Adenosine 5'-(tetrahydrogen triphosphate), disodium salt

Administrative data

Endpoint:

skin sensitisation: in chemico

Type of information:

experimental study

Adequacy of study:

weight of evidence

Study period:

17 March -19 May 2017

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Data source

Materials and methods

GLP compliance:

yes (incl. QA statement)

Type of study:

direct peptide reactivity assay (DPRA)

Test material

In chemico test system

Details on the study design:

SUMMARY: DPRA measures the reaction of the test item with synthetic peptides containing cysteine (Ac-RFAACAA-COOH) or lysine (Ac-RFAAKAA-COOH). The custom peptides contained cysteine or lysine as the nucleophilic reaction centres and phenylalanine to facilitate HPLC detection. Test item and peptide were combined and incubated together for 24 h at room temperature. Following this incubation, the concentration of free (i.e. unreacted) peptide remaining was measured by HPLC immediately prior to the lysine peptide assay.


EXPERIMENTAL PROCEDURES

PEPTIDES:
Source: RS Synthesis
Batch:
- Cysteine: No. P170419-LC180433
- Lysine: No. P161108-LC107617
Purity:
-Cysteine: 96,47%
-Lysine: 98.14%

BUFFERS USED:
- Phosphate buffer: ca 100 mM, pH 7.49
- Ammonium acetate buffer: ca 100 mM, pH 10.17

SOLUBILITY ASSESSMENT:
- ultrapure water was selected as the most suitable solvent for the test material

PREPARATION PEPTIDE STOCK SOLUTIONS:
- CYSTEINE: stock solution of 0.667 mM in phosphate buffer
- LYSINE: stock solution of 0.667 mM in ammonium acetate buffer

CYSTEINE PEPTIDE ASSAY:
-PREPARATION: test item was dissolved in ultrapure water and mixed by inversion and vortex until fully in solution. The concentration of the test solution corrected for purity, was 100 mM (100% from the target). Cinnamic aldehyde was dissolved in acetonitrile with a concentration of 100 mM (100% of target, 100 mM). All test item and control solutions were prepared immediately prior to use.
-PREPARATION OF THE SANDARD CURVE: Dilution buffer was prepared by mixing phosphate buffer (pH 7.49, 8 mL) with acetonitrile (2 mL). Standard 1 (STD1) was prepared by mixing peptide stock solution (1600 µL) with acetonitrile (400 µL). Serial dilutions (1:1, v/v) were prepared from this to make a standard curve (from 0.534 to 0.0167 mM). An additional sample containing only dilution buffer was included as a blank (0 mM) standard. The standard curve was analysed by HPLC immediately prior to the cysteine peptide assay.
-REFERENCE CONTROL: Acetonitrile (250 µL) was mixed with peptide stock solution (750 µL). Three replicates of this were produced for Reference Control A. Reference Control B was prepared as described for Reference Control A. Three replicates were analyzed at the beginning of the testing run, and three at the end of the testing run, to demonstrate peptide stability over the analysis time. Reference Control C samples were prepared containing the solvent that the test item was dissolved in: three replicates containing acetonitrile (250 µL) and peptide stock (750 µL) and three replicates containing ultrapure water (50 µL), acetonitrile (200 µL) and peptide stock (750 µL). These samples were included in every assay run together with the samples containing test item. They are used to verify that the solvent does not impact upon peptide stability during the assay, and to calculate percentage peptide depletion.
- PEPTIDE ASSAY METHOD: The assay contained a 1:10 molar ratio of peptide to test item. Positive control or test item (50 µL) was mixed with acetonitrile (200 µL) and the peptide solution (750 µL). The vials were mixed by vortex. Co-elution controls were prepared by mixing together acetonitrile (200 µL), phosphate buffer (750 µL) and test item (50 µL). All test items and positive control samples were prepared in triplicate. All vials were stored in the dark at ambient temperature for ca 24 h until analyzed by HPLC.

LYSINE PEPTIDE ASSAY:
-PREPARATION: test item was dissolved in ultrapure water and mixed by inversion and vortex until fully in solution. The concentration of the test solution corrected for purity, was 100 mM (100% of target, 100 mM). Cinnamic aldehyde was dissolved in acetonitrile with concentration of 100 mM (100 % of target, 100 mM). All tets item and control solutions were prepared immediately prior to use.
- PREPARATION OF THE STANDARD CURVE: Dilution buffer was prepared by mixing ammonium acetate buffer (pH 10.17, 8 mL) with acetonitrile (2 mL). Standard 1 (STD1) was prepared by mixing peptide stock solution (1600 µL) with acetonitrile (400 µL). Serial dilutions (1:1, v/v) were prepared from this to make a standard curve (from 0.534 to 0.0167 mM). An additional sample containing only dilution buffer was included as a blank (0 mM) standard. The standard curve was analyzed by HPLC.
- REFERENCE CONTROL: like for cysteine
- PEPTIDE ASSAY METHOD: The assay contained a 1:50 molar ratio of peptide to test item. Cinnamic aldehyde or test item (250 µL) were mixed with peptide solution (750 µL). The vials were mixed by inversion and vortex. Co-elution controls were prepared by mixing together ammonium acetate buffer (750 µL) and test item (250 µL). All vials were stored in the dark at ambient temperature for ca 24 h until analysed by HPLC.

