Disodium 4,4'-bis[6-anilino-[4-[bis(2-hydroxyethyl)amino]-1,3,5-triazin-2-yl]amino]stilbene-2,2'-disulphonate

Administrative data

Endpoint:

repeated dose toxicity: oral, other

Remarks:

OECD 422

Type of information:

experimental study

Adequacy of study:

key study

Study period:

From May 22, 2019 to February 14, 2020

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Data source

Materials and methods

GLP compliance:

yes (incl. QA statement)

Limit test:

no

Test material

Test animals

Species:

rat

Strain:

Wistar

Remarks:

SPF quality

Details on species / strain selection:

Laboratory rat has been chosen because our testing laboratory has long experience with this species and because rat is recommended according to the test guideline

Sex:

male/female

Details on test animals or test system and environmental conditions:

TEST ANIMALS
- Source: Charles River SPF breeding, supplied via VELAZ s.r.o.,
- Age at study initiation: males, females: sexually adult; males - 8 weeks on arrival, females – 10
weeks on arrival
- Fasting period before study: animals were without feed two hours before application
- Housing: SPF conditions according to internal SOP No.12
- Diet (e.g. ad libitum): maintenance pelleted diet for rats and mice - Altromin for rats/mice ad libitum
- Water (e.g. ad libitum): drinking water ad libitum
- Acclimation period: 13 days
ENVIRONMENTAL CONDITIONS
- Temperature (°C): 22  3 °C
- Humidity (%): relative humidity 30-70 %
- Photoperiod (hrs dark / hrs light): 12 hour light / 12 hour dark

Administration / exposure

Route of administration:

oral: gavage

Vehicle:

water

Remarks:

water for injection

Details on oral exposure:

PREPARATION OF DOSING SOLUTIONS:
The test item was weighed into glass beaker calibrated to 100 mL and dissolved in vehicle (aqua pro iniectione, ca 80% of total volume) in ultrasonic bath together with occasional mixing by glass rod for 10 minutes. After this the glass beaker was diluted to mark by vehicle and the application form was stirred by magnetic stirrer (400 rpm) for 10 min.
The concentrations of solution at all dose levels were adjusted to ensure the administration of 1 mL per 100 g of body weight. For each dose level concentration, the solution was prepared separately The application forms were prepared daily just before administration and covered with aluminium foil to avoid potential degradation due to light. The administration of the test item to animals was performed during one hour after preparation of application form. The stirring of solutions continued during administration.

Analytical verification of doses or concentrations:

yes

Details on analytical verification of doses or concentrations:

The stability and the homogeneity of application form were determined in CETA analytical laboratories
(Analytical Group I).
Analytical Method
Stability and homogeneity were determined by means of measuring of a peak area of the test item by a high-performance liquid chromatography based on a method developed at the test facility.
The Preparation of Application Form
The application form for analysis was prepared in the same manner as for application to animals – i.e. solution in aqua pro iniectione.
Concentration Level 10 mg/10 mL
Ca 0.10 g of the test item was weighed with wider end of glass Pasteur pipette into a 150mL glass beaker calibrated to 100 mL and the beaker was slowly replenished by the vehicle to mark. The test item was dissolved in ultrasonic bath for 5 min. The solution was stirred by magnetic stirrer at 350 rpm for 5 minutesThe beaker with test item was during dissolving and homogenisation covered by aluminium foil due to possible light unstability.
Concentration Level 1000 mg/10 mL
Ca 10.0 g of the test item was weighed with laboratory spoon into a 150mL glass beaker calibrated to 100 mL. The beaker was slowly replenished by the vehicle (ca 80% of total volume) together with occasional mixing by glass rod. The test item was dissolved in ultrasonic bath together with occasional mixing by glass rod for 10 minutes. After this the glass beaker was diluted to mark by vehicle and the application form was stirred by magnetic stirrer at 390 rpm for 10 min.
The beaker with test item was during dissolving and homogenisation covered by aluminium foil due to possible light unstability.
The Stability of the Application Form
The samples were taken from the middle of the beaker content at required time intervals (0, 30, 60, 90 and 120 minutes) for the determination of stability of both application forms. Two samples were taken at all time intervals.
Conc. level 10 mg/ 10 mL: Time interval 0 min represents for this concentration the time after 5 minutes of ultrasonication and 5 minutes of mixing by magnetic stirrer at 350 rpm.
Conc. level 1000 mg/ 10 mL: Time interval 0 min represents for this concentration the time after 10 minutes of ultrasonication together with occasional mixing with glass rod and 10 minutes of mixing by magnetic stirrer at 390 rpm.
Note: The beaker with test item was during application form preparation and homogeneity and stability measuring covered by aluminium foil due to possible light unstability of test item (information from sponsor).
The Homogeneity of the Application Form
Conc. level 10 mg/ 10 mL: The samples were taken after 5 minutes in ultrasonic bath and 5 minutes of mixing by magnetic stirrer (350 rpm) from 3 given places - the bottom, the middle and the surface of the beaker content. Two samples were taken from each place.
Conc. level 1000 mg/ 10 mL: The samples were taken after 10 minutes in ultrasonic bath together with occasional mixing with glass rod and 10 minutes of mixing by magnetic stirrer (390 rpm) from 3 given places - the bottom, the middle and the surface of the beaker content. Two samples were taken from each place.
Results of Analysis
It follows from the results of analyses (homogeneity and stability) that both application forms (10 mg and 1000 mg /10 mL) of the test item, at defined laboratory conditions (laboratory temperature, preparation of solution by defined manner) are homogenous and stable at least for 120 minutes from the finalization of application form preparation.
The beaker with test item was during dissolving, homogenisation and stability measuring covered by alluminium foil due to possible light unstability of test item.This measure was recommended for further test item application form preparation

Duration of treatment / exposure:

Parental males (totally 49 days of administration):
1st day – 14th day (pre-exposure period) → 15th day - 28th day (pre-mating period, administration) →29th day – 42nd day (mating, administration) → 43rd day – 63rd day (administration period) → 64th day (necropsy)
Satellite males (totally 49 days of administration + 14 days of observation):
1st day – 14th day (pre-exposure period) → 15th day - 63rd day (administration period) → 65th day -77th day (observation period) → 78th day (necropsy)
Parental females:
1st day – 14th day (pre-exposure period) → 15th day - 28th day (pre-mating period, administration) →29th day – 42nd day (mating, administration)→ gestation → lactation → day 12 post partum
Satellite females (totally 49 days of administration + 14 days of observation):
1st day – 14th day (pre-exposure period) → 15th day - 63rd day (administration period) → 65th day - 77th day (observation period) → 78th day (necropsy)
Non-pregnant females (without evidence of copulation):
1st day – 14th day (pre-exposure period) → 15th day - 28th day (pre-mating period, administration) →29th day – 42nd day (mating, administration) → 25 days after the end of mating period
Non-pregnant females (with evidence of copulation):
1st day – 14th day (pre-exposure period) → 15th day - 28th day (pre-mating period, administration) →29th day – 42nd day (mating, administration) → 25th day after confirmed mating

