(1E)-1-chloro-3,3,3-trifluoroprop-1-ene

Administrative data

Endpoint:

two-generation reproductive toxicity

Type of information:

experimental study

Adequacy of study:

key study

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Data source

Materials and methods

Test guidelineopen allclose all

GLP compliance:

yes (incl. QA statement)

Limit test:

no

Test material

Test animals

Species:

rat

Strain:

Wistar

Sex:

male/female

Details on test animals or test system and environmental conditions:

TEST ANIMALS
- Source: Harlan, the Netherlands
- Age at receipt 5 - 6 weeks
- Body weight at study initiation: Male: mean dose groups approx. 207 g; Female: mean dose groups approx. 171 g
- Housing: The animals were housed in macrolon cages with a bedding of wood shavings (Lignocel, Type ¾) and strips of paper (Enviro-dri) and wooden block as environmental enrichment. During premating animals were housed by sex, 4 to a cage, during mating 1 male plus 1 female, following mating females were housed individually and with their litter following delivery.
- Diet: Cereal-based (closed formula) rodent diet (Rat & Mouse No. 3 Breeding Diet, RM3) from a commercial supplier (SDS Special Diets Services, Witham, England). ad libitum, except during exposure
- Water: ad libitum except during exposure
- Acclimation period: 12 days

ENVIRONMENTAL CONDITIONS
- temperature (°C) 22 ± 2
- humidity (%): 45 - 65
- air changes (per hr): 10
- Photoperiod (dark/light): 12/12

Administration / exposure

Route of administration:

inhalation: gas

Type of inhalation exposure (if applicable):

other: combination nose only/ whole body

Vehicle:

air

Details on exposure:

EXPOSURE EQUIPMENT
Animals were exposed to the test atmosphere in head/nose-only exposure units (hereafter called nose-only exposure units) and by whole-body exposure chambers:
- Nose-only exposure: Each exposure unit (Institute’s design) consisted of a cylindrical PVC column with a volume of 75 litres, surrounded by a transparent hood. The test atmosphere was introduced at the bottom of the central column, and was exhausted at the top. Each column included three rodent tube sections of 20 ports each. The animals were secured in plastic animal holders (Battelle), positioned radially through the outer hood around the central column (males and females alternated). The remaining ports were closed. Only the nose of the rats protruded into the interior of the column. Animals were rotated each week with respect to the position in the column, viz. they were moved 5 places each time, and also weekly alternated between the upper, middle and lower sections. The units were illuminated externally by normal laboratory fluorescent tube lighting. The total air flow through the units was at least 1 L/min per animal. The air entering the units was controlled at 22 ± 3 °C and the relative humidity was maintained between 30 and 70 %.
- Whole-body exposure: Animals were exposed whole-body to the test atmosphere in 2.2 m3 whole-body exposure units (Hazleton Systems, Inc., Aberdeen, MD, USA). These chambers are constructed of stainless steel, with glass doors on two sides which allowed observation of the animals during exposure. The test atmosphere was introduced at the top of the exposure chambers, and exhausted at the bottom. Each chamber could accommodate 28 cages to individually house the dams and 56 cages to individually house 28 male and 28 female animals up to approx. week 6. Animals rotated at least every week with respect to their position in the exposure chamber. The units were illuminated externally by normal laboratory fluorescent tube lighting. The ventilation rate was between 12 and 15 times/hour (corresponding to 440 – 550 L/min). The temperature in the chambers was controlled at 22 ± 3 °C and the relative humidity was maintained between 30 and 70 %.

GENERATION OF TEST ATMOSPHERE
- Nose-only exposure: The inhalation equipment was designed to expose rats to a continuous supply of fresh test atmosphere. The cylinder containing the test substance was warmed using a heating jacket to pressurize the cylinder. To generate the test atmosphere, a liquid flow of test substance, controlled by a peristaltic pump (Watson-Marlow 502S, Bredel Pumps Limited, Falmouth, Cornwall, England), was evaporated in a stainless steel evaporator. The temperature of the evaporators was controlled at 20 °C using a thermal bath. The vapor was transported in a stream of humidified compressed air, the flow of which was measured by a mass stream meter (Bronkhorst, Hi Tec, Ruurlo, The Netherlands), supplemented with a mass flow controlled stream of oxygen (mid and high concentration groups). The exposure unit for the control animals was supplied with a measured stream of humidified compressed air only. The generated test atmospheres were directed to the bottom inlets of the exposure units. At the top of the units the test atmospheres were exhausted. The animals were placed in the exposure units after stabilization of the test atmosphere.
- Whole-body exposure: The test atmosphere for each whole-body exposure chamber was generated similarly. Mass flow controlled amounts of gaseous test material were mixed with a main air stream, available as a laboratory provided source of (non-pressurized) filtered air. Oxygen was added for the mid and high concentration groups. To ensure a ventilation rate of 12 - 15 times/hour, air speed was measured continuously in the exhaust of the exposure chamber using a Ventcaptor air speed sensor (Weber Sensors Inc., Acworth, GA, USA). The flow was automatically adjusted to a predefined setpoint by a PID feedback system using an electrical valve (EA20, Georg Fischer AG, Schaffhausen, Switzerland). In addition, air speed in the exhaust of the exposure chambers was checked weekly using a rotary gas meter (IRM-A, Elster-Instromet, Luxembourg, Luxembourg).

