Reaction mass of 1,1,2,2,3,3,4,4-octafluoro-1,4-diiodobutane and 1,6-diiodoperfluorohexane

Administrative data

Endpoint:

short-term repeated dose toxicity: inhalation

Type of information:

experimental study

Remarks:

read-across from supporting substance (structural analogue or surrogate)

Adequacy of study:

key study

Study period:

14-FEB-2007 to 03-DEC-2009

Reliability:

2 (reliable with restrictions)

Rationale for reliability incl. deficiencies:

guideline study

Data source

Referenceopen allclose all

Materials and methods

GLP compliance:

yes

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
- Strain: HsdHan (SPF)
- Source: Harlan Netherlands B.V. / Postbus 6174, NL-5960 AD Horst / THE NETHERLANDS
- Age at study initiation: 7 to 8 weeks for males; 9 to 10 weeks for females
- Weight at study initiation: the weight variation in animals entering the study did not exceed ± 7% of the mean weight of the corresponding sex.
- Fasting period before study: not applicable
- Housing: animals of the same sex were housed in groups of up to 5 in Makrolon type-IV cages with wire mesh tops and standard softwood bedding ("Lignocel", Schill AG, CH-4132 Muttenz / SWITZERLAND).
- Diet: ad libitum (pelleted standard Kliba-Nafag 3433 rat maintenance diet, batch no. 80/06), except during the daily exposure periods and during ca. 16 h prior to clinical laboratory investigations
- Water: ad libitum (community tap-water from Füllinsdorf, chlorinated to ca. 0.5 ppm), except during the daily exposure periods
- Acclimation period: 15 days, under laboratory conditions, after clinical health examination

ENVIRONMENTAL CONDITIONS
- Temperature: 22 ± 3°C
- Humidity: 30 to 70%
- Air changes: 10 to 15 changes per hr
- Photoperiod: 12 hrs dark / 12 hrs light

IN-LIFE DATES: From 21-FEB-2007 to 03-MAY-2007

Administration / exposure

Route of administration:

inhalation: vapour

Type of inhalation exposure:

whole body

Vehicle:

other: compressed filtered air

Remarks on MMAD:

MMAD / GSD: Not applicable

Details on inhalation exposure:

GENERATION OF TEST ATMOSPHERE / CHAMBER DESCRIPTION
- Exposure apparatus: inhalation by whole-body vapour exposure was performed in sealed chambers used for group isolation. These chambers were constructed of stainless steel. Glass doors were equipped with silicone rubber seals. The data of the exposure chambers are summarised in Table 1 below.
- Method of holding animals in test chamber: animals were accustomed to the whole-body inhalation chambers and the exposure conditions for 3 daily periods of ca. 1, 3 and 6 hours, respectively.
- Source and rate of air: the oxygen content was equal to 20.6%.
- Method of conditioning air: no data available
- System of generating particulates/aerosols: for group 2 (ca. 0.2 ppm), gas bags were prepared at a concentration that was defined during technical trials. From the gas bags, the vapour was transferred with a gas pump to a pipe and was then diluted with 420 L/min filtered air to the inlet duct of the exposure chamber.
For groups 3 (ca. 0.632 ppm) and 4 (ca. 2 ppm), the test substance was pumped at a specific rate into a round bottomed glass flask to be vaporised. Compressed air (40 L/min) was supplied into the glass flasks and allowed the liquid to equilibrate to the temperature of the warm walls of the container. The vapour produced then was passed through a pipe and was then diluted with 380 L/min of filtered air to the inlet duct of the exposure chamber.
Gas bags and flasks containing the test substance were kept at room temperature.
- Temperature, humidity, pressure in air chamber: ca. 24.5°C; ca. 33.4%; negative pressure of ca. 2 mm H2O
- Air flow rate: no data available
- Air change rate: 10 to 15 air changes per hour
- Method of particle size determination: not applicable
- Treatment of exhaust air: no data available

TEST ATMOSPHERE
- Brief description of analytical method used: The test item vapour was measured by on-line gas chromatography (GC).
- Samples taken from breathing zone: yes

VEHICLE: not applicable

Analytical verification of doses or concentrations:

yes

Details on analytical verification of doses or concentrations:

The chamber concentration and stability of the test substance over the duration of ca. 6 hours was determined on at least two occasions prior to the start of the animal exposures. The test item was generated in the chambers at nominal concentrations of 0.2, 0.632 / 0.4 and 2 / 0.8 ppm and measured by on-line gas chromatography (GC).
During the treatment period, the concentration of the test substance in the chamber was determined daily, at least 5 times each hour of exposure. Start of recording was after the chamber equilibration time T90 (i.e. 90% equilibration time), and continued until pump off.
The method of analysis corresponded to the following:
- Column: DB-5 (No. 163755)
- Oven: 100°C, isothermal
- Runtime: 3 min
- Injector: 250°C
- Detector: 250°C
- Carrier gas: helium
- Sample loop: ca. 1700 µL
- Retention time: ca. 1.3

Duration of treatment / exposure:

4 consecutive weeks
Due to signs of overt toxicity (body weight loss, emaciation), the vapour concentrations for Groups 3 and 4 were lowered after 12 exposures, starting on Day 13 of exposure (exposures 13 to 20, phase 2).