Frequency of treatment:

7 days per week at the same time (7.00 – 10.00 am)

Doses / concentrationsopen allclose all

No. of animals per sex per dose:

Each main group consisted of 12 males and 12 females; each satellite group consisted of 6 males and 6 females

Control animals:

yes, concurrent vehicle

Details on study design:

- Dose selection rationale:
Based on the result of the DRF study on the substance, the selected highest tested dose for the main study should have been 1000 mg/kg bw/day, since no significant toxicological effects have been observed at this dose and it could have been considered as limit dose. However, it should be noticed that this study has been performed not only to investigate the toxicological properties of the substance in itself, but also and mainly to compare the effects within the members of the category; therefore the highest tested dose has been selected as below reported, taking into account the existing following studies:

• 1-DSA – Subchronic toxicity study – Relevant toxicological effects on kidney at 750 mg/kg bw/day
• 1-DSA – Subchronic toxicity study – Relevant toxicological effects on testes at 750 mg/kg bw/day
• 3a-MSA – Subacute toxicity study – Effects to be confirmed on haematological parameters, liver and kidney starting from 200 mg/Kg bw/day
• 3a-MSA – Two generation toxicity study - Relevant toxicological effects mainly in terms of maternal toxicity at 1000 mg/kg bw/day and minor effects at 300 mg/kg bw/day

Indeed, in this respect all systemic studies concerning repeated dose, reproductive and developmental toxicity (OECD 422, 408 and 414) have been set on similar dose level in order to be able to compare all members of the category on the specific organ effects.
The lowest and the medium doses have been selected in order to have a coherent spacing of doses respect to the highest selected one, also taking into account all the available data on the repeated dose toxicity ( 3a-MSA, 1-DSA).

- Rationale for animal assignment (if not random): random selection according to the internal rule – at the beginning of the study the weight variation of animals in groups of each sex should not exceed ± 20% of the mean weight
- Fasting period before blood sampling for clinical biochemistry: the animals were fasted approximately for 18 hours before blood collection but they were supplied drinking water ad libitum.

Examinations

Observations and examinations performed and frequency:

Health condition control: daily - during the acclimatisation and the experimental part
Body weight: males and satellite animals - the first day of administration and then weekly,
females - the first day of administration and then weekly,
during pregnancy: 0., 7th, 14th, 20th day,
during lactation: 1st, 4th day, 12th day and 13th day
Food consumption: weekly and on the same days as body weight (except the mating period)
satellite males and females – weekly
Water consumption: satellite males and females – twice a week
Clinical observations: males and females - daily during the administration period
Mortality control: twice daily
Detailed clinical observation: before the first application and then weekly (except the mating period)
Functional observation: at the end of administration/observation period
Laboratory examinations:
- vaginal smears: daily – 1st – 14th day of study
daily in mating period (max. 14 days)
on necropsy day
- urinalysis: the last day of administration/observation period – only males
- haematology: males – after the end of application period
parental females – on the 13th day of lactation
satellite animals – after the end of observation period
- biochemistry: males and nonpregnant females – after the end of application period
parental females – on the 13th day of lactation
satellite animals – after the end of observation period
- pathological examination: males and nonpregnant females – after the end of application period
satellite animals – after the end of observation period
- weight of organs: during necropsy
- sperm observation: parental males – during and after necropsy (not performed in satellite males)
- histopathological examination: after necropsy
Sacrifice and pathology
Organs for histopathological examination in all males and females:
Pituitary gland
Adrenal glands
Ovaries
Aorta
Uterus incl. cervix of uterus
Brain (incl. cerebellum and med. oblongata)
Vagina Caecum
Epididymis/Epididymides
Colon
Prostate gland + Seminal vesicles
Duodenum
Testes
Pancreas
Rectum
All gross lesions
Salivary glands
Thyroid gland
Sciatic nerve
Skeletal muscle
Skin
Spinal cord – thoracic
Spleen
Stomach
Thymus
Trachea
Urinary bladder
Female mammary gland area
Femur
Heart
Ileum
Jejunum
Kidneys
Liver
Lungs
Lymph nodes – mesenteric, paraaortal
Oesophagus

Sacrifice and pathology:

Organs for histopathological examination in all males and females:
Pituitary gland
Adrenal glands
Ovaries
Aorta
Uterus incl. cervix of uterus
Brain (incl. cerebellum and med. oblongata)
Vagina Caecum
Epididymis/Epididymides
Colon
Prostate gland + Seminal vesicles
Duodenum
Testes
Pancreas
Rectum
All gross lesions
Salivary glands
Thyroid gland
Sciatic nerve
Skeletal muscle
Skin
Spinal cord – thoracic
Spleen
Stomach
Thymus
Trachea
Urinary bladder
Female mammary gland area
Femur
Heart
Ileum
Jejunum
Kidneys
Liver
Lungs
Lymph nodes – mesenteric, paraaortal
Oesophagus

Statistics:

Males/females from control group were compared with males/females from three treated groups. Satellite males/females from control group were compared with satellite males/females from treated group.
In general:
The parametric tests were used for statistical evaluation of
• body weight of males and females
• mean pup weight
• litter weight
• anogenital distance of pups
• selected haematology parameters
• blood biochemistry parameters
• data from urinalysis (pH, volume)
• data from biometry of organs
As the first step the test for normality (Shapiro-Wilk test) was used. If the data were not normally distributed than the transformation of data was performed (Box-Cox transformation). If still the normal distributed distribution was not achieved than non-parametric tests (Kruskal-Wallis Test, Mann-Whitney test) were used.
For normally distributed data have at first the variance check has been performed (Levene´s test) to verify if standard deviations within each group are equal.One-Way ANOVA (probability level p ≤ 0.05) was used to detect whether there are any significant differences amongst the means. In case of significant differences, the post hoc statistical testing was performed (Fisher's least significant difference - LSD test).
The non-parametric tests were used for statistical evaluation of
• selected reproduction parameters with non-continuous distribution (number of live born pups, number of pups, number of implantations)
• selected haematology parameters with non-continuous distribution (total erythrocyte count, total leucocyte count, total platelet count)
The Kruskal-Wallis test was used for the comparison of the measured effect in all treatment groups with the vehicle control group (as global test) and the two-groups Mann-Whitney test (probability level p ≤ 0.05).

