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EC number: 500-011-5 | CAS number: 9003-80-9
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Endpoint summary
Administrative data
Description of key information
28-day repeated dose toxicity study in rats by oral gavage.
NOAEL: 50 mg/kg (based on adverse microscopic alterations in the liver and associated changes in clinical pathology parameters in both sexes, and reduced body weight gain and food consumption in females at the higher dose levels).
Key value for chemical safety assessment
Repeated dose toxicity: via oral route - systemic effects
Link to relevant study records
- Endpoint:
- short-term repeated dose toxicity: oral
- Type of information:
- experimental study
- Adequacy of study:
- key study
- Study period:
- 20 September 2016 to 29 December 2016
- Reliability:
- 1 (reliable without restriction)
- Rationale for reliability incl. deficiencies:
- guideline study
- Reason / purpose for cross-reference:
- reference to same study
- Qualifier:
- according to guideline
- Guideline:
- OECD Guideline 422 (Combined Repeated Dose Toxicity Study with the Reproduction / Developmental Toxicity Screening Test)
- Version / remarks:
- Organisation of Economic Co-operation and Development (OECD) Guidelines for Testing of Chemicals, Guideline 422, Combined Repeated Dose Toxicity Study with the Reproduction/Developmental Toxicity Screening Test, July 2016.
- Deviations:
- yes
- Remarks:
- see "Any other information" for details
- Qualifier:
- according to guideline
- Guideline:
- other: United States Environmental Protection Agency (EPA) Health Effects Test Guidelines, OPPTS 870.3650
- Version / remarks:
- The United States Environmental Protection Agency (EPA) Health Effects Test Guidelines, OPPTS 870.3650, Combined Repeated Dose Toxicity Study with the Reproduction/Developmental Toxicity Screening Test, July 2000.
- Deviations:
- yes
- Remarks:
- see "Any other information" for details
- GLP compliance:
- yes (incl. QA statement)
- Limit test:
- yes
- Specific details on test material used for the study:
- Purity/composition correction factor: No correction factor required
Test item handling: No specific handling conditions required
Stability at higher temperatures: Not indicated
Stability in vehicle: Polyethylene glycol 400; Stability for at least 6 hours at room temperature is confirmed over the concentration range 1 to 150 mg/mL, Project 512475. - Species:
- rat
- Strain:
- Wistar
- Details on species / strain selection:
- Test system Rat: Crl:WI(Han) (outbred, SPF-Quality). Nulliparous and non-pregnant females and untreated animals were used at initiation of the study.
Rationale: This species and strain of rat has been recognized as appropriate for general and reproduction toxicity studies. This animal model has been proven to be susceptible to the effects of reproductive toxicants. - Sex:
- male/female
- Details on test animals or test system and environmental conditions:
- Test system Rat: Crl:WI(Han) (outbred, SPF-Quality). Nulliparous and non-pregnant females and untreated animals were used at initiation of the study.
Source: Charles River Deutschland, Sulzfeld, Germany.
Age at start pre-test: Females: approximately 10-12 weeks.
Age at start treatment: Males: approximately 10-12 weeks; Females: approximately 12-14 weeks.
Number of animals: 48 females and 40 males.
At the end of the pre-test phase, 40 females with at least two regular estrous cycles were selected at random and further used in the study. The remaining females were removed from the study.
Acclimatization: At least 5 days prior to start of pre-test (females) or treatment (males).
Health inspection: At least upon receipt of the animals.
Randomization: Before initiation of pre-test, by computer-generated random algorithm according to body weight, with all animals within ± 20% of the sex mean.
Identification: During pre-test (females) and treatment (males and females): by earmark and tattoo.
Animal Husbandry
Conditions: Environmental controls for the animal room were set to maintain 18 to 24 °C, a relative humidity of 40 to 70%, at least 10 room air changes/hour, and a 12-hour light/12-hour dark cycle: the photoperiod was between 07:00 and 19:00 hrs daily.
The light/dark cycle was interrupted for study related activities. Any variations to these conditions were maintained in the raw data and had no effect on the outcome of the study.
Accommodation
Pre-test: Females were housed in groups of 5 females/cage in Macrolon plastic cages (MIV type, height 18 cm).
Pre-mating: Animals were housed in groups of 5 animals/sex/cage in Macrolon plastic cages (MIV type, height 18 cm).
Mating: Females were caged together with males on a one-to-one-basis in Macrolon plastic cages (MIII type, height 18 cm).
Post-mating: Males were housed in their home cage (Macrolon plastic cages, MIV type, height 18 cm) with a maximum of 5 animals/cage. Females were individually housed in Macrolon plastic cages (MIII type, height 18 cm).
General: Sterilized sawdust as bedding material (Lignocel S 8-15, JRS - J.Rettenmaier & Söhne GmbH + CO. KG, Rosenberg, Germany) and paper as cage-enrichment/nesting material (Enviro-dri, Wm. Lillico & Son (Wonham Mill Ltd), Surrey, United Kingdom) were supplied. During locomotor activity monitoring, animals were housed individually in a Hi-temp polycarbonate cage (Ancare corp., USA; dimensions: 48.3 x 26.7 x 20.3 cm) without cage-enrichment, bedding material, food and water.
Diet: Free access to pelleted rodent diet (SM R/M-Z from SSNIFF® Spezialdiäten GmbH, Soest, Germany). During motor activity measurements, animals did not have access to food for a maximum of 1.5 hours.
Water: Free access to tap-water. During motor activity measurements, animals did not have access to water for a maximum of 1.5 hours.
Diet, water, bedding and cage-enrichment/nesting material evaluation for contaminants and/or nutrients was performed according to facility standard procedures. There were no findings that could interfere with the study. - Route of administration:
- oral: gavage
- Details on route of administration:
- Oral gavage, using a plastic feeding tube. Formulations were placed on a magnetic stirrer during dosing.
- Vehicle:
- polyethylene glycol
- Details on oral exposure:
- Vehicle: Polyethylene glycol 400, specific gravity 1.125 (Merck, Darmstadt, Germany).
Rationale for vehicle: Based on trial formulations performed at Charles River Den Bosch.
Method of formulation: Formulations (w/w) were prepared daily within 6 hours prior to dosing and were homogenized to a visually acceptable level. Adjustment was made for specific gravity of the vehicle. No correction was made for the purity/composition of the test item.
Appearance of formulations: Solution (Groups 2-4).
Storage conditions: At room temperature. - Analytical verification of doses or concentrations:
- yes
- Details on analytical verification of doses or concentrations:
- Analyses were conducted on a single occasion during the treatment phase (04 November 2016) according to a validated method.
Samples of formulations were analyzed for homogeneity (highest and lowest concentration) and accuracy of preparation (all concentrations).
The accuracy of preparation was considered acceptable if the mean measured concentrations were 90-110% of the target concentration. Homogeneity was demonstrated if the coefficient of variation was ≤ 10%.
Stability of formulations over 6 hours at room temperature under normal laboratory light conditions (concentration range 1-150 mg/mL) was determined as part of the analytical method development and validation study. - Duration of treatment / exposure:
- Males were dosed for 29 days, i.e. 2 weeks prior to mating, during mating, and up to the day prior to scheduled necropsy.
