Ozone

Administrative data

Description of key information

A total of 10 animal studies were reviewed here for data related to carcinogenicity of ozone, and overall, there is limited scientific evidence to indicate the carcinogenic potential of ozone in animals.

On the other hand, carcinogenicity of ozone in humans has been assessed by the US EPA as part of the "Integrated Science Assessment for Ozone and Related Photochemical Oxidants" (EPA 2013, pages 80-85). In this assessment, the authors carefully reviewed the epidemiological studies on the effects of ozone on human health and concluded that, albeit that ozone exposure may contribute to DNA damage, the evidence is inadequate to determine if a causal relationship exists between ambient ozone exposure and cancer. Since there was insufficient evidence for carcinogenic effects of ozone obtained from animal or human epidemiological studies, classification for carcinogenicity is considered not appropriate.

Key value for chemical safety assessment

Carcinogenicity: via oral route

Endpoint conclusion

Endpoint conclusion:

no study available

Carcinogenicity: via inhalation route

Link to relevant study records

Referenceopen allclose all

Reference 1

Endpoint:

carcinogenicity: inhalation

Type of information:

experimental study

Adequacy of study:

key study

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

comparable to guideline study with acceptable restrictions

Qualifier:

equivalent or similar to guideline

Guideline:

EPA OPPTS 870.4200 (Carcinogenicity)

Principles of method if other than guideline:

The State of California and the Health Effects Institute (HEI) nominated ozone to the National Toxicology Program (NTP) for long-term studies in rats and mice to determine the potential toxicity and carcinogenicity of long-term ozone exposure. The studies reported here include exposures at the current EPA standard (0.12 ppm), the maximum concentration considered to be compatible with long-term survival (1.0 ppm) and an intermediate concentration (0.5 ppm). A second ozone inhalation study was included in which 0.5- and 1.0 ppm exposures were continued to 30 months based on lifetime studies in rats in which the majority of lung tumors developed after 24 months. A third study was included in which male rats were administered 2 concentrations of a known pulmonary carcinogen, 4-(N-nitrosomethylamino)-1-(3-pyridyl)-1-butanone (NNK), and exposed to 0.5 ppm ozone to determine the co-carcinogenic potential of ozone.

GLP compliance:

yes

Specific details on test material used for the study:

Ozone was generated by corona discharge using an OREC model 03V5-ozonator (Ozone Research and Equipment Corp., Phoenix, AZ) with 100% oxygen. The 03 concentration in each chamber was monitored by a multiplexed Dasibi model 1003-AH or 1003-PC ultraviolet spectrophotometric analyser (Dasibi Environmental Corp., Glendale, CA). The monitor was calibrated by comparing it with a chemical specific, calibrated monitor (neutral-buffered potassium iodide method) simultaneously sampling the exposure chambers.

Species:

rat

Strain:

Fischer 344

Sex:

male/female

Details on test animals or test system and environmental conditions:

Male and female F344/N rats were obtained from Simonsen Laboratories (Gilroy, CA). Rats were quarantined for 14 days before the beginning of the study. Five male and five female rats were selected for bacterial culture and selected histopathology prior to the beginning of the study. Approximately 3 weeks after receipt, serology samples were collected for viral screening from up to seven male and seven female rats. Rats were approximately 6 weeks old at the beginning of the studies. The health of the animals was monitored during the studies according to the protocols of the NTP sentinel Animal Program.

All animals were housed individually. Water was available ad libitum, and feed (NIH-07 open formula meal diet, Zeigler Brothers, Inc., Gardners, PA; changed weekly) was available ad libitum except during exposure periods. Cage units were rotated vertically (2-year study) or horizontally (life time study) within each chamber weekly.

Environmental conditions:
Average temperature: 23.9 degrees centigrade;
Relative humidity: 40% to 70%;
Fluorescent light: 12 hours/day;
Room air: 12 to 18 changes/hour.

IN-LIFE DATES:
2 Year ozone study
From: 25 January 1990 to 24 January 1992.

Lifetime study
From: 26 October 1989 to 13 March 1992.

2 Year ozone/NKK study
Ozone - From: 28 November 1989 to 27 November 1991.
NKK - From: 27 November 1989 to 13 April 1990.

