Benzyl 4-[(1-butyl-5-cyano-1,6-dihydro-2-hydroxy-4-methyl-6-oxopyridin-3-yl)azo]benzoate

Administrative data

Endpoint:

skin sensitisation: in vivo (non-LLNA)

Type of information:

experimental study

Remarks:

source of read-across

Adequacy of study:

key study

Study period:

29 April to 6 June, 2002

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Justification for type of information:

Justification for the use of a read-across approach is provided in IUCLID section 13.

Data source

Materials and methods

Test guidelineopen allclose all

GLP compliance:

yes (incl. QA statement)

Type of study:

guinea pig maximisation test

Justification for non-LLNA method:

Test conducted on 2002

Test material

In vivo test system

Test animals

Species:

guinea pig

Strain:

Himalayan

Remarks:

lbm: GOHI; SPF-quality guinea pigs (synonym: Himalayan spotted)

Sex:

female

Details on test animals and environmental conditions:

TEST ANIMALS
- Source: RCC Ltd, Biotechnology & Animal Breeding Division, Wölferstrasse 4, 4414 Füllinsdorf, CH
- Number of animals: preliminary test: 3 females; main study: 15 females (10 treatment + 5 control animals)
- Females nulliparous and non-pregnant: yes
- Age at study initiation: 5 to 7 weeks
- Weight at study initiation: preliminary test: 400 to 437 g; main study: 408 to 448 g
- Housing: individually in Makrolon type-4 cages with standard softwood bedding ("Lignocel", Schill AG, 4132 Muttenz, CH)
- Diet: pelleted standard Provimi Kliba 3418, batch nos. 116/01 and 25/02, Guinea Pig Breeding / Maintenance Diet, containing Vitamin C (Provimi Kliba AG, 4303 Kaiseraugst, CH), ad libitum. Results of analyses for contaminants are archived at the test laboratory
- Water: community tap water from Füllinsdorf, ad libitum. Results of bacteriological, chemical and contaminant analyses are archived at the test laboratory
- Acclimation period: preliminary test: none; main study: one week
- Indication of any skin lesions: none at check at beginning of study period

ENVIRONMENTAL CONDITIONS
- Temperature: 20 ± 3 °C
- Humidity: 30-70 %
- Air changes: 10-15 per hour
- Photoperiod (hrs dark / hrs light): 12/12 (music was played during the daytime light period)

Study design: in vivo (non-LLNA)

Inductionopen allclose all

No. of animals per dose:

10 per test group
5 per control goup

Details on study design:

RANGE FINDING TESTS
A. Intrademal injections: 4 intradermal injections (0.1 ml/site) of a 1:1 (v/v) mixture of Freund's Complete Adjuvant / physiological saline were made into the shaved neck of one guinea pig. One week later, intradermal injections (0.1 ml/site) were made into the clipped flank of the same guinea pig at concentrations of A = 5 %, B = 3 %, C = 1 % test item in PEG 300. Dermal reactions were assessed 24 hours later.

B. Epidermal applications: 4 intradermal injections (0.1 ml/site) of a 1:1 (v/v) mixture of Freund's Complete Adjuvant/physiological saline were made into the shaved neck of two guinea pigs. One week later, both flanks of each of the guinea pigs were clipped and shaved just prior to the application. Then, 4 patches of filter paper (3 × 3 cm) were saturated with the test item at D = 25 % (technically the highest possible concentration to be applied sutficiently), E = 15 %, F = 10 % and G = 5 % in PEG 300 and applied to the clipped and shaved flanks. The amount of test item preparation applied was approximately 0.2 g for the test item 25 % and a volume of approximately 0.2 ml was applied for the remaining concentrations. The patches were covered by a strip of aluminum foil and firmly secured by elastic plaster wrapped around the trunk and covered with imperuious adhesive tape. This procedure ensured the intensive contact of the test item. The dressings were removed after an exposure period of 24 hours. 21 h after removal of the dressing the application site was depilated with an approved depilatory cream (VEET Cream, Reckitt & Colman AG, CH-4123 Allschwil) in order to visualise any resulting erythema. The depilatory cream was placed on the patch sites and surrounding areas, and left on for 3-5 minutes. lt was then thoroughly washed off with a stream of warm, running water. Then, the animals were dried with a disposable towel, and returned to their cages. The reaction sites were assessed 24 and 48 hours after removal of the bandage for erythema and oedema according to the method of Magnusson and Kligman. The allocation of the different test item dilutions to the sites (D, E, F, G) on the two animals was alternated in order to minimize site-to-site variation in responsiveness.