Females that delivered were exposed for 50-56 days (most females) or 64 days (one female, no. 67), i.e. during 2 weeks prior to mating (with the objective of covering at least two complete estrous cycles), the variable time to conception, the duration of the pregnancy and at least 13 days after delivery up to and including the day before scheduled necropsy. Females which failed to deliver healthy offspring were exposed for 41 days. - Frequency of treatment:
- Once daily for 7 days per week, approximately the same time each day with a maximum of 6 hours difference between the earliest and latest dose.
- Dose / conc.:
- 5 other: mL/kg body weight.
- Remarks:
- Actual dose volumes were calculated according to the latest body weight.
- Dose / conc.:
- 50 mg/kg bw/day (nominal)
- Dose / conc.:
- 150 mg/kg bw/day (nominal)
- Dose / conc.:
- 500 mg/kg bw/day (nominal)
- No. of animals per sex per dose:
- 48 females and 40 males. (10 males/females per dose group)
- Control animals:
- yes, concurrent vehicle
- Details on study design:
- Based on the results of a dose range finding study in which dose limiting effects were noted at 1000 mg/kg, the dose levels for this combined 28-day oral gavage study with reproduction/developmental toxicity screening test were selected to be 50, 150 and 500 mg/kg.
- Positive control:
- Postive control not used in this study.
- Observations and examinations performed and frequency:
- Mortality / Viability: At least twice daily.
Clinical signs: Clinical observations (detailed clinical signs and arena) were conducted from start of treatment onwards up to the day prior to necropsy at least at 1 hour (± 30 min)) after dosing based on the peak period of anticipated effects. Once prior to start of treatment and at weekly intervals during the treatment period this was also performed outside the home cage in a standard arena.
The time of onset, grade and duration of any observed sign was recorded. Signs were graded for severity and the maximum grade was predefined at 3 or 4. Grades were coded as slight (grade 1), moderate (grade 2), severe (grade 3) and very severe (grade 4). For certain signs, only its presence (grade 1) or absence (grade 0) was scored. In the data tables, the scored grades were reported, as well as the percentage of animals affected in summary tables.
Functional Observations: The following functional observations tests were performed on each individual animal of the selected 5 animals/sex/group:
-hearing ability (HEARING), pupillary reflex (PUPIL L/R), and static righting reflex (STATIC R) (Score 0 = normal/present, score 1 = abnormal/absent).
-fore- and hind-limb grip strength, recorded as the mean of three measurements per animal (Series M4-10, Mark-10 Corporation, J.J. Bos, Gouda, The Netherlands).
-locomotor activity (recording period: 1-hour under normal laboratory light conditions, using a computerized monitoring system, Kinder Scientific LLC, Poway, USA). Total movements and ambulations are reported. Ambulations represent movements characterized by a relocation of the entire body position like walking, whereas total movements represent all movements made by the animals, including ambulations but also smaller or finer movements like grooming, weaving or movements of the head.
The selected males were tested during Week 4 of treatment and the selected females were tested once during the last week of lactation (e.g. PND 6-13). These tests were performed after observation for clinical signs (incl. arena observation, if applicable) and started at 1 hour (± 30 min) after dosing.
Body weights: Males and females were weighed on the first day of exposure (prior to first exposure) and weekly thereafter. Mated females were weighed on Days 0, 4, 7, 11, 14, 17 and 20 post-coitum.
Food consumption: Weekly, except for males and females which were housed together for mating and for females without evidence of mating. Food consumption of mated females was measured on
Days 0, 4, 7, 11, 14, 17 and 20 post-coitum.
Water consumption: Subjective appraisal was maintained during the study, but no quantitative investigation was introduced as no treatment related effect was suspected.
Clinical Laboratory Investigations: Blood samples were collected at the end of the treatment period on the day of scheduled necropsy from the selected 5 animals/sex/group under anaesthesia using isoflurane (Abbott B.V., Hoofddorp, The Netherlands) between 7.00 and 10.30 a.m.
The animals were deprived of food overnight (with a maximum of 24 hours) before blood sampling, but water was available. Blood samples were drawn from the retro-orbital sinus and collected into tubes (Greiner Bio-One GmbH, Kremsmünster, Austria) prepared with K3-EDTA for haematological parameters (0.5 mL), with citrate for clotting tests (0.45 mL) and tubes treated with Li-heparin for clinical biochemistry parameters (0.5 mL). An additional blood sample (0.25 mL) was collected into serum tubes for determination of bile acids.
Haematology
The haematology parameters were determined in blood prepared with K3-EDTA as an anti-coagulant, using the ADVIA® 2120i Hematology System (Siemens Healthcare Diagnostics B.V., Den Haag, The Netherlands): Reported tabulated – see “Any other information” for parameters.
The clotting parameters were determined in plasma prepared with citrate as anticoagulant, using the STA Compact® (Diagnostica Stago S.A.S., Asnières, France): Reported tabulated – see “Any other information” for parameters.
Clinical Biochemistry
The clinical biochemistry parameters were determined using the AU400 (Beckman Coulter Nederland B.V., Woerden, The Netherlands). All parameters were determined in plasma, except for bile acids which were determined in serum: Reported tabulated – see “Any other information” for parameters. - Sacrifice and pathology:
- Termination
The animals were deprived of food overnight (with a maximum of 24 hours) before blood sampling, but water was available.
All animals surviving to the end of the observation period were deeply anaesthetized using isoflurane (Abbott B.V., Hoofddorp, The Netherlands) and subsequently exsanguinated.
Necropsy was conducted on the following days:
Males: Following completion of the mating period (a minimum of 28 days of dose administration).
Females which delivered: PND 14-16.
Females which failed to deliver: Post-coitum Day 26 (females with evidence of mating)
Macroscopic Examination
After sacrifice, all animals were subjected to a full post mortem necropsy, with special attention being paid to the reproductive organs. Descriptions of all macroscopic abnormalities were recorded.
The number of former implantation sites were recorded for all paired females.
Samples of the following tissues and organs were collected and fixed in 10% buffered formalin (neutral phosphate buffered 4% formaldehyde solution, Klinipath, Duiven, The Netherlands).
Selected 5 animals/sex/group:
Identification marks: not processed; Adrenal glands; (Aorta); Brain – cerebellum, mid-brain, cortex (7-levels); Caecum; Cervix; Clitoral gland; (Cowper’s gland); Duodenum; Epididymides; Eyes (with optic nerve (if detectable) and Harderian gland); Mammanry gland area (males and females); Femur including joint; (Glans penis); (Levator ani plus bulbocavernosus muscle complex (LABC)); Heart; Ileum; Jejunum; Kidneys; (Lacrimal gland, exorbital); (Larynx); Liver; Lung, infused with formalin; Lymph nodes – mandibular, mesenteric; (Nasopharynx); (Esophagus); Ovaries; (Pancreas); Payer’s patches [jejunum, ileum] if detectable; Pituitary gland; Preputial gland; Prostate gland; Rectum; (Salivary glands – mandibular, sublingual); Sciatic nerve; Seminal vesicles; Skeletal muscle; (Skin); Spinal cord –cervical, midthoratic, lumbar; Spleen; Sternum with bone marrow; Stomach; Testes; Thymus; Thyroid including parathyroid if detectable; (Tongue); Trachea; Urinary bladder; Uterus; Vagina; All gross lesions.