Frequency of treatment:

6 hours/day and 5 days/week

Doses / concentrationsopen allclose all

No. of animals per sex per dose:

5 per sex per dose

Control animals:

yes, concurrent vehicle

Details on study design:

- Dose selection rationale: vapour concentrations were chosen on the basis of the results of the 5-day dose range finding inhalation toxicity study in the rat (see ESR entitled "I-(CF2)6-I - Repeat. dose tox.: 5-day inhal. - K1 2008RCC").
- Due to signs of overt toxicity (body weight loss, emaciation), the vapour concentrations for Groups 3 and 4 were lowered starting on Day 13 of exposure.

- Rationale for animal assignment (if not random): not applicable
- Rationale for selecting satellite groups, post-exposure recovery period in satellite groups: in order to assess the reversibility of any treatment-related findings satellite groups of animals were maintained for a subsequent period of 4 weeks without treatment.
- Section schedule rationale (if not random): not applicable

Examinations

Observations and examinations performed and frequency:

CAGE SIDE OBSERVATIONS: Yes
- Time schedule: all animals were observed for mortality/morbidity twice daily, once prior to and once following exposure, during the treatment period and at least once daily on non-exposure days of treatment period and during the acclimatisation period and recovery periods.

DETAILED CLINICAL OBSERVATIONS: Yes
- Time schedule: clinical signs were recorded on the first day of the acclimatisation period. During the exposure period, clinical signs were observed twice daily, prior to and following exposure. On non-exposure days of the treatment period and during the recovery period, clinical signs were observed once daily. During exposure, only grossly abnormal signs were observed, as the animals were housed in the whole-body inhalation chambers. Observations included, but were not limited to: changes in the skin and fur, eyes and mucous membranes and also respiratory, circulatory, autonomic and central nervous system, somatomotor activity and behaviour pattern.

BODY WEIGHT: Yes
- Time schedule for examinations: each animal was weighed on the first day of the acclimatisation period (used for randomised), and thereafter at least once weekly during the acclimatisation, treatment and recovery periods.

FOOD CONSUMPTION:
- Food consumption for each animal determined and mean daily diet consumption calculated as g food/kg body weight/day: Yes; food consumption was measured per cage of 5 animals once weekly during the acclimatisation, treatment and recovery periods.

FOOD EFFICIENCY:
- Body weight gain in kg/food consumption in kg per unit time X 100 calculated as time-weighted averages from the consumption and body weight gain data: No

WATER CONSUMPTION: Yes
- Time schedule for examinations: water consumption was measured per cage of 5 animals at least twice weekly during the acclimatisation, treatment and recovery periods.

OPHTHALMOSCOPIC EXAMINATION: Yes
- Time schedule for examinations, dose groups that were examined: ophthalmoscopic examinations was performed in all animals before treatment (during acclimatisation [23-FEB-2007]) and in all surviving animals in week 4 of the treatment period [29-MAR-2007] and in week 4 of the recovery period [27-APR-2007]. Observations were performed after instillation of a mydriaticum, using a Heine Bifocal Type Miroflex ophthalmoscope (Eisenhut Vet. AG, 4123 Allschwil / SWITZERLAND).

HAEMATOLOGY: Yes
- Time schedule for collection of blood, how many animals: blood samples from the retro-orbital plexus were collected for haematology from all animals of all groups under isofluorane (Forene) anaesthesia before necropsy. The samples were collected early in the working day to reduce biological variation caused by circadian rhythm.
- Anaesthetic used for blood collection: Yes (isofluorane)
- Animals fasted: Yes; the animals were fasted in metabolism cages for ca. 16 hours before blood sampling, but water was provided ad libitum.
- Parameters checked: erythrocyte count (RBC), haemoglobin (HB), haematocrit (HCT), mean corpuscular volume (MCV), mean corpuscular haemoglobin (MCH), mean corpuscular haemoglobin concentration (MCHC), reticulocyte count, red blood cell morphology (red cell volume distribution width (RDW), haemoglobin concentration distribution width), reticulocyte maturity index, platelet count, total leukocyte count (WBC), differential leukocyte count, coagulation (prothrombin time (PT), activated partial thromboplastin time (PTT))

