trans-1-(1-oxohexadecyl)-4-[(1-oxohexadecyl)oxy]-L-proline

Administrative data

Endpoint:

skin sensitisation: in vivo (non-LLNA)

Type of information:

experimental study

Adequacy of study:

key study

Study period:

11-12-2007 to 25-02-2008

Reliability:

1 (reliable without restriction)

Data source

Materials and methods

GLP compliance:

yes

Type of study:

guinea pig maximisation test

Justification for non-LLNA method:

Test performed in 2008.
LLNA method (OECD 442 B) was adopted in 2010.

Test material

In vivo test system

Test animals

Species:

guinea pig

Strain:

Dunkin-Hartley

Sex:

female

Details on test animals and environmental conditions:

15 female albino guinea pigs of Dunkin-Hartley strain, supplied by Charles River (F-69592 L’Arbresle) weighed between 252 and 297 at the beginning of the test and were 4 weeks old.
Prior to the test, the animals were kept for a minimum acclimatisation period of 5 days, under stabling and nutritional conditions identical to those of the test.
Before the experimentation process, they were identified individually by marking with picric acid and a tattoo placed on their ear.
The animals were carefully shorn before each test item application.
The animals were housed either in groups of 2 or 3 in polycarbonate containers, the flooring of which
was covered with dust-free cuttings and the top fitted a stainless steel lid with a feeding device and
drinking device of 500 ml.
The environmental parameters of the main test were :
- Temperature : between 20°C and 23°C
- Relative humidity : between 33% and 67%
- Lighting time: 12 hours daily
The drinking water (tap water from public distribution system) and food were supplied freely.
Microbiological verification and chemical analysis were conducted every six months by the Institut Européen de l’Environnement de Bordeaux (I.E.E.B.).

Study design: in vivo (non-LLNA)

Inductionopen allclose all

Challengeopen allclose all

No. of animals per dose:

controls: 5 animals
treated: 10 animals

Details on study design:

(1) Preliminary study
- for the determination of the MNNC, two animals received increasing concentration of the substance by intradermal injection on both sides of the spine. A macroscopic evaluation of the cutaneous reactions was conducted 24 hours later.
- for the determination of the pre-MNIC, the product was applied on the dorso-lumbar zone of 2 animals shorn beforhand, with occlusive dressing for 24 hours. A macroscopic evaluation of the cutaneous reactions was conducted 24 hours after removal of the dressing.
- for the determination of the MNIC, 3 animals were treated according to the same treatment as negative controls for the induction phase (ie 2 intradermic injection (ID) of Freund's Complete Adjuvant (FCA) diluted at 50% in isotonic sodium chloride + 2 ID of isotonic sodium chloride + 2 ID a mixture with equal volumes v/v FCA at 50% and isotonic sodium chloride. 7 days after, the animals were shared and a 24 hours topic application under occlusive dressing of the test product at 6.25% ; 12.5% ; 25% and 50% in distilled water was performed.
A macroscopic evaluation of the cutaneous reactions was conducted 24 hours after removal of the occlusive dressing.
(2) Main study
A- Induction
1st Intradermal Induction:
Day 0
After shearing the scapular zone, three (3) pairs of intradermal injections (ID) of 0.1 ml were performed on the scapular zone in such a way as an injection on each pair is placed to either side of the spine as follows :
GROUP 1 (Negative control):
• 2 ID: Freund’s Complete Adjuvant diluted at 50 % in isotonic sodium chloride.
• 2 ID: isotonic sodium chloride
• 2 ID: a mixture with equal volumes v/v :
- Freund’s Complete Adjuvant at 50% and isotonic sodium chloride,
GROUP 2 (Treated):
• 2 ID: Freund’s Complete Adjuvant diluted by 50 % in isotonic sodium chloride,
• 2 ID: test item at 0.78%,
• 2 ID a test mixture in equal volumes v/v :
- Freund’s Complete Adjuvant at 50% and the test item at 1.56%.
2nd Topical Induction:
Day 6
The scapular zone of all the animals in each group, shorn beforehand, was brushed with a solution of sodium lauryl sulfate at 10% in thick vaseline, in
order to create a local irritation.
Day 7
A topical application under occlusive dressing for 48 hours was performed on the injection sites of each animal.
GROUP 1 (Negative control): 0.5 ml of distilled water
GROUP 2 (treated): 0.5 ml of the test item at 50%
B - Rest phase
The animals of both groups were left for 10 days.
C - Challenge phase
Day 21
The experimental procedure of this phase was identical for both groups GROUP 1 (Negative control) and GROUP 2 (Treated) submitted to this experimentation: on the previously shorn dorso-lumbar zone, an application on either side of the spine, under occlusive dressing, was performed during 24 hours:
- 1 sample cup containing the test item at 50% (MNIC) and at 25% (1/2 MNIC).

