United States
Environmental Protection
fm Agency
EPA/690/R-05/009F
Final
4-14-2005
Provisional Peer Reviewed Toxicity Values for
Bromoform
(CASRN 75-25-2)
Superfund Health Risk Technical Support Center
National Center for Environmental Assessment
Office of Research and Development
U.S. Environmental Protection Agency
Cincinnati, OH 45268
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Acronyms and Abbreviations
bw body weight
cc cubic centimeters
CD Caesarean Delivered
CERCLA Comprehensive Environmental Response, Compensation and Liability Act
of 1980
CNS central nervous system
cu.m cubic meter
DWEL Drinking Water Equivalent Level
FEL frank-effect level
FIFRA Federal Insecticide, Fungicide, and Rodenticide Act
g grams
GI gastrointestinal
HEC human equivalent concentration
Hgb hemoglobin
i.m. intramuscular
i.p. intraperitoneal
i.v. intravenous
IRIS Integrated Risk Information System
IUR inhalation unit risk
kg kilogram
L liter
LEL lowest-effect level
LOAEL lowest-observed-adverse-effect level
LOAEL(ADJ) LOAEL adjusted to continuous exposure duration
LOAEL(HEC) LOAEL adjusted for dosimetric differences across species to a human
m meter
MCL maximum contaminant level
MCLG maximum contaminant level goal
MF modifying factor
mg milligram
mg/kg milligrams per kilogram
mg/L milligrams per liter
MRL minimal risk level
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MTD
maximum tolerated dose
MTL
median threshold limit
NAAQS
National Ambient Air Quality Standards
NOAEL
no-observed-adverse-effect level
NOAEL(ADJ)
NOAEL adjusted to continuous exposure duration
NOAEL(HEC)
NOAEL adjusted for dosimetric differences across species to a human
NOEL
no-observed-effect level
OSF
oral slope factor
p-IUR
provisional inhalation unit risk
p-OSF
provisional oral slope factor
p-RfC
provisional inhalation reference concentration
p-RfD
provisional oral reference dose
PBPK
physiologically based pharmacokinetic
PPb
parts per billion
ppm
parts per million
PPRTV
Provisional Peer Reviewed Toxicity Value
RBC
red blood cell(s)
RCRA
Resource Conservation and Recovery Act
RDDR
Regional deposited dose ratio (for the indicated lung region)
REL
relative exposure level
RfC
inhalation reference concentration
RfD
oral reference dose
RGDR
Regional gas dose ratio (for the indicated lung region)
s.c.
subcutaneous
SCE
sister chromatid exchange
SDWA
Safe Drinking Water Act
sq.cm.
square centimeters
TSCA
Toxic Substances Control Act
UF
uncertainty factor
Hg
microgram
|j,mol
micromoles
voc
volatile organic compound
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PROVISIONAL PEER REVIEWED TOXICITY VALUES FOR
BROMOFORM (CASRN 75-25-2)
Background
On December 5, 2003, the U.S. Environmental Protection Agency's (EPA's) Office of
Superfund Remediation and Technology Innovation (OSRTI) revised its hierarchy of human
health toxicity values for Superfund risk assessments, establishing the following three tiers as the
new hierarchy:
1. EPA's Integrated Risk Information System (IRIS).
2. Provisional Peer-Reviewed Toxicity Values (PPRTV) used in EPA's Superfund
Program.
3. Other (peer-reviewed) toxicity values, including:
~ Minimal Risk Levels produced by the Agency for Toxic Substances and Disease
Registry (ATSDR),
~ California Environmental Protection Agency (CalEPA) values, and
~ EPA Health Effects Assessment Summary Table (HEAST) values.
A PPRTV is defined as a toxicity value derived for use in the Superfund Program when
such a value is not available in EPA's Integrated Risk Information System (IRIS). PPRTVs are
developed according to a Standard Operating Procedure (SOP) and are derived after a review of
the relevant scientific literature using the same methods, sources of data, and Agency guidance
for value derivation generally used by the EPA IRIS Program. All provisional toxicity values
receive internal review by two EPA scientists and external peer review by three independently
selected scientific experts. PPRTVs differ from IRIS values in that PPRTVs do not receive the
multi-program consensus review provided for IRIS values. This is because IRIS values are
generally intended to be used in all EPA programs, while PPRTVs are developed specifically for
the Superfund Program.
Because science and available information evolve, PPRTVs are initially derived with a
three-year life-cycle. However, EPA Regions or the EPA Headquarters Superfund Program
sometimes request that a frequently used PPRTV be reassessed. Once an IRIS value for a
specific chemical becomes available for Agency review, the analogous PPRTV for that same
chemical is retired. It should also be noted that some PPRTV manuscripts conclude that a
PPRTV cannot be derived based on inadequate data.
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Disclaimers
Users of this document should first check to see if any IRIS values exist for the chemical
of concern before proceeding to use a PPRTV. If no IRIS value is available, staff in the regional
Superfund and RCRA program offices are advised to carefully review the information provided
in this document to ensure that the PPRTVs used are appropriate for the types of exposures and
circumstances at the Superfund site or RCRA facility in question. PPRTVs are periodically
updated; therefore, users should ensure that the values contained in the PPRTV are current at the
time of use.
It is important to remember that a provisional value alone tells very little about the
adverse effects of a chemical or the quality of evidence on which the value is based. Therefore,
users are strongly encouraged to read the entire PPRTV manuscript and understand the strengths
and limitations of the derived provisional values. PPRTVs are developed by the EPA Office of
Research and Development's National Center for Environmental Assessment, Superfund Health
Risk Technical Support Center for OSRTI. Other EPA programs or external parties who may
choose of their own initiative to use these PPRTVs are advised that Superfund resources will not
generally be used to respond to challenges of PPRTVs used in a context outside of the Superfund
Program.
Questions Regarding PPRTVs
Questions regarding the contents of the PPRTVs and their appropriate use (e.g., on
chemicals not covered, or whether chemicals have pending IRIS toxicity values) may be directed
to the EPA Office of Research and Development's National Center for Environmental
Assessment, Superfund Health Risk Technical Support Center (513-569-7300), or OSRTI.