Route of administration:

inhalation: gas

Type of inhalation exposure (if applicable):

whole body

Vehicle:

air

Details on exposure:

Animals were exposed in H-2000 chambers. The animals were hold single in stainless steel, wire bottom cages. The build-up of vapour concentration in the chamber at the beginning of exposure to 90% of its final stable concentration (T90) and the decay of concentration at the end of exposure to 10% (T10) were measured prior to the start of each study in chambers with a full complement of mature F344/N rats. These tests were done in conjunction with the pre-start tests for the ozone study. A T90 value of 30 minutes was used based on the experimental data. The T10 value ranged from 5 to 11 minutes.
Chamber concentrations were monitored using an ultraviolet spectrophotometric analyser (Dasibi Model 1003-AH or Dasibi Model 1003-PC systems). Samples were directed to the ozone monitor through computer controlled, multiplexed Teflon valves. A sampling rate of 4 minutes per port assured that all ports were sampled approximately twice per hour. Uniformity of ozone concentration in was measured quarterly during the 2-year and lifetime studies. While the majority of the determinations were within this range, some exceeded this value, and 10.1% was the maximum value found.
The vehicle was conditioned air (single HEPA filters and charcoal).

Analytical verification of doses or concentrations:

yes

Details on analytical verification of doses or concentrations:

Chamber concentrations were monitored using an ultraviolet spectrophotometric analyser (Dasibi Model 1003-AH or Dasibi Model 1003-PC systems) (Glendale, CA). Initially, the UV spectrophotometric analyser (Dasibi Model 1003-AH) was used to monitor the ozone concentration in the exposure chambers, control chamber, room, generator cabinet, and an on-line ozone standard. After approximately 14 months (2-year ozone study), or 16 months (2-year ozone/NNK study and lifetime studies) the Model 1003-AH ozone monitors were replaced with Dasibi Model 1003-PC ozone monitors/generators. This change reduced maintenance and repair costs and maintained an effective system for monitoring ozone.
For both monitoring systems, air sampled at each location was transported to the monitor by transfer lines of Teflon" tubing. Samples were directed to the ozone monitor through a set of eight computer controlled, multiplexed Teflon valves. A sampling rate of 4 minutes per port assured that all ports were sampled approximately twice per hour.

Duration of treatment / exposure:

2 Year ozone study: exposure 6h/d, 5d/w for 105 weeks;
Lifetime study: exposure 6h/d, 5d/w for 125 weeks;
2 Year ozone/NKK study: exposure 6h/d, 5d/w for 105 weeks.

Frequency of treatment:

daily for 5 days/week

Post exposure period:

no post exposure period

Dose / conc.:

0.12 ppm

Dose / conc.:

0.5 ppm

Dose / conc.:

1 ppm

No. of animals per sex per dose:

2 Year ozone study: 50 males and 50 females per dose;
Lifetime study: 50 males and 50 females per dose;
2 Year ozone/NKK study: 48 males

Control animals:

yes, concurrent vehicle

Details on study design:

Concentration levels were based on the National Ambient Air Quality standard (0.12 ppm) and the maximum concentration which the animals would tolerate (1.0 ppm).

Positive control:

n/a

Observations and examinations performed and frequency:

CAGE SIDE OBSERVATIONS: Yes, twice daily for mortalities
DETAILED CLINICAL OBSERVATIONS (not in lifetime study): Yes, initially, monthly through week 92 then every 2 weeks until the end of the study.
BODY WEIGHT: Yes, initially, weekly through week 13, monthly through week 92 then every 2 weeks until the end of the study.
OPHTHALMOSCOPIC EXAMINATION: No
HAEMATOLOGY: No
NEUROBEHAVIOURAL EXAMINATION: No

Sacrifice and pathology:

GROSS PATHOLOGY: No data
HISTOPATHOLOGY: Yes
2 Year ozone study and lifetime study:
Complete histopathology was performed on all rats. In addition to gross lesions and tissue masses, the tissues examined included: adrenal gland, brain, clitoral gland, esophagus, femur, heart, large intestine (cecum, colon, rectum), small intestine (duodenum, jejunum, ileum), kidney, larynx, liver, lungs, lymph nodes (mandibular, mesenteric, bronchial, and mediastinal), mammary gland (with adjacent skin), nose, ovaries, pancreas, parathyroid gland, pituitary gland, preputial gland (rats), prostate gland, salivary gland, spleen, stomach, testes (with epididymis and seminal vesicle), thymus, thyroid gland, trachea, urinary bladder, and uterus
2 Year ozone/NKK study:
Histopathology was performed on all animals. In addition to gross lesions and tissue masses, the tissues examined included lymph nodes (bronchial and mediastinal), lungs, nose, larynx, and trachea.