Tissues/organs mentioned in parentheses were not examined by the pathologist, since no signs of toxicity were noted at macroscopic examination.
All remaining animals:
Cervix; Clitoral gland; Coagulation gland; Cowper’s glands; Epididymides; Glans penis; Levator ani plus bulbocavernosus muscle complex (LABC); Mammary gland area (males and females); Ovaries; Preputial gland; Prostate gland; Seminal vesicles; Testes; Thyroid including parathyroid if detectable; Uterus; Vagina; All gross lesions; Identification marks: not processed.
Organ Weights
Terminal body weights were recorded from all rats at scheduled necropsy.
The following organ weights were recorded from the following animals on the scheduled day of necropsy:
Selected 5 animals/sex/group:
Adrenal glands; Brain; Cowper’s glands; Epididymides; Glans penis; Heart; Kidneysl Levator ani plus bulbocavernosus muscle complex (LABC); Liver; Ovaries; Prostate; Seminal vesicles including coagulating glands; Spleen; Testes; Thymus; Thyroid; Uterus (including cervix)
All remaining animals:
Cowper’s glands; Epididymides; Glans penis; Levator ani plus bulbocavernosus muscle complex (LABC); Prostate; Seminal vesicles including coagulating glands; Testes; Thyroid (including parathyroid if detectable)
Absolute organ weights and organ to body weight ratios are reported.
Histotechnology
All organ and tissue samples, as defined under Histopathology (following section), were processed, embedded and cut at a thickness of 2-4 micrometers. These slides were stained with haematoxylin and eosin (Klinipath, Duiven, The Netherlands). The additional slides of the testes (to examine staging of spermatogenesis) were stained with PAS/haematoxylin (Klinipath, Duiven, The Netherlands).
Histopathology
The following slides were examined by a pathologist:
-The preserved organs and tissues of the selected 5 animals/sex of Groups 1 and 4.
-Additional slides of the testes of the selected 5 males of Groups 1 and 4, including the two males that failed to sire (nos. 01 and 31), to examine staging of spermatogenesis.
-All gross lesions of all animals (all dose groups).
-Spleen and liver of the selected 5 males and females of Groups 2 and 3 and thyroid gland of the selected 5 females of Groups 2 and 3, based on (possible) treatment-related changes in these organs in Group 4.
-The reproductive organs of all males that failed to sire and all females that failed to deliver healthy pups.
All abnormalities were described and included in the report. An attempt was made to correlate gross observations with microscopic findings. - Other examinations:
- Blood Sampling for Thyroid Hormone Analysis: End of study from all animals at planned necropsy; this included females on Day 14-16 of lactation, all females that failed to deliver healthy pups and all males after at least 4 weeks of treatment (including all males that failed to sire).
Blood samples were collected under anaesthesia using isoflurane between 7.00 and 10.30 a.m. The animals were deprived of food overnight (with a maximum of 24 hours) before blood sampling, but water was available. Blood samples (0.9 mL) were drawn from the retroorbital sinus and collected into serum tubes (Greiner Bio-One GmbH, Kremsmünster, Austria).
After clotting and centrifugation, serum was used as listed below.
Males: 1 aliquot of 150 μL serum was used for measurement of thyroxine (T4), and the remaining volume of serum was stored for possible future measurement of thyroidstimulating hormone (TSH).
Females: The serum was stored for possible future measurement of thyroxine (T4) and/or thyroid-stimulating hormone (TSH).
Serum samples were stored at ≤-75 °C. Under these storage conditions, the samples are stable for 6 months. Any samples remaining after 6 months will be discarded.
In general:
Total T4 was measured in serum using the Immulite 1000® (Siemens Healthcare Diagnostics B.V., Den Haag, The Netherlands): Reported tabulated – see “Any other information” for parameters. - Statistics:
- The following statistical methods were used to analyse the data:
-If the variables could be assumed to follow a normal distribution, the Dunnett-test (many-to-one t-test) based on a pooled variance estimate was applied for the comparison of the treated groups and the control groups for each sex.
-The Steel-test (many-to-one rank test) was applied if the data could not be assumed to follow a normal distribution.
-The Fisher Exact-test was applied to frequency data.
-The Kruskal-Wallis nonparametric ANOVA test was applied to motor activity data to determine intergroup differences.
All tests were two-sided and in all cases p < 0.05 was accepted as the lowest level of significance. Group means were calculated for continuous data and medians were calculated for discrete data (scores) in the summary tables. Test statistics were calculated on the basis of exact values for means and pooled variances. Individual values, means and standard deviations may have been rounded off before printing. Therefore, two groups may display the same printed means for a given parameter, yet display different test statistics values. - Clinical signs:
- effects observed, non-treatment-related
- Description (incidence and severity):
- The clinical signs noted incidentally occurred within the range of background findings to be expected for rats of this age and strain which are housed and treated under the conditions in this study and showed no dose-related trend. At the incidence observed, these were considered to be unrelated to treatment.
- Mortality:
- no mortality observed
- Body weight and weight changes:
- no effects observed
- Food consumption and compound intake (if feeding study):
- no effects observed
- Food efficiency:
- not examined
- Water consumption and compound intake (if drinking water study):
- not examined
- Ophthalmological findings:
- not examined
- Haematological findings:
- effects observed, treatment-related
- Description (incidence and severity):
- The following statistically significant differences between treated animals and controls were noted in haematology parameters:
Higher prothrombin time at 500 mg/kg in males.
Higher total white blood cell count (WBC) at 500 mg/kg in males. This finding was likely to be unrelated to treatment as values at 500 mg/kg were well in the normal range, whereas the concurrent control group mean was at the lower end of this range.
Lower mean corpuscular volume (MCV) and mean corpuscular haemoglobin (MCH) at 500 mg/kg in males, and lower mean corpuscular haemoglobin concentration (MCHC) at 500 mg/kg in females. These slight differences (values in treated rats remained within normal limits) were considered not to be toxicologically relevant as they occurred in the absence of treatment-related changes in haemoglobin, haematocrit or number of red blood cells. - Clinical biochemistry findings:
- effects observed, treatment-related
- Description (incidence and severity):
- The following (statistically significant) changes in clinical biochemistry parameters distinguished treated animals from control animals:
Higher alanine aminotransferase (ALAT) at 500 mg/kg in both sexes (group means increased about twofold). Increased ALAT values were also observed in a few animals (one male, one female) at 150 mg/kg.
Higher aspartate aminotransferase (ASAT) at 500 mg/kg in both sexes (group means increased about twofold). Increased ASAT values were also observed in a few animals (one male, two females) at 150 mg/kg and a single female at 50 mg/kg.