INTRODUCTION
The HEAST (U.S. EPA, 1997) lists a subchronic oral reference dose (RfD) value of 2E-1
for bromoform. The subchronic RfD is based on a NOAEL of 25 mg/kg-day for hepatic
vacuolization in male rats administered bromoform five days per week for 13 weeks (NTP,
1989a). The LOAEL in this study was 50 mg/kg-day. The NOAEL was adjusted to a continuous
dose of 17.9 mg/kg-day and divided by a composite uncertainty factor (UF) of 100, which
includes factors of 10 each to account for animal to human extrapolation and interhuman
variability. The source document for derivation of the subchronic oral RfD is a Health and
Environmental Effects Document (HEED) for Bromoform (U.S. EPA, 1989). The HEAST
references IRIS (U.S. EPA, 2003) for the chronic RfD of 2E-2 mg/kg-day. The chronic RfD is
also derived from the subchronic data for hepatic vacuolization in male rats obtained in the 13-
week NTP (1989a) study. A composite UF of 1000, which includes an additional factor of 10 for
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use of data from a subchronic study, was used in the calculation of the chronic value. The
chronic RfD was verified by the RfD Work Group on August 13, 1987.
Several additional sources were reviewed for information on bromoform toxicity. The
CARA list (U.S. EPA, 1991, 1994a) includes no documents for bromoform other than the 1989
HEED. A Health Effects Assessment (HEA) is available for trihalogenated methanes (U.S. EPA,
1987). The HEA lists subchronic and chronic RfDs of 0.056 mg/kg-day and 0.0056 mg/kg-day,
respectively, for bromoform that were derived from subchronic oral exposure data published by
Chu et al. (1982). The Drinking Water Standards and Health Advisories list (U.S. EPA, 2002)
includes bromoform and lists the current chronic RfD value of 2E-2 mg/kg-day. ATSDR (1990)
derived a chronic oral minimal risk level (MRL) for bromoform of 0.2 mg/kg-day based on a
NOAEL of 20 mg/kg-day for hepatic pathology in a chronic study by Tobe et al. (1982). The
World Health Organization (WHO, 2002) has not prepared an Environmental Health Criteria
document on bromoform.
Neither the HEAST, the HEED, nor the HEA report a subchronic inhalation reference
concentration (RfC) for bromoform. The HEAST references IRIS for the chronic RfC. IRIS
indicates that the inhalation database for bromoform is inadequate to calculate an inhalation
reference concentration and lists the current RfC status as not verifiable (U.S. EPA, 2003). The
RfD/RfC Workgroup assigned this status on February 11, 1993. ACGIH (2001) lists a TLV-
TWA of 0.5 ppm (5.2 mg/m3) with skin and A3 cancer notations for bromoform. This
occupational exposure limit is intended to minimize the potential for lacrimation, salivation, and
irritation of the respiratory tract, and possible liver damage as reported in rodent studies. The A3
notation identifies bromoform as a confirmed animal carcinogen with unknown relevance to
humans. MOSH (2002) and OSHA (2002) have adopted 0.5 ppm (5 mg/m3) with a skin notation
for the bromoform REL-TWA and PEL-TWA, respectively.
The HEAST references IRIS (U.S. EPA, 2003) for the oral cancer slope factor, drinking
water unit risk, and inhalation unit risk values for bromoform. These values were verified by the
CRAVE Work Group on August 2, 1989. The oral cancer slope factor of 7.9E-3 (mg/kg-day)"1
and oral unit risk value of 2.3E-7 (i-ig/L)"1 are derived from dose-response data for neoplastic
lesions in the large intestine of female F344/N rats (NTP, 1989a). Appropriate inhalation
exposure data were not available for estimation of carcinogenic potency. Therefore, the
inhalation unit risk of 1. 1E-6 (|_ig/m3)"' was derived from the oral exposure tumor data by route-
to-route extrapolation. The HEAST lists an inhalation slope factor of 3.9E-3 (mg/kg-day)"1 for
bromoform. The calculation of this factor is not clearly described in the documents referenced in
the HEAST. Handwritten comments on a draft of the IRIS file dated May 19, 1989 suggest that
the inhalation slope factor was obtained by adjusting the oral slope factor for a default
bromoform absorption of 50% via the inhalation route. U.S. EPA (1989, 2003) evaluated the
weight of evidence for human carcinogenicity and assigned bromoform to carcinogenicity group
B2 (probable human carcinogen). NTP (2002) does not list bromoform among the chemicals it
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considers to be known human carcinogens or reasonably anticipated to be human carcinogens.
IARC (1991, 1999) has assigned bromoform to weight of evidence Group 3, not classifiable as to
its carcinogenicity to humans.
Literature searches to identify studies relevant to the derivation of provisional toxicity
values for bromoform were conducted for the period 1988 through September 19, 2002.
Databases searched included: TOXLINE, MEDLINE, TSCATS, RTECS, CCRIS, DART,
EMIC/EMICBACK, HSDB, GENETOX and CANCERLIT. Additional literature searches from
2002 through May 2004 were conducted by NCEA-Cincinnati using TOXLINE, MEDLINE,
Chemical and Biological Abstracts databases.
REVIEW OF PERTINENT DATA
Human Studies
No adequate data on the subchronic or chronic effects of bromoform in humans were
located. Some data on the acute or short-term effects of oral exposure are available because
bromoform was used in the early 1900s to sedate children suffering from whooping cough (U.S.
