Study of Thermal Destruction of Bacillus anthracis'
Surrogates Spiked on Building Materials
Paper #1113
Chun W. Lee, Joseph P. Wood*, Doris A. Betancourt, William P. Linak, Paul M.
Lemieux*, Timothy R. Dean, Marc Y. Menetrez, and Jared Novak+
U.S. Environmental Protection Agency, Office of Research and Development, National
Risk Management Research Laboratory, Air Pollution Prevention and Control Division
Research Triangle Park, NC 27711. ^National Homeland Security Research Center. +EPA
student contractor.
Nicole Griffin
ARCADIS G & M, Inc., P.O. Box 13109, Research Triangle Park, NC 27709
ABSTRACT
A significant amount of contaminated material may need to be disposed of after a bio-
terrorism attack. The efficacy of disposal of building materials contaminated with
biological agents by incineration is complicated by matrix effects associated with the
contaminant and the material it is on. It is important to know the relative difficulty of
destroying these biological agents bound to different materials. This project examines the
thermal destruction of surrogate biological agents that are present on several common
building materials including ceiling tiles and wallboard. A laboratory-scale thermal reactor
was constructed to examine the effect of building material, heating temperature and
residence time on the destruction of Bacillus anthracis' surrogates. Results of the study
showed that the destruction of the Bacillus anthracis surrogates, Bacillus subtilis and
Geobacillus stearothermophilus spiked on building materials strongly depends on the type
of material and time-temperature history of the simulants in the reactor.
INTRODUCTION
After a biological terrorist attack occurring in a public building, a significant amount of
contaminated building material and waste may need to be disposed of. Some of the
materials to be disposed of may have already been externally decontaminated. This
material could include a porous material such as contaminated wall board, ceiling tile, and
carpet. It is possible that much of this material could be disposed of in high temperature
thermal incineration facilities, including medical/pathological waste incinerators, municipal
waste combustors, or hazardous waste combustors. Portable incineration units might be
field erected to dispose of these materials on-site in order to minimize exposure. The
disposal of building materials contaminated with harmful biological agents by thermal
incineration is complicated by matrix effects, such as the heat transfer rate associated with
the material on which the agent is bound. It is important to know the relative difficulty of
destroying these biological agents bound on different materials. Selection of appropriate
disposal facilities requires fundamental knowledge of the behavior of the matrix-bound
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contaminants in various thermal environments. A review of existing data showed viable
spores were detected in some of the air emissions and residual ash samples obtained from
microbiological survivability tests conducted at several medical waste incinerators
(MWIs).1 Very little is known about the behavior of the likely contaminants bound in these
various matrices within incineration facilities, and complete destruction of the
contaminants without releasing air emissions of contaminants and contaminated
combustion residues from the disposal of these materials is very important.
This project examined the destruction of surrogate biological agents bound on several
common building materials including ceiling tiles and wallboard. A laboratory-scale
reactor was used in this project to examine building material, heating temperature and
residence time affecting the destruction of surrogate biological contaminants including
Bacillus subtilis and Geobacillus stearothermophilus, surrogates for Bacillus anthracis.
The results from these studies can be used to evaluate incineration technologies for
appropriateness for disposal of contaminated building materials.
EXPERIMENTAL
The primary objective of this project was to heat different building materials in a bench-
scale tube furnace at specified gas temperatures and time periods. The building materials
were inoculated with bacteriological spores (surrogates for Bacillus anthrax) at a level of
104 - 106 spores/cm2 prior to heating in the furnace, and after heating, the materials were
subsequently analyzed to determine survivability of the spores. The overall purpose of the
project was to determine the effect that different building materials have on the heat
resistance of Bacillus anthrax surrogates. A secondary objective of the project is to obtain
internal temperature profiles (temperature versus time) of the building materials when
subjected to the specified gas temperatures. These temperature profile tests of the building
materials were conducted prior to the microbial survivability tests.
Thermal Reactor System
A bench-scale reactor was constructed for studying the destruction of anthrax surrogates
bound on different building materials. A schematic of the reactor system is shown in Figure
1. The heating source of the reactor was a Thermcraft electrical furnace, which is 46 cm
long and has a 30 cm long heating element. A borosilicate glass tube of 5 cm outside
diameter (4 cm inside diameter), and 71 cm long is placed in the tube furnace for heating of
the samples. At each end of the glass tube is a ball and socket joint with a 0.6 cm nipple to
allow for insertion of thermocouples (T/C). The glass tube also has a 5 cm long, 0.6 cm
diameter nipple at each end (perpendicular to the tube) to allow for connection of 0.6 cm
Teflon tubing for nitrogen gas flow. All tubing connections in the apparatus use
compression type fittings.