Higher alkaline phosphatase (ALP) at 500 mg/kg in both sexes (group means increased about twofold). Increased ALP values were also observed in a few animals (one male, one female) at 150 mg/kg and two females at 50 mg/kg.
Higher total bilirubin at 500 mg/kg in both sexes (group means increased about twofold).
Higher bile acids at 500 mg/kg in males (group mean increased nearly fourfold).
Lower total protein and albu min at 500 mg/kg in both sexes (group means decreased about 5-10%). Total protein was also lower (about 5%) at 150 mg/kg (not statistically significant in females).
Lower fasting glucose at 150 and 500 mg/kg in females (group means decreased about 15 and 30%, respectively). - Urinalysis findings:
- not examined
- Behaviour (functional findings):
- effects observed, non-treatment-related
- Description (incidence and severity):
- The variation in motor activity did not indicate a relation with treatment. All groups showed a similar habituation profile with a decreasing trend in activity over the duration of the test period.
- Immunological findings:
- not examined
- Organ weight findings including organ / body weight ratios:
- effects observed, treatment-related
- Description (incidence and severity):
- There were test item-related organ weight changes consisting of:
decreased weights of the prostate gland, Cowper’s gland and ani plus bulbocavernosus muscle complex (LABC) in males treated at 500 mg/kg
decreased weights of the thymus and liver in females treated at 500 mg/kg.
Other statistically significant differences in absolute or relative organ weights noted at 500 mg/kg (i.e. increased relative kidneys weight in males, and decreased absolute adrenals and uterus weights in females) were in line with lower terminal body weights. - Gross pathological findings:
- effects observed, non-treatment-related
- Description (incidence and severity):
- There was a test item-related macroscopic finding in the thymus (reduced in size) of one female treated at 500 mg/kg.
The remainder of the recorded macroscopic findings were within the range of background gross observations encountered in rats of this age and strain. These necropsy findings were therefore considered to be unrelated to treatment. - Neuropathological findings:
- not examined
- Histopathological findings: non-neoplastic:
- effects observed, treatment-related
- Description (incidence and severity):
- Test item-related microscopic findings were noted in the liver at 150 and 500 mg/kg, and in the spleen at 500 mg/kg. These changes occurred in both sexes.
In the liver, single cell necrosis (mainly centrilobular) and increased mitosis was present in males and females starting from 150 mg/kg up to moderate and slight degree, respectively.
Pigmentation of macrophages and/or Kupffer cells was observed in males at 500 mg/kg at minimal degree and in females starting from 150 mg/kg up to slight degree. Additionally, in females hypertrophy/hyperplasia of Kupffer cells was observed starting from 150 mg/kg up to slight degree.
In the spleen, a decreased incidence of extramedullary hematopoiesis was present in males and females at 500 mg/kg, and an increased severity of pigmentation was present in females at 500 mg/kg (minimal to slight pigmentation is considered to be normal background).
There were no other test item-related histologic changes. The remainder of the recorded microscopic findings were within the range of background pathology encountered in rats of this age and strain. There was no test item-related alteration in the prevalence, severity, or histologic character of those incidental tissue alterations. - Histopathological findings: neoplastic:
- not examined
- Other effects:
- effects observed, non-treatment-related
- Description (incidence and severity):
- Thyroid hormone analyses:
Serum levels of T4 in F0 males were statistically significantly lower at 500 mg/kg (relative difference from controls: 22%).
The statistically significantly higher T4 level in males at 50 mg/kg was considered to be unrelated to treatment due to the absence of similar changes at the higher dose levels. - Details on results:
- Body weight gain was decreased, to about the same extent, in females at 150 and 500 mg/kg throughout the lactation period. This was accompanied by decreased body weights at 500 mg/kg (up to 10% lower than controls at Day 13 of lactation) and decreased food consumption between lactation Days 7-13 at 150 and 500 mg/kg. Food consumption during gestation, on the other hand, was increased in females at 500 mg/kg and, to a lesser extent, 150 mg/kg.
Adverse, treatment-related microscopic changes were observed in the liver starting at 150 mg/kg, generally in both sexes. These changes were characterized by single cell necrosis (up to moderate degree), increased mitosis (up to slight degree), pigmentation of Kupffer cells/macrophages (up to slight degree; not observed in 150 mg/kg males) and hypertrophy/hyperplasia of Kupffer cells (females only). Liver weight was slightly decreased in females at 500 mg/kg but this could not clearly be related to the microscopic liver findings.
At 500 mg/kg (in both sexes), the histopathological changes in the liver were accompanied by increases in the plasma levels of alanine and aspartate aminotransferase (ALAT, ASAT), alkaline phosphatase (ALP), bilirubin and bile acids, and decreases in total protein and albumin. To a lesser extent, a decrease in total protein and increases in plasma enzymes were also observed 150 mg/kg (enzymes were increased in a few animals). Additionally, fasting glucose was decreased in females at 150 and 500 mg/kg. The increased ASAT and ALP values in a few females at 50 mg/kg were not corroborated by histopathological changes and therefore considered to be non-adverse.
Microscopic examination of the spleen showed a treatment-related decrease in the incidence of extramedullary hematopoiesis in both sexes and a slightly increased severity of pigmentation in females at 500 mg/kg. In the absence of adverse changes in haematology parameters, these findings were considered to be non-adverse.
Males treated at 500 mg/kg had lower weights of the prostate gland, Cowper’s gland and ani plus bulbocavernosus muscle complex (LABC). These treatment-related organ weight changes occurred in the absence of macroscopic or microscopic correlate and were therefore considered not to be adverse. Females at 500 mg/kg had lower thymus weights, which correlated with a reduced size of the thymus in one animal. In the absence of a microscopic correlate, the decrease in thymus weight was regarded as non-adverse.
The serum level of thyroid hormone T4 was decreased by about 20% in males at 500 mg/kg.
The weight or morphology of the thyroid were not affected by treatment. Therefore, the decrease in T4 was regarded as non-adverse.
Prothrombin time (PT) was increased in males at 500 mg/kg. There was no evidence of impaired coagulation. Possibly, the prolonged PT was associated with the adverse effect on the liver (decreased hepatic synthesis of clotting factors). - Key result
- Dose descriptor:
- NOAEL
- Effect level:
- 50 mg/kg bw/day (nominal)
- Based on:
- test mat.
- Sex:
- male/female
- Basis for effect level:
- body weight and weight gain
- clinical biochemistry
- gross pathology
- histopathology: neoplastic
- Key result
- Critical effects observed:
- yes
- Lowest effective dose / conc.:
- 150 mg/kg bw/day (nominal)
- System:
- hepatobiliary
- Organ:
- liver
- Treatment related:
- yes
- Dose response relationship:
- yes
- Relevant for humans:
- not specified
- Conclusions:
- Parental NOAEL: 50 mg/kg (based on adverse microscopic alterations in the liver and associated changes in clinical pathology parameters in both
sexes, and reduced body weight gain at the higher dose levels). - Executive summary:
SUMMARY
Title
Combined 28-day repeated dose toxicity study with the reproduction/developmental toxicity screening test of formaldehyde, oligomeric reaction products with acetone and diphenylamine in rats by oral gavage.