EPA, 1989, 1994b). A typical dose for mild sedation was one drop (about 180 mg) given three to
six times daily, or approximately 54 mg/kg-day (U.S. EPA, 1994b). Several deaths or near-
deaths related to this practice have been documented. The most prominent clinical sign of
poisoning in fatal cases was profound depression of the central nervous system. Death usually
resulted from respiratory failure. The fatal doses were not quantified, but have been estimated to
be 20 to 40 drops of bromoform or approximately 150 to 300 mg/kg-day (U.S. EPA, 1989,
1994b). Low-level inhalation exposure is reported to result in irritation, lacrimation, and
reddening of the face (Sax and Lewis, 1989). Dykan (1964) reported that workers in bromoform
production exhibited changes in the central nervous system and liver. No supporting details were
provided on the duration or level of exposure, the number of workers evaluated, or potential
confounding factors.
A number of epidemiological studies have examined the potential association of
reproductive or developmental outcomes with consumption of tap water containing
trihalomethanes, including bromoform (reviewed in Nieuwenhuijsen et al., 2000 and Bove et al.,
2002). Studies that have examined associations of reproductive or developmental outcomes with
trihalomethanes have in most cases used total trihalomethane concentration (a composite
measure which includes the brominated trihalomethanes and chloroform) as the exposure metric.
One study is available which examined the potential association specifically between bromoform
concentration in disinfected tap water and reproductive outcome. Waller et al. (1998) conducted
a prospective study in pregnant women to examine the association between exposure to
trihalomethanes in drinking water and spontaneous abortion (pregnancy loss at 20 or less
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completed weeks of gestation). No association with incidence of spontaneous abortion was
observed for bromoform when data were adjusted for gestation or maternal age at interview,
smoking, history of pregnancy loss, and maternal race or after adjustment for the presence of
other trihalomethanes in tap water.
Animal Studies
NTP (1989a) administered bromoform to male and female F344/N rats by corn oil gavage
for 13 weeks (5 days/week). The study was conducted using a standard NTP protocol and was
GLP compliant. The test animals (10/sex/dose) received doses of 0, 12, 25, 50, 100, or
200 mg/kg-day. The administered doses in both male and females correspond to duration-
adjusted doses of 0, 8.6, 17.9, 35.7, 71.4, and 143 mg/kg-day, respectively. Complete
histopathology was performed on rats in the vehicle control and high-dose groups. Liver
histopathology was performed on rats in all treatment groups. No rats died before the end of the
study and body weights were not significantly affected in either sex. All high-dose animals and
male rats dosed with 100 mg/kg-day were lethargic. A dose-related increase in the incidence of
hepatocellular vacuolization was observed in male rats (incidence: vehicle control, 3/10; 12
mg/kg-day, 6/10; 25 mg/kg-day, 5/10; 50 mg/kg-day, 8/10; 100 mg/kg-day, 8/10; 200 mg/kg-day,
10/10). The response in males reached statistical significance at 50 mg/kg-day when data were
analyzed using Fisher's Exact Test (U.S. EPA, 2003). This lesion was characterized by the
presence of well-demarcated vacuoles in the cytoplasm of hepatocytes. The number of these
vacuoles was reported to be greater in the 200 mg/kg-day group than in other dose groups.
Hepatocellular vacuolization was not observed in female rats. No data were presented for any
other histopathologic lesion in males or females. NOAEL and LOAEL values of 25 mg/kg-day
and 50 mg/kg-day (duration adjusted values of 17.9 and 35.7 mg/kg-day) were identified in this
study based on hepatocellular vacuolization in male rats.
In a parallel study, NTP (1989a) administered bromoform to male and female B6C3Fj
mice by corn oil gavage for 13 weeks (5 days/week). The study was conducted using a standard
NTP protocol and was GLP compliant. Test animals (10/sex/dose) received doses of 0, 25, 50,
100, 200, or 400 mg/kg-day. The administered doses correspond to duration-adjusted doses of 0,
17.9, 35.7, 71.4, 143, and 286 mg/kg-day, respectively. Complete histopathology was conducted
on the vehicle control and high-dose groups. In addition, liver histopathology was conducted on
male mice receiving doses of 100 mg/kg-day and higher. One female mouse died at 100 mg/kg-
day; no other deaths occurred at any dose level. Final mean body weights in dosed animals did
not differ statistically from the vehicle control, although the final body weight in high-dose males
was reduced by 8%. A dose-related increase in the incidence of minimal to moderate
hepatocellular vacuolization was seen in male mice. This lesion was not observed in female
mice. The histologic changes associated with this lesion in males involved only a few cells or
were diffuse. The incidence of this lesion was 5/10 at 200 mg/kg and 8/10 at 400 mg/kg. The
incidences of hepatocellular vacuolization in the vehicle control and 100 mg/kg-day groups were
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not explicitly reported and are assumed to be 0/10. NOAEL and LOAEL values of 100 mg/kg-
day and 200 mg/kg-day (duration adjusted values of 71.4 and 143 mg/kg-day), respectively, were
identified in this study based on hepatocellular vacuolization in male mice.
Chu et al. (1982) administered bromoform to male and female weanling Sprague-Dawley
rats (20 rats/sex/group) in drinking water for 90 days. The tested concentrations were 0, 5, 50,
500, or 2500 ppm. No information was provided on measures taken to monitor or validate the
concentrations of bromoform in drinking water. Half of the animals in each group (10/sex/dose)
were sacrificed at the end of the exposure period and the remaining animals were given tap water
for another 90 days to assess recovery. Based on estimation of bromoform intake per rat by the
study authors and data provided for body weight gain, the administered concentrations resulted in
doses of approximately 0, 0.65, 6.1, 57, and 218 mg/kg-day for males and 0, 0.64, 6.9, 55, and
283 mg/kg-day for females. A trend toward decreased body weight gain was observed, but this
response did not reach statistical significance in any exposure group. Lymphocyte counts were
significantly decreased in high-dose males and females when evaluated 90 days after cessation of
treatment. Lactate dehydrogenase activity was significantly decreased in high-dose males and
females at cessation of treatment and the effect was still evident after the 90-day recovery period.
Mild histologic changes occurred in the liver and thyroid of male and female animals. The
observed hepatic lesions included increased cytoplasmic volume and vacuolization due to fatty
infiltration. The incidence and severity of hepatic lesions tended to increase with dose (Table 1).