CLINICAL CHEMISTRY: Yes
- Time schedule for collection of blood, how many animals: blood samples from the retro-orbital plexus were collected for clinical biochemistry from all animals of all groups under isofluorane (Forene) anaesthesia before necropsy. The samples were collected early in the working day to reduce biological variation caused by circadian rhythm.
- Animals fasted: Yes; the animals were fasted in metabolism cages for ca. 16 hours before blood sampling, but water was provided ad libitum.
- Parameters checked: glucose, total cholesterol, creatinine, phospholipids, urea, total bilirubin, triglycerides, alanine aminotransferase, aspartate aminotransferase, alkaline phosphatase, lactate dehydrogenase (LDH), glutamate dehydrogenase, creatinine kinase, gamma-glutamyl-transferase, chloride, calcium, sodium, potassium, total protein, phosphorus, albumin, globulin, albumin/globulin ratio.
- Additional investigations: alpha-glutathione S-transferase (alpha-GST) (by immuno assay), inhibin B (by ELISA), tri-iodothryronine (T3), thyroxine (T4), thyroid-stimulating hormone (TSH), testosterone by immunoassay.

URINALYSIS: Yes
- Time schedule for collection of urine: sampling during the 16-h period before blood sampling
- Metabolism cages used for collection of urine: Yes
- Animals fasted: Yes
- Parameters checked: volume, relative density, osmolality, colour, appearance, pH, protein, glucose, ketone, nitrite, bilirubin, erythrocytes, urobilinogen, leukocytes

NEUROBEHAVIOURAL EXAMINATION: No

Sacrifice and pathology:

GROSS PATHOLOGY: Yes; all animals of all groups were necropsied. The surviving animals were fasted overnight before necropsy, but water was provided. All animals were anaesthetised by an intraperitoneal injection of sodium pentobarbitone and sacrificed by exsanguination.
HISTOPATHOLOGY: Yes; samples of the following tissues and organs were collected from all animals at necropsy and fixed in neutral phosphate buffered 4% formaldehyde solution unless otherwise stated. Lungs were instilled with the fixative at a hydrostatic pressure of 30 cm.
Adrenal glands
Aorta
Brain (cerebrum, cerebellum, brain stem)
Cecum
Colon
Duodenum
Epididymides (fixed in Bouin's solution)
Oesophagus
Extraorbital lacrimal glands
Eyes with optic nerves (fixed in Davidson's solution)
Femur, including joint
Harderian glands (fixed in Davidson's solution)
Heart
Ileum
Jejunum
Kidneys
Larynx (three transversal sections, at least levels II, III and IV)
Liver
Lungs
Lymph nodes - bronchial, mandibular, mesenteric
Mammary gland area
Nasal cavities (infused with formalin) with "paranasal sinuses" (Levels I to IV)
Nasopharyngeal duct and pharynx (1 longitudinal section)
Ovaries
Pancreas
Pituitary gland
Prostate
Rectum
Salivary glands - mandibular, sublingual
Sciatic nerve
Seminal vesicles (fixed in Bouin's solution)
Skeletal muscle (thigh region)
Skin
Spinal cord - cervical, midthoracic, lumbar
Spleen
Sternum with bone marrow
Stomach
Testes (fixed in Bouin's solution)
Thymus
Thyroid gland with parathyroid gland
Tongue
Trachea (one transversal section below larynx)
Tracheal bifurcation, carina and mainstem bronchi
Urinary bladder (infused with formalin)
Uterus with uterine cervix
Vagina
All gross lesions

Other examinations:

ORGAN WEIGHTS: the following organ weights were recorded at the scheduled dates of necropsy. Organ to body weight and organ to brain weight ratios were calculated. Paired organs were weighed together.
Adrenal glands
Brain
Epididymides
Heart
Kidneys
Liver
Lungs
Ovaries
Spleen
Testes
Thymus
Uterus