Guidelines
The study was based on the following guidelines:
• OECD 422, Combined Repeated Dose Toxicity Study with the Reproduction/Developmental Toxicity Screening Test, July 2016.
• OPPTS 870.3650, Combined Repeated Dose Toxicity Study with the Reproduction/Developmental Toxicity Screening Test, July 2000.
• EC No 440/2008 B.7: "Repeated Dose (28 days) Toxicity (oral)", May 2008.
• OECD 407, Repeated Dose 28-day Oral Toxicity Study in Rodents, October 2008.
• OPPTS 870.3050, Repeated dose 28-day oral toxicity study in rodents, July 2000.
Rationale for dose levels
Based on the results of a dose range finding study in which dose limiting effects were noted at 1000 mg/kg, the dose levels for this combined 28-day oral gavage study with reproduction/developmental toxicity screening test were selected to be 50, 150 and 500 mg/kg.
Study outline
The test item, formulated in polyethylene glycol 400, was administered daily by oral gavage to SPF-bred Wistar Han rats. One control group and three treated groups were tested, each consisting of 10 males and 10 females.
Males were treated for 29 days, i.e. 2 weeks prior to mating, during mating, and up to termination. Females were treated for 50-56 days (most females) or 64 days (one female), i.e. during 2 weeks prior to mating, during mating, during post-coitum, and during at least 13 days of lactation. Females which failed to deliver offspring were treated for 41 days.
Evaluated parameters
The following observations and examinations were evaluated: mortality / viability, clinical signs (daily), functional observations and locomotor activity (end of treatment), body weight and food consumption (at least at weekly intervals), clinical pathology (end of treatment), measurement of thyroid hormone T4 (males at the end of treatment), macroscopy at termination, organ weights and histopathology on a selection of tissues.
Formulations were analyzed once during the study to assess accuracy and homogeneity.
Results/discussion
Accuracy and homogeneity of formulations were demonstrated by analyses.
Body weight gain was decreased, to about the same extent, in females at 150 and 500 mg/kg throughout the lactation period. This was accompanied by decreased body weights at 500 mg/kg (up to 10% lower than controls at Day 13 of lactation) and decreased food consumption between lactation Days 7-13 at 150 and 500 mg/kg. Food consumption during gestation, on the other hand, was increased in females at 500 mg/kg and, to a lesser extent, 150 mg/kg.
Adverse, treatment-related microscopic changes were observed in the liver starting at 150 mg/kg, generally in both sexes. These changes were characterized by single cell necrosis (up to moderate degree), increased mitosis (up to slight degree), pigmentation of Kupffer cells/macrophages (up to slight degree; not observed in 150 mg/kg males) and hypertrophy/hyperplasia of Kupffer cells (females only). Liver weight was slightly decreased in females at 500 mg/kg but this could not clearly be related to the microscopic liver findings.
At 500 mg/kg (in both sexes), the histopathological changes in the liver were accompanied by increases in the plasma levels of alanine and aspartate aminotransferase (ALAT, ASAT), alkaline phosphatase (ALP), bilirubin and bile acids, and decreases in total protein and albumin. To a lesser extent, a decrease in total protein and increases in plasma enzymes were also observed 150 mg/kg (enzymes were increased in a few animals). Additionally, fasting glucose was decreased in females at 150 and 500 mg/kg. The increased ASAT and ALP values in a few females at 50 mg/kg were not corroborated by histopathological changes and therefore considered to be non-adverse.
Microscopic examination of the spleen showed a treatment-related decrease in the incidence of extramedullary hematopoiesis in both sexes and a slightly increased severity of pigmentation in females at 500 mg/kg. In the absence of adverse changes in haematology parameters, these findings were considered to be non-adverse.
Males treated at 500 mg/kg had lower weights of the prostate gland, Cowper’s gland and ani plus bulbocavernosus muscle complex (LABC). These treatment-related organ weight changes occurred in the absence of macroscopic or microscopic correlate and were therefore considered not to be adverse. Females at 500 mg/kg had lower thymus weights, which correlated with a reduced size of the thymus in one animal. In the absence of a microscopic correlate, the decrease in thymus weight was regarded as non-adverse.
The serum level of thyroid hormone T4 was decreased by about 20% in males at 500 mg/kg.
The weight or morphology of the thyroid were not affected by treatment. Therefore, the decrease in T4 was regarded as non-adverse.
Prothrombin time (PT) was increased in males at 500 mg/kg. There was no evidence of impaired coagulation. Possibly, the prolonged PT was associated with the adverse effect on the liver (decreased hepatic synthesis of clotting factors).
Conclusion
Based on the results, the following No Observed Adverse Effect Level (NOAEL) was derived:
Parental NOAEL: 50 mg/kg (based on adverse microscopic alterations in the liver and associated changes in clinical pathology parameters in both sexes, and reduced body weight gain and food consumption in females at the higher dose levels).
Reference
CLINICAL SIGNS SUMMARY
MALES
|
|
PRE MATING |
REPRO PERIOD |
||||||||||||||||||||||||||
SIGN (MAX. GRADE) |
WEEK: |
1 |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
1 |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
(LOCATION) |
DAY: |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
GROUP 1 (CONTROL) Secretion / excretion Salivation (3) |
G: %: |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
1 1 |
. . |
. . |
. . |
. . |
. . |
. . |
GROUP 2 (50 MG/KG) Skin /fur Scabs (3) (Tail) |
G: %: |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
1 1 |
1 1 |
1 1 |
1 1 |
1 1 |
1 1 |
. . |
. . |
GROUP 3 (150 MG/KG) No clinical signs noted |
|
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|
|
|
|
GROUP 4 (500 MG/KG) Secretion / excretion Salivation (3) |
G: %: |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
. . |
1 1 |
CLINICAL SIGNS SUMMARY
FEMALES
|
|
PRE MATING |
REPRO PERIOD |
||||||||||||||||||||||||||
SIGN (MAX. GRADE) |
WEEK: |
1 |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
1 |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
. |
(LOCATION) |
DAY: |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
GROUP 1 (CONTROL) No clinical signs noted |
|
|
|
|
|
|
|
|
|
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|
|
|
|
|
|
|
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|
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GROUP 2 (50 MG/KG) No clinical signs noted |
|
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|
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|
|
|
GROUP 3 (150 MG/KG) No clinical signs noted |
|
|
|
|
|
|
|
|
|
|
|
|
|
|
|
|
|
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|
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|
|
|
|
|
GROUP 4 (500 MG/KG) No clinical signs noted |
|
|
|
|
|
|
|
|
|
|
|
|
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|
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|
|
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|
|
G: Median value of the highest individual daily grades.