Details on mating procedure:

At the end of the premating period, each female was caged with one male from the same group. Animals were caged together until mating occured or 1 week had elapsed. In the F1-generation the mating period was extended for one day. Mating pairs were clearly identified. Every consecutive morning during the mating period, vaginal smears were made for determination of the presence of sperm. The day on which sperm was detected in the vaginal smear was considered as gestation day 0. Upon evidence of copulation the females were caged individually for the birth and rearing of their pups. Sperm positive females that turned out to be non-pregnant were killed after more than 21 days after copulation. Females that did not show evidence of copulation after the end of the mating period were also housed individually until sacrifice (more than 21 days after the last day of the mating period). Dams were allowed to raise one litter.

Analytical verification of doses or concentrations:

yes

Details on analytical verification of doses or concentrations:

The actual concentration of the test material in the test atmosphere was monitored with a total carbon analyser (for groups 2 and 3: Ratfisch RS55T, Munich, Germany; for group 4: Sick Instruments Benelux, Hedel, The Netherlands). The responses of the analysers were recorded on a PC every minute using a CAN transmitter (G.Lufft Mess- und Regeltechnik GmbH, 70719 Fellbach, Germany). Test atmosphere samples were taken continuously from the exposure unit at the animals’ breathing zone and were passed to the total carbon analyser through a sample line. The mean response was calculated by averaging values read every minute. Prior to the various exposures, the total carbon analysers were calibrated for a particular target concentration by sampling from three concentrations in duplicate in a range including the target concentration. The concentrations were prepared by injecting a known amount of 1233zd(E) into a PET sample bag containing a measured amount of air. These calibrations were checked weekly by measuring the concentration from a sample bag close to the target concentration. If the measured concentration from the sample bags deviated more than 5 % from the calculated concentration during the study and this was confirmed with a second sample bag, the total carbon analyser was calibrated again.

Duration of treatment / exposure:

6 hours/day

Frequency of treatment:

F0 generation animals were exposed nose-only to the test material in air for 6 hrs/day/5 days/wk for at least 10 weeks prior to mating and daily during mating. Daily exposure continued for F0 females up to gestation day (GD) 19 for 6 hrs/day (nose only). From lactation day 5 (PN5), females were exposed daily (6 hrs/day) to the test substance by whole body exposure until the end of the lactation period (PN21) or their sacrifice shortly thereafter. The F1-generation male and female pups were exposed by whole body exposure (6 hrs/day, 5 days/wk) from postnatal day 22 up to ca. 6 wks of age. Subsequently, the F1 animals were exposed in a similar manner as that described for the F0 generation.
Non-mated females were exposed (nose-only) until the end of the nose-only exposure period. Non-pregnant animals were exposed by nose-only exposure until GD 19 of the presumed gestation period; thereafter the exposure was not resumed.

Details on study schedule:

Selection of parents from the F1 generation: On or shortly after PN day 21 the F1-pups were weaned and 28 males and 28 females were selected at random from as many litters as possible in each group to rear the next generation.
F1 parental animals not mated until at least 10 weeks after selection from the F1 litters.

Doses / concentrationsopen allclose all

No. of animals per sex per dose:

28

Control animals:

yes, sham-exposed

Details on study design:

Exposure level selection rational: High exposure level same as used in 13-week inhalation toxicity study which resulted in heart lesions.

CULLING
On postnatal (PN) day 4, litters of more than 8 pups were adjusted by eliminating extra pups by random selection to yield, as nearly as possible, 4 males and 4 females per litter. Pups euthanised at culling were examined externally for abnormalities and subsequently preserved in a neutral aqueous phosphate buffered
4 % solution of formaldehyde.

WEANING AND SELECTION OF PUPS
On or shortly after PN day 21 the F1-pups were weaned and 28 males and 28 females were selected at random selection from as many litters as possible in each group to rear the next generation (see Annex 5). Furthermore, F1- and F2-generation pups were randomly selected for necropsy. Four spare pups per sex and dose group were selected at weaning of the F1-pups. From PN 22, these pups were exposed to the same concentrations as their mothers and
pups from the groups treated with the test substance were discarded on day 7 of the pre-mating period of the F1-generation. Selected spare F1-pups of the control group were exposed until day 6 of the pre-mating period (for possible replacement) and were sacrificed at the end of the in-life phase of the study (satellite animals).