The incidences of combined hepatic lesions in the 500 ppm and 2500 ppm exposure groups were
significantly greater (p<0.05) than the vehicle control incidence for both male and female rats
when independently analyzed using Fisher's Exact Test by SRC. The severity of combined
hepatic lesions was significantly greater in 2500 ppm males and in 500 and 2500 ppm females.
Lesions of the thyroid included decreased follicular size and colloid density and occasional focal
collapse of follicles. Neither the incidence nor severity of thyroid lesions in treated animals
differed significantly from the controls. Histologic changes in most dose groups were mild and
similar to controls when evaluated after the 90-day recovery period, although males in the high-
dose group continued to exhibit an increased incidence of hepatic lesions with greater severity
relative to the vehicle control. The NOAEL and LOAEL values in this study are approximately 7
mg/kg-day and 55 mg/kg-day, respectively, based on increased incidence and severity of hepatic
lesions (combined) in male and female rats.
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Table 1. Incidence and Severity of Hepatic Lesions in the Subchronic Oral Exposure
Study Conducted by Chu et al., 1982
Concentration
(PPm)
Estimated Dose
(mg/kg-day)
Males/Females
Males
Females
Incidence
Severity3
Incidence
Severity
0
(vehicle control)
0
2/9
(22%)
1.2 ±0.44
0/10
(0%)
1.0 ±0.0
5
0.65/0.64
5/10
(50%)
1.6 ±0.70
3/10
(30%)
1.3 ±0.48
50
6.1/6.9
4/10
(40%)
1.4 ±0.52
0/10
(0%)
1.0 ±0.0
500
57/55
7/10b
(70%)
1.8 ±0.63
4/10b
(40%)
1.5 ± 0.71°
2500
218/283
o ^
O
SO ^S-
2.7 ± 0.71°
6/10b
(60%)
1.7 ± 0.67°
a Severity grading ranges from 1 (normal) to 10 (malignant tumors or complete necrosis)
b Significantly different from vehicle control (p 0.05) by Fisher's Exact Test (analysis performed by SRC)
c Significantly different from vehicle control (p 0.05) (analysis performed by study authors)
Tobe et al. (1982) evaluated the chronic effects ofbromoform administered in the diet to
male and female Slc:Wistar SPF rats (40/sex/group) for 24 months. Bromoform was
administered in microencapsulated form at dietary levels of 0.0%, 0.04%, 0.16%, or 0.65%).
Control groups (70 rats/sex) received feed amended with microcapsules that did not contain
bromoform. Data were reported from interim sacrifice of 9 animals/sex in the control group and
5 animals/sex/dose in the exposure groups at 18 months. All surviving animals were sacrificed
at 24 months. Necropsy, hematology, and serum biochemistry were conducted at the interim and
final sacrifices. Based on the published data for body weight and food consumption, the
administered levels ofbromoform correspond to doses of approximately 0, 22, 90, and
364 mg/kg-day for males and 0, 38, 152, and 619 mg/kg-day for females. Marked suppression
(>65%) of body weight gain was seen in males and females at the high dose (364 and 619 mg/kg-
day) and mild suppression of body weight gain (roughly 15-20%) was seen in males and females
at the mid dose (90 and 152 mg/kg-day). No dose-related hematological changes were observed
at either 18 or 24 months. At the 18 month interim time point, dose-related increases in absolute
and relative liver weights occurred in females at > 152 mg/kg-day. Dose-related changes in
serum parameters in males included decreased glucose concentration, non-esterified fatty acid
(NEFA) concentration, and cholinesterase (CHE) activity and increased gamma-glutamyl
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transpeptidase (GGTP), leucine aminopeptidase (LAP), and glucose-6-phosphate dehydrogenase
(G6PDH) activities. Dose-related changes in females included decreased serum
albumin/globulin ratio, glucose concentration, and CHE activity and increased total protein
concentration, GGTP activity, and G6PDH activity. Prominent necropsy findings at 18 months
included dose-related yellowing of the liver males and females; roughening of the liver surface in
males; and hypertrophy and transparency of the lobules of the liver in females. At study
termination, increased absolute and relative liver weights were observed in mid- and high-dose
(at >152 mg/kg-day) females. Dose-related alterations in serum biochemistry in males included
decreased levels of NEFA and CHE activity. Decreased glucose and NEFA concentrations and
increased GGTP activity, LAP activity, glycylproline-dipeptidyl aminopeptidase activity, and
potassium concentration showed dose-related trends in females. The most prominent findings at
necropsy were yellowing of the surface of the liver in all high-dose animals and mid-dose
females; roughening of the liver surface in all high-dose animals; small white spots on the liver
in some high-dose (364 mg/kg-day) males and mid- and high-dose (at > 152 mg/kg-day)
females; and transparent lobules in mid- and high-dose females. No histopathology data for
bromoform have been published from this study. The body weight and serum biochemistry data
obtained for male animals in this study suggest NOAEL and LOAEL values of 22 mg/kg-day and
90 mg/kg-day, respectively.
NTP (1989a) administered bromoform to male and female F344/N rats (50/sex/group) by
gavage in corn oil at doses of 0, 100, or 200 mg/kg-day for 103 weeks (5 days/week). The study
was conducted using a standard NTP protocol and was GLP compliant. The administered doses
correspond to duration-adjusted doses of 0, 71.4, and 143 mg/kg-day, respectively. Necropsy and
histopathological examination were performed on all animals at study termination. Final mean
body weight was decreased by 25% in high-dose females and by 21% in high-dose males when
compared to the corresponding controls. Survival of high-dose males was significantly lower
than that of the vehicle controls after week 91 of the study. Survival of dosed female rats was
similar to the vehicle control group. Treatment-related clinical signs included lethargy in males
and females and increased aggressiveness in males. Increased incidences of hepatic fatty change
and chronic inflammation were observed in males and females at both doses (Table 2). The
incidence of mixed cell foci were increased in females at both doses. The incidence of hepatic
necrosis was increased in high-dose males, while a dose-related decrease in the incidence of
hepatic necrosis was observed in females. Nonneoplastic changes in other tissues were not
reported. This study identified a LOAEL of 100 mg/kg-day (duration-adjusted value of 71.4
mg/kg-day), the lowest dose tested, for hepatic fatty change and chronic inflammation.