%: Percent of affected animal (0=less than 5%, 1=between 5% and 15%,….,A=more than 95%)
.: Observation performed, sign no present
BODY WEIGHTS (GRAM) SUMMARY
MALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
|
PRE MATING |
|||||
DAY 1 WEEK 1 |
MEAN ST. DEV N |
320 11.5 10 |
318 8.3 10 |
314 14.4 10 |
320 12.3 10 |
DAY 8 WEEK 2 |
MEAN ST. DEV N |
340 16.1 10 |
337 12.3 10 |
337 15.7 10 |
344 15.5 10 |
MATING PERIOD |
|||||
DAY 1 WEEK 1 |
MEAN ST. DEV N |
358 21.1 10 |
351 18.8 10 |
350 17.6 10 |
347 17.1 10 |
DAY 8 WEEK 2 |
MEAN ST. DEV N |
368 23.0 10 |
365 21.7 10 |
362 19.7 10 |
354 15.5 10 |
DAY 15 WEEK 3 |
MEAN ST. DEV N |
378 24.2 10 |
376 35.6 10 |
373 20.0 10 |
366 16.1 10 |
FEMALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
|
PRE MATING |
|||||
DAY 1 WEEK 1 |
MEAN ST. DEV N |
212 11.4 10 |
218 10.1 10 |
216 10.4 10 |
219 7.7 10 |
DAY 8 WEEK 2 |
MEAN ST. DEV N |
218 8.3 10 |
225 13.2 10 |
223 11.0 10 |
222 8.9 10 |
MATING PERIOD |
|||||
DAY 1 WEEK 1 |
MEAN ST. DEV N |
225 9.9 10 |
230 13.4 10 |
228 13.8 10 |
226 12.0 10 |
DAY 8 WEEK 2 |
MEAN ST. DEV N |
|
|
232 --- 1 |
222 --- 1 |
DAY 15 WEEK 3 |
MEAN ST. DEV N |
|
|
|
245 --- 1 |
DAY 22 WEEK 4 |
MEAN ST. DEV N |
|
|
|
283 --- 1 |
HAEMATOLOGY SUMMARY
MALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
|
END OF TREATMENT |
|||||
WBC 10E9/L |
MEAN ST. DEV N |
5.8 1.8 4 |
6.4 1.1 5 |
8.1 1.7 5 |
8.6* 1.7 5 |
Neutrophils %WBC |
MEAN ST. DEV N |
27.0 19.3 4 |
15.6 5.7 5 |
13.1 4.1 5 |
13.3 2.5 5 |
Lymphocytes %WBC |
MEAN ST. DEV N |
70.3 20.1 4 |
81.8 5.8 5 |
83.9 4.6 5 |
84.4 2.7 5 |
Monocytes %WBC |
MEAN ST. DEV N |
1.4 0.6 4 |
1.7 0.4 5 |
2.1 0.9 5 |
1.6 0.4 5 |
Eosinophils %WBC |
MEAN ST. DEV N |
1.2 0.6 4 |
0.8 0.2 5 |
0.8 0.3 5 |
0.6 0.1 5 |
Basophils %WBC |
MEAN ST. DEV N |
0.1 0.1 4 |
0.1 0.1 5 |
0.1 0.0 5 |
0.1 0.1 5 |
Red blood cells 10412/L |
MEAN ST. DEV N |
8.83 0.22 4 |
8.90 0.12 5 |
8.99 0.31 5 |
9.21 0.32 5 |
Reticulocytes %RBC |
MEAN ST. DEV N |
2.5 0.5 4 |
2.8 0.6 5 |
2.7 0.4 5 |
3.0 0.4 5 |
RDW % |
MEAN ST. DEV N |
12.5 0.4 4 |
12.4 0.7 5 |
11.8 0.4 5 |
12.4 0.8 5 |
Haemoglobin mmol/L |
MEAN ST. DEV N |
9.8 0.4 4 |
9.6 0.3 5 |
9.6 0.2 5 |
9.7 0.1 5 |
Haematocrit L/L |
MEAN ST. DEV N |
0.463 0.015 4 |
0.457 0.007 5 |
0.467 0.011 5 |
0.469 0.015 5 |
MCV fL |
MEAN ST. DEV N |
52.4 0.6 4 |
51.3 0.7 5 |
52.0 1.0 5 |
50.9* 0.9 5 |
MCH fmol |
MEAN ST. DEV N |
1.11 0.04 4 |
1.08 0.02 5 |
1.07 0.02 5 |
1.06* 0.03 5 |
MCHC mmol/L |
MEAN ST. DEV N |
21.15 0.60 4 |
21.07 0.52 5 |
20.57 0.25 5 |
20.80 0.45 5 |
Platelets 10E9/L |
MEAN ST. DEV N |
769 69 4 |
730 59 5 |
782 88 5 |
835 122 5 |
PT s |
MEAN ST. DEV N |
17.1 1.0 4 |
17.0 0.3 5 |
17.9 0.4 5 |
18.5** 0.3 4 |
APTT s |
MEAN ST. DEV N |
14.0 1.6 4 |
15.0 1.7 5 |
15.4 2.2 5 |
13.2 0.5 4 |
+/++ Steel-test significant at 5% (+) or 1% (++) level
*/** Dunnett-test based on pooled variance significant at 5% (*) or 1% (**) level
HAEMATOLOGY SUMMARY
FEMALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
|
END OF TREATMENT |
|||||
WBC 10E9/L |
MEAN ST. DEV N |
7.1 1.4 5 |
7.4 2.4 5 |
6.0 1.3 5 |
8.7 2.1 5 |
Neutrophils %WBC |
MEAN ST. DEV N |
41.4 11.5 5 |
41.4 3.9 5 |
48.2 19.7 5 |
46.2 8.3 5 |
Lymphocytes %WBC |
MEAN ST. DEV N |
53.8 10.7 5 |
54.0 3.6 5 |
46.6 20.6 5 |
49.2 7.9 5 |
Monocytes %WBC |
MEAN ST. DEV N |
3.6 1.8 5 |
3.5 0.7 5 |
4.2 1.4 5 |
3.7 1.6 5 |
Eosinophils %WBC |
MEAN ST. DEV N |
0.9 0.5 5 |
0.9 0.4 5 |
1.0 0.3 5 |
0.8 0.1 5 |
Basophils %WBC |
MEAN ST. DEV N |
0.1 0.1 5 |
0.1 0.1 5 |
0.1 0.0 5 |
0.1 0.0 5 |
Red blood cells 10412/L |
MEAN ST. DEV N |
7.73 0.71 5 |
7.65 0.43 5 |
8.08 0.29 5 |
7.85 0.27 5 |
Reticulocytes %RBC |
MEAN ST. DEV N |
3.7 0.9 5 |
4.1 0.6 5 |
3.7 0.3 5 |
3.3 0.7 5 |
RDW % |
MEAN ST. DEV N |
14.2 0.4 5 |
14.7 1.9 5 |
13.3 1.1 5 |
14.1 2.3 5 |
Haemoglobin mmol/L |
MEAN ST. DEV N |
9.5 0.9 5 |
9.4 0.1 5 |
9.7 0.4 5 |
9.3 0.5 5 |
Haematocrit L/L |
MEAN ST. DEV N |
0.443 0.046 5 |
0.447 0.013 5 |
0.463 0.021 5 |
0.448 0.021 5 |
MCV fL |
MEAN ST. DEV N |
57.3 1.5 5 |
58.5 1.8 5 |
57.3 1.4 5 |
57.1 2.3 5 |
MCH fmol |
MEAN ST. DEV N |
1.23 0.04 5 |
1.24 0.06 5 |
1.20 0.03 5 |
1.19 0.06 5 |
MCHC mmol/L |
MEAN ST. DEV N |
21.40 0.51 5 |
21.12 0.37 5 |
21.00 0.19 5 |
20.77* 0.29 5 |
Platelets 10E9/L |
MEAN ST. DEV N |
840 136 5 |
941 79 5 |
850 68 5 |
842 175 5 |
PT s |
MEAN ST. DEV N |
17.0 0.8 4 |
16.9 0.7 5 |
16.6 0.4 5 |
17.4 0.6 5 |
APTT s |
MEAN ST. DEV N |
13.0 1.7 4 |
12.9 2.0 5 |
13.3 2.4 5 |
14.1 1.0 5 |
+/++ Steel-test significant at 5% (+) or 1% (++) level
*/** Dunnett-test based on pooled variance significant at 5% (*) or 1% (**) level
CLINICAL BIOCHEMISTRY SUMMARY
MALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
|
END OF TREATMENT |
|||||
ALAT U/L |
MEAN ST. DEV N |
40.4 2.1 5 |
53.0 22.4 5 |
52.8 17.6 5 |
98.8** 11.0 5 |
ASAT U/L |
MEAN ST. DEV N |
77.2 3.7 5 |
92.5 31.1 5 |
99.5 18.8 5 |
152.4** 35.2 5 |
ALP U/L |