Examinations

Parental animals: Observations and examinations:

- General clinical observations: Each animal was observed daily in the morning hours by cage-side observations and, if necessary, handled to detect signs of toxicity. On working days and on all exposure days, all cages were checked again in the afternoon for dead or moribund animals to minimize loss of animals from the study. In the period before the start of exposure on Saturdays, Sundays and public holidays only one check per day was carried out. All abnormalities, signs of ill health or reactions to treatment were recorded.
- Body weight: Body weights of male and female rats were recorded four days before the start of administration of the test substance at randomization, at the start of the study (day 0) and weekly thereafter during the premating period. Males were weighed once per week during the postmating period until sacrifice. Females were weighed once per week during postmating and mated females were weighed on days 1, 7, 14 and 21 during presumed gestation and on day 0, 4, 7, 14 and 21 of lactation. In addition, the animals were weighed on their scheduled necropsy date in order to calculate the correct organ to body weight ratios.
- Food consumption: The food consumption was measured from day 0 onwards on the same days as the body weight was measured. Erroneously, no food consumption was measured of the not mated F1-females in the postmating period. The results are expressed in g per animal per day and g per kg body weight per day.

Oestrous cyclicity (parental animals):

Vaginal smears to evaluate the estrus cycle length and normality were made daily for about 3 weeks prior to mating. Smears were made and stained of all females, but only the smears of the control group (group 1) and the high-dose group (group 4) were evaluated. Since no treatment-related abnormalities were observed, the vaginal smears of the animals of the low- and mid-dose group were not examined.

Sperm parameters (parental animals):

- Epididymal sperm motility, count and morphology: At scheduled necropsy, epididymal sperm was derived from the left cauda epididymis of all males of all groups. For this purpose the cauda epididymis was dissected, weighed and thereafter minced in M199 medium containing 0.5 % bovine serum albumin. Sperm motility and, after sonification and DNA staining, the cauda epididymal sperm reserves (sperm count) was measured for all males of all groups, using the Hamilton Thorne Integrated Visual Optical System (IVOS). In addition, a smear of the sperm solution was prepared and stained for all males, but only the smears of the control group (group 1) and the high-dose group (group 4) males were examined for morphology. No treatment-related changes were observed in the high-dose group, therefore the examination of sperm morphology was not extended to the low- and mid-dose groups.
- Testicular sperm count: At necropsy, the left testis of all males of all groups was placed on dry ice and subsequently stored in a freezer (<-70 °C) for later determination of the number of homogenisation-resistant spermatids. The testes to be analysed were thawed just before further processing. Following removal of the tunica albuginea, the testicular parenchyma was weighed, minced and homogenised in Saline Triton X-100 solution. Following DNA-staining, the homogenisation-resistant sperm heads were enumerated using the IVOS and the daily sperm production was calculated. The evaluation of homogenisation-resistant spermatids was performed in the control (group 1) and high-dose (group 4). No treatment-related changes were observed in the high-dose group, therefore the evaluation of homogenisation-resistant spermatids was not extended to the low- and mid-dose groups.

Litter observations:

- Parturition and litter evaluation: At the end of the gestation period (GD 21), females were examined twice daily for signs of parturition. To keep nest disturbance to a minimum the litters were examined only once daily for dead pups.
- Litter size, sexes and weight: The total litter size and numbers of each sex as well as the number of stillbirths, live- and dead pups and grossly malformed pups were evaluated on days 0, 4, 7, 14 and 21 of lactation. The pups were individually weighed on days 0, 4, 7, 14, and 21 of lactation. Mean pup weight was calculated per sex and for both sexes combined. The number of runts [defined as pup weight less than mean pup weight of the control group minus 2 standard deviations] was calculated.
- Sexual maturation: The following landmarks for sexual maturation were recorded in the selected F1-generation animals: males: balanopreputial separation from PN day 38 onwards; females: vaginal patency from PN day 30 onwards.

Postmortem examinations (parental animals):

- Gross necropsy and histology of parental animals: Males were sacrificed after successful mating and females were sacrificed at or shortly after weaning on PN day 21. All surviving parent male and female rats were euthanised by exsanguination from the abdominal aorta under CO2/O2 anaesthesia and then examined grossly for pathological changes. A necropsy was performed on animals that died intercurrently (if not precluded by autolysis) or that had to be killed because they were moribund. Samples of the following tissues and organs of all parent animals were preserved in a neutral aqueous phosphate-buffered 4% solution of formaldehyde except for the testes which were preserved in Bouin's fixative: adrenals, brain, epididymides *(left cauda which was used for sperm analysis), heart*, kidneys, liver, ovaries including oviduct*, pituitary gland*, prostate*, seminal vesicles and coagulating glands*, spleen, testes*(left testis was used for sperm analysis), thyroid, uterus* (after counting of the implantation sites), vagina*, organs and tissues showing macroscopic abnormalities. All organs mentioned above except the vagina were weighed (paired organs together) as soon as possible after dissection to avoid drying. Tissues marked with an asterisk (*) were embedded in paraffin wax, sectioned at 5µm, and stained with haematoxylin and eosin, except for sections of the testes, which were stained with PAS (Periodic Acid Schiff). Microscopic examination was performed on these organs of all rats of the control and high-dose groups. As no treatment-related abnormalities were observed, the histopathological examination was not extended to the low- and mid-dose groups. In addition, reproductive organs of males that failed to sire (did not mate or mated females were not pregnant) and females that were non-mated or non-pregnant, of the low- and mid-dose groups, were microscopically examined.

