4,4'-[(isopropylidene)bis(p-phenyleneoxy)]diphthalic dianhydride

Administrative data

Link to relevant study record(s)

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Reference 1

Endpoint:

hydrolysis

Type of information:

experimental study

Adequacy of study:

key study

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Justification for type of information:

The study was performed on the primary hydrolysis product of BPA-DA, 4,4-Bisphenol A Tetra-Acid (BPA-TA; CAS 38103-05-8). Testing on BPA-TA was in addition to testing on BPA-DA as BPA-DA was concluded to be hydrolytically unstable at pH 2, 5-6 and 9.

Reason / purpose for cross-reference:

reference to other study

Reason / purpose for cross-reference:

other: read-across target

Qualifier:

according to guideline

Guideline:

OECD Guideline 111 (Hydrolysis as a Function of pH)

Deviations:

no

GLP compliance:

yes

Remarks:

OECD GLP

Analytical monitoring:

yes

Buffers:

Buffer solutions used during this study were prepared in the following manner: pH 4 - 180 mL of 0.05 M sodium acetate (3.40 g of sodium acetate trihydrate dissolved and diluted to a final volume of 500 mL with purified reagent water) was added to 820 mL of 0.05 M acetic acid (2.88 mL of acetic acid diluted to 1000 mL with purified reagent water). The pH of the resultant solution was 3.44 and was adjusted to 4.00 with 1 N sodium hydroxide; pH 7 - 1000 mL of 0.1 M potassium dihydrogen phosphate solution (13.65 g potassium phosphate dissolved in 1000 mL purified reagent water) was added to 580 mL of 0.1 M sodium hydroxide (100 mL of 1.0 M sodium hydroxide dissolved in 1000 mL purified reagent water) and diluted to 2000 mL with purified reagent water. The pH of the resultant solution was 7.01 and required no adjustment; and pH 9 - 100 mL of 0.5 M boric acid solution (30.9 g of boric acid dissolved in 1000 mL purified reagent water) was diluted to 1000 mL with purified reagent water. The pH of the resultant solution was 9.00 and required no adjustment.

Buffers were autoclaved at approximately 120°C at 15 psi for 30 minutes. Prior to dosing, the buffer solutions were purged with sterile nitrogen for approximately 5 minutes to exclude oxygen. The sterility of the prepared buffers was confirmed on day 0 and day 5. Sterility was evaluated using aerobic count plates. A 0.5-mL aliquot of each dosed sample was pipetted onto the center of the bottom film and spread using a spreader. Plates were incubated at room temperature for at least 48 hours and then observed for microbial growth on days 0 and 5. Plates were interpreted as positive, indicating the presence of microbial growth, or as negative, indicating the absence of microbial colony formation.

Details on test conditions:

Hydrolysis in Buffers Experiment:
All standard reagent solutions were prepared using sterilised reagent water. The filter-sterilised water typically shows greater than 16.7 Mohm-cm resistivity and less than 1 mg/L total organic carbon, which is the established detectable limit at this laboratory. All chemicals were obtained from commercial sources and are at least reagent grade.

A 2.5 mg/mL BPA-TA primary stock solution was prepared by placing 0.2521 g of the test substance in a 100-mL volumetric flask and bringing it to volume with methanol. This stock solution was used to fortify calibration standards, test and QC samples during the preliminary test.

Prior to testing, the vials and pipettes used to transfer solutions were autoclaved at approximately 121 °C at 15 psi for 30 minutes, to minimize the potential for microbial degradation of the test substance. Individual 10-mL amber vials (eight vials per buffer solution) were filled with 4.96 mL of the appropriate buffer solution (i.e., pH 4, 7 or 9). To each 10-mL vial was added 40 microL of the 2.5 mg/mL BPA-TA stock solution to provide a nominal concentration of 20.0 mg/L. The vials were capped with aluminum crimp caps fitted with Teflon-lined rubber septa and vortexed for 20 seconds. The vials were placed in an incubator designed to maintain a temperature of 50°C for a period of 5 days. Analysis of the test solutions for BPA-TA concentration was performed on day 0 and day 5. In addition, two QC samples were prepared at a concentration of 20.0 mg/L in buffers of varying pH (i.e., 4, 7 or 9). The QC samples were prepared at each sampling interval and were analyzed along with the test samples. The results of the QC sample analyses were used to judge the precision and quality control maintained during the analytical process. All samples were mixed with 1.25 mL of 0.5% phosphoric acid in acetonitrile prior to HPLC analysis. Acceptance criteria for the recovery of QC samples were set at 80.0 to 120% of the prepared concentration. All hydrolysis solutions and QC samples were analyzed for BPA-TA using high performance liquid chromatography with ultraviolet detection (HPLC/UV) based on methodology validated at the testing laboratory. The method validation study was conducted prior to the initiation of the test and established an average recovery of 99.8% ± 5.93% from pH 5, 7, and 9 buffer solutions. Conditions and procedures used throughout the analysis of the test and quality control (QC) samples during this study were the same as those described in the method validation study with the following exceptions: 1) the pH buffers used during the hydrolysis study were pH 4, 7 and 9, while the pH buffers used during the method validation were pH 5, 7, and 9. The method validation was conducted to support Kow testing, requiring pH 5, and hydrolysis testing required pH 4, and 2) the nominal concentration used during the hydrolysis test was 20.0 mg/L, while the method validation range was up to 10.0 mg/L. Since both studies used acetate buffer solutions and QC samples (nominal concentration of 20.0 mg/L) were all within the required range, these exceptions did not negatively impact the study results.