NTP (1989a) administered bromoform doses of 0, 50, or 100 mg/kg-day to male B6C3Fj
mice (50/dose) by corn oil gavage for 103 weeks (5 days/week). Female B6C3Fj mice (50/dose)
received corn oil gavage doses of 0, 100, or 200 mg/kg-day for 103 weeks (5 days/week). The
study was conducted using a standard NTP protocol and was GLP compliant. The administered
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Table 2. Incidence of Hepatic Lesions in Rats in the Two-Year Corn Oil Gavage
Study of Bromoform (NTP, 1989a)
Males
Females
Lesion
Vehicle
100
200
Vehicle
100
200
Control
mg/kg-day
mg/kg-day
Control
mg/kg-day
mg/kg-day
Fatty Change
23/50
49/50
50/50
19/50
39/49
46/50
(46%)
(98%)
(100%)
(38%)
(80%)
(92%)
Active Chronic
0/50
29/50
23/50
9/50
8/49
27/50
Inflamation
(100%)
(58%)
(46%)
(18%)
(16%)
(54%)
Necrosis
7/50
3/50
20/50
11/50
3/49
2/50
(14%)
(6%)
(40%)
(22%)
(6%)
(4%)
Mixed Cell
10/50
11/50
8/50
8/50
25/49
28/50
Focus
(20%)
(22%)
(16%)
(16%)
(51%)
(56%)
doses correspond to duration-adjusted doses of 0, 71.4, and 143 mg/kg-day, respectively. At
study termination, all animals were necropsied and a complete histological examination of
tissues was performed on vehicle control and high-dose mice. Selected tissues were examined in
low-dose mice. Decreased survival was observed in females of both dosed groups when
compared to the vehicle control group. Survival in dosed males was comparable to the vehicle
control group. The decline in survival of females was attributed in part to a utero-ovarian
infection in the test animals. No treatment-related clinical signs were noted in either sex. Final
mean body weights for low- and high-dose females were 10% and 16% lower than the control
values, respectively; final mean body weight was not affected in males. Increased incidences of
minimal to mild fatty change were noted in the livers of dosed females relative to controls
(vehicle control, 1/49; low-dose, 9/50; high-dose, 24/50). The incidence of focal or multifocal
follicular cell hyperplasia was increased in the thyroid of high-dose females (vehicle control,
5/49; low-dose, 4/49; high-dose, 19/47). Hyperplasia of the glandular stomach occurred at
slightly increased incidences in dosed mice. No other statistically or biologically significant
nonneoplastic changes were reported in mice of either sex in response to treatment. The LOAEL
for this study is 100 mg/kg-day (duration-adjusted value of 71.4 mg/kg-day), the lowest dose
tested, based on decreased body weight and histologic changes in female rats.
The available inhalation exposure data for animals are reviewed in IRIS (U.S. EPA,
2003) and the HEED for Bromoform (U.S. EPA, 1989). von Oettingen (1955) reported that
exposure of rats to bromoform vapors may result in irritation of the respiratory tract and
lacrimation. As reported in IRIS, bromoform had a narcotic effect on rabbits subjected to a
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single inhalation exposure at concentrations ranging from 1064 to 1741 ppm (Dykan, 1964).
Rats exposed to a bromoform vapor concentration of 240 ppm for 10 days developed central
nervous system effects and dystrophic and vascular alterations of the liver and kidney (Dykan,
1964). Exposure of rats to a vapor concentration of 24 ppm (4 hours/day) for two months
induced hepatic disorders characterized by decreased blood clotting and impaired glycogenesis in
the liver and altered renal filtration capacity (Dykan, 1962). No adverse effects were evident
after two months of exposure to a vapor concentration of 4.8 ppm (Dykan, 1964). U.S. EPA
(1989, 2003) noted that these data were obtained from study abstracts that did not provide
sufficient information for critical evaluation of the studies.
The developmental toxicity of bromoform has been assessed in rats. Ruddick et al.
(1983) administered 0, 50, 100, or 200 mg/kg-day to pregnant Sprague-Dawley rats (15/dose) by
corn oil gavage on gestation days 6 through 15. Maternal weight gain, organ weights,
hematology, and clinical chemistry parameters were unaffected by treatment. Increased
incidences of a 14th rib, wavy ribs, interparietal deviations, and sternebral variations were
reported in treated animals. The study authors did not report statistical analysis of these data.
Analysis of the published data using Fisher's Exact Test indicates that the litter incidence of
sternebral variations (control, 1/15; 50 mg/kg-day, 3/15; 100 mg/kg-day, 5/14; 200 mg/kg-day,
8/15) was significantly different (p = 0.007) from the control at 200 mg/kg-day. The responses
for other fetotoxic endpoints did not reach statistical significance (p 0.05) by this test. Based
on this analysis, the NOAEL for developmental toxicity in this study is 100 mg/kg-day and the
LOAEL is 200 mg/kg-day for increased incidence of sternebral variations in the offspring of
pregnant females treated with bromoform. The NOAEL for maternal toxicity is 200 mg/kg-day,
the highest dose tested.
NTP (1989b) evaluated the reproductive toxicity of bromoform in CD-I mice using a two
generation continuous breeding protocol. Male-female pairs (20 pairs/dose) were administered
daily doses of 50, 100, or 200 mg/kg-day by corn oil gavage during a seven-day precohabitation
and a 98-day cohabitation period. Vehicle control animals (40 pairs/dose) received corn oil only.