Postmortem examinations (offspring):

- Gross necropsy and histology op pups and weanings: All stillborn pups and pups found dead were stored in a freezer (<-18 °C) for macroscopical examination for structural and pathological changes. Gross necropsy was also performed on pups of dams that were sacrificed during lactation (these pups were sacrificed at the time of the dam’s death). Organs and tissues showing macroscopic abnormalities were preserved in a neutral aqueous phosphate buffered 4 % solution of formaldehyde. After selection of the pups for the next generation, from the remaining pups 1 male and 1 female pup of each litter (as far as present) were subjected to a thorough necropsy. Pups were euthanized by exsanguination from the abdominal aorta under CO2/O2 anaesthesia and then examined grossly for pathological changes. Special attention was paid to the organs of the reproductive system. The following organs were preserved in a neutral aqueous phosphate-buffered 4 % solution of formaldehyde: brain, spleen, thymus, organs and tissues showing macroscopic abnormalities. The brain, spleen, and thymus were weighed as soon as possible after dissection to avoid drying.

Statistics:

Tests were generally performed as two-sided tests with results taken as significant where the probability of the results is p<0.05 (*) or p<0.01 (**).
- Continuous data was subjected to a decision tree or parametric statistical test.
- Dichotomous data was evaluated using the statistical test Chi-square-Fisher.
- Incidences of microscopic observations in adult animals were evaluated by Fisher’s exact probability test.

Reproductive indices:

For each mating the following data was presented for each group:
- number of females mated (=number of females placed with males)
- number of males mated (= number of males placed with females)
- number of females inseminated (= number of successful copulations)
- number of females pregnant (demonstrated by the presence of implantation sites observed at necropsy)
- number of males with inseminated females
- number of males with pregnant females
- number of females with liveborn and (all) stillborn pups
- number of implantation sites
- number of corpora lutea
- number of pups delivered (live- and stillborn)
- number of lost pups
- mean number of litters with liveborn pups at day n

The following parameters were calculated:
- female mating index = number of females inseminated *100/number of females placed with males
- female fertility index = number of pregnant females*100/number of inseminated females
- male mating index = number of males with inseminated females*100/number of males placed with females
- male fertility index = number of males with pregnant females*100/number of males placed with females
- pre-coital time = mating days until day 0 post coitum (time between the start of mating and successful copulation)
- gestation index = number of females with liveborn pups*100/number of delivering pregnant females
- pre-implantation loss = number of corpora lutea- number of implantation sites*100/number of corpora lutea
- prenatal loss = number of implantation sites - number of pups delivered*100/number of implantation sites
- perinatal loss = number of stillborn pups*100/ number of pups delivered
- % liveborn pups (i.e. live birth index) = number of pups born alive*100/total number of pups delivered
- viability index day 4-21= number of pups surviving 21 days*100/number of liveborn after culling day 4
- sex ratio day n = number of live male pups on day n*100/ number of live pups on day n

Results and discussion

Results: P0 (first parental generation)

General toxicity (P0)

Clinical signs:

no effects observed

Description (incidence and severity):

During premating, several females started to develop sparsely haired areas and/or encrustations on the back from week 3 onwards (in all dose-groups). This was due to the ventilation holes in the exposure tubes. The incidence decreased after adapting the tubes by closing the holes. On 6 February 2012 and 7 February 2012, two females of the high-dose group were found dead (lactation days 16 and 17, respectively). At necropsy, no apparent cause of death could be found. Treatment-related clinical signs were not observed in this generation, including the animals found dead. All signs observed were within the range of expected for animals of this strain and age.

Dermal irritation (if dermal study):

not examined

Mortality:

mortality observed, treatment-related

Description (incidence):

Two females of the high-dose group were found dead

Body weight and weight changes:

no effects observed

Description (incidence and severity):

Premating period:
Males: No statistically significant differences were observed on mean body weight during the study. Body weight change in low-dose males was statistically significantly decreased from day 49 to 56 and increased from day 56 to 63 during the study. This was considered as incidental finding, based on the absence of an effect on mean body weights and a dose-relation.
Females: No significant differences were observed on body weight or body weight change during premating.
Gestation period:
No statistically significant differences in mean body weights and body weight changes were observed between the exposed groups and the control group.
Lactation period:
No statistically significant differences in mean body weights and body weight changes were observed between the exposed groups and the control group.

