Zinc acrylate

Administrative data

Endpoint:

eye irritation: in vitro / ex vivo

Type of information:

experimental study

Adequacy of study:

key study

Study period:

From Dec. 07, 2017 to Dec. 07, 2017

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Data source

Materials and methods

Test guidelineopen allclose all

GLP compliance:

yes (incl. QA statement)

Test material

Test animals / tissue source

Species:

cattle

Strain:

other: Bos primigenius Taurus (fresh bovine corneas)

Details on test animals or tissues and environmental conditions:

Test System: Bos primigenius Taurus (fresh bovine corneas). Fresh bovine eyes were obtained from the slaughterhouse Müller Fleisch GmbH, Enzstr. 2-4, 75217 Birkenfeld, Germany, on the Day of the test. The cattle were between 12 and 60 months old. The eyes were transported to the test facility in Hanks’ Balanced Salt Solution with 1% Penicillin-Streptomycin solution (Penicillin 100 U/mL, Streptomycin 100 µg/mL) in a suitable cooled container. After the arrival of the corneas, they were examined and only corneas which were free from damages were used. The corneas were excised with a scalpel and cut from the globe with a 2-3 mm ring of sclera around the outside. Each cornea was transferred to a cornea holder in which pre-warmed cMEM (32 ± 1°C) without phenol red was filled. The holders were then incubated for 1 h in the incubation chamber at 32 ± 1°C.

Test system

Vehicle:

Hank's balanced salt solution

Remarks:

Batch no.: 20171207, 10-fold concentrated, diluted in demineralised water (1:10)

Controls:

yes, concurrent positive control

yes, concurrent negative control

Amount / concentration applied:

Test substance Preparation: The test substance was a solid non-surface-active substance. It was tested as a suspension with a concentration of 20% in HBSS. The suspension was prepared freshly on the Day of the assay.

Duration of treatment / exposure:

Incubation time: 4 h

Number of animals or in vitro replicates:

For each treatment group [negative control solution (HBSS), test substance and positive control (20% imidazole solution)], three replicates were used.

Details on study design:

OPACITY TEST
After the initial incubation, the medium was changed and the baseline opacity for each cornea was recorded. After removal of the pre-incubation medium (cMEM without phenol red), 750 µL negative control solution, test substance suspension and positive control solution were applied to each replicate. The test or control preparations were given directly on the epithelium in such a manner that as much as possible of the cornea was covered with test or control substances. Exposure time on the corneas was 4 h at 32 ± 1°C. After thorough rinsing with cMEM with phenol red and final rinsing with cMEM without phenol red, both chambers were filled with cMEM without phenol red, and the final opacity value of each cornea was recorded.

PERMEABILITY TEST
After the recording of the final opacity value, the cMEM without phenol red was removed from the front chamber, and 1 mL sodium fluorescein solution was added to the front chamber for the detection of permeability of the corneas. For the open chamber method, a sodium fluorescein solution with a concentration of 5 mg/mL was used. The chambers were then closed again and incubated for 90 min. at 32 ± 1°C. After incubation, the content of the posterior chamber was thoroughly mixed. Then, its optical density at 492 nm was measured with the microtiter plate photometer.

Results and discussion

In vitro

Other effects / acceptance of results:

In the negative control, no signs of eye irritation were observed. The positive control induced serious eye damage, which would be classified as GHS category I.

Any other information on results incl. tables

Opacity and Permeability Values

 

The illuminance (unit: LUX) values measured before and after exposure

Parameter	Negative Control			Test substance			Positive Control
	1. Rep.	2. Rep.	3. Rep.	1. Rep.	2. Rep.	3. Rep.	1. Rep.	2. Rep.	3. Rep.
(I) Measured values before exposure	968	995	972	999	1022	975	994	989	979
(I) Measured values after exposure	969	938	926	250	243	267	358	390	352

Rep. = Replicate

 

Opacity Values Negative Control

Parameter	Negative Control
	1. Rep.	2. Rep.	3. Rep.
Opacity before exposure	3.85	2.67	3.67
Opacity after exposure	3.80	5.23	5.81
Opacity Difference	-0.04	2.56	2.14
Mean Opacity Difference	1.55

 

Opacity Values Test substance and Positive Control

Parameter	Test substance			Positive Control
	1. Rep.	2. Rep.	3. Rep.	1. Rep.	2. Rep.	3. Rep.
Opacity before exposure	2.51	1.56	3.54	2.72	2.93	3.36
Opacity after exposure	128.11	132.93	117.44	77.57	67.97	79.56
Opacity Difference	125.60	131.37	113.90	74.85	65.04	76.20
Opacity Difference corrected	124.05	129.82	112.35	73.30	63.49	74.65
Mean Opacity Difference corrected	122.08			70.48

 

For the permeability measurement, three replicates for each treatment group were measured three times. cMEM without phenol red was measured as blank value.