Challenge controls:

Negative controls : 5 animals

1st Intradermal Induction:
Day 0
After shearing the scapular zone, three (3) pairs of intradermal injections (ID) of 0.1 ml were performed on the scapular zone in such a way as an injection on each pair is placed to either side of the spine as follows :

GROUP 1 (Negative control):
• 2 ID: Freund’s Complete Adjuvant diluted at 50 % in isotonic sodium chloride.
• 2 ID: isotonic sodium chloride
• 2 ID: a mixture with equal volumes v/v :
- Freund’s Complete Adjuvant at 50% and isotonic sodium chloride,


2nd Topical Induction:
Day 6
The scapular zone of all the animals in each group, shorn beforehand, was brushed with a solution of sodium lauryl sulfate at 10% in thick vaseline, in order to create a local irritation.
Day 7
A topical application under occlusive dressing for 48 hours was performed on the injection sites of each animal.
GROUP 1 (Negative control): 0.5 ml of distilled water

Rest phase
The animals of control groups were left for 10 days.

Challenge phase
Day 21
The experimental procedure of this phase was identical for both groups GROUP 1 (Negative control) and GROUP 2 (Treated) submitted to this experimentation: on the previously shorn dorso-lumbar zone, an application on either side of the spine, under occlusive dressing, was performed during 24 hours:
- 1 sample cup containing the test item at 50% (MNIC) and at 25% (1/2 MNIC).

Positive control substance(s):

yes

Remarks:

alpha-hexylcinnamaldehyde

Results and discussion

Positive control results:

positive control at 50% : 100% of animals sensitized after 24h
positive control at 50% : 90% of animals sensitized after 48h
positive control at 25% : between 90% and 100% of animals sensitized 24h
positive control at 25% : between 70% and 100% of animals sensitized 48h

In vivo (non-LLNA)

Resultsopen allclose all

Any other information on results incl. tables

The aim of the study was to evaluate the possible allergenic activity of the test substance after intradermic injection and topical administration in guinea pigs. After induction (intradermic injection at 0.78% and topical application at 50%) of 10 Guinea Pigs of treated group with the test item and a 10-day rest phase, the challenge phase, under occlusive dressing for 24 hours, consisted to a single topical application of the test item diluted at 50% and at 25% in distilled water. The experimental protocol was established according the O.E.C.D. guideline n°406 dated July 17th, 1992 and the method B.6 of the E.E.C. n°96/54 dated July 30th, 1996. Slight erythema was noted in 40% of the animals of the treated group (4/10) and of the animals of the control group (2/5), 24 hours after the challenge phase, on the treated area with the test item at 50%. These reactions were totally reversible at the reading time 48 hours and were significant of an irritant reaction type. No cutaneous intolerance reaction was recorded in the animals of the treated group, on the treated area at 25%. No cutaneous intolerance reaction was recorded in animals from the negative control group, on the treated area at 25%. In conclusion, in view of these results, under these experimental conditions, the test item LCA07033 must not be classified, in accordance with the criteria for classification, packaging and labelling of dangerous substances and preparations of the E.E.C. Directives 67/548, 2001/59 and 99/45. No symbol and risk phrase are required.

Applicant's summary and conclusion

Interpretation of results:

not sensitising

Remarks:

Migrated information

Conclusions:

In view of these results, under these experimental conditions, the test substance must not be classified, in accordance with the criteria for classification, packaging and labelling of dangerous substances and preparations of the E.E.C. Directives 67/548, 2001/59 and 99/45. No symbol and risk phrase are required.

Executive summary:

The aim of the study was to evaluate the possible allergenic activity of the test substance after intradermic injection and topical administration in guinea pigs. After induction (intradermic injection at 0.78% and topical application at 50%) of 10 Guinea Pigs of treated group with the test item and a 10-day rest phase, the challenge phase, under occlusive dressing for 24 hours, consisted to a single topical application of the test item diluted at 50% and at 25% in distilled water. The experimental protocol was established according the O.E.C.D. guideline n°406 dated July 17th, 1992 and the method B.6 of the E.E.C. n°96/54 dated July 30th, 1996. Slight erythema was noted in 40% of the animals of the treated group (4/10) and of the animals of the control group (2/5), 24 hours after the challenge phase, on the treated area with the test item at 50%. These reactions were totally reversible at the reading time 48 hours and were significant of an irritant reaction type. No cutaneous intolerance reaction was recorded in the animals of the treated group, on the treated area at 25%. No cutaneous intolerance reaction was recorded in animals from the negative control group, on the treated area at 25%. In conclusion, in view of these results, under these experimental conditions, the test item LCA07033 must not be classified, in accordance with the criteria for classification, packaging and labelling of dangerous substances and preparations of the E.E.C. Directives 67/548, 2001/59 and 99/45. No symbol and risk phrase are required.