Disilver oxide

Administrative data

Endpoint:

basic toxicokinetics in vivo

Type of information:

experimental study

Adequacy of study:

key study

Study period:

2020-2021

Reliability:

1 (reliable without restriction)

Rationale for reliability incl. deficiencies:

guideline study

Cross-referenceopen allclose all

Data source

Materials and methods

Objective of study:

absorption

bioaccessibility (or bioavailability)

tissue distribution

GLP compliance:

yes (incl. QA statement)

Test material

Radiolabelling:

no

Test animals

Species:

rat

Strain:

Sprague-Dawley

Details on species / strain selection:

Crl:CD IGS (SD)

Sex:

male/female

Details on test animals or test system and environmental conditions:

TEST ANIMALS
- Source: Charles River UK
- Age at study initiation: 8-10 weeks old at start of treatment
- Weight at study initiation: min. 170 g for females and 200 g for males
- Housing: up to four animals of the same sex per cag. Within each group, cages will be blocked together (by sex). The distribution of the groups within and between racks and the position of the racks within the room will be determined to equalize environmental influences across the study while minimizing the opportunity for inter-group contamination.
- Diet (e.g. ad libitum): SDS VRF-,1 pelleted diet, non-restricted availability (diet contains no added antibiotic or other chemotherapeutic or prophylactic agent)
- Water (e.g. ad libitum): potable water from the public supply, non-restricted availability via polycarbonate bottles with sipper tubes (except during urine collection)
- Acclimation period: at least 5 days before commencement of treatment
- Health status: visually inspected at least twice daily for evidence of ill-health

ENVIRONMENTAL CONDITIONS
- Temperature (°C): monitored and maintained within the range of 20-24ºC
- Humidity (%): monitored and maintained within the range of 40-70%
- Air changes (per hr): air filtered, not recirculated
- Photoperiod (hrs dark / hrs light): 12 hours light : 12 hours dark
- Fasting period : none

IN-LIFE DATES: study performed in phases, with first phase started on 30 Sep 2020 and last (repeated) phase ended on 20 Aug 2021

Administration / exposure

Route of administration:

oral: gavage

Vehicle:

water

Details on exposure:

PREPARATION OF DOSING SOLUTIONS:
Notes:
- Chloride and phosphate containing vehicles and reagents were avoided due to the potential for silver precipitation effects.
- Dissolved silver and silver particles adsorb onto material surfaces including glass and metals, and as such use of these was avoided.
- Formulations were protected from light during preparation (use of yellow-light instead).
- The formulation procedures are documented in the study data and will be included in the final report.
- The pH of the final formulations was measured and recorded in the data.
- A series of formulations at the required concentrations is prepared by dilution of individual weighing of the Test Item and dispensed in polypropylene screw top jars or similar

Method of preparation:
The required amount of test item was weighed out, (Ag Acetate was ground in a pestle and mortar) and then added to ca 50% of the final volume of vehicle and magnetically stirred to mix/disperse. The ‘weighing’ vessel was rinsed, and the rinsing is added to the container before bringing to volume with the vehicle. The mixture was then transferred to a magnetic stirrer and stirred for a minimum of 20 minutes, recording the start and finish times in the raw data. Formulation analysis sampling will occur whilst under constant stirring, prior to dispensing and aliquoting into suitable containers for dose administration (stirrer bars will be included).

Frequency of preparation:
- Repeat dose formulations were prepared weekly and split into daily aliquots.
- The suitability and homogeneity of formulations were confirmed as part of studies, undertaken separately by third parties designated by the Sponsor, and by the Principal Investigator for dose formulation analysis.

Storage of formulation: Silver solutions – ambient temperature (15 to 25°C), protected from light.

Duration and frequency of treatment / exposure:

Two treatments:
- single oral dose: single occasion on day 1
- repeat oral doses: 28 days; frequency: once daily at approximately the same time each day

Doses / concentrationsopen allclose all

No. of animals per sex per dose / concentration:

4 males + 4 females

Control animals:

yes, concurrent vehicle

Details on study design:

Rationale for Dose Level Selection and Route:
The dose levels for silver acetate (AgAc) have been chosen to support a program of reproductive toxicology studies on this compound. Based on existing toxicity data for AgAc, from repeated administration studies in rodents the dose levels are expected to be well tolerated.