ENZYMATIC ASSAY:
It was hypothesised that the test substance could act as an inhibitor of the (hepatic) deiodinase leading to potential accumulation of T4 and concomitant decrease in T3. This suggested mode of action was investigated by determination of in vitro conversion of T4/T3 catalysed by rat and human liver microsomes in presence of the test substance.
Rat (Wistar) liver microsomes were prepared by RCC and tested for P-450 content and stored at -80°C until use. Human liver microsomes were obtained from Chemie Brunschwig AG (Basel, SWITZERLAND) and stored at -80°C until use.
Activity of 5’-deiodinase was determined by release of acid soluble iodide [125 I-] from 3,3’,5’-[125 I]-triiodo-L-thyronine ([125 I]-reverse T3) upon incubation with liver microsomes. Test item concentrations from 0 up to 1 mM were incubated with liver microsomes (4.4 µg protein) in a final volume of 100 µL of 0.1 M potassium hydrogen phosphate buffer/0.01 EDTA (pH 7.0), 1 mM DTT, 1 µM freshly prepared reverse T3 and [125 I]-reverse T3 (13.5 fmol/assay) at 37°C for 20 min. The reactions were stopped by addition of 50 µL 6-propyl-2-thiouracil (PTU) at 10 µM/8% BSA (50:50, v/v). The proteins were precipitated by addition of 400 µL 10% trichloroacetic acid and centrifugation at 3000 g for 15 min at 4°C. Released acid soluble iodide [125 I-] in the supernatant was determined by gamma-counting following purification by cation exchange chromatography.
A known inhibitor of 5’-deiodinase, PTU at 3-4 µM, was used as a positive control.

To test linearity of 5’-deiodinase activity rat liver microsomes were incubated with [125 I]-reverse T3 for 10, 20 and 40 min at protein concentrations of 0, 11, 22, 44, 88 and 176 µg/mL. 5’-deiodinase activity of rat liver microsomes was proportional to the incubation time and to the protein concentration up to 40 min at 44 µg protein/mL, up to 88 µg protein/mL at an incubation time of 20 min and up to 176 µg protein/mL at an incubation time of 10 min. Therefore 5’-deiodinase activity was investigated at a protein concentration of 44 µg/mL and an incubation time of 20 min, and with test item concentrations of 0, 1, 3, 7, 15, 63, 250 and 1000 µM.

% deiodination = ((sample cpm – blank cpm) x 100)/total cpm
where total cpm = cpm in incubation

Activity of 5’-deiodinase: % deiodination/protein concentration per assay/incubation time [% deiodination/ng protein/min]

Statistics:

The Dunnett test (many-to-one t-test) based on a pooled variance estimate was used to analyse body weight, organ weights and food and water consumption and clinical laboratory parameters.
The Steel test (many-one rank test) was applied instead of the Dunnett test for those clinical laboratory parameters that could not be assumed to follow a normal distribution.
The Fisher's exact test was applied to macroscopic findings and ophthalmoscopy data where appropriate.
Group means and standard deviations were calculated for continuous data.

Results and discussion

Results of examinations

Clinical signs:

effects observed, treatment-related

Description (incidence and severity):

There were no unscheduled deaths during the course of this study. However, in group 2, several females were emaciated towards the end of the treatment period. In group 4, the majority of animals of both genders were emaciated towards the end of the treatment period. The majority of animals of both genders from group 4 were still emaciated during the beginning of the recovery period. No further clinical signs were considered to be related to exposure to the test substance.

Mortality:

mortality observed, treatment-related

Description (incidence):

There were no unscheduled deaths during the course of this study. However, in group 2, several females were emaciated towards the end of the treatment period. In group 4, the majority of animals of both genders were emaciated towards the end of the treatment period. The majority of animals of both genders from group 4 were still emaciated during the beginning of the recovery period. No further clinical signs were considered to be related to exposure to the test substance.

Body weight and weight changes:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Food consumption and compound intake (if feeding study):

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Food efficiency:

not examined

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

not specified

Ophthalmological findings:

no effects observed

Description (incidence and severity):

The findings noted were corneal opacity and persistent pupillary membrane. The incidence or distribution of these findings did not distinguish treated animals from controls.

Haematological findings:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Clinical biochemistry findings:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Urinalysis findings:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Behaviour (functional findings):

not examined

Organ weight findings including organ / body weight ratios:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Gross pathological findings:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Histopathological findings: non-neoplastic:

effects observed, treatment-related

Description (incidence and severity):

see in "Details on results"

Histopathological findings: neoplastic:

no effects observed

Details on results:

BODY WEIGHT (Table 2 in "Any other information on results incl. tables")
After 4 weeks of treatment, body weight and body weight gain were considerably reduced in both genders of all treated groups, related to dose, attaining statistical significance in both genders of groups 3 and 4, and in males of group 2 for body weight gain.
After 4 weeks of recovery, body weight was significantly lower in males of group 4 compared to control (group 1). During recovery, body weight gain was considerably higher in both genders of group 4.
For details, see in Table 2.