Food consumption and compound intake (if feeding study):

no effects observed

Description (incidence and severity):

Premating period:
Males and females of the F0-generation: No statistically significant differences on mean food consumption (expressed as g/animal/day and g/kg BW/day) were observed in males and females during the premating, except for an incidental increase in mean food consumption (g/kg BW/day) in males of the low-and mid-dose groups between days 42 and 49.
Gestation period:
No statistically significant effect on mean food consumption (expressed as g/animal/day and g/kg BW/day) was observed during the gestation period.
Lactation period:
No statistically significant effect on mean food consumption (expressed as g/animal/day) was observed during the lactation period.

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

Endocrine findings:

not examined

Urinalysis findings:

not examined

Behaviour (functional findings):

not examined

Immunological findings:

not examined

Organ weight findings including organ / body weight ratios:

no effects observed

Histopathological findings: non-neoplastic:

no effects observed

Histopathological findings: neoplastic:

effects observed, non-treatment-related

Description (incidence and severity):

Microscopic analysis revealed no treatment-related changes. In agreement with the macroscopic findings, the lungs of animal 177 were hyperaemic. No obvious cause of death could be established. In agreement with the macroscopic findings, the lungs of animal 189 were hyperaemic. No abnormalities could be detected in the stomach. The caecum was necrotic. The thymus showed microhaemorrhages and the adrenals were hyperaemic. No obvious cause of death could be established.

Other effects:

not examined

Reproductive function / performance (P0)

Reproductive function: oestrous cycle:

effects observed, non-treatment-related

Description (incidence and severity):

A statistically significantly decreased mean cycle length was observed in females of the high-dose group. This was not considered as treatment-related, because a cycle length of 4-5 days is normal for this strain. In the control group more females with a cycle length of 6 or more days were observed compared to the high-dose group.

Reproductive function: sperm measures:

no effects observed

Description (incidence and severity):

Epididymal sperm motility:
No statistically significant differences were observed in sperm motility between the exposed groups and the control group.
Epididymal sperm count:
Epididymal sperm count in the exposed groups and the control group was comparable in this genaration.
Sperm morphology:
No statistically significant differences were observed in sperm morphology between the high-dose group and the control group in this generation.
Homogenisation resistant sperm:
Homogenisation resistant sperm count and daily sperm production in the testis werecomparable between the high-dose group and the control group

Reproductive performance:

no effects observed

Description (incidence and severity):

Fertility:
Each group comprised 28 males and females that were mated. Twenty seven, 26, 24 and 26 females of the control, low-, mid-, and high-dose group, respectively were found inseminated, of which 25, 21, 21, and 19, respectively were pregnant. The mean number of mating days until day 0 post coitum was comparable between all groups. No treatment-related differences were observed in the female and male mating indices. Both female and male fertility indices tended to be decreased in the high-dose group.
Delivery and litter data:
Delivery Report: No treatment-related effects were observed on the duration of the gestation period and gestation index. All pregnant females delivered a litter. One, 1, 3 and 3 females of the control, low-, mid- and high-dose group delivered a litter with stillborn pups, of which one female of the mid-dose group and one female of the high-dose group delivered one stillborn pup only.
Litter Report: No treatment-related effects of the test substance were observed on the mean number of corpora lutea, implantation sites, preimplantation loss, mean number of pups delivered, prenatal and perinatal loss in this generation. Five females were killed interim, because they had complete litter loss during the lactation period: Females 129 of the mid-dose group and female 203 of the highdose group both delivered 1 stillborn pup. Females 125, 153 and 159 of the middose group lost their complete litter due to cannibalism at PN 4, 7 and 4, respectively. None of these dams nor pups showed clinical signs or abnormal body weight.

Details on results (P0)

Cannibalism was mainly observed in this generation. No relationship could be observed between cannibalism and decreased food intake of the dams or cage position in the animal room. The incidence of cannibalism as observed in the middose group of this generation was within the range of historical control data of this strain and therefore not considered to be an adverse effect. The number of pups delivered and the number of stillborn pups were not considered to be adversely affected by test substance exposure.

Effect levels (P0)

open allclose all

Results: P1 (second parental generation)

General toxicity (P1)

Clinical signs:

effects observed, non-treatment-related

Description (incidence and severity):

On 5 June 2012, one female of the high-dose group was found dead (lactation day 19). At necropsy, no apparent cause of death could be found. No treatment-related clinical signs were observed in this generation during the study. All signs observed were within the range of expected for animals of this strain and age. Because several animals had not achieved sexual maturation minimally at PN 56 (females) or PN80 (males), vaginal patency and balanopreputial separation were registered as clinical signs from this period onwards.