Details on dosing and sampling:

TOXICOKINETIC STUDY (Absorption, distribution, excretion)
- Tissues and body fluids sampled: blood, brain, bone marrow, small intestine, liver, spleen, ovaries, testes, uterus
- Time and frequency of sampling: blood: Day 15: PD, 6 hours post-dose, Day 28: PD, 3, 6, 9, 12, 24, 72, 96 hours post-dose. (10 time points) ; tissues: at termination (after 28 days treatment)

ANALYTICAL METHOD
Total Ag concentrations were determined in whole blood and tissues by ICP-MS after microwave digestion with nitric acid and hydrochloric acid. This method was successfully validated with a lower limit of quantification (LLOQ) of 10 ng/mL for silver in rat blood4 and 30 ng/g for silver in rat tissue.

Statistics:

- Ag analysis data were acquired and integrated using MassHunter (version C.01.05 Agilent). Peak area results were exported to Watson LIMS (Version 7.5 SP1, Thermo Scientific) in text file format. Watson LIMS was used to calculate standard curve parameters and concentration data for Silver. The concentration and statistical data were generated by computerized techniques.
- AUC(0-t): area under the concentration-time curve from hour 0 to the last measurable concentration, estimated by the linear trapezoidal rule.

Results and discussion

Main ADME resultsopen allclose all

Toxicokinetic / pharmacokinetic studies

Details on absorption:

- Comparisons via normalised administered doses (i.e. Ag equivalent dose) can be made between Ag acetate and bulk Ag (AgMP). Based on these matched dose assessments, the extent of systemic exposure was about 10 to 30-fold lower in the case of Ag metal powder versus AgAc
- The maximum observed Ag concentration in blood occurs between 3-9h post-dosing for repeat dose groups.

Details on distribution in tissues:

- Levels of Ag distributed into tissues and organs are similar for AgAc and AgNO3 (but considerably lower in the case of AgMP ).
- The study shows that the testis and brain are minor sites of distribution. In contrast, the ovary has been shown to be an important site of distribution. However, ancillary investigations strongly suggest silver is present in the ovary as chemically stable silver sulphide/selenide complexes with very low local bioavailability.

Details on excretion:

not investigated

Toxicokinetic parametersopen allclose all

Metabolite characterisation studies

Metabolites identified:

no

Remarks:

n.a.

Details on metabolites:

n.a.

Any other information on results incl. tables

Systemic exposure / Ag in blood

- Figure 1 (attached below) shows the extent of systemic exposure as area under the concentration time curve (AUC) values after repeated dose administration of silver acetate (AgAc) for 28 days.

- Comparisons via normalised administered doses (i.e. Ag equivalent dose) can be made between different Ag test items. Based on these matched dose assessments, the extent of systemic exposure was similar for AgAc and AgNO3 but about 10 to 30-fold lower in the case of Ag metal powder versus a reference ionic Ag salt.

- Table 2 shows the blood Ag concentrations at predicted steady state (day 15) after repeated dose administration of AgAc. The maximum observed concentration occurs between 3-9h post-dosing for repeat dose groups, hence the 6h values for the respective test substances are shown as an indicator of peak exposure.

Table 2.  Blood Ag concentrations at day 15 after repeated oral dose administration of silver acetate (AgAc).

Dose level	Mean 6h blood [Ag]		Mean [Ag]6h/
(mg/kg Test Item bw/d)	ng/mL		Ag Equiv. Dose
			ng/mL
	♂	♀	♂	♀
Control	<LLOQ	<LLOQ	--	--
		(n=3)
5	113	204	34.8	62.8
	± 15	± 26
55	317	423	8.9	11.8
	± 93	± 72
175	652	918	5.7	8.1
	± 171	± 103
	(n=3)	(n=3)

- Comparing these data to the data for other Ag test items, this demonstrates that oral dosing of AgAc and AgNO3 lead to similar systemic exposure and AgMP leads to appreciably lower Ag amplitude of systemic exposure in comparison to ionic Ag forms.

 

Tissue exposure / Ag distribution

Table 3 shows the Ag tissue levels / distribution after repeated dose administration of AgAc.