The pH of the test solutions was measured on test day 0 (before and after dosing) and day 5. The pH was determined to the nearest 0.01 pH unit using a Jenco Model 60 pH meter. The temperature was monitored continually.

The percent of nominal at each time point is calculated by:
% nominal = (Ct / C0)* 100
where:
C0 = initial concentration, mg/L
Ct = measured concentration at time t in days

Duration:

5 d

pH:

4

Temp.:

50 °C

Initial conc. measured:

20 g/L

Duration:

5 d

pH:

7

Temp.:

50 °C

Initial conc. measured:

20 g/L

Duration:

5 d

pH:

9

Temp.:

50 °C

Initial conc. measured:

20 g/L

Test performance:

The temperature of the water bath used to control the temperature of the test solutions ranged from 49.9 to 50.3°C. Measurements of pH recorded in the test solutions showed that the buffering capacity had not been decreased.

The hydrolysis was performed in pH 4 (0.05 M acetate), pH 7 (0.05 M phosphate) and pH 9 (0.05 M borate) sterile aqueous buffer solutions at an application rate of 20 mg/L (20 ppm). At selected intervals, duplicate samples were analysed directly by high performance liquid chromatography with ultraviolet detection (HPLC/UV) to quantify the test substance present in the aqueous samples.

Concentrations of BPA-TA measured during the hydrolysis test showed that less than 10% degradation of BPA-TA was observed after 5 days incubation at 50 ± 0.5°C in sterile pH 4, pH 7 and pH 9 buffer samples. The test substance was considered to be hydrolytically stable (half-life greater than 1 year) and no additional testing was performed.

Analysis of QC samples resulted in measured concentrations that were consistent with the acceptable range. Based on these results, it was established that the appropriate precision and quality control was maintained during the analysis of the test solutions.

Transformation products:

no

Key result

pH:

4

Temp.:

50 °C

DT50:

> 1 yr

Remarks on result:

other: Less than 10 % degradation in 5 days

Key result

pH:

7

Temp.:

50 °C

DT50:

> 1 yr

Remarks on result:

other: Less than 10 % degradation in 5 days

Key result

pH:

9

Temp.:

50 °C

DT50:

> 1 yr

Remarks on result:

other: Less than 10 % degradation in 5 days

Concentrations of BPA-TA measured by HPLC/UV in the test and QC samples at 50ºC during the hydrolysis test

Sample	Day/ Sample No.	Target Concentration (mg a.i./L)	Area	Concentration (mg a.i./L)	% of Nominal
pH 4 buffer	Day0	20.0	2614263	19.395	96.98
	Day0	20.0	2714379	20.133	100.67
	Average				98.82
	Day5	20.0	2665233	19.776	98.88
	Day5	20.0	2672121	19.827	99.14
	Average				99.01
QC Sample	1114QC	20.0	2607271	19.344	96.72
	1119QC	20.0	2655726	19.706	98.53
pH 7 buffer	Day0	20.0	2653228	19.683	98.42
	Day0	20.0	2697684	20.010	100.05
	Average				99.23
	Day5	20.0	2733794	20.282	101.41
	Day5	20.0	2738655	20.317	101.59
	Average				101.5
QC Sample	1114QC	20.0	2673616	19.833	99.17
	1119QC	20.0	2716701	20.155	100.78
pH 9 buffer	Day0	20.0	2674464	19.839	99.20
	Day0	20.0	2691034	19.961	99.81
	Average				99.50
	Day5	20.0	2713129	20.129	100.65
	Day5	20.0	2716123	20.151	100.76
	Average				100.70
QC Sample	1114QC	20	2545432	19.961	99.81
	1119QC	20	2688286	19.946	99.73
Note: Samples were incubated at 50 ± 0.5°C for 5 days before HPLC analysis.

Validity criteria fulfilled:

yes

Conclusions:

Less than 10% degradation of the parent was observed after 5 days (half-life greater than 1 year) in the sterile pH 4, pH 7 and pH 9 buffer samples. Based on the results of this study, the BPA-TA was considered to be hydrolytically stable and no additional testing is required.