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ASTM E1398-91(2003)

(Practice)

Standard Practice for the in vivo Rat Hepatocyte DNA Repair Assay

Standard Practice for the in vivo Rat Hepatocyte DNA Repair Assay

SCOPE
1.1 This practice covers a typical procedure and guidelines for conducting the rat in vivo hepatocyte DNA repair assay. The procedures presented here are based on similar protocols that have been shown to be reliable (1, 2, 3, 4, 5).  
1.2 Mention of trade names or commercial products are meant only as examples and not as endorsements. Other suppliers or manufacturers of equivalent products are acceptable.
1.3 This standard does not purport to address all of the safety problems associated with its use. It is the responsibility of the user of this standard to establish appropriate safety and health practices and determine the applicability of regulatory limitations prior to use.

General Information

Status
Historical
Publication Date
09-Sep-2003
ICS
11.220 - Veterinary medicine
Technical Committee
F04 - Medical and Surgical Materials and Devices
Drafting Committee
F04.16 - Biocompatibility Test Methods
Current Stage
Ref Project

Relations

Replaces
ASTM E1398-91(1998) - Standard Practice for the in vivo Rat Hepatocyte DNA Repair Assay
Effective Date
10-Sep-2003
Replaced By
ASTM E1398-91(2008) - Standard Practice for <i>In Vivo</i> Rat Hepatocyte DNA Repair Assay (Withdrawn 2014)
Effective Date
01-Aug-2008
Referred By
ASTM F1439-03(2018) - Standard Guide for Performance of Lifetime Bioassay for the Tumorigenic Potential of Implant Materials
Effective Date
10-Sep-2003