Dermal irritation (if dermal study):

not examined

Mortality:

mortality observed, non-treatment-related

Body weight and weight changes:

no effects observed

Description (incidence and severity):

Premating period:
Males: No statistically significant differences were observed on mean body weight during the study. From days 49 to 56 body weight change was statistically significantly decreased in high-dose males. A statistically significantly increased body weight change was observed in low-, mid-, and high dose males from day 56 to 63. These findings were not dose-related and are therefore considered to be of no toxicologically significance.
Females: No significant differences were observed on body weight or body weight change during premating, except for an incidental statistically significant increase in body weight change in high-dose females from day 63 to 70 of the study.
Gestation period:
No statistically significant difference in mean body weight was observed between the exposed groups and the control group. An incidental statistically significant increase in body weight change was observed in mid-dose females from day 7 to 14 only.
Lactation period:
No statistically significant differences in mean body weights and body weight changes were observed between the exposed groups and the control group.

Food consumption and compound intake (if feeding study):

effects observed, non-treatment-related

Description (incidence and severity):

Premating period: Males and females: No statistically significant differences on mean food consumption (expressed as g/animal/day and g/kg/day) were observed in males and females during the premating. Food consumption (expressed as g/kg BW/day) was statistically significantly increased in high-dose males from day 7 to 14 and in low-, mid, and high-dose males from day 56 to 63 of the study. These findings were considered to be incidental, because no relation with the concentration of the test substance was observed.
Gestation period:
Food consumption (expressed as g/animal per day) was statistically significantly increased in mid-dose females from day 7 to 14 during gestation, which was considered to be incidental. No effect on mean food consumption (expressed as g/kg BW/day) was observed during the gestation period.
Lactation period:
No statistically significant effect on mean food consumption (expressed as g/animal/day) was observed during the lactation period

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

Endocrine findings:

not examined

Urinalysis findings:

not examined

Behaviour (functional findings):

not examined

Immunological findings:

not examined

Organ weight findings including organ / body weight ratios:

effects observed, non-treatment-related

Description (incidence and severity):

The following statistically significant differences were observed in organ weights: Relative weight of the adrenals was decreased in males of the mid-dose-group. Due to the absence of this finding in the high-dose group, this was considered to be not related to treatment. Both absolute and relative weight of the epididymis were decreased in low-dose males. This was an incidental finding, because no dose-response was observed. Relative liver weight was increased in females of the high-dose group (about 7 % compared to the control group). Absolute and relative thyroid weights were decreased in females of the high dosegroup (about 8 % compared to the control group)

Gross pathological findings:

effects observed, non-treatment-related

Description (incidence and severity):

Intercurrent deaths:
One female animal of the high-dose group (no. 677) was found dead on 5 June 2012 (lactation day 19). At necropsy, the stomach was swollen and its mucosa was brown. The jejunum was red. The caecum was swollen and the ovaries were red. The lungs showed red patches and were not collapsed properly. The uterus had a dark appearance.
Scheduled necropsies:
Macroscopic analysis revealed no treatment-related changes.

Neuropathological findings:

not examined

Histopathological findings: non-neoplastic:

effects observed, non-treatment-related

Description (incidence and severity):

Microscopic analysis revealed no treatment-related changes. In agreement with the macroscopic findings, the lungs of animal 677 were hyperaemic. No abnormalities could be detected in the stomach or the jejunum. The caecum was necrotic. The ovaria were hyperaemic. Microscopic examination of the uterus revealed no explanation for the dark appearance. No obvious cause of death could be established.

Histopathological findings: neoplastic:

not examined

Other effects:

not examined

Reproductive function / performance (P1)

Reproductive function: oestrous cycle:

no effects observed

Description (incidence and severity):

No differences were observed in estrus cyclicity parameters.

Reproductive function: sperm measures:

no effects observed

Description (incidence and severity):

Epididymal sperm motility:
A statistically significantly decreased linearity (ratio VSL/VCL) was observed in the mid- and high-dose groups. Because none of the other sperm motility parameters were affected and the number of pregnant females and pups per litter were comparable between the groups, this finding was considered not to be treatment-related. Furthermore, histopathological examination of the epididymides and testes did not show treatment-related abnormalities.
Epididymal sperm count:
Epididymal sperm count in the exposed groups and the control group was comparable.
Sperm morphology:
No statistically significant differences were observed in sperm morphology between the high-dose group and the control group in both F0- and F1-generations.
Homogenisation resistant sperm:
Homogenisation resistant sperm count and daily sperm production in the testis were comparable between the high-dose group and the control group.