Other examinations:

n/a

Statistics:

The probability of survival was estimated by the product-limit procedure of Kaplan and Meier (1958). Statistical analyses for possible dose-related effects on survival used Cox's method for testing two groups for equality and Tarone's life table test to identify dose-related trends. P values for the survival analyses are two sided.

Analysis of Neoplasm incidences was by logistic regression analysis. Neoplasm prevalence was modelled as a logistic function of chemical exposure and time. Both linear and quadratic terms in time were incorporated initially, and the quadratic term was eliminated if the fit of the model was not significantly enhanced. The neoplasm incidences of exposed and control groups were compared on the basis of the likelihood score test for the regression coefficient of dose (prevalence analysis of Dinse and Lagakos). In addition to logistic regression, other methods of statistical analysis were used. These methods include the life table test (Cox; Tarone), appropriate for rapidly lethal neoplasms, and the Fisher exact test and the Cochran Armitage trend test, procedures based on the overall proportion of neoplasm-bearing animals. Tests of significance included pairwise comparisons of each exposed group with controls and a test for an overall dose-related trend. Continuity corrected tests were used in the analysis of neoplasm incidence, and reported P values are one sided. The procedures described above were also used to evaluate selected non-neoplastic lesions.
All non-neoplastic lesions in this study were considered to be incidental to the cause of death or not rapidly lethal. The primary statistical analysis used was logistic regression analysis. For lesions detected at the interim evaluation, the Fisher exact test was used.
Organ and body weight data were analysed using procedures test of Dunnett or William's, Jonckheere's test and the Mann­ Whitney U test.

Clinical signs:

effects observed, treatment-related

Description (incidence and severity):

Hypoactivity was observed in male and female rats exposed to ozone. Rats, particularly those exposed to 1.0 ppm, were less active during and immediately after exposure.

Mortality:

mortality observed, treatment-related

Description (incidence):

Hypoactivity was observed in male and female rats exposed to ozone. Rats, particularly those exposed to 1.0 ppm, were less active during and immediately after exposure.

Body weight and weight changes:

effects observed, treatment-related

Food consumption and compound intake (if feeding study):

not examined

Food efficiency:

not examined

Water consumption and compound intake (if drinking water study):

not examined

Ophthalmological findings:

not examined

Haematological findings:

not examined

Clinical biochemistry findings:

not examined

Urinalysis findings:

not examined

Behaviour (functional findings):

not examined

Organ weight findings including organ / body weight ratios:

not specified

Gross pathological findings:

not specified

Histopathological findings: non-neoplastic:

effects observed, treatment-related

Histopathological findings: neoplastic:

no effects observed

Details on results:

Summary of the 2-Year and Lifetime Carcinogenesis Studies of Ozone

Doses 0, 0.12 (2-year study only), 0.5 and 1.0 ppm ozone by inhalation

2-Year males Lifetime males 2-Year females Lifetime females
Body weights 1.0 ppm group 1.0 ppm group 1.0 ppm group 1.0 ppm group
slightly lower than lower than controls slightly lower than slightly lower than
controls controls controls
Survival rates 8/49, 5/50, 7/50, 7/50 0/50, 0/50, 1/50 28/50, 24/50, 30/50, 6/50, 6/50, 7/50
27/50
Nonneoplastic effects
Nose: goblet cell Nose: goblet cell Nose: goblet cell Nose: goblet cell
hyperplasia (1/50, hyperplasia (1/50, hyperplasia (1/50, hyperplasia (0/50,
4/50, 41/50, 48/50); 46/49, 48/49); lateral 2/50, 45/50, 50/50); 47/49, 50/50); lateral
lateral wall wall hyperplasia lateral wall wall hyperplasia
hyperplasia (0/50, (10/50, 48/49, 47/49); hyperplasia (2/50, (4/50, 49/49, 50/50);
8/50, 50/50, 49/50) squamous metaplasia 8/50, 48/50, 50/50) squamous metaplasia
squamous metaplasia (10/50, 23/49, 40/49) squamous metaplasia (5/50, 25/49, 35/50)
(2/50, 6/50, 36/50, Larynx: squamous (2/50, 11/50, 21!50, Larynx: squamous
46/50) metaplasia (0/50, 45/50) metaplasia (2/49,
Larynx: squamous 20/48, 43/47) Larynx: squamous 16/47, 48/50)
metaplasia (0/50, Lung: metaplasia metaplasia (4/50, Lung: metaplasia
2/50, 16/50, 43/50) (0/50, 45/50, 50/50); 5!50, 9/50, 43/50) (0/50, 44/50, 50/50);
Lung: metaplasia histiocytic infiltration Lung: metaplasia histiocytic infiltration
(0/50, 9/50, 46/50, (0/50, 38/50, 49/50); (0/50, 6/50, 48/50, (0/50, 38/50, 49/50);
47/50); interstitial interstitial fibrosis 48/50); interstitial interstitial fibrosis
fibrosis (0/50, 2/50, (0/50, 44/50, 50/50) fibrosis (0/50, 0/50, (0/50, 41/50, 50/50)
40/50, 44/50) 42/50, 47/50)
Neoplastic effects
None None None None

Level of evidence of carcinogenic activity
No evidence No evidence No evidence No evidence

Ozone/NKK study

Lung: Alveolar epithelial metaplasia and interstitial fibrosis occurred in all groups of rats exposed to ozone (with or without NNK), but were not observed in vehicle controls or in animals exposed to NNK alone. The incidence of alveolar cellular infiltration was greater in males exposed to ozone than in the vehicle control males. There was a dose-related increased incidence of atypical alveolar hyperplasia in groups of rats receiving NNK, and the increase was significant. An increased incidence of alveolar/bronchiolar adenoma or carcinoma (combined) also occurred in rats administered 1.0 mg/kg NNK, with or without ozone. The administration of ozone did not affect the occurrence of pulmonary neoplasms or nonneoplastic lesions in rats administered NNK.

Nose: The incidence of hyperplasia in groups of rats exposed to ozone with and without NNK was greater than the incidence in males not exposed to ozone. Incidences of hyperplasia among groups of rats exposed only to NNK were low and similar to that of the controls. The nasal lesions were similar to those seen in rats exposed to ozone by inhalation for 2 years.

Conclusions:

The results of the large "NTP study" (2-year and lifetime inhalation studies) on rats showed that there was no evidence of carcinogenic activity of ozone in male or female F344/N rats exposed to 0.12, 0.5, or 1.0 ppm.

Executive summary:

The toxicity and carcinogenicity of ozone was evaluated in Fischer 344/N rats and B6C3Fl mice exposed 6 hr/day, 5 days/week, to 0.12 (2 years only), 0.5 or 1.0 ppm ozone by inhalation for 2-year and lifetime exposures. A 2-year cocarcinogenicity study (male rats only) included the subcutaneous administration of 0, 0.1 or 1.0 mg/kg body weight. of 4-(N-methyl-Nnitrosamino)- 1-(3-pyridyl)-1-butanone (NNK) for the first 20 weeks along with inhalation exposure to 0 or 0.5 ppm ozone followed by additional 84 weeks of ozone exposure alone.

Ozone exposure in rats did not cause an increased incidence of lung neoplasms. In the co-carcinogenicity study, ozone exposure did not have an additive carcinogenic effect. We conclude, that under the conditions of these studies: (a) ozone exposure is not carcinogenic to either male or female F-344/N rats, (b) ozone does not enhance the incidence of pulmonary neoplasms in F-344/N rats exposed to a known pulmonary carcinogen (NNK), and (c) mild site-specific toxic lesions characteristic of ozone exposure persist in the nasal passage and lung throughout the lifetime of the rat with continued ozone exposure