Results and discussion

Results of examinations

Clinical signs:

no effects observed

Description (incidence and severity):

The clinical observation results were noted for all 12 animals per group and satellite animals.
Males
No clinical changes were recorded in control or treated males during the application period.
Satellite males
No clinical changes were recorded in satellite control or satellite treated males during the application
period.
Females
In all control and treated females no clinical changes were recorded during the entire study.
Satellite females
No clinical changes were recorded in satellite control or satellite treated females during the application
period.

Health Condition Control
The health condition control results were noted for all 12 animals per group and satellite animals. The males and females were not distributed into groups during the check-in, acclimatisation and the pre-exposure period with monitoring of oestrous cycle in females. No signs of diseases were re
corded during that time.
Males
No signs of disease and clinical signs of intoxication were recorded during the application period in all treated males.
Satellite males
No signs of disease and clinical signs of intoxication were recorded during the application period in all treated males. During the observation period (recovery; weeks 8 and 9) no changes of health status were noted in satellite treated males.
Females
No signs of disease and clinical signs of intoxication were recorded during the application period in all treated females.
Satellite females
No signs of disease and clinical signs of intoxication were recorded during the application period in all treated males. During the observation period (recovery; weeks 8 and 9) no changes of health status were noted in satellite treated males.

Mortality:

mortality observed, non-treatment-related

Description (incidence):

Males
Male No. 46 (the dose level 250 mg/kg/day) was found dead on day 30 of application. Due to partial cannibalism, the cause of death was not established.
Females
There were no unscheduled deaths during the study.

Body weight and weight changes:

no effects observed

Description (incidence and severity):

Males
In the beginning of study, mean body weight of all groups of animals was similar. Slightly higher body weight was recorded in animals at the dose levels 80 and 250 mg/kg/day in comparison with the control group during the whole application period. Comparable body weight was recorded in animals at th
e dose level 750 mg/kg/day and control group. Statistically significant differences in necropsy body weight were not found in treated males.
Satellite males
Body weights of satellite treated males were slightly lower in comparison with the satellite control males during the whole study. Statistically significant differences in necropsy body weight were not found in satellite treated males.
Females
Different body weight on the 1st day of administration was caused by sequential inclusion of animal groups to the study. Before the mating period, body weights of females in all treated groups was similar to the control group. During the pregnancy and lactation periods, body weights of treated females in all groups was comparable with the control females. Statistically significant differences in necropsy body weight were not found in treated females.
Satellite females
Body weight of satellite treated females was comparable with satellite control animals for the entire application and recovery periods. Statistically significant differences in necropsy body weight were not found in satellite treated females.

Mean Body Weight Increment
Males
Weight increments of treated males were not adversely influenced by the test item treatment.
Satellite males
Weight increments of satellite treated males in application and recovery period were variable and not adversely influenced by the test item administration.
Females
Weight increments in treated females were variable in comparison with the control females and not affected by the test item treatment.
Satellite females
Weight increments in treated females were variable and not affected by the test item treatment.
Pregnancy
Mean body weight of all treated groups was similar with controls. Weight increments of treated females was comparable with the control females
Lactation
Only mothers (females with live pups born) were included in the evaluation of body weight increment s during lactation period. Mean body weight of females at the dose level 750 mg/kg/day was insignificantly decreased on day 4 and 12 of lactation in comparison with the control females.
Weight increments of treated mothers at tall dose levels were lower at the end of lactation period in comparison with the control females.

Food consumption and compound intake (if feeding study):

no effects observed

Description (incidence and severity):

Males
The food consumption of treated males was similar or slightly higher in comparison with the control males during the whole application period of study.
Satellite males
The food consumption of satellite treated males was comparable to the control group during application period and slightly lower during the recovery period (8th – 9th week).
Females
During the pre-mating period, pregnancy and lactation period the food consumption of treated females was similar with the control females.
Satellite females
The food consumption of satellite treated females was similar or slightly higher in comparison with the control group during the entire application and recovery periods.

Description (incidence and severity):

Males
The food conversion of treated males was comparable with the control males in the pre-mating period and not negatively influenced by the test item treatment.During the period after mating, the food conversion of males in the treated group was similar with the control group of males (except the conversion at the dose level 250 mg/kg/day at the 6th week of study).
Satellite males
The food conversion of satellite treated males was quite similar to the satellite control (exc. the 9th and the 9th week of study).
Females
The food conversion of treated females in the pre-mating period was variable but not adversely influenced by the test item treatment.
During the pregnancy period, the food conversion of treated females was similar with the control group.
During the lactation period, the food conversion of treated females at all dose levels was decreased in comparison with the control females.
Satellite females
The food conversion of satellite treated females was variable compared to satellite control females, but not adversely influenced by the test item treatment.

Description (incidence and severity):

Satellite males
The water consumption of satellite treated males was lower compared to the satellite control group during the entire application and recovery period.
Satellite females
The water consumption of satellite treated females was higher compared to the satellite control group during the entire application and recovery period.

Description (incidence and severity):

Males
The value of the total leucocyte count was not affected by the test item treatment. The five-population differential of white blood cells were not affected by the test item treatment. The count of lymphocytes, monocytes, neutrophils, eosinophils and basophiles were similar in treated group of males and control group of males.
The red blood components were changed mainly in males at the dose level 80 mg/kg /day. An increase in the total value of erythrocytes (RBC) (p ≤ 0.05) was detected. This increase is related to the increased concentration of haemoglobin (p ≤ 0.05, out of historical control range) and value of haematocrit (p ≤ 0.05). There was an increase in the percentage value of reticulocytes in males at the dose level 750 mg/kg – even out of historical control range, but not statistically significant. The values of haemocoagulation parameters were not significantly affected by the test item treatment.
Values over the historical range (HGB concentration in the lowest dose level and reticulocytes in the highest dose level) were isolated values very close to the upper limit, without dose-dependent and biological significance. These findings were reversible (not observed in satellite animals).
Satellite males
The APTT value recorded in satellite treated males was statistically significantly decreased in comparison with the satellite control group of males. Other values were similar with satellite control males. All values were in a range of historical control.
Females
The value of the total leucocyte count was not affected by the test item treatment. The five-population differential of white blood cells were not affected by the test item treatment except the value of monocytes. The percentage value of monocytes was significantly decreased (p ≤ 0.05) in females at the
dose level 750 mg/kg /day compared to control females.
The red blood components in treated females were not changed in comparison with the control females except significantly increased value of MCV (p ≤ 0.05) at the dose level 250 mg/kg/day.
Haematocoagulation parameter were not affected by the test item treatment.
The value over the historical range (MCV in the middle dose level) was isolated value close to the upper limit without dose dependence.
Satellite females
A decreased value of RBC (p ≤ 0.05) and associated increased value of MCV (p ≤ 0.05) were recorded in satellite treated females in comparison with the satellite control females. Decreased value of neutrophils (p ≤ 0.05) was also recorded in satellite treated females.
Other values were similar with satellite control females and in a range of historical control.