FOOD CONSUMPTION
During the 4-week treatment period, food consumption was non-significantly reduced in both genders of groups 2 to 4 compared to control (group 1). Relative food consumption was slightly and non-significantly reduced in both genders of groups 2 and 3 and increased in both genders of group 4 compared to control (group 1).
During the recovery period, food consumption and relative food were non-significantly reduced in males of group 4 and increased in females of group 4.

HAEMATOLOGY (Table 3 in "Any other information on results incl. tables")
After 4 weeks of treatment, several haematological parameters were significantly altered in treated animals of both sexes. Overall, treated males displayed significant decreases in erythrocyte count (RBC), haemoglobin (HB), haematocrit (HCT), neutrophil (Neut) count, and in prothrombin time (PT), as well as an increase in reticulocyte (RETI). Treated females showed similar haematological impairments: significant decreases in RBC, HB, HCT, and Neut count, as well as a significant increase in RETI, lymphocyte (Lymph) and monocyte (Mono) counts.
After 4 weeks of recovery, some haematological parameters remained significantly altered; others appeared in treated animals of both sexes. Males of group 4 showed significant decreases in HB, HCT, HDW, total leukocyte count (WBC), basophil (Baso) count, Lymph count, and Mono count. While females of group 4 only displayed a significant decrease in HB.

CLINICAL CHEMISTRY (Table 4 in "Any other information on results incl. tables")
After 4 weeks of treatment, several biochemistry parameters were significantly altered in treated animals of both sexes. Overall, treated males displayed significant increases in glucose, lactate dehydrogenase activity (LDH), chloride, calcium, globulin, as well as significant decreases in urea, total cholesterol, aspartate aminotransferase activity (ASAT), creatinine kinase activity (CK), inorganic phosphorus, and an albumin decrease in group 3 followed by an increase in group 4. Treated females showed the following haematological impairments: significant increases in glucose, triglycerides, alkaline phosphatase (ALP), calcium, inorganic phosphorus, protein, and globulin, as well as significant decreases in urea, creatinine, total cholesterol, CK, sodium, chloride, albumin, and albumin/globulin ratio.
After 4 weeks of recovery, some biochemistry parameters remained significantly altered. Males of group 4 showed only a significant increase in inorganic phosphorus. While females of group 4 displayed significant decreases in calcium, protein, and albumin levels, and a significant elevation in inorganic phosphorus.

In addition, serum α-GST levels were found to be non-significantly decreased in males and females of all treated groups when compared to controls. Regardless of the gender, mean constitutive Inhibin B levels were increased in animals treated for 4 weeks with 0.4 and 0.8 ppm test substance (i.e., groups 3 and 4). After a recovery period of 4 weeks, Inhibin B levels from animals treated with 0.8 ppm test substance returned to control values. The clear decrease of Inhibin B concentrations provided further evidence of gonadotoxicity by the test substance at dose levels of 0.4 and 0.8 ppm. Moreover, T3 levels were significantly decreased in males and females of group 4. Whereas a significant increase in T4 levels was observed in males of groups 3 and 4 and in females of all treated groups. There was no measurement of T3 and T4 levels after the 4-week recovery period.

URINALYSIS
The relative density significantly decreased in males of group 2. Osmolality significantly decreased in males and females of group 2.

ORGAN WEIGHTS (Table 5 in "Remarks on results including tables and figures")
After 4 weeks of exposure, the weight of various organs was significantly altered in treated animals of both sexes. When expressed as organ/body weight ratio, the weight of thymus, adrenals, epididymis, and testes significantly decreased in treated males, while the weight of brain, heart, lungs, liver, kidneys, adrenals, and spleen significantly increased in the same treated groups. Overall, treated females displayed moderate but significant decreases in thymus and ovaries weights and slight but significant increases in brain, liver, and spleen weights (i.e., when expressed as organ/body weight ratio).
After 4 weeks of recovery, some organ weights parameters remained significantly altered. When expressed as organ/body weight ratio, epididymis and testes weights were still significantly decreased and, as seen during the treatment period, the weight of brain, lungs, thymus, and adrenals significantly increased in males of group 4 at the end of the recovery period. The only significant effect seen in females of group 4 was the remaining increase in liver weight (i.e., liver/body weight ratio).

GROSS PATHOLOGY (Table 6 in "Remarks on results including tables and figures")
After 4 weeks of exposure, all males of group 4 and almost all males from group 3 showed a size reduction of testes, epididymis, prostate and seminal vesicles. Two males of group 2 showed seminal vesicles with a reduced size. In all females of group 4, thymus was reduced in size. In groups 3 and 3, a single female demonstrated enlarged liver and ovaries with a reduced size. In one female of group 4, the pituitary gland was thickened.
After 4 weeks of recovery, males of group 4 still showed a size reduction of testes, epididymis, prostate and seminal vesicles. Further, thymus and lymph node discoloration, as well as spleen constriction and skin alopecia/sore were observed in one male of group 4. Two females of group 4 displayed a thickened pituitary gland and alopecia.

