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Biofilms and microbial testing in the dairy industry'

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Title: Biofilms and microbial testing in the dairy industry'

1
Biofilms and microbial testing in the dairy
industry.

S. Flint Guelph University
2nd April 2007

2
Outline

Introduction to Fonterra
Biofilm research group
Features of dairy biofilms
Current strategies to control biofilms
Alternative strategies
Current research
Alternative test methods

3
Introduction to Fonterra
4
Long History, New Beginning
1927 Amalgamated Dairies established in London
to market New Zealand butter and cheese
2000 Milk supply by two major companies New
Zealand Dairy Group Kiwi Cooperative Dairies
1963 New Zealand Dairy Board established
1800s Dairying in NZ began
2001 Fonterra formed
2006 Total business aligned under one brand
1882 SS Dunedin sailed to London with first
refrigerated shipment of butter in the world
1930 Many towns have dairy factories in New
Zealand
1970-1990 Dairy factories merged
5
Fonterra Today

Co-operative owned by 11,600 supplier
shareholders
Total Sales of 12.7 billion
Process nearly 2 billion kilograms of milk solids
annually
Export 95 of production to more than 100 markets
around the world
Employ 18,600 people worldwide

6
Innovation in Fonterra
CUSTOMERS
FonterraIngredients
FonterraSpecialty Products
FonterraBrands
FonterraFood Service
Ingredients Innovation
Brands Innovation
Group Innovation
Manufacturing Innovation
Fonterra Group Manufacturing
7
Palmerston North
Population 73,000
City Square
8
Globally Recognised Facilities People
9
One of Worlds Largest Registered Dairy Pilot
Plants
10
A Cluster of Science Organisations
11
Biofilm research groups
12
Biofilm Research Groups

Steve Flint - Fonterra

Phil Bremer - University of Otago

Dunedin
John Brooks Massey University
13
Biofilm Research at Fonterra current strategy

Alternative Cleaning systems (CIP chemicals)
Bioactive Surfaces (substrate focus)
Disruptive Technologies (process/environment
manipulation)
Technical advancement (microbial interactions)

14
Biofilm research at Fonterra
Laboratory reactor system
15
Biofilm research at Fonterra
Robbins device
16
Biofilm research at Fonterra
Bactrac impedance system
17
Features of dairy biofilms
18
Features of Dairy Biofilms

Process biofilms
Generally single species
Limited thickness and density ( 106 cells/cm2)
Rapid growing
Environmental biofilms
Mixed species
Thick layer

19
Process Biofilms

Streptococcus thermophilus
Pasteuriser plate heat exchangers (PHEs)
Recycle loops in scraped surface plants
Thermophilic bacilli
Preheating and evaporation sections of milk
powder plants
Pasteuriser PHEs
Hot separators
Cream heaters in anhydrous milk fat (AMF) plants
Hot ultrafiltration plants

20
Process Biofilms S. thermophilus

Thermoduric
Optimum growth temperature of 40-45ºC
Grow on the cooling side of pasteurisers
Causes off flavours excess open texture in
cheese

21
Process biofilms Thermophilic bacilli

True thermophiles
Geobacillus spp.
Anoxybacillus flavithermus
Facultative thermophiles
Bacillus spp.
Optimum growth temperature of 40 65 ºC
Difficult to eliminate
Fast growth rate (approximately 15 - 20 min
generation time)
Heat and chemical resistant spores
Wide temperature growth range

22
Environmental Biofilms

Membranes in reverse osmosis (RO) and
ultrafiltration (UF) plants
Mixed species
Bacillus sp.
Enterobacteriaceae, Pseudomonas
Lactococcus
Blastoshizomyces captitatum
Limits operating time
Contamination of product

23
Strategies to control biofilms
24
Current strategies to control dairy biofilms

Frequent cleaning
Use of sanitisers
Cold processing
Ultrafiltration
Centrifugal milk separation
Reducing surface area over the optimal
temperature zone for biofilm growth
Direct steam injection (DSI)
Steam infusion.
Dual PHEs

25
Current cleaning procedures

Water rinse
NaOH (1.5) 75ºC
Water rinse
Nitric acid (0.5) 70ºC
Water rinse
Sanitiser flush - 200 ppm free available chlorine
(FAC)
Water rinse