Description (incidence and severity):

Males
Significantly changed values (p ≤ 0.05) of T-Pro (increased), Crea (decreased, under the historical control range), T-Bil (decreased), Na (increased) and Cl (increased) were detected in males at the dose level 750 mg/kg/day compared to control animals. The changed values (p ≤ 0.05) of T-Bil (decreased) and Na (increased) were also recorded in males at the dose level 250 mg/kg/day. In male s at the dose level 80 mg/kg/day was detected changed values (p ≤ 0.05) of T-Bil (decreased) and Cl (increased).
The value altered at all dose levels (statistically significantly) was bilirubin (T-Bil) - decreased at all treated levels compared to control animals.
The value of creatinine recorded under the historical control range was very close to the lower limit, without dose dependency and reversible change (not observed in satellite animals)
Values of other biochemical parameters of treated males were in a historical control range and not significantly altered in comparison with the controls.
Satellite males
A statistically significant increased value of bile acid (BA) only was recorded in satellite treated males in comparison with the satellite control males. Values of other biochemical parameters of satellite treated males were similar to the satellite control group.
Females
Significantly changed biochemical values were recorded only sporadically in treated females in comparison with the control females.
Significantly (p ≤ 0.05, over the historical control range) increased value of TG only was reported in females at the dose level 750 mg/kg/day. Significantly (p ≤ 0.05) decreased value of GLU was recorded in females at the dose level 80 mg/kg/day only.
The value of triglyceride recorded over the historical control range was very close to the upper limit, without dose dependency and reversible change (not observed in satellite animals). Values of other biochemical parameters of treated females were comparable to the control group.
Satellite females
Statistically significantly (p ≤ 0.05) increased values of Ca and BA were noted in satellite treated females in comparison with the satellite control females. Values of other biochemical parameters of treated satellite females were in a historical control range and comparable to the control group.

Description (incidence and severity):

Urinalysis was performed only in males (six of each group) during the last week of the study. Statistical evaluation was performed for pH and volume of urine.
Males
A statistically significantly increased pH of urine was detected in males at the dose level 750 mg/kg/day. The volume of urine was insignificantly decreased in males at the dose level 750 mg/kg/day. The presence of proteins was recorded in treated males as well as in control males. The presence of blood and leucocytes were recorded in males at the dose levels 80 and 250 mg/kg/day.
Satellite males
The presence of leucocytes was recorded in satellite treated males as well as in satellite control males.

Behaviour (functional findings):

no effects observed

Description (incidence and severity):

Males
Reactions to touch, noise, pain and pupillary reflex of treated males were the same as in the control group. The number of upstanding in treated males was comparable to the control. Emiction and defecation in treated males was similar with the control males. The values of grip strength of pectoral legs
and pelvic legs did not show any significant differences between control and treated males.
Satellite males
No significant differences were detected in examined parameters.
Females
Reactions to touch, noise, pain and pupillary reflex of treated females were the same as in the control females. The number of upstanding in treated females was similar with the control females. The values of grip strength of pectoral and pelvic legs were without significant differences between control and treated females.
Satellite females
No significant differences were detected in examined parameters.

Description (incidence and severity):

Males
Statistically significantly increased absolute weight of adrenal glands was recorded in males at the dose levels 80 and 750 mg/kg/day in comparison with the control males. Absolute weights of other organs were in dosed males comparable with the control males.
Satellite males
A statistically significantly changed absolute weight of organs were not recorded in dosed males in comparison with the satellite control males. Absolute weights of organs at dosed group of males was similar with the control males.
Females
Statistically significantly decreased absolute weight of pituitary gland was recorded in females at the dose level 750 mg/kg/day in comparison with the control females. An insignificant decrease in the weight of the thyroid gland was recorded in females at the dose level 750 mg/kg/day in comparison with
the control group of females. Absolute weights of other organs were in dosed females comparable with the control females.
Satellite females
Statistically significant differences were recorded in the absolute weight of kidneys in satellite females. Absolute weight of kidneys was increased in treated females in comparison with the control females.

Relative Organ Weight
Males
The relative weights of the adrenal glands and epididymis were statistically significantly increased in males at the dose level 750 mg/kg /day in comparison with the control males. The relative weight of the adrenal glands was insignificantly increased also in males at the dose levels 80 and 250 mg/kg/day.
Satellite males
A statistically significant increase in the relative weight of epididymis was detected in satellite treated males.
Females
A statistically significantly changed relative weight of organs were not recorded in dosed females in comparison with the control females. Insignificantly decreased relative weight of pituitary gland was recorded in females at the dose level 750 mg/kg/day.
Satellite females
No statistically significant differences were recorded in satellite treated females

Gross pathological findings:

no effects observed

Description (incidence and severity):

Males
Control: no macroscopic findings were recorded in all 6 males.
80 mg/kg /day: no macroscopic findings were recorded in all 6 males.
250 mg/kg /day: no macroscopic findings were recorded in 5 males (one male died during the study – partial cannibalism was observed, the cause of death could not be determined).
750 mg/kg /day: no macroscopic findings were recorded in all 6 males.
Satellite males
Control satellite: no macroscopic findings were recorded in all 6 males.
120 mg/kg /day satellite: no macroscopic findings were recorded in all 6 males.
Females
Control: no macroscopic findings were recorded in all 6 females.
80 mg/kg /day: no macroscopic findings were recorded in all 6 females.
250 mg/kg /day: no macroscopic findings were recorded in all 6 females.
750 mg/kg /day: no macroscopic findings were recorded in all 6 females.
Satellite females
Control satellite: no macroscopic pathological findings were recorded in all 6 females (dilatation of uterus – non-pathological finding was recorded in two of six females).
750 mg/kg /day satellite: no macroscopic pathological findings were recorded in all 6 females (dilatation of uterus – non-pathological finding was recorded in two of six females).