Reproductive performance:

no effects observed

Description (incidence and severity):

Each group comprised 28 males and females that were mated. Twenty five, 28, 27 and 27 females of the control, low-, mid-, and high-dose group, respectively were found inseminated, of which 22, 23, 25, and 26, respectively were pregnant. No statistically significant differences were found in the mean number of mating days until day 0 post coitum, however, 5 of the animals of the control group were inseminated relatively late (between mating days 5 and 8). No treatment-related differences were observed in the female and male mating and fertility indices.
- Delivery Report: The mean number of gestation days and gestation index were comparable between the exposed and control group. All pregnant females delivered a litter. One, 3,1 and 1 females of the control, low-, mid- and high-dose group delivered a litter with both live and stillborn pups.
Litter Report: No treatment-related effects of the test substance were observed on the mean number of corpora lutea, implantation sites, preimplantation loss, mean number of pups delivered, prenatal and perinatal loss of the F2 pups. One dam of the high-dose group (no. 715) was killed interim 24 May 2012, because she had complete litter loss during the lactation period (one pup delivered which was missing at day 1 of lactation). Pup 217-07 had been selected as female 715. This pup had a low pup weight when selected and body weight was low during premating and gestation. This dam had a low body weight at the start of lactation (144.7 gram; 32% decrease versus mean control body weights on day 0 of lactation) and her single pup was missing on day 1 of lactation. No histopathological abnormalities were observed in this female.

Effect levels (P1)

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Results: F1 generation

General toxicity (F1)

Clinical signs:

no effects observed

Description (incidence and severity):

The number of runts was comparable between the exposed groups and the control group. Treatment-related pup clinical signs were not observed. All signs observed were within the range of the expected for this strain and age. The right eye of pup 123-05 had encrustations at PN14 and was missing at PN21. Because this pup was selected for the F1-generation as female 655 this clinical sign persisted. A high incidence of early pup mortality (PN0-4) in the mid-dose group was observed. This was due to a high incidence of cannibalism and not considered an adverse effect. The pups of dams 177 and 189 were killed interim, because the dams were found dead. The mean number of live pups was comparable in the exposed groups compared to the control group at PN4, 7, 14 and 20. Viability index from PN4-21 and sex ratio were comparable between the groups.

Dermal irritation (if dermal study):

not examined

Mortality / viability:

no mortality observed

Body weight and weight changes:

no effects observed

Description (incidence and severity):

No statistically significant differences in mean pup weights and pup weight changes were observed between the pups of the exposed groups and the control group.

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

Sexual maturation:

no effects observed

Anogenital distance (AGD):

not examined

Nipple retention in male pups:

not examined

Organ weight findings including organ / body weight ratios:

no effects observed

Description (incidence and severity):

No statistically significant differences in absolute and relative mean pup organ weights and pup weight changes were observed between the pups of the exposed groups and the control group.

Gross pathological findings:

no effects observed

Description (incidence and severity):

No abnormalities were observed

Histopathological findings:

no effects observed

Description (incidence and severity):

No abnormalities were observed

Other effects:

not examined

Developmental neurotoxicity (F1)

Behaviour (functional findings):

not examined

Developmental immunotoxicity (F1)

Developmental immunotoxicity:

not examined

Effect levels (F1)

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Results: F2 generation

General toxicity (F2)

Clinical signs:

effects observed, non-treatment-related

Description (incidence and severity):

A statistically significant number of runts was observed in female pups of the mid-dose group on PN4 and PN7. This finding was not dose-related and therefore not considered as adverse effect. Treatment-related pup clinical signs were not observed. All signs observed were within the range of the expected for this strain and age. There was no treatment related-effect on the number of dead pups between PN0-4. The mean number of live pups was comparable in the exposed groups compared to the control group at PN4, 7, 14 and 20. Viability index from PN4-21 and sex ratio were comparable between the groups.

Dermal irritation (if dermal study):

not examined

Mortality / viability:

no mortality observed

Body weight and weight changes:

effects observed, non-treatment-related

Description (incidence and severity):

Statistically significantly increased mean pup body weights were observed only in females of the high-dose group at lactation days 0, 4, and 7. Mean pup body weight was statistically significantly increased when combining male and females pup weights in the high-dose group at day 4 and 7. No statistically significant differences in pup weight changes were observed between the pups of the exposed groups and the control group.

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

Sexual maturation:

no effects observed

Description (incidence and severity):

In the male and female animals, no statistically significant difference was observed between the day of achievement of balanopreputial separation or vaginal patency between the exposed groups and the control group.

Anogenital distance (AGD):

not examined

Nipple retention in male pups:

not examined

Organ weight findings including organ / body weight ratios:

no effects observed

Description (incidence and severity):

No statistically significant differences in absolute and relative mean pup organ weights and pup weight changes were observed between the pups of the exposed groups and the control group.

Gross pathological findings:

no effects observed

Description (incidence and severity):

No abnormalities were observed

Histopathological findings:

no effects observed

Description (incidence and severity):

No abnormalities were observed

Developmental neurotoxicity (F2)

Behaviour (functional findings):

not examined

Developmental immunotoxicity (F2)

Developmental immunotoxicity:

not examined

Effect levels (F2)

Overall reproductive toxicity

Applicant's summary and conclusion

Conclusions:

Exposure of rats to 2000, 5000 or 15000 ppm of the test substance for 6 h/day, 5 days a week during pre-mating and daily during mating, gestation up to GD19 and lactation (from PN5 onward) resulted in mortality of two F0-females and one F1-female of the high-dose group at the end of the lactation period. Based on these results, the No Observed Effect Level (NOEL) for parental toxicity for exposure to the test substance by inhalation, under the conditions of this two-generation reproduction toxicity study in rats, is considered to be 5000 ppm (26550 mg/m3). The NOEL for fertility and development for exposure to the test substance by inhalation, under the conditions of this two-generation reproduction toxicity study in rats, is considered to be 15000 ppm (79650 mg/m3), because no adverse effects on fertility parameters or offspring were observed.