CHROMATOGRAPHIC AND DETECTOR PARAMETERS
- Column: Phenomenex Luna C18 (2) (2 x 100 mm, 3 µm)
- Run Time: 20 min
- Mobile Phase Conditions: Mobile Phase A: trifluoracetic acid (0.1%, v/v) in Milli-Q H2O
Mobile Phase B: trifluoracetic acid (0.085%, v/v) in acetonitrile
- Flow Rate: 0.35 mL/min
- Column Temperature: 30°C
- Auto Sampler Temperature: Room temperature
- Injection Volume: 7 µL
- UV Wavelength: 220 nm
- HPLC Gradient: see below

CALCULATIONS:
The concentration of peptide remaining in each sample following incubation was calculated from integrated peak area, with reference to the peptide standard curve. Percent peptide depletion was calculated from the following formula:
Peptide Depletion (%) = 1 – ( Peak Area (Sample) / Mean Peak Area (Reference Control C)) x 100

Results and discussion

Positive control results:

The mean depletion value for the positive control was 66.3% showing a high reactivity (Sensitiser)

In vitro / in chemico

Other effects / acceptance of results:

No co-elution of the test item with either peptide was observed.

SYSTEM SUITABILITY FOR THE CYSTEINE ASSAY
The calibration linearity, r2, for the cysteine standard curve was 0.9982. This met the acceptance criteria for r2 which was >0.990.
The mean peptide concentration of Reference Control A was 0.461 mM ± 0.049 mM (mean ± SD). These samples met the acceptance criteria of 0.5 mM ± 0.05 mM.
The calculated peptide concentration in the Reference Control C samples was 0.480 mM ± 0.002 mM (acetonitrile), and 0.477 mM ± 0.006 mM (ultrapure water). These samples met the acceptance criteria of 0.5 mM ± 0.05 mM. In addition, for the six Reference Control B and three Reference Control C in acetonitrile, the coefficient of variation (CV) was 1.6%. This met the acceptance criteria of <15.0%.
The mean percentage peptide depletion value of the three replicates for cinnamic aldehyde fell within the lower bound and upper bound values of 60.8% and 100.0% for cysteine, with a peptide depletion value of 80.7 ± 7.7% (mean ± SD). The standard deviation of replicate positive control samples achieved the acceptance criteria of <14.9%.
Finally, the standard deviation of replicate test item samples was 14.9% for ATP, Di Na

SYSTEM SUITABILITY FOR THE LYSINE ASSAY
The calibration linearity, r2, for the lysine standard curve was 1. This met the acceptance criteria for r2 which was >0.990.
The mean peptide concentration of Reference Control A was 0.490 mM ± 0.002 mM (mean ± SD). These samples met the acceptance criteria of 0.5 mM ± 0.05 mM.
The calculated peptide concentration in the Reference Control C samples was 0.487 mM ± 0.003 mM (acetonitrile) and 0.495 mM ± 0.004 mM (ultrapure water). These samples met the acceptance criteria of 0.5 mM ± 0.05 mM. In addition, for the six Reference Control B and three Reference Control C samples in acetonitrile, the CV was 0.5% (acceptance criteria for CV was <15%).
The mean percentage peptide depletion value of the three replicates for cinnamic aldehyde fell within the lower bound and upper bound values of 40.2% and 69.0% for lysine, with the SD <11.6%. The actual percentage peptide depletion value reported for cinnamic aldehyde was 51.8% ± 1.2% (mean ± SD). The standard deviation of replicate positive control samples achieved the acceptance criteria of <11.6%.
Finally, the standard deviation of replicate test item samples was 0.8% for ATP, Di Na.

PROTOCOL DEVIATIONS
The study was performed in accordance with the protocol with the following deviation:
- The protocol states that prior to analysis HPLC samples will be inspected visually however there is no evidence to suggest that this has been carried out. As results met the acceptance criteria it can be assumed that there was no precipitate, therefore there was no impact on study integrity.
- The protocol also states that the time between sample preparation and analysis should not exceed 35 h. For the cysteine run reported in this study, the time prior to analysis of the last sample was ca 41 h. However, there was no evidence of sample degradation (from the peptide peak areas) towards the end of the batch, therefore the samples and results were still acceptable. There is no impact on study integrity.

