth, the microorganisms
are counted and results are reported as the number of CFU
per area sampled.
2017/3/4 21
RODAC
(Replicate Organism Detection and Counting)
• flat agar surface is above the edges of the dish (so you can press
it on flat surfaces) and a grid, allowing counting of cfu per cm².
2017/3/4 22
RODAC Plates
• One objective of surface sampling is to determine the efficiency of
routine cleaning procedures in removing contamination.
- Sampling is done before and after cleaning.
- The medium in the plates contains neutralizing agents,
which inactivate residual disinfectants on the surface to be
tested, allowing comparative results before and after
cleaning.
• RODAC plates are also used to monitor the contamination level of
personnel gowns and Personal Protective Equipment (PPE) before
or during manufacturing production.
2017/3/4 23
Swabbing method
(Viable, Surface-Bound Particles)
Surface Monitoring
ISO 14644, Fed Std-209E, USP <1116>
• The swabbing method can be used to supplement contact
plates for sampling of irregular surfaces, especially irregular
surfaces of equipment.
• The area that will be swabbed is defined with a sterile template
of appropriate size.
• In general, it is in the range of 24–30 cm2.
• After sample collection the swab is placed in an appropriate
diluent or transport medium and is plated onto the desired
nutrient agar.
2017/3/4 24
2017/3/4 25
Rapid Microbiological Methods
Contact Slide(25cm2) Petrifilm plate
• USP<61> <62> <71> <1227>
2017/3/4 26
Growth Media
• Use a growth medium with low selectivity i.e. capable of
supporting a broad spectrum of microorganisms including
bacteria, fungi, yeast and molds.
- SCDM(TSA) is suitable for environmental monitoring in
most cases because it supports the growth of a wide range
of bacteria, yeast, and molds.
- Sabouraud Dextrose Agar (SDA) supports yeast and fungal
colonies.
2017/3/4 27
Growth Media
• When necessary to detect or search for a particular type of
microorganism a selective culture medium should be used.
- Malt Extract Agar(MEA) is used as a general purpose growth
media to isolate and cultivate yeasts and molds from
clinical samples, as well as a wide range of environmental
sources.
2017/3/4 28
Culture Condition
USP 39 <1116>
• Typically, for general microbiological growth media such
as SCDM, incubation temperatures in the ranges of
approximately 20 –35℃ have been used with an incubation
time of not less than 72 hours.
• The temperature ranges given above are by no means
absolute.
• For many mesophilic organisms, recovery is possible over a
range of approximately 20℃ .
2017/3/4 29
Culture Condition
USP 39 <1116>
•In the absence of confirmatory evidence, microbiologists
may incubate a single plate at both a low and a higher
temperature. Incubating at the lower temperature first may
compromise the recovery of Gram(+) cocci that are
important because they are often associated with humans.
•Typically, for general microbiological growth media such as
SCDM, incubation temperatures in the ranges of
approximately 20–35℃ have been used with an incubation
time of not less than 72 hours.
- TSA plates are incubated at 30-35°C for 3 days.
- SDA plates are incubated at 20-25°C for 5 days.
(A review of cleanroom microflora: Types, treans, and Pattens. PDA J Pharm Sci Technol ,2011)
2017/3/4 30
Identification
• FDA Pharmaceutical CGMPs, 2004
2017/3/4 31
• FDA Pharmaceutical CGMPs, 2004
2017/3/4 32
• USP 39 <1116> Identification of microbial isolates
2017/3/4 33
Gowning Procedure
2017/3/4 34
2017/3/4
35
2017/3/4 36
Questions
2017/3/4 37
USP39 <1117>
• Special care should be taken with media that is used in
environmental monitoring studies. Media used for
environmental monitoring of critical areas should preferably
be double-wrapped and terminally sterilized. If terminal
sterilization is not performed, media should be subjected to
pre-incubation and 100% inspection prior to use within a
critical area. This will prevent extraneous contamination
from being carried into controlled environments and will
prevent false-positive results. A raised agar level for surface
contact plates should be verified.