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Figure 1. Schematic of Experimental Apparatus to Investigate Thermal Destruction of Bacillus
anthracis Surrogates on Various Building Materials
Hood
N2 Gas How
Gas How
Electrical
Furnace
Rotameter
Tl———ouple * Data
Acquisition/Computer
Filter
Thermo-
couple ¦
1
z
N2 Gas
Cylinder
Condensate
Trap
lass Tube
* For T emperature Profile T est Only
Test Procedures
The building material samples tested included ceiling tile and wallboard (drywall). Each
set of the two building material samples was cut from the same source. Each sample
consisted of two layers, each of which is 7.6 cm long by 3.8 cm wide by 0.6 cm thick, and
stacked together. The building material samples were placed in rectangular aluminum
-3
sample pans. Nitrogen (N?) gas regulated with a rotameter at 500 cm/min flowed through
the glass tube to prevent combustion of the sample placed inside the tube. A filter (0.22
micron pore size) was placed at the outlet of the glass tube to capture any spores entrained
in the nitrogen carrier gas.
For the tests to determine the internal temperature profiles of the materials, a hole was
drilled between the two layers of material to allow for insertion of the T/C. The tip of a
0.16 cm diameter T/C was placed between the two layers of building material. The layers
were fastened together and the sample was placed in the center of the tube furnace.
Temperatures were measured using Omega brand Type E T/C. A 0.3 cm diameter T/C was
used to measure the gas temperature within the glass tube. The tip of the T/C was placed in
the center of the tube (in terms of height), and just left of the sample. The furnace has its
own thermocouple placed at the center of the top heating element and its temperature
reading is displayed on the temperature control box. This temperature was also recorded
(manually) during the experiments. Once the gas temperature within the glass tube reached
the desired temperature, the sample pan with the building material was inserted into the
glass tube to the center of the oven and gas and material temperature data were recorded
every 5 seconds with an Iotech data acquisition system (DAS).
For the spore survivability tests, no internal material temperatures were measured, although
the same materials, gas temperatures and heating procedure were used for the
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corresponding temperature profile tests. The spores were placed between the two layers of
the material and then fastened together prior to a survivability test. When the specified
heating period for a test had been reached, the sample was removed from the furnace and
analyzed for the spore survivability.
Prior to each spore survivability test all the components of the furnace glass tube except
T/Cs were steam sterilized for 60 minutes at 121 °C and 15 lb/in2. Due to the heat
sensitivity of the T/Cs, they were sanitized with 95% (v/v) ethanol.
Materials and Analytical Methods
Bacterial Strains, Growth Conditions and Preparation of Spore Suspensions
Bacillus anthracis surrogates were used in this study to prepare spore suspensions. These
were Bacillus subtilis (ATCC 19659) and Geobacillus stearothermophilus (ATCC 7953).
Bacillus subtilis spores were harvested from 72 hr cultures grown on 10% Columbia Broth
with 0.1 mM Mn+2 (ASTM E 2197) at 35 °C + 2 °C. After the third centrifugation, the
pellet was resuspended in sterile deionized water (1/10 volume of the original culture
medium) and placed in a water bath at 80 °C for 10 min to heat-kill vegetative cells. The
final spore concentration was approximately 108 spores/mL. Geobacillus
stearothermophilus spores were harvested from 72 hr cultures grown on sporulation broth3
at 55 °C + 2 °C using the procedure as previously described. The final spore concentration
was approximately 106 spores/mL.
Building Materials Preparation and Inoculation
The bulk building materials (BBM) used in this study included ceiling tile and wallboard.
Ceiling tiles that had been in use for approximately 1 year in a laboratory were made
available due to construction changes. These were Class A, standard-white, fire-retardant,
textured-faced ceiling tiles composed of wood fiber (0 - 60%) and fibrous glass (0 - 13%)
as specified by the manufacturer. New drywall was used for these tests which consisted of
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gypsum core (5 mg/m ) wrapped with a paper lining (cellulose - 5 mg/m ) as specified by
the manufacturer.
All the BBM were cut into sample sizes measuring 7.62 x 3.81 cm, weighed, individually
wrapped in aluminum foil and steam sterilized by autoclaving. The sterile BBM were
inoculated with either 1.0 ml of Bacillus subtilis spores for a final concentration of 108
spores/ml or 1.0 ml of Geobacillus stearothermophilus spores for a final concentration of
106 spores/ml. Once inoculated the BBM pieces were placed on a sterile tray and allowed
to dry overnight within a biological safety cabinet. Once dried, the samples were prepared
by stacking two (7.62 x 3.81 cm) pieces with the inoculated sides facing each other and
then tested in thermal destruction experiments.