HISTOPATHOLOGY: NON-NEOPLASTIC (Table 6 in "Remarks on results including tables and figures")
After 4 weeks of exposure, a minimal centrilobular hepatocellular hypertrophy seen in 2 females of group 2 and a diffuse hepatocellular hypertrophy noted in 2 males of group 2 and in all males and females of groups 3 and 4. This was considered to be possibly adaptive. The hypertrophy seen in males and females of group 4 was associated with minimal to slight midzonal hepatocellular fatty change.Enhanced alveolar histiocytosis occurred in lungs of males and females from group 4.
The pituitary gland of one female from group 4 showed a minimal diffuse hypertrophy of pars distalis.
In addition, diffuse tubular atrophy of testes was seen in 4 males of group 3 and all males of group 4. Atrophy of epididymis occurred in 4 males of groups 3 and 4. An atrophy of seminal vesicles was seen in the majority of all males from all treated groups. An atrophy of prostate was observed in all males of groups 3 and 4. A reduction of the number of corpora lutea in ovaries was described in 1 female of group 3 and 3 females of group 4.
Adrenal cortices presented a minimal diffuse hypertrophy in 2/5 animals of group 3 and in the majority of males and females from group 4. Minimal to slight atrophy of thymus occurred in all males and females of group 4. Both findings were considered to be possibly consequent to stress and/or decreased body weights.
After the 4-week recovery period, the findings in lung, adrenal glands (males only), and male reproductive organs were still present, but mostly in a decreased incidence and/or severity. All other microscopic findings noted in various organs and in all groups examined were considered to be incidental in nature since their morphology, severity, and incidence did not distinguish treated rats from controls.


ENZYMATIC ASSAY
In the additional in vitro analysis, constitutive rat 5’-deiodinase activity in the absence of the test item was found to be 2.578% deiodination/ng protein/min. The test substance clearly inhibited 5’-deiodinase activity in isolated rat liver microsomes, in a concentration-dependent manner. A half maximal inhibitory concentration (IC50) of ca. 5 µM could be calculated for the test item, whereas with 4 µM PTU about 50% of the activity was inhibited.
Human liver microsomes showed ca. 5 times lower constitutive 5’-deiodinase activity than rat liver microsomes (i.e., 0.348% deiodination/ng protein/min). Due to the low activity in human microsomes and the concomitantly variations of individual measurements, a calculation of IC50 could not be performed. However, only a slight inhibition of the deiodinase activity by the test item could be estimated.
Therefore, the test substance was suggested to be an inhibitor of 5’-deiodinase activity in rat liver microsomes whereas in human liver microsomes only a slight inhibition of 5’-deiodinase activity was observed.

Effect levels

open allclose all

Target system / organ toxicity

Any other information on results incl. tables

Table 2: Body weight and body weight gain after 4 weeks of treatment and 4 weeks of recovery

Gender

After 4 weeks of treatment

After 4 weeks of recovery

Males

Females

Males

Females

Group

1

2

3

4

1

2

3

4

1

4

1

4

Body weight relative to control

-

-5.8%

-15.5%*

-30.7%*

-

+0.3%

-13.5%*

-14.2%*

-

-12.9%*

-

-2.5%

Body weight gain

+30.9%

+21.6%*

+3.9%*

-12.1%*

+12.0%

+9.3%

-2.0%*

-6.8%*

+15.3%

+45.1%*

+4.9%

+24.8%*

* = statistically significant

 

Table 3: Summary of significant haematology data after 4 weeks of treatment and 4 weeks of recovery

Gender

After 4 weeks of treatment

After 4 weeks of recovery

Males

Females

Males

Females

Group

1

2

3

4

1

2

3

4

1

4

1

4

RBC (T/L)

8.65

8.17

7.62*

7.58*

8.01

7.45*

7.30*

7.29*

8.95

8.45

8.03

8.01

HB (mmol/L)

9.4

9.2

8.7*

8.2*

9.3

8.8*

8.6*

8.5*

9.7

9.4*

9.5

9.1*

HCT (rel.)

0.42

0.40

0.38*

0.36*

0.41

0.39*

0.39*

0.38*

0.43

0.42*

0.42

0.40

Coagulation - PT (rel.)