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ASTM E1398-91(2003) - Standard Practice for the in vivo Rat Hepatocyte DNA Repair AssayASTM E1398-91(2003) - Standard Practice for the in vivo Rat Hepatocyte DNA Repair Assay
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ASTM E1398-91(2003) - Standard Practice for the in vivo Rat Hepatocyte DNA Repair Assay
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NOTICE: This standard has either been superseded and replaced by a new version or withdrawn.
Contact ASTM International (www.astm.org) for the latest information
Designation:E1398–91 (Reapproved 2003)
Standard Practice for
In Vivo Rat Hepatocyte DNA Repair Assay
This standard is issued under the fixed designation E1398; the number immediately following the designation indicates the year of
original adoption or, in the case of revision, the year of last revision.Anumber in parentheses indicates the year of last reapproval.A
superscript epsilon (e) indicates an editorial change since the last revision or reapproval.
1. Scope from the patterns of activation and detoxification that actually
occurinhepatocytes.Anextensiveliteratureisavailableonthe
1.1 This practice covers a typical procedure and guidelines
use of in vitro DNA repair assays (9-19).
forconductingtheratinvivohepatocyteDNArepairassay.The
2.2 Afurther advance was the development of an in vivo rat
procedures presented here are based on similar protocols that
hepatocyte DNA repair assay in which the test chemical is
have been shown to be reliable (1, 2, 3, 4, 5).
administered to the animal and the resulting DNA repair is
1.2 Mention of trade names or commercial products are
assessed in hepatocytes isolated from the treated animal (20).
meant only as examples and not as endorsements. Other
Numerous systems now exist to measure chemically induced
suppliers or manufacturers of equivalent products are accept-
DNA repair in specific tissues in the whole animal (4). The
able.
average of in vivo assays is that they reflect the complex
1.3 This standard does not purport to address all of the
patterns of uptake, distribution, metabolism, detoxification,
safety concerns associated with its use. It is the responsibility
and excretion that occur in the whole animal. Further, factors
of the user of this standard to establish appropriate safety and
such as chronic exposure, sex differences, and different routes
health practices and determine the applicability of regulatory
of exposure can be studied with these systems. This is
limitations prior to use.
illustrated by the potent hepatocarcinogen 2,6-dinitrotoluene
2. Significance and Use (DNT). Metabolic activation of 2,6-DNT involves uptake,
metabolism by the liver, excretion into the bile, reduction of
2.1 Measurement of chemically induced DNA repair is a
the nitro group by gut flora, readsorption, and further metabo-
means of assessing the ability of a chemical to reach and alter
lism by the liver once again to finally produce the ultimate
the DNA. DNA repair is an enzymatic process that involves
genotoxicant (21). Thus, 2,6-DNT is negative in the in vitro
recognition and excision of DNA-chemical adducts, followed
hepatocyte DNArepair assay (22) but is a very potent inducer
by DNA strand polymerization and ligation to restore the
of DNA repair in the in vivo DNA repair assay (23, 24).A
original primary structure of the DNA(6).This process can be
problem with tissue-specific assays is that they may fail to
quantitated by measuring the amount of labeled thymidine
detect activity of compounds that produce tumors in other
incorporated into the nuclear DNA of cells that are not in
target tissues. For example, no activity is seen in the in vivo
S-phaseandisoftencalledunscheduledDNAsynthesis(UDS)
DNA repair assay with the potent mutagen benzo(a)pyrene
(7). Numerous assays have been developed for the measure-
(BP), probably because limited tissue distribution and greater
ment of chemically induced DNA repair in various cell lines
detoxification in the liver yields too few DNA adducts to
and primary cell cultures from both rodent and human origin
produce a measurable response (3). In contrast, BP is readily
(4). The primary culture rat hepatocyte DNA repair assay has
detected in the less tissue-specific in vitro hepatocyte DNA
proven to be particularly valuable in assessing the genotoxic
repair assay (11). An extensive literature exists on the use of
activity of chemicals (8). Genotoxic activity often results from
the in vivo hepatocyte DNA repair assay (1-3, 5, 9, 25-33).
metabolites of a chemical. The in vitro rat hepatocyte assay
provides a system in which a metabolically competent cell is
3. Procedure
also the target cell. Most other in vitro short-term tests for
3.1 Treatment:
genotoxicityemployaratliverhomogenate(S-9)formetabolic
3.1.1 All personnel must be knowledgeable in the proce-
activation, which differs markedly in many important ways
dures for safe handling and proper disposal of carcinogens,
potential carcinogens, and radiochemicals. Disposable gloves
ThispracticeisunderthejurisdictionofASTMCommitteeF04onMedicaland
and lab coats must be worn.
Surgical Materials and Devices and is the direct responsibility of Subcommittee
3.1.2 Any strain or sex of rat may be used. The largest
F04.16 on Biocompatibility Test Methods.
database is for male Fischer-344 rats.Young adult animals are
Current edition approved Sept. 10, 2003. Published September 2003. Originally
published in 1991. Last previous edition published in 1998 as E1398–91 (1998).
preferred. It is possible that factors such as sex, age, and strain
The boldface numbers in parentheses refer to the list of references found at the
of the rat could affect the outcome of the DNA repair
end of this practice.
Copyright © ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959, United States.
E1398–91 (2003)
experiments. Therefore, for any one series of experiments 3.2.2 DMN exhibits a maximum UDS response 1 h after
(including controls) these variables should be kept constant. treatment. However, the response remains elevated and mea-
surable for at least 16 h after treatment. More commonly,
3.1.3 Administration is usually by gavage with chemicals
however, chemicals (for example, 2,6-DNT and
dissolved or suspended in an appropriate vehicle such as water
2-acetylaminofluorene (2-AAF)) show a peak response 12 to
or corn oil, depending on solubility.An advantage of the assay
16 h post-treatment.The time from treatment to perfusion may
is that various routes of administration may be chosen. Thus,
bevariedtoobtainatimecourseofinducedrepair.Theroutine
chemicals may also be administered by intraperitoneal injec-
protocol for primary screening involves a time point between
tion or inhalation or in the diet. For gavage administration, 0.2
12 and 16 h with an optional time point between 1 and 4 h.
to 1.0 mL of test chemical solution is administered per 100 g
3.2.3 Anesthetize the rat by intraperitoneal injection with a
bodyweight.Controlsreceivetheappropriatevehiclesolution.
Stock corn oil should be replaced with fresh monthly. 50-mg/mLsolution of sodium pentobarbital (0.2 mLper 100 g
body weight) 10 min prior to the perfusion procedure. Other
3.1.4 ForDNArepairstudies,animalsmaybetakenofffeed
proven anesthetics are also acceptable. Make sure that the
for a few hours prior to sacrifice to make the process of
animal is completely anesthetized, so that it feels no pain.
perfusion a little easier with less food in the stomach. The
3.2.4 Secure the animal with the ventral surface up on
period without food should never exceed 12 h because of the