Executive summary:

In this two-generation study, performed in accordance with OECD Guideline 416 and GLP, 28 Wistar rats/sex/group were exposed by inhalation to 0 (air), 2000, 5000 or 15000 ppm of the test substance. Male animals were exposed to the test substance in air (nose-only) for at least 10 weeks prior to mating during 6 hours/day and 5 days/week, and daily during mating for 6 hours/day. Males were exposed until sacrifice after at least 11 weeks (for sperm analyses and necropsy). The females were exposed to the test substance in air (nose-only) for at least 10 weeks prior to mating for 6 hours/day and 5 days/week, and daily during mating and up to gestation day (GD) 19 for 6 hours/day. From day 5 of lactation onwards, females were exposed daily by whole body exposure for 6 hours/day to the test substance until the end of the lactation period (PN21) or the sacrifice of the females shortly thereafter. From PN day 22 up to ca. 6 weeks of age, the F1-generation male and female pups were exposed by whole body exposure during 6 hours/day and 5 days/week. Subsequently, F1-generation male animals were exposed by nose-only exposure until the end of the premating period during 6 hours/day and 5 days/week, and daily for 6 hours/day during mating and up to sacrifice after at least 11 weeks (for sperm analyses and necropsy). F1-generation female animals were exposed by nose-only exposure until the end of the premating period during 6 hours/day and 5 days/week, and daily during mating and up to GD19 for 6 hours/day. From PN5 onwards, F1-generation females were exposed daily 6 hours/day to the test substance by whole body exposure until sacrifice on or shortly after PN21. Clinical signs did not reveal treatment-related changes. Two females of the high-dose group in the F0-generation and one female of the high-dose group in the F1 -generation were found dead on lactation days 16, 17 and 19. Histopathological observation of these animals revealed no obvious cause of death. Due to the incidence of mortality in the high-dose group only, this was considered to be related to exposure to the test substance. No treatment-related effects were observed on body weights, body weight changes and food consumption. No adverse effects of the test substance were observed on oestrus cycle parameters of the F0- and F1-female animals and on sperm parameters of the male F0- and F1 -animals. The number of pregnant F0-females was 25, 21, 21, and 19 in the control, low-,mid- and high-dose group, respectively. The number of pregnant F1-females was 22, 23, 25 and 26 in the control, low-, mid- and high-dose group, respectively. Precoital time, gestation index and duration of gestation, male and female fertility indices, incidences of dams with live- and stillborn pups were not affected by exposure to the test substance by inhalation in either generation. In both generations, the mean number of pups delivered, the incidences of liveborn and stillborn pups, the number of live and dead pups at delivery, the number of pups lost during the lactation period, the sex ratio, pup clinical observations, pup organ weight and macroscopic observations were considered not to be affected by exposure to the test substance. The increased pup body weights observed in F1-female pups on PN day 0, 4 and 7 were considered not to be an adverse effect of the test substance, based on the absence of a clear dose-reponse and reduction of the effect on PN14 and 21. No statistically significant differences were observed among the various groups in timing of balanopreputial separation or vaginal patency. Organ weights of parental animals of both generations were considered not to be affected by exposure to the test substance. The slight significant differences observed in liver, kidney and thyroid weight were not consistently observed in both generations, not dose-related and not accompanied by corroborative histopathological effects. Therefore no toxicological significance is attached to these slight organ weight changes. At necropsy of the parental animals no test substance related gross changes were observed in the F0- and F1-generation animals. Microscopic examination did not reveal any test substance related findings in the male and female animals of the F0- and F1-generations. In conclusion, exposure of rats to 2000, 5000 or 15000 ppm to the test substance for 6 h/day, 5 days a week during premating and daily during mating, gestation up to GD19 and lactation (from PN5 onwards) resulted in mortality of two F0-females and one F1-female of the high-dose group at the end of the lactation period. Based on these results, the No Observed Effect Level (NOEL) for parental toxicity for exposure to the test substance by inhalation, under the conditions of this two-generation reproduction toxicity study in rats, is considered to be 5000 ppm (26550 mg/m3). The NOEL for fertility and development for exposure to the test substance by inhalation, under the conditions of this two-generation reproduction toxicity study in rats, is considered to be 15000 ppm (79650 mg/m3), because no adverse effects on fertility parameters or offspring were observed.