0.75

0.70

0.67*

0.72

0.78

0.71*

0.70

0.74

0.80

0.80

0.80

0.79

HDW (mmol/L)

2.10

1.93

1.97

2.11

1.82

1.70

1.77

1.92

2.18

1.75*

1.69

1.71

RETI - Abs (g/L)/Rel.

178/0.21

245*/0.030

267*/0.035*

303*/0.041*

210/0.026

215/0.029

273/0.037*

466*/0.064*

190/0.021

234/0.028

193/0.024

172/0.021

WBC (g/L)

7.62

6.72

6.60

6.10

5.72

4.59

5.38

5.00

7.79

5.37*

4.42

4.41

Neut - Abs (g/L)/Rel.

1.12/0.144

0.98/0.152

0.69*/0.107

0.82/0.134

0.89/0.159

0.62/0.134

0.59/0.108*

0.93/0.183

1.45/0.184

1.04/0.218

0.58/0.129

0.86/0.192

Baso - Abs (g/L)/Rel.

0.03/0.003

0.03/0.004

0.02/0.003

0.02/0.003

0.02/0.003

0.02/0.004

0.02/0.004

0.02/0.003

0.03/0.004

0.01*/0.002

0.02/0.005

0.02/0.004

Lymph - Abs (g/L)/Rel.

6.25/0.822

5.49/0.812

5.68/0.860

5.05/0.828

4.60/0.801

3.83/0.834

4.58/0.851*

3.75/0.749

5.98/0.770

4.11*/0.740

3.65/0.828

3.35/0.762

Mono - Abs (g/L)/Rel.

0.10/0.014

0.10/0.015

0.10/0.015

0.11/0.019

0.09/0.015

0.05/0.011

0.10/0.018

0.20*/0.041

0.18/0.024

0.11*/0.020

0.08/0.018

0.09/0.020

* = statistically significant; rel. = relative

 

Table 4: Summary of significant biochemistry data after 4 weeks of treatment and 4 weeks of recovery

Gender	After 4 weeks of treatment								After 4 weeks of recovery
	Males				Females				Males		Females
Group	1	2	3	4	1	2	3	4	1	4	1	4
Glucose (mmol/L)	6.91	7.33	8.99*	6.30	5.91	6.81	8.06*	7.38	6.02	5.52	5.74	5.80
Urea (mmol/L)	6.30	4.90*	5.80	6.33	7.12	6.09	5.82*	6.40	5.83	6.48	8.91	7.35
Creatinine (µmol/L)	24.4	24.9	25.9	26.4	28.7	25.6*	25.7	22.8*	24.8	26.3	34.0	29.7
Cholesterol (mmol/L)	1.49	0.44*	0.40*	1.13	1.59	0.62*	0.97	1.34	1.59	1.74	1.35	1.47
Triglycerides (mmol/L)	0.38	0.79	0.64	0.72	0.32	0.33	0.39	1.29*	0.97	0.46	0.49	0.47
ASAT (U/L)	70.8	61.7	61.3	60.1*	62.3	55.0	51.0	60.0	68.1	74.6	63.6	57.6
LDH (U/L)	130.6	121.4	128.3	212.7*	149.4	87.8	152.6	201.3	122.2	128.0	122.0	129.2
ALP (U/L)	96.7	91.4	88.3	103.8	34.7	41.5	45.3	64.4*	79.6	68.7	23.2	28.3
CK (U/L)	152.7	123.8	99.8*	129.2	126.4	82.4*	90.5	120.9	126.2	141.3	118.9	146.0
Sodium (mmol/L)	143.2	143.1	144.6	144.2	144.6	145.0	144.7	142.9*	142.9	143.9	142.6	142.6
Potassium (mmol/L)	3.58	3.40	3.63	3.56	3.19	3.27	3.69*	3.57	3.46	3.31	2.92	3.06
Chloride (mmol/L)	102.8	103.9	104.6*	103.8	105.1	105.3	105.2	101.5*	102.1	103.1	103.2	104.1
Calcium (mmol/L)	2.61	2.55	2.56	2.72*	2.69	2.69	2.65	2.87*	2.65	2.60	2.72	2.63*
Phosphorus (mmol/L)	2.22	1.97*	1.97*	2.07	1.67	1.53	1.61	1.98*	1.93	2.13*	1.31	1.59*
Protein (g/L)	61.94	62.30	62.24	71.23*	70.38	73.11	68.84	75.27*	66.45	62.68	74.10	68.71*
Albumin (g/L)	39.30	37.75	36.44*	42.35*	48.87	49.43	42.34*	47.21	41.31	38.77	50.57	45.24*
Globulin (g/L)	22.64	24.55*	25.80*	28.88*	21.51	23.68	26.50*	28.05*	25.14	23.92	23.53	23.47
Albumin/globulin ratio	1.74	1.54	1.42	1.47	2.27	2.10	1.60*	1.69*	1.65	1.63	2.17	1.97
Inhibin B (pg/mL)	179	143	54*	89*	179	143	54*	89*	-	184	-	184
T3	108.9	99.0	90.8	57.5*	101.4	110.9	104.9	63.1*	-	-	-	-
T4	6.6	10.2*	9.9*	7.7	3.5	6.6*	7.7*	7.0*	-	-	-	-