DEMONSTRATION OF TECHNICAL PROFICIENCY
Charles River Laboratories demonstrated technical proficiency in the DPRA test, using the panel of proficiency chemicals listed in OECD 442C (Toner, F, 2015)

Any other information on results incl. tables

Test Item	% Peptide Depletion Cysteine (Mean  ± SD)	% Peptide Depletion Lysine (Mean ± SD)	Mean of Cysteine and Lysine	DPRA Classification (Cysteine and Lysine Prediction Model)
ATP	8.6 ± 14.9	0.9 ± 0.8	4.75	Minimal Reactivity (Non-Sensitizer)
Cinnamic Aldehyde (Positive control)	80.7 ± 7.7	51.8 ± 1.2	66.3	High Reactivity (Sensitizer)

Using the cysteine and lysine prediction model (see Table below) the test material was categorised as minimally reactive and a non-sensitiser.

Mean depletion values (Cys Lys)	Mean Depletion values (cys only)	Reactivity classification	DPRA Prediction
<6.38 %	<13.89%	Minimal	Non Sensitizer
6.38 -22.62%	13.89 -23.09%	Low	Sensitizer
22.62 -42.47%	23.09%-98.24%	Moderate	Sensitizer
>42.47	>98.24%	High	Sensitizer

Applicant's summary and conclusion

Interpretation of results:

other: minimally reactive: non-sensitizer

Conclusions:

In conclusion, according to the DPRA cysteine and lysine prediction model, ATP, Di-Na (CAS 987-65-5) was classified as minimally reactive and was, therefore, a non-sensitiser.

Executive summary:

Skin sensitisation is a type IV (delayed) hypersensitivity reaction that results from the interaction of a sensitising agent with host proteins to form an immunogenic complex.

Small molecules that can interact with proteins in this way are referred to as haptens, and are generally not immunogenic in isolation. Hapten-modified proteins are recognised as foreign by antigen presenting cells, leading to T-cell activation and localised inflammation at the site of all subsequent exposures to the hapten.

Most skin sensitising agents are electrophiles, i.e. will accept an electron pair from a nucleophile to form a covalent bond. The amino acids cysteine and lysine are thought to be the nucleophiles most frequently modified in proteins during sensitisation, and the ability of small molecules to react with these amino acids forms the basis of the Direct Peptide Reactivity Assay (DPRA).

The objective of this study was to assess the peptide binding capability of ATP, Di-Na (CAS 987-65-5) using synthetic cysteine and lysine peptides and to classify the test item to one of the four reactivity classes leading to a DPRA prediction according to the following prediction model.

Mean depletion values (Cys Lys)	Mean Depletion values (cys only)	Reactivity classification	DPRA Prediction
<6.38 %	<13.89%	Minimal	Non Sensitizer
6.38 -22.62%	13.89 -23.09%	Low	Sensitizer
22.62 -42.47%	23.09%-98.24%	Moderate	Sensitizer
>42.47	>98.24%	High	Sensitizer

The reaction of the test item with synthetic peptides containing cysteine (Ac-RFAACAA-COOH) or lysine (Ac-RFAAKAA-COOH) was performed.  The custom peptides contained cysteine or lysine as the nucleophilic reaction centres and phenylalanine to facilitate detection by HPLC analysis.

The solubility of the test item was previously assessed under Charles River Study No. 799765 and ultrapure water selected as the most suitable solvent for use in both peptide assays (Vinall, J, 2017). The test item and peptides were combined and incubated together for ca 24 h at ambient temperature.  The test item was prepared at a concentration of 100 mM.  Following this incubation, the concentration of free (i.e. unreacted) peptide remaining was measured by HPLC.  From the results obtained, a reactivity class was assigned and a DPRA prediction was made according to the above criteria.  Both peptide assays were successfully run with all acceptance criteria being met.

The results obtained are presented in the following table:

Test Item	% Peptide Depletion Cysteine (Mean  ± SD)	% Peptide Depletion Lysine (Mean ± SD)	Mean peptide depletion (%)	DPRA Classification (Cysteine and Lysine Prediction Model)
ATP	8.6 ± 14.9	0.9 ± 0.8	4.75	Minimal Reactivity (Non-Sensitizer)
Cinnamic Aldehyde (Positive control)	80.7 ± 7.7	51.8 ± 1.2	66.3	High Reactivity (Sensitizer)

All acceptance criteria were fulfilled.  There was no evidence of co-elution of ATP, Di-Na with either Cysteine or Lysine peptide.  Peptide depletion was calculated as 0.9% and 8.6% in Lysine and Cysteine Assays, respectively, resulting in a mean peptide depletion of 4.75%.  This value places ATP, Di-Na in the minimal reactivity classification resulting in a DPRA prediction of Non-Sensitiser.

In conclusion, according to the DPRA cysteine and lysine prediction model, ATP, Di-Na (CAS 987-65-5) was classified as minimally reactive and was, therefore, a non-sensitiser.