MEAN ST. DEV N |
136 34 5 |
162 27 5 |
180 22 5 |
285** 73 5 |
Total protein g/L |
MEAN ST. DEV N |
64.2 2.6 5 |
62.1 1.3 5 |
60.8 1.8 5 |
57.3** 1.9 5 |
Albumin g/L |
MEAN ST. DEV N |
33.9 1.2 5 |
62.1 1.3 5 |
60.8* 1.8 5 |
57.3* 1.9 5 |
Total bilirubin umol/L |
MEAN ST. DEV N |
2.3 0.3 5 |
2.3 0.3 5 |
3.1 0.4 5 |
5.8** 1.2 5 |
Urea mmol/L |
MEAN ST. DEV N |
6.9 1.6 5 |
5.8 0.9 5 |
7.5 1.1 5 |
8.6 1.4 5 |
Creatinine umol/L |
MEAN ST. DEV N |
37.5 2.3 5 |
36.9 1.9 5 |
38.6 1.6 5 |
35.8 1.2 5 |
Glucose mmol/L |
MEAN ST. DEV N |
8.71 1.36 5 |
9.61 0.80 5 |
9.02 0.66 5 |
7.81 0.36 5 |
Cholesterol mmol/L |
MEAN ST. DEV N |
2.39 0.52 5 |
1.81 0.28 5 |
1.96 0.21 5 |
2.55 0.51 5 |
Bile Acids umol/L |
MEAN ST. DEV N |
34.9 17.2 5 |
23.2 15.0 5 |
30.2 13.0 5 |
128.8* 93.5 5 |
Sodium mmol/L |
MEAN ST. DEV N |
140.8 0.6 5 |
140.6 0.3 5 |
140.5 0.6 5 |
140.0 1.3 5 |
Potassium mmol/L |
MEAN ST. DEV N |
4.12 0.25 5 |
4.00 0.06 5 |
3.94 0.16 5 |
4.09 0.16 5 |
Chloride mmol/L |
MEAN ST. DEV N |
103 1 5 |
103 0 5 |
103 1 5 |
103 2 5 |
Calcium mmol/L |
MEAN ST. DEV N |
2.59 0.10 5 |
2.53 0.02 5 |
2.52 0.05 5 |
2.52 0.03 5 |
Inorg.Phos mmol/L |
MEAN ST. DEV N |
1.97 0.09 5 |
1.86 0.10 5 |
1.88 0.15 5 |
2.12 0.15 5 |
Total T4 ug/dL |
MEAN ST. DEV N |
4.09 0.60 10 |
5.13* 0.69 10 |
4.71 1.12 10 |
3.20* 0.52 10 |
*/** Dunnett-test based on pooled variance significant at 5% (*) or 1% (**) level
CLINICAL BIOCHEMISTRY SUMMARY
FEMALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
|
END OF TREATMENT |
|||||
ALAT U/L |
MEAN ST. DEV N |
71.5 9.0 5 |
67.9 23.8 5 |
99.1 40.2 5 |
144.5* 71.4 5 |
ASAT U/L |
MEAN ST. DEV N |
114.5 20.0 5 |
132.4 62.3 5 |
175.3 66.1 5 |
216.6* 65.4 5 |
ALP U/L |
MEAN ST. DEV N |
119 36 5 |
178 76 5 |
171 48 5 |
265* 127 5 |
Total protein g/L |
MEAN ST. DEV N |
64.1 3.4 5 |
63.4 1.5 5 |
60.1 3.9 5 |
57.0** 2.1 5 |
Albumin g/L |
MEAN ST. DEV N |
32.7 1.3 5 |
32.6 1.0 5 |
31.1 1.4 5 |
29.5** 0.8 5 |
Total bilirubin umol/L |
MEAN ST. DEV N |
2.4 0.7 5 |
2.7 0.5 5 |
2.8 0.3 5 |
4.5** 1.4 5 |
Urea mmol/L |
MEAN ST. DEV N |
10.3 1.5 5 |
10.2 1.1 5 |
11.1 2.1 5 |
12.4 2.1 5 |
Creatinine umol/L |
MEAN ST. DEV N |
43.3 2.5 5 |
44.2 2.1 5 |
45.1 4.4 5 |
45.0 4.4 5 |
Glucose mmol/L |
MEAN ST. DEV N |
9.12 0.76 5 |
8.11 0.86 5 |
45.1 4.4 5 |
45.0 4.4 5 |
Cholesterol mmol/L |
MEAN ST. DEV N |
2.41 0.34 5 |
2.66 0.35 5 |
3.10 0.60 5 |
3.02 0.82 5 |
Bile Acids umol/L |
MEAN ST. DEV N |
38.6 35.7 5 |
50.1 7.9 5 |
47.2 24.0 5 |
120.6 165.0 5 |
Sodium mmol/L |
MEAN ST. DEV N |
135.4 1.4 5 |
137.3 2.0 5 |
135.7 2.4 5 |
135.7 1.6 5 |
Potassium mmol/L |
MEAN ST. DEV N |
4.04 0.28 5 |
3.91 0.20 5 |
4.22 0.19 5 |
4.35 0.22 5 |
Chloride mmol/L |
MEAN ST. DEV N |
98 2 5 |
98 2 5 |
99 2 5 |
100 3 5 |
Calcium mmol/L |
MEAN ST. DEV N |
2.74 0.09 5 |
2.70 0.13 5 |
2.67 0.06 5 |
2.65 0.11 5 |
Inorg.Phos mmol/L |
MEAN ST. DEV N |
2.64 0.47 5 |
2.84 0.44 5 |
2.80 0.52 5 |
2.84 0.49 5 |
Total T4 ug/dL |
MEAN ST. DEV N |
--- --- 0 |
--- --- 0 |
--- --- 0 |
--- --- 0 |
*/** Dunnett-test based on pooled variance significant at 5% (*) or 1% (**) level
MACROSCOPIC FINDINGS SUMMARY
MALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
END OF TREATMENT |
||||
Animals examined |
10 |
10 |
10 |
10 |
Animals without findings |
8 |
8 |
8 |
9 |
Animals affected |
2 |
2 |
2 |
1 |
Liver Diaphragmatic hernia |
0 |
1 |
0 |
0 |
Kidneys Pelvic dilation |
0 |
1 |
0 |
0 |
Epididymides Nodule(s) |
0 |
1 |
0 |
0 |
Cowper’s gland Enlarged |
0 |
1 |
0 |
0 |
Thyroid gland Discolouration Agenesis |
0 1 |
0 0 |
1 0 |
0 0 |
Thymus Focus/foci Discolouration |
0 1 |
0 0 |
0 0 |
1 0 |
Skin Nodule(s) |
0 |
0 |
1 |
0 |
FEMALES
|
GROUP 1 CONTROL |
GROUP 2 50 MG/KG |
GROUP 3 150 MG/KG |
GROUP 4 500 MG/KG |
END OF TREATMENT |
||||
Animals examined |
10 |
10 |
10 |
10 |
Animals without findings |
7 |
10 |
8 |
6 |
Animals affected |
3 |
0 |
2 |
4 |
Stomach Focus/foci |
1 |
0 |
1 |
0 |
Jejunum Discolouration |
0 |
0 |
1 |
0 |
Uterus Contains fluid |
0 |
0 |
0 |
1 |
Clitoral glands Nodule(s) Focus/foci |
0 0 |
0 0 |
0 1 |
1 0 |
Thymus Reduced in size Discolouration |
0 0 |
0 0 |
0 1 |
1 0 |
Mandibular lymph n Discolouration |
2 |
0 |
0 |
0 |
Skin Scab formation |
0 |
0 |
0 |
1 |
#/## Fischer’s Exact test significant at 5% (#) or 1% (##) level
Endpoint conclusion
- Endpoint conclusion:
- no adverse effect observed
- Dose descriptor:
- NOAEL
- 50 mg/kg bw/day
- Study duration:
- subacute
- Species:
- rat
- Quality of whole database:
- K1 - OECD & US EPA test guidelines in accordance with GLP accreditation.
Repeated dose toxicity: inhalation - systemic effects
Endpoint conclusion
- Endpoint conclusion:
- no study available
Repeated dose toxicity: inhalation - local effects
Endpoint conclusion
- Endpoint conclusion:
- no study available
Repeated dose toxicity: dermal - systemic effects
Endpoint conclusion
- Endpoint conclusion:
- no study available
Repeated dose toxicity: dermal - local effects