Table 3. Terminal Ag tissue levels following repeated oral dose administration for 28 days of silver acetate (AgAc)

 

Dose (mg/kg bw/d) /Sex		Bone marrow	Brain	GI tract	Spleen	Testis	Liver
Control M	Mean	BLQ	BLQ	BLQ	BLQ	BLQ	BLQ
5 M	Mean	62.0	142	2770	283	168	55.4
	SD	13.5	36.0	1720	71.2	75.9	15.3
55 M	Mean	3500	637	19200	38700	1510	9470
	SD	1540	57.2	7680	11000	215	4120
175 M	Mean	21400	1460	83200	96400	1530	22700
	SD	15400	33.1	5270	55200	237	7630

Dose(mg/kg bw/d) /Sex		Bone Marrow	Brain	GI Tract	Spleen	Ovaries	Uterus	Liver
Control F	Mean	BLQ	BLQ	BLQ	BLQ	BLQ	BLQ	BLQ
5 F	Mean	126	169	3800	990	2200	188	305
	SD	110	21.2	1490	455	1080	121	232
55 F	Mean	4500	805	50700	60800	24300	8000	16500
	SD	1420	35.9	11200	10400	2610	3300	3610
175 F	Mean	46800	1460	104000	142000	39700	11100	21900
	SD	19800	114	12600	93500	19800	2320	13100

BLQ    <5.00 ng/mL

- Comparing these data to the data for other Ag test items, this demonstrates that levels of Ag distributed into tissues and organs are similar for AgAc and AgNO3 but considerably lower in the case of Ag metal powder.

Applicant's summary and conclusion

Conclusions:

This in-vivo toxicokinetic study (in rats) by oral gavage comparing silver metal powder, nanosilver, silver nitrate and silver acetate shows a lower absorption/distribution and lower systemic exposure to tissues and organs for silver metal powder than for the other silver substances. The amount of Ag+ in blood and tissues is much higher for silver acetate/silver nitrate than for silver metal powder at comparable Ag dosing levels. Although all silver-containing substances have the ability to release Ag+, the extent of released silver ions is significantly different between substances. Therefore, a direct read-across of mammalian toxicity datasets for simple ionic silver salts like silver acetate or silver nitrate and nanosilver to silver metal powder/massive is not supported (from a scientifically valid toxicokinetic perspective).

Executive summary:

This in-vivo toxicokinetic study is an oral route investigation using adult CD Sprague Dawley rats. The design conformed to OECD TG 417 and was conducted in compliance to GLP. The study was designed as a comparative toxicokinetic assessment of the test items Silver Acetate (AgAc), Silver Nitrate (AgNO3), Micron-sized Silver (AgMP) and Nanoparticulate Silver (AgNP). This included assessment of bioavailability following single oral doses relative to single intravenous doses and systemic exposure following single and repeat oral doses. Groups of 4 male and 4 female CD Sprague Dawley rats were administered the test items, either as a single intravenous dose, a single oral dose or repeated daily oral doses for 4 weeks.

The systemic exposure (28 days) results show a difference in the extent of absorption and systemic circulation for silver acetate and nitrate versus silver metal powder. Based on a matched dose assessment, the extent of systemic exposure was about 10 to 30-fold lower in the case of silver metal powder versus silver acetate (as reference ionic silver compound).

The silver tissue levels after repeated dose administration are considerably lower in the case of silver metal powder (AgMP) than for silver acetate. This suggests that AgMP represents a correspondingly lower health hazard, i.e. AgMP (and by extrapolation also massive Ag with a tremendously lower particle size/reactive surface area) is expected to cause less effects at corresponding Ag dose levels than AgAc.

In conclusion, it is assumed that the systemic toxicity of silver substances is driven by the release potential of Ag ionic species as the primary moiety for systemic circulation and tissue exposure, and hence hazard assessment. The comparative TK study is a high quality GLP investigation and the first which permits a direct comparison of systemic circulation and tissue distribution of Ag ionic species between soluble Ag salts (AgNO₃and Ag acetate), AgNP and AgMP. This new evidence demonstrates that oral intake of AgMP results in markedly lower absorption, distribution and systemic tissue/organ exposure to silver than more bioavailable forms like AgAc. As a generic observation, the following trend is being observed: AgAc > AgNO₃>> AgNP >>> AgMP.

The study findings show that the direct read-across of mammalian toxicity data with soluble silver salts (like silver acetate and silver nitrate) and nanosilver to silver metal (powder and massive) is not justified (based on their individual toxicokinetic profiles).