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Spore Recovery after the Thermal Destruction Tests
Immediately after the thermal destruction tests, the samples were aseptically placed in a
sterile jar with cold water for quenching. To recover the spores the sample was transferred
to a sterile polyethylene bag and if necessary more sterile water was added to prepare a
1/10 (weight of sample to volume of water, w/v) dilution of the sample. The bag with
sample was inserted in a masticator-blender (Nasco Sampling Products, Modesto, CA) and
homogenized for 15 sec at 10 beats per sec.4 The homogenate was then diluted as needed
and plated in triplicate on Trypticase Soy Agar (TSA). Unheated, inoculated BBM
samples were homogenized at the same time to determine the spore concentration prior to
the thermal destruction tests.
For recovery of Bacillus subtilis spores, TSA plates were incubated at 35 °C + 2 °C for 24
hr. For recovery of Geobacillus stearothermophilus spores, TSA plates were incubated at
55 °C + 2 °C for 24 hr. Spore concentration before and after the heating was determined by
colony-forming units (CFU, CFU = number of colonies x dilution factor).5
Analysis of Heated BBM Samples
Spore survivability was determined by Log 10 reduction (LR) using the CFU prior to the
heating and the CFU after the heating as in the equation shown below.6
LR = loglO (c) - loglO (t)
Where:
c = CFU of inoculated building material prior to heating
t = CFU of inoculated building materials after heating
RESULTS AND DISCUSSION
Temperature Profiles
The internal temperature profiles of the ceiling tile and wallboard were measured at several
gas temperatures (148, 204, 260, and 315 °C) in a constant N2 flow (500 cc/min). The two
building materials showed significantly different temperature profiles under the same
heating conditions. Examples of the temperature profiles for the ceiling tile and wallboard
heated at 204 °C gas temperature are shown in Figures 2 and 3, respectively. Ceiling tile
approached close to the gas temperature of 204 °C in about 6 min (360 sec). However, the
wallboard only reached 125 °C after it was heated at the same gas temperature for 15 min
(900 sec). It appears that wallboard which is made of gypsum (CaSO^FbO), contained
high moisture content (20 wt. %), and evaporation of water was observed at the same time
when the internal temperature profile of wallboard flattened out. It is likely that the heat
provided by the furnace was used to evaporate the moisture contained in the wallboard, not
to raise the temperature of the material.
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Figure 2. Internal Temperature Profile of Ceiling Tile Measured at 204 °C Initial Gas
Temperature
250
U
e 150
ce
a
a
S
H
100
Gas
200
0
100 200 300
Heating Time (sec)
400
Figure 3. Internal Temperature Profile of Wallboard Measured at 204 °C Initial Gas
Temperature
o
CO
Cl>
200 400 600 800
Heating Time (sec)
1000
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Bacillus anthracis Surrogate Spores Survivability Tests
The survivability of Bacillus subtilis bound on ceiling tile and wallboard was tested at gas
heating temperatures of 148, 204, 260, and 315 °C. Results of the survivability tests for the
ceiling tile and wallboard are shown in Figures 4, and 5, respectively. Figure 4 indicates
that the destruction (expressed in Log 10 reduction, LR) of Bacillus subtilis spiked on
ceiling tile occurs rapidly when they are heated at gas temperatures above 200 °C. Almost
complete destruction (with a LR value of greater than 8) of the ceiling tile bound spores
occurs within 2 min of heating at 315 °C. Similar level of destruction occurs within 5 and
10 min when the gas heating temperature is reduced to 260 and 204 °C, respectively. The
rate of destruction decreases significantly when the heating temperature is reduced further
to 148 °C, and reduction of a LR value of 6 is achieved in about 25 min.
Figure 4. Effect of Heating Temperature and Time on Reduction of Bacillus subtilis Spiked
on Ceiling Tile
9
8
7
6
J
4
3
2
1
0
0 5 10 15 20 25 30 35
Heating Time (minutes)
Results shown in Figure 5 indicate that the Bacillus subtilis spiked on wallboard have
significantly slower destruction rates than those for the ceiling tile bound spores (Figure 4)
under the similar gas heating temperatures. Destruction of the wallboard bound spores
with the LR value of 6 occurs in about 30 min when the sample is heated at 315 °C gas
temperature. Similar high level of destruction occurs at about 60 min of heating when the
gas heating temperature is reduced to 204 °C. Very little spore destruction is observed
when the heating temperature is reduced further to 146 °C even at extended heating period
of over 100 min.