The Fj generations from the vehicle control and 200 mg/kg-day groups were also treated and
evaluated. In the F0 generation, the body weights at delivery of dams in the 200 mg/kg-day group
were consistently less than the value for the control group. The reduction in body weight was
statistically significant after the delivery of four out of the five total litters. No evidence of
systemic toxicity was reported for F0 males. There was no apparent effect of treatment on
fertility, litters per pair, live pups per litter, proportion of live births, sex of live pups, or pup
body weights. In the Fj generation, male and female mice receiving 200 mg/kg-day had
increased relative liver weights and decreased relative kidney weights. Terminal body weights of
dosed Fj males were significantly lower than the corresponding control values. Minimal to mild
hepatocellular degeneration was observed in 19/20 dosed males. Postnatal survival was
significantly decreased in the 200 mg/kg-day group. No other effects on fertility or reproduction
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were observed. The NOAEL and LOAEL values in this study are 100 mg/kg-day and 200
mg/kg-day, respectively, for reproductive toxicity.
Other Studies
The available toxicokinetic data for bromoform are limited. Absorption of bromoform
occurs from the respiratory tract, gastrointestinal tract, and skin (von Oettingen, 1955). Mink et
al. (1986) estimated gastrointestinal absorption of radiolabeled bromoform to be 60 to 90% in
mice and rats given a single oral dose, as determined from recovery of radioactivity from exhaled
air, urine, and tissues. No quantitative data are available for absorption via the inhalation or
dermal routes. Once absorbed, bromoform and its metabolites are rapidly distributed. In rats,
bromoform distributed to adipose tissue, kidney, brain, and liver after a single gavage dose of
radiolabeled compound (Parra et al., 1986). Radioactivity has also been detected in the urinary
bladder, lungs, skeletal muscle, pancreas, stomach, and thymus of rodents after administration of
a single gavage dose of radiolabeled bromoform (Mink et al., 1986). Bromoform is metabolized
to carbon dioxide, carbon monoxide, and hydrogen bromide via a cytochrome P-450-dependent
pathway (U.S. EPA, 1989). The primary site for metabolism is the liver. Metabolism to toxic
species appears to be mediated by both oxidative and reductive pathways, as inferred from
studies of bromoform and structurally-related trihalomethanes. Preliminary evidence obtained
using transfected strains of Salmonella typhimurium suggests that production of toxic metabolites
may also be mediated by a glutathione S-transferase- dependent pathway (DeMarini et al., 1997).
Excretion of bromoform and its metabolites occurs primarily via the lungs, with a small fraction
excreted in the urine (Mink et al., 1986).
DERIVATION OF PROVISIONAL SUBCHRONIC AND CHRONIC
ORAL RfD VALUES FOR BROMOFORM
A chronic RfD of 2E-2 mg/kg-day is listed for bromoform on IRIS (U.S. EPA, 2003),
based a NOAEL of 25 mg/kg-day for hepatic vacuolization in male rats administered bromoform
five days per week for 13 weeks (NTP, 1989a). The presence of a chronic RfD on IRIS
precludes derivation of a provisional chronic RfD for this chemical.
In considering derivation of a provisional subchronic RfD, no new human or animal data
on the subchronic toxicity of bromoform were identified in the literature search. None of the
existing human data are adequate for derivation of a subchronic RfD value for bromoform. The
existing subchronic animal data include well-conducted subchronic gavage studies in rats and
mice (NTP, 1989a) and data from a drinking water exposure study conducted in rats (Chu et al.,
1982). Additional data are available from a reproductive toxicity study in mice (NTP, 1989b)
and a developmental toxicity study in rats (Ruddick et al., 1983). The NTP (1989a) data for rats
11
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identify histologic changes in the liver as the most sensitive response to bromoform exposure
among the endpoints evaluated in these studies.
As previously noted, the subchronic RfD currently listed in the HEAST was derived by
U.S. EPA (1989) using a NOAEL of 25 mg/kg-day for hepatocellular vacuolization in male
F344/N rats administered bromoform by corn oil gavage five days per week for 13 weeks (NTP,
1989a). The LOAEL for this lesion was 50 mg/kg-day. A composite UF of 100 was applied to
the duration adjusted dose of 17.9 mg/kg-day to give the subchronic RfD of 0.2 mg/kg-day. A
modifying factor (MF) was not used in the calculation.
A benchmark dose (BMD) modeling approach (U.S. EPA, 2000) was used as an
alternative to the conventional NOAEL/LOAEL approach for derivation of the provisional
subchronic RfD. The NTP (1989a) data for hepatocellular vacuolization in male rats exposed to
bromoform for 13 weeks were selected for this purpose (3/10, 6/10, 5/10, 8/10, 8/10, and 10/10
in the time-adjusted dosage as 0, 12, 25, 50, 100, and 200 mg/kg-day dose groups, respectively).
These data were obtained in a well-documented study conducted under Good Laboratory Practice
guidelines and describe a statistically and biologically significant dose-related trend in the
selected endpoint. In addition, this study utilized a larger number of doses than other candidate
studies, including three doses below 100 mg/kg-day that provide information on the shape of the
dose-response curve in the region of greatest interest. Available models in the U.S. EPA
Benchmark Dose Software (BMDS) program (Version 1.3.1) were fit to the incidence data for
hepatocellular vacuolization to estimate the duration-adjusted dose producing a 10 percent extra
risk of developing the lesion (i.e., the BMD). BMDS modeling results were evaluated according
to the criteria outlined in U.S. EPA (2000). The best fit to the data was obtained with the
Quantal-Linear model (Table 3). This model gave values of 4.4 mg/kg-day for the BMD and 2.6
mg/kg-day for the BMDL10, the lower 95 percent confidence interval on the BMD. Figure 1 plots
predicted (from the fitted Quantal-Linear model) and observed lesion incidence as a function of
the duration-adjusted dose, as well as the BMD and the BMDL10.