Description (incidence and severity):

Full histopathology of the preserved organs and tissues was performed for high dose and control animals and satellite animals.
Histopathological examination of the preserved organs and tissues was performed for males Nos. 1-6 and the first six mothers that delivered pups in the repeated dose toxicity part of the study.
Because no treatment related histological findings were recorded in animals at the highest dose level (750 mg/kg/day), histological examination of organs was not performed for the animals from the dose level 80 and 250 mg/kg/day.
The incidence of affected males is expressed in numeric form and ranged in sequence of dose levels 0-750 mg/kg /day and 0S-750S in satellite groups.
Males
For examination of the repeated toxicity of the test item, the full histopathology was performed for the first six males of control (No 1-6) and high dose (No 61-66).
Only sporadic findings were recorded in the control group of males as well as in dosed group of males.
Hydronephrosis in kidneys was detected in 1-0 males. Focal chronic inflammation in liver was recorded in 0-1 male, slight focal chronic inflammation of prostate gland in 1-1 male and extramedullary hemopoiesis in spleen in 0-1 male.
The incidence of other microscopical findings was very sporadic.
No treatment-related changes were found in male genital tract.
Satellite males
The satellite animals (control - No. 81-86 and high dosed – No.91-96) as a part of the repeated dose toxicity study were histopathologically examined. The full histopathology was performed. Only sporadic findings were recorded. Hydronephrosis in kidneys in 1-1 males, extramedullary hemopoiesis in spleen in 1-2 male, tubular atrophy in testes in 0-1 male were recorded. The incidence of other microscopical findings was very sporadic and these findings are mentioned in individual tables.
Test item orally administered to male rats in the dose of 750 mg/kg/day did not cause any pathological changes in the male genital tract organs, in the pituitary gland, did not cause gross or histopathological changes in the kidneys of rats indicative of a toxic effect and did not cause gross or histopa
thological changes in the gastrointestinal tract.
Females
For examination of the repeated toxicity of the test item, the full histopathology was performed for the first six females delivered pups from control (Nos. 103,104,105,106,107,108) and high dose group (Nos. 161,165,166,167,168,169).
In one female from the dose level 250 mg/kg/day (No.150) was examined uterus (macroscopical finding – dilatation). Marked hydrometra was detected.
The incidence of affected females is expressed in numeric form and ranged in sequence of dose levels 0-750 mg/kg /day and 0S-750S in satellite groups.
Only sporadic findings were recorded in the control group of females as well as in dosed group of females. Hydronephrosis in kidneys was detected in 1-3 females. The changes related to pregnancy were found in both control and high treated females: accumulation of siderophages in mesometrium of uterus in 6-6 females, hemosiderin in mucosa in 6-6 females and lobular hyperplasia of mammary gland in 6-6 females. The incidence of other microscopical findings was very sporadic and these findings are mentioned in individual tables
Satellite females
The satellite animals (control - No. 181-186 and high dosed – No.191-196) as a part of the repeated dose toxicity study were also histopathologically examined. The full histopathology was performed. Hyaline casts in kidneys in 0-1 female and hydropherosis in kidneys in 0-1 female were detected.
Hydrometra of iterus was observed in 2-3 females. The incidence of other microscopical findings was very sporadic and these findings are mentioned in individual tables.

Histopathological findings: neoplastic:

no effects observed

Description (incidence and severity):

Neoplastic tissues were not observed during the histopathology

Other effects:

no effects observed

Description (incidence and severity):

Biochemical Examination – Thyroid hormones
Blood (serum) samples from all adult parental males were assessed for thyroid hormones thyroxine
(T4 total) and rat thyroid stimulating hormone (TSH). Mean concentrations of T4 and TSH hormones at all dosed groups were not significantly changed in
comparison with the control group of males.