absorbent paper attached to a cork board. Fold the paper in on
possibility of altered metabolism or uptake. Water should be
each edge to contain perfusate overflow. Thoroughly wet the
continuously available.
abdomen with 70% ethanol and wipe with gauze for cleanli-
3.1.5 Dose selection will depend on the characteristics of
nessandtodiscourageloosefurfromgettingontheliverwhen
each chemical and the purpose of the experiment. If one is
the animal is opened.
investigating whether a chemical can produce a genotoxic
3.2.5 Make a V-shaped incision through both skin and
effect in the animal, even at massive doses and by routes of
muscle from the center of the lower abdomen to the lateral
administration that may overwhelm natural defense mecha-
aspects of the rib cage. Do not puncture the diaphragm or cut
nisms, then high doses (such as the LD50, or higher) that do
theliver.Foldbacktheskinandattachedmuscleoverthechest
not kill the animal before the 16-h sacrifice point may be
to reveal the abdominal cavity.
employed. Even in such a case, doses above 1000-mg/kg body
3.2.6 Placeatubeapproximately1cmindiameterunderthe
weightarenotrecommended.Insomeinstanceshepatotoxicity
back to make the portal vein more accessible.
at high doses may result in inhibition of cell attachment or
DNA repair. More commonly, the purpose of employing the 3.2.7 Movetheintestinesgentlyouttotherighttorevealthe
whole animal is to evaluate the genotoxic effects of realistic portal vein.Adjust the tube under the animal so that the portal
exposures and routes of administration in the target tissue. In vein is horizontal.
this case, doses above 500 mg/kg and the intraperitoneal route 3.2.8 Put a suture in place (but not tightened) in the center
of administration are not recommended. The usual range of
of the portal vein and another around the vena cava just above
doses is from 10 to 500 mg compound per kilogram body the right renal branch.
weight. Target doses with a new compound are usually the
3.2.9 Perform perfusions with a peristaltic pump, the tubing
LD50 and 0.2 3the LD50, with 500 mg/kg as an upper limit.
of which is sterilized by circulation of 70% ethanol followed
The potent mutagen dimethylnitrosamine (DMN) (often used
by sterile water. Place a valve in the line so that the operator
as a positive control) can be detected with doses as low as 1
mayswitchfromtheEGTAsolutiontothecollagenasesolution
mg/kg. Normally, an initial range finding experiment is con-
without disrupting the flow. Solutions should be kept at a
ducted using single animals to cover a range of times and
temperature that results in a 37°C temperature at the hepatic
doses.Ifapositiveresponseisseen,additionalexperimentsare
portal vein.
conducted to establish the dose-response relationship. If no
3.2.9.1 Aperistalticpumpwithachargeablepumpheadand
response is seen, the highest dose(s) is repeated. The final
silicone tubing is suitable for performing the perfusion.
report should contain results from at least three animals per
3.2.9.2 Begin the flow of the 37°C EGTA solution at 8
datapoint.
mL/min and run to waste.
3.1.6 Thus far, no examples have been seen of a compound 1
3.2.10 Cannulate the portal vein with a 20 GA 1 ⁄4-in.
thatproducesaUDSresponseinfemaleratsbutnotmales.For
catheter about 3 mm below the suture. Remove the inner
thosecaseswhereacomparisonhasbeenmade,malesrespond
needle and insert the plastic catheter further to about ⁄3 the
more strongly than females in this assay.Thus, for the purpose
length of vein and tie in place by the suture. Blood should
of routine screening only male rats need to be used.
emerge from the catheter. Insert the tube with the flowing
3.1.7 Treated animals should be maintained in a ventilated
EGTA in the catheter (avoid bubbles) and tape in place.
area or other suitable location to prevent possible human
3.2.11 Immediately cut the vena cava below the right renal
exposure to expired chemicals. Contaminated cages, bedding,
branch and allow the liver to drain of blood for 1.5 min. The
excreta, and carcasses should be disposed of safely according
liver should rapidly clear of blood and turn a tan color. If all
to standard published procedures.
lobes do not clear uniformly, the catheter has probably been
3.2 Liver Perfusion:
inserted too far into the portal vein.
3.2.1 Any proven technique which allows the successful 3.2.12 Tightenthesuturearoundthevenacavaandincrease
isolation and culture of rat hepatocytes can be used. An the flow to 20 mL/min for 2 min.The liver should swell at this
example of one such procedure is given in 3.2.2-3.2.17. point. In some cases gentle massaging of the liver or adjusting
E1398–91 (2003)
the orientation of the catheter may be necessary for complete for control cultures. With practice and the proper technique,
clearing. At this point the vena cava above the suture may be viabilitiesofabout90%canroutinelybeobtained.Attachment
clipped to release some of the pressure in the liver. of the cells to the substrate is an active process. Thus, if a
3.2.13 Switch the flow to the 37°C collagenase solution for sufficientnumberofcellsattachtoconducttheexperiment,this
is a further indication of the viability of the culture.
12 min. During this period, cover the liver with sterile gauze
wetted with sterile saline or WEI (see Annex A1) and place a 3.3.10 Placea25-mmroundplasticcoverslipintoeachwell
40-W lamp 2 in. above the liver for warming. It is valuable to of 6-well culture dishes. 10.5 by 22-mm plastic coverslips and
screen each new batch of collagenase to be ensured that it will 26 by 33-mm eight-chamber culture dishes can also be used.
function properly. Be sure to keep the proper side up as marked on the package.
FourmillilitresofWEC(seeAnnexA1)areaddedtoeachwell.
3.2.14 Allowtheperfusatetoflowontothepaperandcollect
by suction into a vessel connected by means of a trap to the Hepatocyteswillnotattachtoglassunlesstheslideshavebeen
boiled. The use of collagen-coated thermanox coverslips im-
vacuumline.Theperfusateshouldbedisposedofashazardous
waste. proves cell attachment and morphology.
3.2.15 Aftertheperfusioniscompleted,removethecatheter 3.3.10.1 Theseproceduresyieldpreparationsconsistingpri-
marily of hepatocytes.Approximately 400000 viable cells are
and gauze. Remove the liver carefully by cutting away the
membranes connecting it to the stomach and lower esophagus, seeded into each well and distributed over the coverslip by
shaking or stirring gently with a plastic 1-mL pipet. Glass
cutting away the diaphragm, and cutting any remaining attach-
ments to veins or tissues in the abdomen. pipettes can scratch the coverslips.
3.2.16 Hold the liver by the small piece of attached dia- 3.3.11 Incubate the cultures for 90 to 120 min in a 37°C
incubator with 5% CO and 95% relative humidity to allow
phragm and rinse with sterile saline or WEI (see Annex A1).
the cells to attach.
3.2.17 Place the liver in a sterile petri dish and take to a
sterile hood to prepare the cells. 3.4 Labeling the Cultures:
3.3 Preparation of Hepatocyte Cultures: 3.4.1 After the 90-min attachment, wash cultures once with
3.3.1 Place the perfused liver in a 60-mm petri dish and 4mLWEI(seeAnnexA1)perwelltoremoveunattachedcells
and debris. This is done by tilting the culture slightly, aspirat-
rinse with 37°C WEI (see Annex A1). Remove extraneous
tissues (fat, muscle, and so forth). ing the media, and adding the fresh media at 37°C. Be careful
not to direct the stream from the pipet directly onto the cells.
3.3.2 Place the liver in a clean petri dish and add 30 mL of
3.4.2 Remove the WEI (see Annex A1) and replace with 2
fresh collagenase solution at 37°C.
...