12
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Table 3. Summary of BMD Modeling Results Obtained for Incidence of Hepatocellular
Vacuolization in Male Rats Using the U.S. EPA Benchmark Dose Software
Modela
Chi Square
P
AICb
BMDC
BMDL10d
Gamma
1.92
0.589
67.7261
1.9
0.00031
Logistic
2.48
0.648
66.1399
7.3
4.7
Log Logistic
2.40
0.494
68.4402
4.4
0.039
Probit
2.45
0.654
66.0888
7.8
5.3
Quantal Linear
2.18
0.703
65.8698
4.4
2.6
Quantal Quadratic
3.45
0.483
67.1516
19.9
13.6
Weibull
2.02
0.568
67.8044
2.8
0.013
a Available models in the U. S. EPA Benchmark Dose Software Program (version 1.3.1)
b AIC, Aikake Information Criterion
c BMD, Benchmark Dose. The BMD is a maximum likelihood estimate of the dose producing a 10 percent extra
risk of hepatic vacuolization in male F344/N rats.
d BMDL10 = lower 95 percent confidence interval on the BMD.
13
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Quantal Linear Model with 0.95 Confidence Level
O.E
<
i=
o
Quantal Linear
0.6
0.4
0.2
BMDL
BMP
1 3:1 0 09/04 2002
50
100
dose
150
200
Figure 1. BMD Modeling Results for Hepatocellular Vacuolization in Male Rats
Administered Bromoform by Corn Oil Gavage for 13 weeks (NTP, 1989a)
14
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A provisional subchronic RfD of 0.03 mg/kg-day for bromoform is calculated using the
duration adjusted BMDL10 of 2.6 mg/kg-day for hepatocellular vacuolization in male rats
exposed to bromoform for 13 weeks (NTP, 1989a):
BMDL10
subchronic p-RfD =
UFxMF
2.6 mg/kg-day
100 x 1
0.03 mg/kg-day (3E-2 mg/kg-day)
A composite UF of 100 incorporating factors of 10 each for extrapolation from animals to
humans and for human variability; and a modifying factor (MF) of 1 are used in the calculation.
Use of the BMDL10 in this calculation accounts for inherent uncertainty in the study results and
ensures (with 95% confidence) that the desired benchmark response of 10% extra risk is not
exceeded. A database uncertainty factor was not applied because supporting systemic studies
were available and developmental (in only one species, however) and reproductive endpoints had
been studied and found not to be sensitive targets for this chemical.
Confidence in the principal study for the subchronic RfD (NTP, 1989a) is medium-to-
high. The study used both sexes of two species, included comprehensive histopathological
examination of livers in all animals, identified liver lesions as the critical effect in both species
with associated NOAELs and LOAELs, and was reported in adequate detail, including the lesion
incidence data. However, the study did not investigate clinical chemistries or perform urinalysis.
Confidence in the database is medium-to-high. Several studies support the choice of hepatic
lesions as the critical effect, and reproductive and developmental endpoints have been studied
and found not to be sensitive targets. Medium-to-high confidence in the subchronic p-RfD
follows.
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DERIVATION OF PROVISIONAL SUBCHRONIC AND CHRONIC
INHALATION RfC VALUES FOR BROMOFORM
U.S. EPA (2003) concluded in a previous review of inhalation data for bromoform that
insufficient data were available for derivation of a chronic p-RfC. The available inhalation data
are from abstracts of studies conducted by Dykan (1962, 1964). In summarizing these studies,
U.S. EPA (2003) noted that no details were available for exposure generation or characterization,
specific effect measures, or results. In addition, there were insufficient toxicokinetic data to
perform a route-to-route extrapolation from existing oral data, and the potential for local
respiratory (portal-of-entry) effects was not adequately characterized. No new subchronic or
chronic inhalation studies, reproductive or developmental studies that employed an inhalation
route of exposure, or relevant toxicokinetic studies were identified in the literature search. The
database for bromoform, therefore, remains inadequate for derivation of subchronic or chronic
p-RfC values.
DERIVATION OF A PROVISIONAL CARCINOGENICITY ASSESSMENT
FOR BROMOFORM
A cancer assessment, including derivation of an oral slope factor and inhalation unit risk,
is available for bromoform on IRIS (U.S. EPA, 2003), precluding derivation of a provisional
carcinogenicity assessment for this chemical.
REFERENCES
ACGIH (American Conference of Governmental Industrial Hygienists). 2001. 2001 Threshold
Limit Values for Chemical Substances and Physical Agents and Biological Exposure Indices.
ACGIH, Cincinnati, OH.
ATSDR (Agency for Toxic Substances and Disease Registry). 1990. Toxicological Profile for
Bromoform and Chlorodibromomethane. U.S. Department of Health and Human Services,
Public Health Service. Atlanta, GA. Online, http://www.atsdr.cdc.gov/toxprofiles/tpl30.html
Bove, F., Y. Shim and P. Zeitz. 2002. Drinking water contaminants and adverse pregnancy
outcomes: a review. Environ. Health Perspect. 110 (Suppl. 1): 61-74.
Chu I., D.C. Villeneuve, V.E. Secours et al. 1982. Trihalomethanes: II. Reversibility of
toxicological changes produced by chloroform, bromodichloromethane and bromoform in rats.
J. Environ. Sci. Health B. 17: 225-240.
16
-------�
4-14-2005
DeMarini, D.M., M.L. Shelton, S.H. Warren et al. 1997. Glutathione S-transferase-mediated
induction of GC—>AT transitions by halomethanes in Salmonella. Environ. Mol. Mutagen.
30(4): 440-447.
Dykan, V.A. 1962. Changes in liver and kidney functions due to methylene chloride and
bromoform. Nauchn. Tr. Ukr. Nauchn. - Issled. Inst. Gigieny Truda i Profzaboleuanil. 29: 82-
90. (Cited in U.S. EPA, 1989, 2003)
Dykan, V.A. 1964. Problems on toxicology, clinical practice and work hygiene in the
production of bromine-organic compounds. Gig. Sb. 100-103. (Cited in U.S. EPA, 1989, 2003)
IARC (International Agency for Research on Cancer). 1991. Bromoform. Chlorinated drinking
water; chlorination by-products; some other halogenated compounds; cobalt and cobalt
compounds. IARC Monographs on the Evaluation of Carcinogenic Risks to Humans. 52:
213-242.