Effect levels

Target system / organ toxicity

Any other information on results incl. tables

Results of main study

	doses (mg/kg bw/day)				satellite - dose (mg/kg day) - 6 M + 6 F		notes
	0	80	250	750	0	750
Repeated-dose part - first six males and six mothers who delivered pups/group + satellite
Body Weight M (group mean ± standard deviation (g))	477.93 ± 40.48	492.99 ± 43.33	488.60 ± 40.12	471.01 ± 28.54	513.20 ± 26.37	494.61 ± 80.65	Necropsy body weight
Body Weight F (group mean ± standard deviation (g))	323.27 ± 18.58	326.88 ± 23.51	328.92 ± 23.40	323.06 ± 30.79	291.46 ± 21.74	299.94 ± 15.52	Necropsy body weight
Body Weight Gain	No effects	No effects	No effects	No effects	No effects	No effects
Food Consumption M (group mean (grams/animal/day)	28.48	31.34	32.06	30.21	27.91	24.68	at 7th for males and 9th week for satellite males
Food Consumption F (group mean (grams/animal/day))	69.04	63.64	69.51	67.34	18.80	20.63	at 12th lactation day for females and 9th week for satellite females
Food Conversion M (group mean (%))	7.04	5.42	5.23	9.32	6.02	0	at 7th for males and 9th week for satellite males
Food Conversion F (group mean (%))	0.17	0	0	0	0	7.95	at 12th lactation day for females and 9th week for satellite females
Water Consumption M (group mean (mL/animal/day))	-	-	-	-	32.38	25.48	at 9th week
Water Consumption F (group mean (mL/animal/day))	-	-	-	-	36.90	50.71	at 9th week
Mortality	0	0	one male found dead  on day 30 of application	0	0	0	Due to partial cannibalism, the cause of death was not established.
Signs of toxicity M+F	No signs of disease and clinical signs of intoxication	No signs of disease and clinical signs of intoxication	No signs of disease and clinical signs of intoxication	No signs of disease and clinical signs of intoxication	No signs of disease and clinical signs of intoxication	No signs of disease and clinical signs of intoxication	at 7th or 9th week
Nature, severity and duration of clinical observations (whether reversible or not)	No clinical changes	No clinical changes	No clinical changes	No clinical changes	No clinical changes	No clinical changes	at 7th or 9th week
Functional observations	No effects	No effects	No effects	No effects	No effects	No effects
Results of ophthalmological examination	Not examined	Not examined	Not examined	Not examined	Not examined	Not examined
Haematological tests with relevant baseline values	No effects	(M): Significantly changed values of red blood components	(F): Statistically significantly increase of MCV	(F): significantly decrease of monocytes	No effects	(M): APTT was statistically significantly decrease of APTT (F): Statistically significantly decreased value of RBC associated with increased value of MCV	Haematological examination of treated animals showed only sporadic differences in haematological values in treated animals compared to control animals. Haematological examination of males did not reveal statistically significant differences in haematological values in comparison with the control animals. In satellite treated males, only the value of APTT was statistically significantly decreased in comparison with the control satellite animals. Haematological examination of females at the highest dose level did not reveal statistically significant differences in haematological values in comparison with the control animals except the value of monocytes
white blood components (% WBC)	(M) Monocytes: 5.32 Neutrophils: 22.46 Reticulocytes: 22.43 (F) Monocytes: 6.02 Neutrophils: 51.52 Reticulocytes: 3.13	(M) Monocytes: 9.07 Neutrophils: 17.91 Reticulocytes: 2.93 (F) Monocytes: 5.29 Neutrophils: 51.59 Reticulocytes: 3.52	(M) Monocytes: 6.45 Neutrophils: 21.48 Reticulocytes: 2.70 (F) Monocytes: 3.64 Neutrophils: 53.83 Reticulocytes: 3.83	(M) Monocytes: 5.39 Neutrophils:18.03 Reticulocytes: 3.70* (F) Monocytes: 2.56 Neutrophils: 68.55 Reticulocytes: 3.63	(M) Monocytes:6.21 Neutrophils: 18.48 Reticulocytes:2.47 (F) Monocytes: 5.59 Neutrophils: 14.74 Reticulocytes: 2.37	(M) Monocytes:8.22 Neutrophils: 24.87 Reticulocytes: 2.10 (F) Monocytes: 4.93 Neutrophils: 10.78 Reticulocytes: 2.53
red blood components	(M) RBC:7.43 HGB: 14.83 HCT: 38.13 MCV:51.47 APTT: 16.80 (F) RBC: 6.64 HGB:14.35 HCT: 37.55 MCV: 56.68 APTT: 18.70	(M) RBC: 7.94* HGB: 16.05* HCT: 42.53* MCV:53.67 APTT: 18.20 (F) RBC: 6.43 HGB: 14.98 HCT: 37.78 MCV: 59.05 APTT: 18.72	(M) RBC: 7.79 HGB:15.54 HCT: 39.98 MCV: 51.42 APTT: 16.16 (F) RBC: 6.20 HGB: 14.87 HCT: 37.80 MCV: 61.05* APTT: 19.65	(M) RBC: 7.34 HGB: 14.85 HCT: 38.08 MCV: 51.98 APTT: 17.85 (F) RBC: 6.44 HGB: 15.05 HCT: 38.68 MCV: 60.30 APTT: 18.47	(M) RBC: 7.56 HGB: 14.12 HCT: 38,32 MCV: 51.08 APTT: 17.28 (F) RBC: 7.29 HGB:14.07 HCT: 38.08 MCV: 52.27 APTT: 17.27	(M) RBC: 7.89 Hgb: 14.30 HCT: 39.32 MCV: 49.92 APTT: 15.78* (F) RBC: 6.61* HGB: 13.62 HCT: 35.68 MCV: 54.10* APTT: 17.05
Urinalysis M	No effects	presence of blood and leucocytes	presence of blood and leucocytes	Increased pH of urine. Insignificantly decreased volume of urine. Presence of proteins recorded.	Presence of leucytes	Presence of leucytes	Presence of proteins, blood and leukocytes were recorded in treated males as well as in control males. These findings were not associated with the application of the test item.
Clinical biochemistry tests with relevant baseline values	No effects	(M): decrease of Total Bilirubin and increase of Chloride ions (F): decreased value of Glucose	(M): decrease of Total Bilirubin and increase of Natrium ions	(M) decreased Creatinine, Total Bilirubin; increased Total Protein, Natrium ions and Chloride ions. (F): increase of Triglycerides	No effects	(M): increased value of bile acid (BA) (F): increased values of Calcium ions and Bile acids	Biochemical examination of males, statistically significantly changed values (compared to control) were detected. During the biochemical examination of females, significantly changed biochemical values were recorded only sporadically in treated females.
T-Pro (g/L)	M: 70.24 F: 62.88	M: 70.36 F: 61.09	M: 70.85 F: 62.24	M: 61.69* F: 60.41	M: 68.95 F: 75.50	M: 68.14 F: 78.48
TG (mmol/L)	M: 0.80 F: 0.90	M: 0.97 F: 1.05	M: 1.35 F: 0.99	M: 0.82 F: 1.92*	M: 0.75 F: 1.21	M: 0.95 F: 1.35
Creatinine (μmol/L)	M: 30.80 F: 42.23	M: 32.20 F: 44.73	M: 30.54 F: 40.65	M: 25.77* F: 42.18	M: 32.32 F: 38.53	M: 31.75 F: 33.58
GLU (mmol/L)	M: 7.31 F: 5.38	M: 6.86 F: 4.40*	M: 6.65 F: 5.78	M: 6.63 F: 5.62	M: 7.81 F: 6.96	M: 7.36 F: 7.13
Ca (mmol/L)	F 2.54	F 2.53	F 2.55	F 2.49	F: 2.84	F: 2.93*
BA (μmol/L)	M: 61.33 F: 126.47	M: 32.21 F: 110.01	M: 35.83 F: 101:12	M: 36.71 F: 95.06	M: 17.25 F: 19.09	M:30.87* F: 60.55*
T-Bil (μmol/L)	M: 2.85 F: 2.64	M: 2.19* F: 2.61	M:2.22* F: 2.88	M: 2.12* F: 2.46	M: 2.15 F: 3.62	M: 2.11 F: 3.07	(T-Bil) - decreased at all treated levels compared to control animals.
Sodium (mmol/L)	M: 136.83 F: 132.67	M: 138.33 F: 132.83	M: 139.20* F: 133.67	M: 140.17* F: 134.00	M: 137.67 F: 137.50	M: 138.50 F: 138.17
Chloride (mmol/L)	M: 100.67 F: 95.33	M: 103.00* F:95.17	M: 102.20 F: 95	M: 104.17* F: 94.17	M: 101.00 F: 111101.83	M: 99.50 F: 102.17
Organ weights	No effects	Statistically significantly increased absolute weight of adrenal glands	Statistically significantly increased absolute weight of adrenal glands	(M): Statistically significantly increased absolute weight of adrenal glands (F): Statistically significantly decreased absolute weight of pituitary gland	No effects	(F): Statistically significant differences were recorded in the absolute weight of kidneys	Biometry of organs of treated animals showed sporadic significant changes in absolute and relative weight of organs. The weight of adrenal gland (absolute and relative) was significantly increased in all dose groups of males. Increase of relative weight of epididymis was recorded in males. In females, significant decrease of the absolute weight of pituitary gland was observed. Statistically significantly increased of absolute weight of kidneys was reported in satellite females.
adrenal glands	(M) 0.0653± 0.0096	(M) 0.0786± 0.0099*	(M) 0.0778± 0.0089	(M) 0.0912± 0.0112*	(M) 0.0761± 0.0075	(M) 0.0793± 0.0067
kidneys	(F) 2.0725± 0.1683	(F) 2.1054±0.1407	(F) 2.2246± 0.2625	(F) 2.1533± 0.1439	(F) 1.9362±0.2789	(F) 2.2185± 0.2279*
pituitary gland	(F) 0.0165± 0.0022	(F) 0.0163±0.0007	(F) 0.0154± 0.0007	(F) 0.0142± 0.0011*	(F) 0.0157±0.0020	(F) 0.0169± 0.0004
Relative organ weight	No effects	Insignificantly increased o frelative weight of the adrenal glands	Insignificantly increased of relative weight of the adrenal glands	Statistically significantly increased relative weight of the adrenal glands and epididymis.	No effects	Statistically significant increase in the relative weight of epididymis
males - adrenal glands	0.0137±0.0020	0.0160±0.0021	0.0161±0.0029	0.0193±0.0016*	0.0149±0.0016	0.0164±0.0034
males - epididymis	0.1695±0.0105	0.1630±0.0160	0.1773±0.0156	0.1925±0.0223*	0.3265±0.0153	0.3463±0.0127*
Necropsy findings	No effects	No effects	1M died during the study– partial cannibalism was observed, the cause of death could not be determined	No effects	No effects	No effects
Histopathological findings (out of 6 animals)							Histological examination revealed only sporadic findings in treated animals as well as in control animals. Test item orally administered in the dose of 750 mg/kg/day did not cause any pathological changes in the male and female genital tract organs, in the pituitary gland, did not cause gross or histopathological changes in the kidneys of rats indicative of a toxic effect and did not cause gross or histopathological changes in the gastrointestinal tract.
Kidneys: hydronephrosis	1M/1F	Not examined	Not examined	0/3F	1	1M/1F
Liver: focal chronic inflammation	0	Not examined	Not examined	1	1F	0
Lungs: blood aspiration	3M/1F	Not examined	Not examined	4M/1F	5M/1F	6M/2F
Prostate gland: focal chron. inflammation	1	Not examined	Not examined	1	1	0
Spleen: extramedullary hemopoiesis	0	Not examined	Not examined	1M/2F	1	2
Testes: tubular atrophy	0	Not examined	Not examined	0	0	1
Trachea: blood aspiration	3	Not examined	Not examined	4M/2F	5	5
Mammary gland: lobular hyperplasia	6	Not examined	Not examined	6	0	0
Thymus: cysts	0	Not examined	Not examined	1	3	1
Uterus: focal accumulation of lipophages and siderophages in mesometrium	6	Not examined	Not examined	6	0	0
Uterus: hemosiderin in mucosa	6	Not examined	Not examined	6	0	0