2017/3/4 38

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1116 Added.pdf

  • 2. USP Regulations • <51> Antimicrobial effectiveness testing • <61> Microbiological examination of nonsterile products: microbial enumeration tests • <62> Microbiological examination of nonsterile products: tests for specified microorganisms • <71> Sterility tests • <1113> Microbial characterization identification and strain typing • <1116> Microbiological control and monitoring of aseptic processing environments • <1117> Microbiological Best Laboratory Practices • <1227> Validation of microbial recovery from pharmacopeial articles 2017/3/4 2
  • 3. Purpose of EM • Critical process within the pharmaceutical industries. • Determines the microbial and particulate content of cleanroom air and surfaces. • Highlights conditions contributing to excessive microbial & particulate levels due to ineffective cleaning, or personnel/equipment issues (Trending). • Alerts to conditions exceeding classifications. • Proactive tool for Quality Assurance. 2017/3/4 3
  • 4. Who Does It? • Quality Control – Demonstrate product safety – Environmental Monitoring – Testing • Quality Assurance – Oversight responsibilities – ensure compliance with GMPs – Review and Approve all Records, Reports, written procedures, specifications – Audit methods, results, systems and processes 2017/3/4 4
  • 5. To be monitored • Non-viable airborne particulates • Viable airborn particulates • Viable surface bound particulates on cleanroom surfaces and personnel • Contamination Sources – People ~75% – Ventilation ~15% – Room Structure ~5% – Equipment ~5% 2017/3/4 5
  • 6. USP 39 <1116> • Studies indicate that gowned humans slough particulate and microbial contamination at a rather consistent rate. • Where equipment is the primary source of particulate matter, the resulting particulates are essentially all nonviable. • It is not possible to clearly distinguish between background total particulate contamination generated largely by mechanical operations and the total particulates contributed by personnel. both a total particulate component and a microbiological component. 2017/3/4 6
  • 7. Classifications & Control Level USP39 <1116> 2017/3/4 7
  • 8. USP34 <1116> Microbial considerations and Action levels for Controlled Environment 2017/3/4 8 FDA(2004) 1 10 100
  • 9. USP39 <1116> Suggested Initial Contamination Recovery Rates(CRR) in Aseptic Environments Room Classification Active air Sample (%) Settle Plates(9cm) 4hr Exposure(%) Contact Plates or Swab(%) Glove or Garment (%) Isolator/Closed RABS (ISO 5 or better) <0.1 <0.1 <0.1 <0.1 ISO 5 <1 <1 <1 <1 ISO 6 <3 <3 <3 <3 ISO 7 <5 <5 <5 <5 ISO 8 <10 <10 <10 <10 2017/3/4 9
  • 10. EU and FDA recommended limits for microbial contamination PIC/S Annex 1 PE 009-13(2017) (top) ,FDA Pharmaceutical CGMPs (2004) (bottom) Grade Air Sample cfu/m3 Settle Plates (Ø 90mm), cfu/4hrs Contact Plates (Ø 55mm), cfu/plate Glove Print 5 Fingers, cfu/glove A <1 <1 <1 <1 B 10 5 5 5 C 100 50 25 - D 200 100 50 - Clean Area Classification (0.5Îźm particles/cfu) ISO Designation Air Sample cfu/m3 Settle Plates (Ø 90mm), cfu/4hrs 100 ISO 5 1 1 1000 ISO 6 7 3 10000 ISO 7 10 5 100000 ISO 8 100 50 2017/3/4 10
  • 11. Sampling Plain • Frequency • Time • Sites • Method 2017/3/4 11
  • 12. Sampling Frequency • The frequency of sampling depends on the manufacturing process conducted within an environment. • Classified environments in which closed manufacturing operations are conducted, including fermentation, sterile API processing, and chemical processes, require fewer monitoring sites and less frequent monitoring because the risk of microbial contamination from the surrounding environment is comparatively low. 2017/3/4 12
  • 13. Sampling Frequency (cont.) • It is not possible to recommend microbial control levels for each type of manufacturing environment. depending on the production activities • Monitoring should reflect the microbiological control requirements of manufacturing or processing activities. • Formal risk assessment techniques can result in a scientifically valid contamination control program. 2017/3/4 13
  • 14. USP39 <1116> ESTABLISHMENT OF SAMPLING PLAN AND SITES 2017/3/4 14
  • 15. Sampling Time • Sampling should take place with the facility in the operational condition (personnel present and normal operations being carried out). • Microbial sampling should occur when materials are in the area, processing activities are ongoing, and a full complement of personnel is working within the aseptic processing environment. • The operational condition for sterile hoods and transfer devices can be considered to be when an operator is working in any part of the clean air device. • Sampling in the static condition should be performed at an agreed frequency to monitor baseline contamination levels. 2017/3/4 15
  • 16. Sampling Sites • Microbial monitoring of manufacturing clean rooms, RABS, and isolators should include compressed gases, surfaces, room or enclosure air, and any other materials and equipment that might produce a risk of contamination. • The location and movement of personnel within the clean room correlate with contamination risk to the environment and to the processes conducted within that environment. • The location and movement of personnel within the clean room correlate with contamination risk to the environment and to the processes conducted within that environment. 2017/3/4 16
  • 17. Methods of EMM • Air - Air sampler(active method): testing of the number of organisms per volume of air sampled. -Settling plate(passive method): settling plates can be used as qualitative, or semi-qualitat • Surface -Contact plate: product contact surface, floors, walls, and equipment should be tested on a regular basis. -Swabbing 2017/3/4 17