Optical density at 492 nm of Blank

Parameter	cMEM without phenol red
1. Measurement	0.041
2. Measurement	0.035
3. Measurement	0.042
Mean	0.039

 

Optical density at 492 nm of Negative Control, Test substance and Positive Control

Parameter	Negative Control			Test substance			Positive Control
	1. Rep.	2. Rep.	3. Rep.	1. Rep.	2. Rep.	3. Rep.	1. Rep.	2. Rep.	3. Rep.
1 Measurement	0.068	0.050	0.060	0.040	0.050	0.060	1.435	2.137	1.411
2. Measurement	0.064	0.047	0.054	0.036	0.048	0.057	1.463	2.140	1.413
3. Measurement	0.069	0.048	0.050	0.039	0.049	0.057	1.465	2.143	1.396
1. Measurement – blank	0.0287	0.0107	0.0207	0.0007	0.0107	0.0207	1.3957	2.0977	1.3717
2. Measurement – blank	0.0247	0.0077	0.0147	-0.0033	0.0087	0.0177	1.4237	2.1007	1.3737
3. Measurement – blank	0.0297	0.0087	0.0107	-0.0003	0.0097	0.0177	1.4257	2.1037	1.3567
Mean of each replicate	0.0277	0.0090	0.0153	-0.0010	0.0097	0.0187	1.4150	2.1007	1.3673
Mean of the 3 replicates	0.0173			--			--
Corrected	--	--	--	-0.0183	-0.0077	0.0013	1.3977	2.0833	1.3500
Corrected mean of the 3 replicates	--			-0.0082			1.6103

IVIS Value

The calculated IVIS for each replicate and the corresponding means

Test Group	IVIS	Mean IVIS	Relative Standard Deviation IVIS
Negative Control HBSS	0.37	1.81	69.47%
	2.69
	2.37
Test substance Zinc acrylate	123.78	121.95	7.22%
	129.71
	112.37
Positive Control 20% imidazole solution	94.27	94.64	0.35%
	94.74
	94.90

Validityof the Study: The validity criteria and findings

Parameter	Criterion	Found	Assessment
IVIS of negative control HBSS	≤3	1.81	ok
IVIS of positive control 20% imidazole solution	70.92 – 157.64	94.64	ok

Applicant's summary and conclusion

Interpretation of results:

Category 1 (irreversible effects on the eye) based on GHS criteria

Conclusions:

Under study conditions, the test substance was determined to induce serious eye damage on the cornea of the bovine eye.

Executive summary:

A study was conducted to determine the eye irritation potential of test substance using the in vitro Bovine Corneal Opacity and Permeability (BCOP) test method according to OECD Guideline 437, in compliance with GLP. The BCOP test method can identify chemicals inducing serious eye damage and chemicals not requiring classification for eye irritation or serious eye damage. Fresh bovine eyes were obtained from the slaughterhouse on the day of the test. The cattle were between 12 and 60 months old. The corneas were screened for test requirements, prepared and mounted in corneal holders. Prior to treatment, the test system was previously incubated with cMEM without phenol red at 32 ± 1°C for 1 h and Corneal opacity was determined. The test substance preparation [20% suspension in Hank’s Balanced Salt Solution (HBSS)] was incubated on the cornea for 4 h at 32 ± 1°C. After removal of the test substance, opacity and permeability values were measured. For each treatment group [negative control solution (HBSS), test substance and positive control (20% imidazole solution)], three replicates were used. In the negative control, no signs of eye irritation were observed. The positive control induced serious eye damage, which would be classified as GHS category I .The negative control and the positive control met the validity criteria. The calculated IVIS (In Vitro Irritancy Score) was 121.95. Under study conditions, the test substance was therefore determined to induce serious eye damage on the cornea of the bovine eye (Geitlinger, 2018).