Results of DRF study

	doses (mg/kg bw/day)				notes
	0	100	300	1000
For dams (per dose)
Mortality	No effects	No effects	No effects	No effects
Body Weight F [group mean ± standard deviation (g)]	440.02 ± 27.78	437.92 ± 28.66	455.82 ± 26.38	446.52 ± 34.00	at 20th day of pregnancy
Clinical signs: description, severity, time of onset and duration	No effects	No effects	No effects	No effects
Haematological findings	No effects	RBC and PLT were slightly lower	RBC and PLT were slightly lower	No effects	The haematological examination did not show significant differences among dose levels.
Number of pregnant dams	6	6	6	6
Implantations [mean ± SD]	17.33 ± 1.21	16.83 ± 2.32	16.83 ± 4.96	16.33 ± 3.78
Resorptions [mean ± SD]	0.33 ± 0.82	0.17 ± 0.41	0.17 ± 0.41	0.83 ± 0.98
Corpora lutea [mean ± SD]	17.50 ± 1.52	17.83 ± 2.04	17.17 ± 4.17	17.17 ± 2.48
For foetuses/offspring (per dose)
Total number of live foetuses	102	100	100	92
Total number of dead foetuses	0	0	0	1
External, soft tissue and skeletal malformations and other relevant alterations	No effects	No effects	No effects	Only one dead foetus in one litter in female. This foetus was fully developed, similar in size to other live fetuses at the same litter (partial autolysis was recorded).	No macroscopic changes of soft tissues and external alteration were found during the pathological examination of foetuses at all dose levels.

Applicant's summary and conclusion

Conclusions:

NOAEL for general toxicity ≥ 750 mg/kg body weight/day

Executive summary:

The test item was tested for effects on reproduction and subacute toxicity using the OECD Test Guideline No. 422.

Wistar rats (SPF quality) were used for testing. The test item was administered in the form of a solution in water for injection. Oral application by stomach tube was performed daily.The animals were without feed two hours before application and two hours after application of the test item.The main study includes four main groups (3 treated groups (doses 80, 250, 750 mg/kg/day) and one control group (vehicle only)) and two satellite groups of animals (one control group (vehicle only) and one treated group (750 mg/kg/day)). The dose levels for the study were determined on the basis of the results of dose-range finding experiments (see the Annex 2) and approved by the Sponsor. Each main group consisted of 12 males and 12 females; each satellite group consisted of 6 males and 6 females.

 

The first six males and six mothers who delivered pups per group (as per internal SOP) and a satellite groups of animals (control and treated) are part of the repeated dose toxicity study and examined with respect to toxicity of the test item. Satellite animals were used for observation of reversibility, persistence or delayed occurrence of systemic toxicity effects up to 14 days post treatment. All twelve males and females per group are a part of the reproduction study and examined with respect to reproduction parameters.

 

The treated groups were administered daily for the following periods: males and females – 2 weeks prior to the mating period and during the mating period; pregnant females – during pregnancy and up to the 12^thday of lactation; males – after mating period – 49 days in total; nonpregnant females (mated females without parturition) – for 25 days after confirmed mating; non-mated females – for 25 days after the end of the mating period. After the end of the administration period, the animals in the main groups were sacrificed and satellite animals were observed for the next 14 days without treatment.   

 

During the study, clinical observation and health status controls were performed daily. The body weight and food consumption were measured weekly or at the specified time intervals. Detailed clinical observation was carried out weekly. Functional observations were performed at the end of the application and observation periods. Vaginal smears were prepared daily, 2 weeks before start of the administration period (oestrous cycle monitoring), during the mating period (until the presence of spermatozoa) and at necropsy. Reproduction parameters relevant to pups (number of pups, weight of litters and weight of pups, sex and vitality of pups, measurement of anogenital distance, nipple retention, serum levels of thyroid hormones (T4 and TSH in pups) were also recorded. The study was completed with urinalysis, haematological and biochemical analysis and gross necropsy of animals. In all males of the main groups, the sperm parameters, sperm motility and sperm morphology were examined. Selected organs from adult animals and pups were removed for weighing and histopathological examination.