Endpoint conclusion
- Endpoint conclusion:
- no study available
Additional information
Repeated dose toxicity-oral
Combined 28-day repeated dose toxicity study with the reproduction/developmental toxicity screening test of formaldehyde, oligomeric reaction products with acetone and diphenylamine in rats by oral gavage.
The test item, formulated in polyethylene glycol 400, was administered daily by oral gavage to SPF-bred Wistar Han rats. One control group and three treated groups were tested, each consisting of 10 males and 10 females.
Males were treated for 29 days, i.e. 2 weeks prior to mating, during mating, and up to termination. Females were treated for 50-56 days (most females) or 64 days (one female), i.e. during 2 weeks prior to mating, during mating, during post-coitum, and during at least 13 days of lactation. Females which failed to deliver offspring were treated for 41 days.
Evaluated parameters
The following observations and examinations were evaluated: mortality / viability, clinical signs (daily), functional observations and locomotor activity (end of treatment), body weight and food consumption (at least at weekly intervals), clinical pathology (end of treatment), measurement of thyroid hormone T4 (males at the end of treatment), macroscopy at termination, organ weights and histopathology on a selection of tissues.
Results/discussion
Body weight gain was decreased, to about the same extent, in females at 150 and 500 mg/kg throughout the lactation period. This was accompanied by decreased body weights at 500 mg/kg (up to 10% lower than controls at Day 13 of lactation) and decreased food consumption between lactation Days 7-13 at 150 and 500 mg/kg. Food consumption during gestation, on the other hand, was increased in females at 500 mg/kg and, to a lesser extent, 150 mg/kg.
Adverse, treatment-related microscopic changes were observed in the liver starting at 150 mg/kg, generally in both sexes. These changes were characterized by single cell necrosis (up to moderate degree), increased mitosis (up to slight degree), pigmentation of Kupffer cells/macrophages (up to slight degree; not observed in 150 mg/kg males) and hypertrophy/hyperplasia of Kupffer cells (females only). Liver weight was slightly decreased in females at 500 mg/kg but this could not clearly be related to the microscopic liver findings.
At 500 mg/kg (in both sexes), the histopathological changes in the liver were accompanied by increases in the plasma levels of alanine and aspartate aminotransferase (ALAT, ASAT), alkaline phosphatase (ALP), bilirubin and bile acids, and decreases in total protein and albumin. To a lesser extent, a decrease in total protein and increases in plasma enzymes were also observed 150 mg/kg (enzymes were increased in a few animals). Additionally, fasting glucose was decreased in females at 150 and 500 mg/kg. The increased ASAT and ALP values in a few females at 50 mg/kg were not corroborated by histopathological changes and therefore considered to be non-adverse.
Microscopic examination of the spleen showed a treatment-related decrease in the incidence of extramedullary hematopoiesis in both sexes and a slightly increased severity of pigmentation in females at 500 mg/kg. In the absence of adverse changes in haematology parameters, these findings were considered to be non-adverse.
Males treated at 500 mg/kg had lower weights of the prostate gland, Cowper’s gland and ani plus bulbocavernosus muscle complex (LABC). These treatment-related organ weight changes occurred in the absence of macroscopic or microscopic correlate and were therefore considered not to be adverse. Females at 500 mg/kg had lower thymus weights, which correlated with a reduced size of the thymus in one animal. In the absence of a microscopic correlate, the decrease in thymus weight was regarded as non-adverse.
The serum level of thyroid hormone T4 was decreased by about 20% in males at 500 mg/kg.
The weight or morphology of the thyroid were not affected by treatment. Therefore, the decrease in T4 was regarded as non-adverse.
Prothrombin time (PT) was increased in males at 500 mg/kg. There was no evidence of impaired coagulation. Possibly, the prolonged PT was associated with the adverse effect on the liver (decreased hepatic synthesis of clotting factors).
Conclusion
Based on the results, the following No Observed Adverse Effect Level (NOAEL) was derived:
Parental NOAEL: 50 mg/kg (based on adverse microscopic alterations in the liver and associated changes in clinical pathology parameters in both sexes, and reduced body weight gain and food consumption in females at the higher dose levels).
Justification for classification or non-classification
Based on the results of this study, the substance is classified as STOT RE 2 in accordance with the CLP Regulation.
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