Based on the results obtained the concentration selected for induction and challenge in the main study was 25 % and 5 %, respectively.

MAIN STUDY
A. INDUCTION EXPOSURE
(I) Intradermal injections (day 1)
- No. of exposures: 3 pair of injections per animal (0.1 ml/site)
- Site: injections were made along the border of an area of dorsal, scapular skin measuring 4 × 6 cm
- Preparation of site: fur was clipped (6 × 8 cm area)
- Concentrations: 5 % (w/w)
- Injections to treatment animals: (1) 1:1 (v/v) Freund's Complete Adjuvant:physiological saline; (2) 5 % test item in PEG 300; (3) 5 % test item in 1:1 (v/v) Freund's Complete Adjuvant:physiological saline
- Injections to control animals: (1) 1:1 (v/v) Freund's Complete Adjuvant:physiological saline; (2) PEG 300; (3) 1:1 (w/w) mixture of PEG 300 in 1:1 (v/v) Freund's Complete Adjuvant:physiological saline
- Frequency of injections: once
- Evaluation: skin response after 24 and 48 hours

(II) Epidermal applications (day 8)
- No. of exposures: 1
- Site: an area of dorsal, scapular skin measuring 4 × 6 cm, over the injection sites
- Preparation of site: fur was clipped and shaved
- Application: 2 × 4 cm patch of saturated filter paper and covered with aluminium foil, then firmly secured by an elastic plaster wrapped around the trunk of the animal and secured with impervious adhesive tape
- Concentrations: 25 % (w/w)
- Exposure period: 48 hours
- Frequency of applications: once
- Test groups: ca. 0.3 g test item as 25 % (w/w) test item in PEG 300
- Control group: 0.3 ml PEG 300
- Evaluation: skin response after 24 and 48 hours

B. CHALLENGE EXPOSURE
(II) Epidermal applications (day 22)
- No. of exposures: 2 (one on each flank)
- Sites: 5 × 5 cm area on both the left and right flank of each guinea pig
- Preparation of site: fur was clipped and shaved
- Application (both treatment and control animals): two 3 × 3 cm patches saturated in 0.2 ml containing either 5 % (w/w) test item in PEG 300 (left flank) or PEG 300 alone (right flank) and covered with aluminium foil, then firmly secured by an elastic plaster wrapped around the trunk of the animal and secured with impervious adhesive tape
- Concentrations: 5 % (w/w)
- Exposure period: 24 hours
- Frequency of applications: once
- Hair removal: 21 h after removal of the dressing the application site was depilated with an approved depilatory cream (VEET Cream, Reckitt & Colman AG, CH-4123 Allschwil) in order to visualise any resulting erythema. The depilatory cream was placed on the patch sites and surrounding areas, and left on for 3-5 minutes. lt was then thoroughly washed off with a stream of warm, running water. Then, the animals were dried with a disposable towel, and returned to their cages. The reaction sites were assessed 24 and 48 hours after removal of the bandage for erythema and oedema according to the method of Magnusson and Kligman.
- Evaluation: erythema and oedema observations were recorded at 24 h and 48 h after removal of dressing. An allergic reaction was defined by visible reddening of the challenge site. lf the dermal reactions of test animals following the challenge were more marked and/or persistent than those of the control animals, the animals were considered to show evidence of contact hypersensitivity. lf the dermal reactions of test animals following the challenge were not clearly different from the reactions seen in the control group animals, the results for the test animals were considered "inconclusive". The test animals were considered to show no evidence of contact hypersensitivity if the dermal reactions to the challenge application were identical or less marked and/or persistent than the reactions obserued in the control animals.

Positive control substance(s):

yes

Remarks:

alpha-hexylcinnamaldehyde

Results and discussion

Positive control results:

All test animals (at the 24-hour reading) and 6 out of 10 animals (at the 48-hour reading) showed discrete/patchy erythema after the challenge treatment with 0.1 % (w/w) positive control in PEG 300. No skin effect was observed in the control group.

In vivo (non-LLNA)

Resultsopen allclose all

Any other information on results incl. tables

SKIN EFFECTS AFTER INTRADERMAL INDUCTION - PERFORMED ON TEST DAY 1

The expected and common findings were obserued in the control and test group after the different applications using FCA intradermally. These findings consisted of erythema, oedema, necrotizing dermatitis, encrustation and exfoliation of encrustation. No detailed description of the effects is given in the report as these FCA effects are wellknown.