 

Results

Repeated oral administration of the test item to rats by gavage at the dose levels of 80, 250 and 750 mg/kg/day did not cause any mortality (except one male from the dose level 250 mg/kg/day – male No.46, who was found dead on day 30 of application; the cause of death was not determined due to partial autolysis of organs).This death was accidental and not treatment-related.

 

The six males per group (Nos. 1-6, 21-26, 41-46, 61-66) and first six mothers per group that delivered pups were examined from the main groups (control: Nos. 103, 104, 105, 106, 107, 108; the lowest dose: Nos. 122, 123, 124, 125, 126, 128; the middle dose: Nos. 141, 144, 145, 147, 148, 149 and the highest dose: Nos. 161, 165, 166, 167, 168, 169). Also, satellite animals (control: males - Nos. 81-86, females – Nos. 181-186 and high dosed: males - Nos. 91-96 and females Nos. 191-196) were part of the examination of the repeated dose toxicity of the test item.

 

Test item treatment did not produce clinical changes in health status of animals, did not affect the normal growth of treated parental males and females.

 

Haematological examination of treated animals showed only sporadic differences in haematological values in treated animals compared to control animals.

Haematological examination of males at the highest dose level 750 mg/kg/day did not reveal statistically significant differences in haematological values in comparison with the control animals. The five-population differential of white blood cells, the value of total leucocyte count and total erythrocyte count were not affected by the test item treatment. Statistically significantly changed values of red blood components were recorded only in males of the dose level 80 mg/kg/day. An increase in the total value of erythrocytes (RBC)(p ≤ 0.05) was detected. This increase is related to the increased concentration of haemoglobin (p ≤ 0.05) and value of haematocrit (p ≤ 0.05). The values of haemocoagulation parameters were not affected by the test item treatment. In satellite treated males, only the value of APTT was statistically significantly decreased in comparison with the control satellite animals. Other values of treated animals were similar with the satellite control animals.

Haematological examination of females at the highest dose level 750 mg/kg/day did not reveal statistically significant differences in haematological values in comparison with the control animals except the value of monocytes. The examination of five-population differential of white blood cells detected statistically significantly decreased value of monocytes (p ≤ 0.05) in females at the dose level 750 mg/kg/day only. The value of total leucocyte count and red blood components were not affected by the test item treatment. Statistically significantly increased value of MCV (p ≤ 0.05) was recorded in females at the dose level 250 mg/kg/day. The values of haemocoagulation parameters were not affected by the test item treatment. In satellite treated females a decreased value of RBC (p ≤ 0.05) and associated increased value of MCV (p ≤ 0.05) were recorded in satellite treated females in comparison with the satellite control females.Decreased value of neutrophils (p ≤ 0.05) was also recorded in satellite treated females.Other values were similar with satellite control females.

The haematological examination did not reveal toxic effect of the test item on administered animals. The isolated findings were not dose-dependent and were found in all dose levels. These findings were reversible and were not associated with any pathological and/or histopathological findings of haematogenous organs.

 

During biochemical examination of males, statistically significantly changed values (compared to control) were detected. Significantly changed values (p ≤ 0.05) of T-Pro (increased), Crea (decreased), T-Bil (decreased), Na (increased) and Cl (increased) were detected in males at the dose level 750 mg/kg/day compared to control animals. The changed values (p ≤ 0.05) of T-Bil (decreased) and Na (increased) were also recorded in males at the dose level 280 mg/kg/day. In males at the dose level 80 mg/kg/day was detected changed values (p ≤ 0.05) of T-Bil (decreased) and Cl (increased). The value altered at all dose levels (statistically significantly) was bilirubin (T-Bil) - decreased at all treated levels compared to control animals.A statistically significant increased value of bile acid (BA) only was recorded in satellite treated males in comparison with the satellite control males. Values of other biochemical parameters of satellite treated males were similar to the satellite control group.

During the biochemical examination of females, significantly changed biochemical values were recorded only sporadically in treated females. Significantly (p ≤ 0.05) increased value of TG only was reported in females at the dose level 750 mg/kg/day. Significantly (p ≤ 0.05) decreased value of GLU was recorded in females at the dose level 80 mg/kg/day only. Values of other biochemical parameters of treated females were comparable to the control group. Statistically significantly (p ≤ 0.05) increased values of Ca and BA were noted in satellite treated females in comparison with the satellite control females. Values of other biochemical parameters of treated satellite females were comparable to the control group.

Biochemical examination of treated animals did not show a toxicologically significant effect of the test substance on the treated animals. Changes were found out in all dose levels, without dose dependency and were reversible.

 

An increased pH of urine (p ≤ 0.05) and insignificantly decreased volume of urine were detected in males at the dose level 750 mg/kg/day. The presence of proteins, blood and leucocytes were recorded in treated males as well as in control males and were not associated with the application of the test item.

 

Biometry of organs of treated animals showed sporadic significant changes in absolute and relative weight of organs.

In males, statistically significantly (p ≤ 0.05) increased absolute weight of adrenal glands only was recorded at the dose levels 80 and 250 mg/kg/day. Also relative weight of adrenal glands was significantly (p ≤ 0.05) increased in males at the dose level 750 mg/kg/day. Increased relative weight of epididymis was recorded in males at the dose level 750 mg/kg/day.

In satellite treated males, a statistically significant increase in the relative weight of epididymides only was recorded.

In females, significant difference in absolute weight of pituitary gland only was recorded.Absolute weight of pituitary gland was significantly(p ≤ 0.05) decreased in females at the dose level 750 mg/kg/day compared to control females. Statistically significantly increased absolute weight of kidneys was recorded in satellite females.

No significant changes in relative weight of organs were detected in treated females.

The test item had no toxicology significant effect of weight of organs of treated animals. This was confirmed by pathological and/or histopathological examination, where no findings were found that would indicate a toxic effect of the test item on organs of dosed animals.

 

During the macroscopic examination, no findings related to the test item treatment were found out. 

Histological examination revealed only sporadic findings in treated animals as well as in control animals.Test item orally administered in the dose of 750 mg/kg/day did not cause any pathological changes in the male and female genital tract organs, in the pituitary gland, did not cause gross or histopathological changes in the kidneys of rats indicative of a toxic effect and did not cause gross or histopathological changes in the gastrointestinal tract.

Conclusion

According to the study results the NOAEL (No Observed Adverse Effect Level) value for REPEATED DOSE TOXICITY in MALES and FEMALES was established as 750 mg/kg body weight/day.No biologically significant changes attributable to the effect of test item administrationwere observed