26
Alternative strategies

Alternative Cleaning systems (CIP chemicals)
Bioactive Surfaces (substrate focus)
Disruptive Technologies (process/environment
manipulation)
Technical advancement (microbial interactions)

27
Alternative strategies

Alternative Cleaning systems (CIP chemicals)
Bioactive Surfaces (substrate focus)
Disruptive Technologies (process/environment
manipulation)
Technical advancement (microbial interactions)

28
Cleaning procedures activated water

Cleaning sanitising solution
Salt solution converted to
Catholyte (pH 11.0
NaOH 0.1)
Anolyte (pH 2.5
FAC 500 ppm)

29
Activated water potential applications

Replacing NaOH with Catholyte for cleaning
Replacing hypochlorite sanitisers with Anolyte to
control bacteria
Improve control of bacteriophage with Anolyte

30
Activated water - catholyte for biofilm removal

Method based on microtitre plate assay (Pitts
et al. 2003)
Microtitre plate incubated with culture to allow
biofilm to form
Serial dilutions of catholyte into microtitre
plate
Biofilm stained with crystal violet then rinsed
with water ethanol
Biofilm remaining detected by measuring the OD
_at_540nm

Bacteria
Catholyte concentration
31
Effect of catholyte on biofilm removal
32
Activated water - catholyte for biofilm removal

Effective at concentrations of gt10 (equivalent
to 0.01 NaOH)
Some variation between different bacteria

33
Activated water - anolyte as a sanitiser

Method
Serial 2-fold dilutions of anolyte into
microtitre plate
106 cells of bacteria added
Incubation 1 h at room temperature
Survivors detected by Alma Blue (Redox indicator)

Bacteria
Anolyte concentration
34
Activated water - anolyte as a sanitiser

Efficacy less than sodium hypochlorite based on
FAC levels
Minimal effect of organics
Biofilm inactivation needs higher concentration
than planktonic cells

35
Activated water - anolyte efficacy against
bacteriophage

Method
Phages exposed to activated water at room
temperature
Surviving phage numbers were determined after
exposure times of one minute and five minutes
Sodium hypochlorite was used as the control
sanitiser
Up to 6 log reduction
Superior to sodium hypochlorite at an equivalent
FAC level

36
Alternative strategies

Alternative Cleaning systems (CIP chemicals)
Bioactive Surfaces (substrate focus)
Disruptive Technologies (process/environment
manipulation)
Technical advancement (microbial interactions)

37
Altering surfaces

Coating stainless steel with a protein
Using impregnated stainless steel
Molecular brush
Anti-stick solutions

38
Coating surfaces with a protein

Coating stainless steel with different proteins

39
Coating surfaces with lysozyme
Rinse manufacturing plant with lysozyme
Lysozyme removes biofilm
40
Coating surfaces with lysozyme

1 Lysozyme effective for 18 h
Re-use of lysozyme solution at least 10 times
Storage life of the solution at 10ºC is at least
50 days
Not currently used because of risk of lysozyme in
product

41
Impregnated stainless steel

University of Surrey provided samples
Tested attachment of thermo-resistant
streptococci to ion impregnated samples and
compared with 316 stainless steel
CrN 4 log reduction
CrC 2 log reduction

42
Surface modifications to stainless steel

Kenifine Coatings - proprietary Nickel plated
surfaces to produce sanitary stainless steel
surfaces
1 log reduction in attachment
Electroless Ni-P based composite coatings
prepared by University of Auckland
Preliminary trials no difference in attachment

43
Molecular brush

Developed by Wageningen University

Complex coacervate micelles unfold on surface
Brush layer
Substrate
Complex coacervate layer
Figure adapted from a presentation by de Kiezer
(2006)
44
Molecular brush
Control
Treated
No difference
Pseudomonas fluorescens
2 log reduction
Streptococcus thermophilus
45
Anti-stick solutions

Commercial anti-stick preparations (Automate
Process 731B from Ecolab) containing
Sodium dichloroisocyanurate
Sodium metasilicate
Traditionally used in butter manufacturing plants
Preliminary trials - treated stainless steel
samples resulted in 2 log reduction of
Geobacillus sp. attachment

46
Alternative strategies

Alternative Cleaning systems (CIP chemicals)
Bioactive Surfaces (substrate focus)
Disruptive Technologies (process/environment
manipulation)
Technical advancement (microbial interactions)

47
Disrupting technologies temperature spike

Control of Streptococcus thermophilus in
pasteurisers

48
Disrupting technologies temperature spike

The preheat section of the pasteuriser was
increased from 34ºC to 55C for 10 min every hour
for 20 h.