* = statistically significant

Applicant's summary and conclusion

Conclusions:

Based on the results of this study, a no-observed-adverse-effect-concentration (NOAEC) could not be established for the test substance. Therefore, the NOAEC of the test item was considered to be lower than 0.198 ppm.
Target organs identified in all dose groups of this 4-week rat inhalation study with the test substance were the male reproductive organs (adverse character) and the liver (adaptive nature). Furthermore, adverse effects on the thyroid hormone metabolism were observed in all dose groups.

Executive summary:

The purpose of this 4-week inhalation toxicity study was to evaluate the range of toxicity and to indicate potential target organs (if any) associated with the exposure of the test substance when administered to rats by whole-body inhalation for 6 hours/day for 5 days/week for 4 consecutive weeks. In order to assess the reversibility of any treatment-related findings, satellite groups of animals were maintained for a subsequent period of 4 weeks without treatment.

 

Groups of 5 male and 5 female Wistar rats were exposed to the test substance at target concentrations of 0.2, 0.632, 2 ppm for groups 2 to 4, respectively. The rats of group 1 served as air controls. Additional satellite groups of 5 males and 5 females were kept in groups 1 and 4 to investigate the potential for recovery. Mortality, clinical signs, body weight, food consumption, water consumption, ophthalmoscopic examinations, clinical laboratory investigations, organ weights, macroscopic and microscopic findings were recorded.

 

The mean analytical vapour concentrations of the test substance were 0.198, 0.635 and 1.99 ppm for groups 2 to 4 during phase 1 (exposure days 1 to 12), then 0.198, 0.434 and 0.78 ppm during phase 2 (exposure days 13 to 20). Due to signs of overt toxicity (body weight loss, emaciation), the vapour concentrations for groups 3 and 4 were lowered starting on day 13 of exposure. Temperature, relative humidity and oxygen concentration during exposure were considered to be suitable for this type of study.

 

There were no unscheduled deaths during the course of the study.

 

After 4 weeks of exposure, a pronounced increase in total serum T4 levels was observed in females of all dose groups and in males of groups 3 and 4. Conversely, considerably lower total serum T3 levels were observed in both genders of group 4. The pronounced increase in T4 was considered to lead to an increase in the basal metabolic rate which resulted in reduced body weight development as observed in both genders of all dose groups.

 

In tissues outside the thyroid, particularly in the liver and kidneys, T4 is converted in T3, an active metabolite, by mono-deiodination of the outer phenol ring. It was hypothesised that the substance acted as inhibitor if the (hepatic) de-iodinase leading to an accumulation of T4 and a concomitant decrease in T3. This suggested mode of action was investigated by determination of in vitro conversion of T4/T3 catalysed by rat and/or human liver microsomes in presence of the test substance. The test substance was showed in vitro to inhibit the 5’-deiodinase activity in rat liver microsomes, whereas in human liver microsomes only a slight inhibition of 5’-deiodinase activity was observed.

 

The liver was established as target organ of the test substance by the observation of hepatocellular hypertrophy, reflected by increased liver weight, in both genders of all dose groups although it was considered to be of adaptive nature.

 

Atrophy of testes, epididymis, prostate glands and seminal vesicles in males of groups 3 and 4 correlated with reduced size of those glands. For testes and epididymis, there was a considerable decrease in weight in relation to dose. These findings in male reproductive organs were still present after 4 weeks of recovery and were deemed to be of adverse character. Testicular lesions were confirmed by the significant decrease in Inhibin B levels at the 2 highest doses. Levels returned to normal after the 4 -week recovery period.

In addition, atrophy along with reduced size was also observed in seminal vesicles of males from group 2 and was deemed to be of adverse character.

 

The atrophy in male reproductive organs was considered to be induced by the changes in thyroid hormones via altered endocrine feedback-regulation of TSH/TRH. Hypertrophy of the pituitary gland was observed in one female from group 4.

  

Based on the results of this study, a no-observed-adverse-effect-concentration (NOAEC) could not be established for the test substance. Therefore, the NOAEC of the test item was considered to be lower than 0.198 ppm (0.00448 mg/L).