  • 18. Air Sampler (Viable airborne particulates) Active Air Monitoring ISO 14644, Fed Std-209E, USP <1116> • Used to sample a defined volume of air, embedding viable particulates onto sterile media strips. • The media strips are incubated to promote the growth of viable particulates • The microorganisms are counted and results are reported as the number of CFU per volume of air sampled. 2017/3/4 18
  • 19. Settling Plates (Viable airborne particulates) Passive Air Monitoring ISO 14644, Fed Std-209E, USP <1116> • Settling plates filled with media are used to sample the microbial fallout over time. • The plates are incubated to promote growth • Microorganisms are counted and results are reported as the number of CFU per time sampled. • The average size of microbial particle will deposit, by gravity, onto surfaces at a rate of approximately 1 cm/s. 2017/3/4 19
  • 20. Sampling Sites for Settling Plates • Areas where there is little air movement (i.e. "dead spaces") or where airflows converge or are excessively turbulent. These conditions are most likely to occur: – adjacent to doors – in pass through hatches – at low level return air grilles – between HEPA's in clean rooms – in corners of rooms • Areas within the clean room where there is personnel activity or where specific operations are carried out. 2017/3/4 20
  • 21. RODAC Plates (Viable, Surface-Bound Particles) Surface Monitoring ISO 14644, Fed Std-209E, USP <1116> • Contact plates (RODAC Plates) filled with media are used to sample tabletops, walls, benches, floors, garments, and gowned personnel. • Measure the number of microorganisms per area sampled. • Plates are incubated to promote growth, the microorganisms are counted and results are reported as the number of CFU per area sampled. 2017/3/4 21
  • 22. RODAC (Replicate Organism Detection and Counting) • flat agar surface is above the edges of the dish (so you can press it on flat surfaces) and a grid, allowing counting of cfu per cm². 2017/3/4 22
  • 23. RODAC Plates • One objective of surface sampling is to determine the efficiency of routine cleaning procedures in removing contamination. - Sampling is done before and after cleaning. - The medium in the plates contains neutralizing agents, which inactivate residual disinfectants on the surface to be tested, allowing comparative results before and after cleaning. • RODAC plates are also used to monitor the contamination level of personnel gowns and Personal Protective Equipment (PPE) before or during manufacturing production. 2017/3/4 23
  • 24. Swabbing method (Viable, Surface-Bound Particles) Surface Monitoring ISO 14644, Fed Std-209E, USP <1116> • The swabbing method can be used to supplement contact plates for sampling of irregular surfaces, especially irregular surfaces of equipment. • The area that will be swabbed is defined with a sterile template of appropriate size. • In general, it is in the range of 24–30 cm2. • After sample collection the swab is placed in an appropriate diluent or transport medium and is plated onto the desired nutrient agar. 2017/3/4 24
  • 26. Rapid Microbiological Methods Contact Slide(25cm2) Petrifilm plate • USP<61> <62> <71> <1227> 2017/3/4 26
  • 27. Growth Media • Use a growth medium with low selectivity i.e. capable of supporting a broad spectrum of microorganisms including bacteria, fungi, yeast and molds. - SCDM(TSA) is suitable for environmental monitoring in most cases because it supports the growth of a wide range of bacteria, yeast, and molds. - Sabouraud Dextrose Agar (SDA) supports yeast and fungal colonies. 2017/3/4 27
  • 28. Growth Media • When necessary to detect or search for a particular type of microorganism a selective culture medium should be used. - Malt Extract Agar(MEA) is used as a general purpose growth media to isolate and cultivate yeasts and molds from clinical samples, as well as a wide range of environmental sources. 2017/3/4 28
  • 29. Culture Condition USP 39 <1116> • Typically, for general microbiological growth media such as SCDM, incubation temperatures in the ranges of approximately 20 –35℃ have been used with an incubation time of not less than 72 hours. • The temperature ranges given above are by no means absolute. • For many mesophilic organisms, recovery is possible over a range of approximately 20℃ . 2017/3/4 29
  • 30. Culture Condition USP 39 <1116> •In the absence of confirmatory evidence, microbiologists may incubate a single plate at both a low and a higher temperature. Incubating at the lower temperature first may compromise the recovery of Gram(+) cocci that are important because they are often associated with humans. •Typically, for general microbiological growth media such as SCDM, incubation temperatures in the ranges of approximately 20–35℃ have been used with an incubation time of not less than 72 hours. - TSA plates are incubated at 30-35°C for 3 days. - SDA plates are incubated at 20-25°C for 5 days. (A review of cleanroom microflora: Types, treans, and Pattens. PDA J Pharm Sci Technol ,2011) 2017/3/4 30
  • 31. Identification • FDA Pharmaceutical CGMPs, 2004 2017/3/4 31
  • 32. • FDA Pharmaceutical CGMPs, 2004 2017/3/4 32
  • 33. • USP 39 <1116> Identification of microbial isolates 2017/3/4 33
  • 38. USP39 <1117> • Special care should be taken with media that is used in environmental monitoring studies. Media used for environmental monitoring of critical areas should preferably be double-wrapped and terminally sterilized. If terminal sterilization is not performed, media should be subjected to pre-incubation and 100% inspection prior to use within a critical area. This will prevent extraneous contamination from being carried into controlled environments and will prevent false-positive results. A raised agar level for surface contact plates should be verified. 2017/3/4 38