(s)
49
Disrupting technologies temperature spike

Temperature spike controlled S. thermophilus
growth

50
Current research
51
Biofilm Research at Fonterra current strategy

Alternative Cleaning systems (CIP chemicals)
Bioactive Surfaces (substrate focus)
Disruptive Technologies (process/environment
manipulation)
Technical advancement (microbial interactions)

52
Current research (Jon Palmer)

Identification of cell surface adhesins on A.
flavithermus (Jon Palmer)
Successful isolation of a mutant with a 10-fold
decrease in attachment
Detection of two proteins not present in the
mutant

53
Current research (Brent Seale)

Understand factors controlling thermophilic spore
attachment
Spores attach quickly to surfaces.
Attach in similar numbers to all surfaces
Increasing ionic strength increases attachment
Developing anti-adhesive stainless steel surfaces
Examine proprietary metallic surfaces and polymer
coatings

54
Current research (Xumei Tang)

Reverse Osmosis / Ultrafiltration biofilm
investigation
Isolate, identify and characterise microflora
from membrane samples
Develop a laboratory model which can mimic
factors (e.g. pH, temperature, pressure,
concentration) found in RO/UF membrane plants
Investigate critical factors for biofilm
colonisation
Identify strategies to reduce biofilm formation

55
Future work?

Altering surfaces
immobilising lysozyme onto UF/RO membranes
Disruptive technology
pulsed flow
Bacteriophage in biofilms

56
Acknowledgements

John Brooks
Phil Bremer
Frank van de Ven
Sara Scott
Kylie Walker
Bryan Waters

Anita Clarke
Jon Palmer
Brent Seale
Xuemei Tang

57
Method Development
58
Rapid Micro Methods - Categories

Methods for typing/characterisation/detection
Well researched
Methods for enumeration
Not so well researched

59
Faster, Smarter (cheaper)

Fonterra spends x per year on testing milk
powder.
Faster Smarter a series of initiatives to
reduce costs for manufacturing.
Faster test results means a reduction in test
numbers.
Greater control over processing means less need
for exhaustive testing on final product.
Rapid trace back when things go wrong.

60
Industry wish list for rapid bacterial
enumeration assays

Lower detection limit 1-100 cells/ml
Specificity selective
Assay time 30 minutes max
Protocol Simple
Measurement Direct
Format Automated
Cell viability Yes
Cost Cheap
Precision /- 0.2 Log

61
Potential rapid enumeration methods - studies at
Fonterra (thermophile focus)

Impedance /metabolite based assays
ATP assays
Quantitative PCR
BioGeorge in-line monitor
Dip-stick assays
Flow Cytometry
Biosensors

62
Potential rapid enumeration methods - studies at
Fonterra (thermophile focus)

Impedance /metabolite based assays
ATP assays
Quantitative PCR
BioGeorge in-line monitor
Dip-stick assays
Flow Cytometry
Biosensors

63
Flow cytometry most promising

Flow cytometry provides a unique opportunity to
achieve this.
Results available in under 2 hours.
Plate counts 2 5 days.
Flow cytometry is well established in other
industries.
Cosmetics
Raw milk
Fruit juices
Brewing and winemaking

64
Flow Cytometry - BactiFlow

Detection Limit 100 - 1000 cells/ml
Specificity Non selective
Assay time 1-3 h
Protocol Simple
Measurement Direct
Format Semi Automatic
Cell viability Yes
Cost 100,000
Precision lt /- 0.5 log

65
Flow Cytometry - outline.

Direct fluorescent labelling of viable
micro-organisms.

Cell Membrane
Substrate
66
Flow Cytometry - outline.

Fluorescent labelling

67
Flow Cytometry - outline.

Sample hydro-dynamicallyfocused.
Laser excites fluorescently labelled cells.
Fluorescent emission signal split up into red
and green wavelengths.
Fluorescence information collected by sensitive
photo-multipliers and converted into data.