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Figure 5. Effects of Heating Temperature and Time on Reduction of Bacillus
subtilis Spiked on Wallboard
0 20 40 60 80 100 120 140
Heating Time (min)
The survivability of Geobacillus stearothermophilus spiked on ceiling tile and wallboard
was also tested at the similar temperature range for the Bacillus subtilis. Results of the
survivability tests for the Geobacillus stearothermophilus spiked on ceiling tile and
wallboard are shown in Figures 6 and 7, respectively. Similar to the Bacillus subtilis, the
destruction of the Geobacillus stearothermophilus spiked on ceiling tile (shown in Figure
6) occurs very fast, and the destruction rate decreases with decreasing heating temperature.
Complete destruction of the spores occurs in less than 5 min at heating temperatures of 260
and 315 °C, which increases to about 7 min when the heating temperature is reduced to 204
°C. The similarly fast destruction rates observed for the two different spores spiked on
ceiling tile (Figures 4 and 6) suggest that the thermal destruction of the Bacillus anthracis
surrogate spores bound on a building material depends strongly on the heat transfer
characteristics of the material. The high spore destruction rates observed for the two
different surrogate spores bound on ceiling tile are consistent with the fast heat transfer
rates measured for this building material in the internal temperature profile tests (see Figure
2).
Results shown in Figure 7 indicate that the destruction rates of Geobacillus
stearothermophilus bound on wallboard are much slower than those for the same organism
bound on ceiling tile. For example, complete destruction of the wallboard bound spores
occurs within 10 min at 315 °C, which increases to over 20 min when the gas heating
temperature is reduced to 260 °C. Spore destruction occurs at much slower rates when the
temperature is reduced further to 204 and 148 °C. The slow rates of destruction
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Figure 6. Effects of Heating Temperature and Time on Reduction of Geobacillus
Stearothermophilus Spiked on Ceiling Tile
Heating Time (min)
Figure 7. Effect of Heating Temperature and Time on Reduction of
Geobacillus stearothermophilus Spikbed on Wallboard
Heating Time (min)
observed for wallboard bound Geobacillus stearothermophilus are similar to those
observed for Bacillus subtilis bound on the same building material (Figure 5). The slow
destruction rates are consistent with the slow heat transfer rates measured for this material
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(Figure 3), which provide further support that the thermal destruction of Bacillus anthracis
surrogate spores bound on a building material depends strongly on the heat transfer rate of
the material.
CONCLUSIONS
A laboratory-scale thermal reactor was constructed to evaluate the effect of building
material, heating temperature, and time on the destruction of Bacillus anthracis' surrogates.
The building materials tested included ceiling tile and wallboard, and tests for another
building material, carpet, are ongoing. Results of the initial tests conducted for measuring
the internal temperature profiles of the ceiling tile and wallboard indicate that ceiling tile
has much faster heat transfer rate than the wallboard. The survivability of two different
Bacillus anthracis surrogates, Bacillus subtilis and Geobacillus stearothermophilus spiked
on these two building materials was also tested. Results of the tests showed that the
destruction of the two Bacillus anthracis surrogates spiked on the building materials
strongly depends on the heat transfer characteristics of the material. The destruction of the
two surrogates spiked on ceiling tile occurs at much faster rates than those of the surrogates
spiked on wallboard. The different anthrax thermal destruction behaviors observed for
these two building materials are consistent with their different heat transfer characteristics.
REFERENCES
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Organisms in Medical Waste Incinerators: A Review of Available Data," presented at the
International Conference in Incineration and Thermal Treatment Technologies, Phoenix,
AZ, May, 2004. www.IT3.umd.edu.
2. Priest, F.G.; Grigovora, R. In Methods for Studying the Ecology of Endospore-
forming Bacteria; Grigovora, R; Norris, J.R. Ed.; Methods in Microbiology (22); Academic
Press: San Diego CA, 1990; pp 565-591.
3. Atlas, R.M. Sporulation Media. Handbook of Microbiological Media. 1997; pp 145.
4. Betancourt, D.A.; Dean, T.R.; Menetrez, M.Y. Journal of Microbiological Methods
(in press).
5. Koch,A.L. In Growth Measurements: Gerhardt, P.; Murray, R.G.E.; Wood, W.A.;
Krieg, N.R., Ed.; Methods for General and Molecular Bacteriology. American Society of
Microbiology: Washington, DC, 1994; pp 248 - 277.
6. DeVries, T.A.; Hamilton, M.A. Estimating the Antimicrobial Log Reduction. Part 1
Quantitative Assays. Quantitative Microbiology 1999, vol. 1, pp 29-45.
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