SKIN EFFECTS AFTER EPIDERMAL INDUCTION - PERFORMED ON TEST DAY 8

CONTROL GROUP

No erythematous or oedematous reaction was observed in the animals treated with PEG 300 only.

TEST GROUP

As the test item at 25 % stained the skin in yellow, it was not possible to determine whether erythema was present or not. However, no oedema was obserued. The animals were not depilated in the epidermal induction phase.

SKIN EFFECTS AFTER THE CHALLENGE - PERFORMED ON TEST DAY 22

CONTROL GROUP

No skin reactions were observed in the animals when treated with either PEG 300 only or when treated with the test item at 5 % in PEG 000. Yellow discoloration produced by the test item was noted directly after removal of the patch. To remove the discoloration all animals were depilated 3 hours prior to challenge reading.

TEST GROUP

Discrete/patchy erythema were observed in eight out of 10 animals at the 24- and 48-hour reading after treatment with the test item at 5 % in PEG 300. No skin reaction were obserued when treated with PEG 300. Yellow discoloration produced by the test item was noted directly after removal of the patch. To remove the discoloration all animals were depilated 3 hours prior to challenge reading.

VIABILITY / MORTALITY / MACROSCOPIC FINDINGS

There were no deaths during the course of the study, hence no necropsies were performed.

CLINICAL SIGNS, SYSTEMIC

No signs of systemic toxicity were observed in the animals.

BODY WEIGHTS

3 animals of the control group and 7 animals of the test group showed a loss of body weight (1.4 % to 6.9 %) during the acclimatization period. They recovered between the treatment start and the end of the study. The body weight of the other animals was within the range commonly recorded for animals of this strain and age.

Applicant's summary and conclusion

Interpretation of results:

other: Skin Sensitiser Category 1B (H317), according to the CLP Regulation (EC 1272/2008)

Conclusions:

The test item elicited positive reactions in 8 out of 10 animals 24 and 48 hours after a challenge application in the GPMT.

Executive summary:

The skin sensitising potential of the test item was evaluated in an experimental study, a GPMT, according to the OECD guideline 406 (1992) and the EU method B.6 (1996). In a preliminary test, one female Himalayan spotted albino guinea pig was administered 4 intradermal injections of equal parts Freund's Complete Adjuvant and physiological saline to the shaved neck; one week later, 3 intradermal injections were made into the clipped flank containing either 5, 3, 1 % test item in PEG 300. 24 hours later, all three concentrations/sites showed positive reactions. Two additional guinea pigs were administered 4 intradermal injections of equal parts Freund's Complete Adjuvant and physiological saline to the shaved neck; one week later, 4 patches of filter paper (3 × 3 cm) saturated with test item (25, 15, 10 and 5 %) in PEG 300 were applied to clipped, shaved flanks for 24 hours under an occlusive dressing. 24 and 48 hours after removal, positive reactions were observed at concentration sites of 10 % and over. Based on the results obtained the concentration selected for induction and challenge in the main study was 25 % and 5 %, respectively.

In the main study, 10 treatment animals and 5 controls were administered three pairs of intradermal injections containing (i) equal parts Freund's Complete Adjuvant and physiological saline, (ii) 5 % test item in PEG 300 (controls: PEG 300 alone), and (iii) 5 % test item in equal parts Freund's Complete Adjuvant and physiological saline (controls: PEG 300 in place of test item). One week later, an epidermal application of 25 % test item in PEG 300 was applied to the same area for 48 hours (control animals recevied PEG 300 alone). Finally, a challenge was performed on day 22 of the study period whereby all animals received a dermal application of 5 % test item in PEG 300 to the left flank and PEG 300 alone to the right flank for 24 hours under an occlusive dressing. The hair was depilled and skin reactions were observed 24 and 48 hours after removal.

After the induction period, no control or treatment animals showed positive reactions, and no readings of erythema could be discerned from the treatment animals due to local yellow discolouration. Following the induction, no control animals showed positive reactions on either flank at either 24 or 48 hours; no positive reactions were observed among treatment animals on the right flank, however, positive reactions were observed in 8 out of 10 animals on the left flank at both 24 and 48 hours after removal of the challenge application.

Based on the positive reactions in 8 out of 10 animals following the challenge application, the test item shows great potential to elicit skin reactions and is considered a skin sensitiser.