Labelled Sample
Green Detector
488 nm laser
Red Detector
Waste
68
Flow Cytometry - outline.
Sample placed into holder.
Data analyzed by computer.
Easy to interpret results displayed on screen.
69
Flow Cytometers.

D-Count (AES Chemunex, France)
Fully automated
High throughput (50 samples/hour)
Bactiflow (AES Chemunex, France)
Manual sample preparation
Lower throughput (15 samples/hour)
RBD 3000 (AATI, USA)
Fully automated
Low throughput (6 samples/hour)
Higher sensitivity

70
Fonterra and flow cytometry.

Bactiflow instruments in routine usage
Fonterra Clandeboye (2005)
Fonterra Whareroa (2004)
Fonterra Te Rapa (2005)
Fonterra Innovation (PN) (2004)
D-Count instrument in routine usage
Fonterra Whareroa (2001)
RBD 3000 instrument (research)
Fonterra Innovation (PN) (2006)

71
Methods

Total Viable Count (Protocol B)
Total Viable Count for milkpowder (Protocol A)
Thermophile Count (Protocol T)
Mould Count (Protocol Y)
Mesophile Count (Protocol C)

72
Protocol B (TVC Basic)Outline

Fastest, simplest test for bacterial enumeration.
Add labelling reagents (buffer, counterstain,
fluorochrome)
Incubate for 20 minutes at 30C.
Add reducing agent to quench unbound
fluorochrome.
Read each sample in the instrument (1 minute per
sample)

73
Protocol C (TVC Basic) Limitations

Does not distinguish between thermophilic/mesophil
ic bacteria.
Milk powders have very high background
fluorescence.

74
Protocol A (TVC Advanced)Outline

Adapted from Protocol B (TVC Basic)
Pre-treatment at 37C/10 minutes with A31
proprietary chemical enzyme based.
Centrifiltration Pre-treated sample passed
through 25µm nylon mesh filter, and centrifuged
at 1000g for 8 minutes.
Successfully reduces background fluorescence for
most milkpowders.

75
Protocol A (TVC Advanced)Performance
76
Protocol A (TVC Advanced)Limitations

Does not distinguish between thermophilic/mesophil
ic bacteria.

77
Protocol T (Thermophile Protocol)Outline

Adapted from Protocol A by Fonterra Innovation
(Flint et al. 2005)
Changed pre-treatment temperature to 62.8C from
37C.
Changed labelling temperature to 40C from 30C.

78
Protocol T (Thermophile protocol)Performance
79
Protocol Y (Mould Protocol)Outline

Adapted by Fonterra innovation from Chemunex
standard method to count yeast and moulds in
cultured dairy products.
Changed sample size from 1ml to 10mL in order to
achieve greater sensitivity. (Fonterra limits
around 50 cfu/g for mould)

80
Protocol Y (Mould Protocol)Performance
81
A cool reception

Traditional plate count method has been in use
for decades at the 3 main laboratories.
A potentially very beneficial opportunity exists
in using Flow Cytometry one test instead of two.
Reduced costs
Even faster grading
Potential changes to the fundamental way testing
is carried out has encountered mixed responses
from the industry.
Scepticism.
Resistance to change.

82
A cool reception

Bactiflow technology requires competent
laboratory trained staff.
Original plan for 10 Bactiflows throughout
Fonterra manufacturing sites, 3 currently.
On site validation trial problems poor
correlations initially.
Poor sample selection sensitivity of test is
poor below 103 counts/g.
Inconsistent testing of both reference and flow
cytometry methods.
Resource and space issues.

83
More challenges.

Flow cytometers are expensive to buy and to run.
Management want business as usual immediately.
Only one supplier of equipment and reagents.
Manufacturer based in France.
Plate count method is imperfect.

84
Future

Instruments at factories without laboratories.
More products to be tested. E.g. whey, lactose,
butter, cheese etc
More specialised testing. E.g. enterobacteriaceae,
spore testing, specific mesophile test

85
Rapid Bacterial Detection (RBD) 3000
86
Sample trays
Un-attended analysis of 42 samples
Priority tray
87
Different labelling options