IARC (International Agency for Research on Cancer). 1999. Bromoform. Re-evaluation of
some organic chemicals, hydrazine and hydrogen peroxide. IARC Monographs. 71: 1331-1338.
Mink, F.L., J. Brown and J. Rickabaugh. 1986. Absorption, distribution and excretion of
14C-trihalomethanes in mice and rats. Bull. Environ. Contam. Toxicol. 37: 752-758.
Nieuwenhuijsen, M.J., M.B. Toledano, N.E. Eaton et al. 2000. Chlorination disinfection
byproducts in water and their association with adverse reproductive outcomes: A review. Occup.
Environ. Med. 57: 73-85.
NIOSH (National Institute for Occupational Safety and Health). 2002. Online NIOSH Pocket
Guide to Hazardous Chemicals. Index of Chemical Abstract Numbers (75-25-2). Online.
http://www.cdc.gov/niosh/npg/npgd0066.html
NTP (National Toxicology Program). 1989a. Toxicology and Carcinogenesis Studies of
Tribromomethane (Bromoform) (CAS No:75-25-2) in F344/N Rats and B6C3F1 Mice (Gavage
Studies). U.S. Dept. of Health and Human Services, Public Health Service, National Institutes of
Health. Technical Report Series, No. 350.
NTP (National Toxicology Program). 1989b. Bromoform: Reproduction and Fertility
Assessment in Swiss CD-I Mice When Administered by Gavage. National Institute of
Environmental Health Sciences. Research Triangle Park, NC. Report No. NTP-89-068.
NTP (National Toxicology Program). 2002. Management Status Report. Online.
http://ntp-server.niehs.nih.gov/cgi/iH Indexes/ALL SRCH/iH ALL SRCH Frames.html
17
-------�
4-14-2005
OSHA (Occupational Safety and Health Administration). 2002. OSHA Standard 1910.1000
Table Z-l. Part Z, Toxic and Hazardous Substances. Online.
http://www.osha-slc.gov/OsliStd data/1910 1000 TABLE Z-l.html
Parra, P., E. Martinez, C. Sunol et al. 1986. Analysis, accumulation and central effects of
trihalomethanes. 1. Bromoform. Toxicol. Environ. Sci. 11(2): 79-91. (Cited in U.S. EPA,
1989)
Ruddick, J.A., D.C. Villeneuve and I. Chu. 1983. A teratological assessment of four
trihalomethanes in the rat. J. Environ. Sci. Health. 1318(3): 333-349.
Sax, N.I. and R.J. Lewis. 1989. Dangerous Properties of Industrial Materials, Seventh Ed.
Van Nostrand Reinhold, New York. (Cited in U.S. EPA, 2003)
Tobe, M., Y. Suzuki, K. Aida et al. 1982. Studies on the Chronic Oral Toxicity of
Tribromomethane, Dibromochloromethane and Bromodichloromethane. Unpublished
Intraagency Report to the National Institute of Hygienic Sciences. Tokyo Medical and Dental
University, Tokyo, Japan.
U.S. EPA. 1987. Health Effects Assessment for Trihalogenated Methanes. Prepared by the
Office of Health and Environmental Assessment, Environmental Criteria and Assessment Office,
Cincinnati, OH for the Office of Solid Waste and Emergency Response, Washington, DC.
U.S. EPA. 1989. Health and Environmental Effects Document for Bromoform. Prepared by the
Office of Health and Environmental Assessment, Environmental Criteria and Assessment Office,
Cincinnati, OH for the Office of Solid Waste and Emergency Response, Washington, DC.
U.S. EPA. 1991. Chemical Assessments and Related Activities (CARA). Office of Health and
Environmental Assessment, Washington, DC. April.
U.S. EPA. 1994a. Chemical Assessments and Related Activities (CARA). Office of Health and
Environmental Assessment, Washington, DC. December.
U.S. EPA. 1994b. Final Draft for the Drinking Water Criteria Document on Trihalomethanes.
Health and Ecological Division, Office of Science and Technology, Office of Water,
Washington, DC.
U.S. EPA. 1995. The Use of the Benchmark Dose Approach in Health Risk Assessment. Office
of Research and Development, Research Triangle Park, Washington, DC. EPA/630/R-94/007.
18
-------�
4-14-2005
U.S. EPA. 1997. Health Effects Assessment Summary Tables (HEAST). FY-1997 Update.
Prepared by the Office of Research and Development, National Center for Environmental
Assessment, Cincinnati, OH for the Office of Emergency and Remedial Response, Washington,
DC. July, 1997. EPA-540-R-97-036. NTIS PB97-921199.
U.S. EPA. 2000. U.S. Environmental Protection Agency. Benchmark Dose Technical Guidance
Document. External Peer Review Draft. October. EPA/630/R-00/001.
U.S. EPA. 2002. 2002 Edition of the Drinking Water Standards and Health Advisories. Office
of Water, Washington, DC. Summer 2002. EPA 822-R-02-038. Online.
http ://www.epa. gov/waterscience/drinking/ standards/dwstandards .pdf
U.S. EPA. 2003. Integrated Risk Information System (IRIS). Office of Research and
Development. National Center for Environmental Assessment, Washington, DC. Online.
http://www.epa.gov/iris/
Von Oettingen, W.F. 1955. The halogenated aliphatics, olefinic, cyclic aromatic, and aliphatic-
aromatic hydrocarbons including the halogenated insecticides, their toxicity and potential
dangers. U.S. Department of Health, Education and Welfare, Public Health Service,
Washington, DC. Publication No. 414. (Cited in U.S. EPA, 1989, 2003)
Waller, K., S.H. Swan, G. DeLorenze et al. 1998. Trihalomethanes in drinking water and
spontaneous abortion. Epidemiology. 9(2): 134-140.
WHO (World Health Organization). 2002. Online catalogs for the Environmental Health
Criteria Series. Online: http://www.who.int/dsa/cat98/chemtox8.htm#
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