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1.1 This practice is intended to determine the potential for a substance, or material extract, to elicit contact dermal allergenicity.  
1.2 The values stated in SI units are to be regarded as standard. No other units of measurement are included in this standard.  
1.3 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health and environmental practices and determine the applicability of regulatory limitations prior to use.  
1.4 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

  • Standard
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  • Standard
    3 pages
    English language
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ASTM
ASTM E2385-11(2016)(Guide)
Standard Guide for Estimating Wildlife Exposure Using Measures of Habitat Quality

SIGNIFICANCE AND USE
6.1 Explicit consideration of landscape features to characterize the quality of habitat for assessment species can enhance the ecological relevance of an EcoRA. This can help avoid assessing exposure in areas in which a wildlife species would be absent because of a lack of habitat or to bound exposure estimates in areas with low habitat quality. The measure of habitat quality is used in place of the commonly used Area Use Factor (AUF). Greater ecological realism and more informed management decisions can be realized through better use of landscape features to characterize sites.
SCOPE
1.1 Ecological Risk Assessments (EcoRAs) typically focus on valued wildlife populations. Regulatory authority for conducting EcoRAs derives from various federal laws [for example, Comprehensive Environmental Response, Compensation and Liability Act 1981, (CERCLA), Resource Conservation Recovery Act (RCRA), and Federal Insecticide, Fungicide, and Rodenticide Act, (FIFRA)]. Certain procedures for conducting EcoRAs (1-4)2 have been standardized [E1689-95(2003) Standard Guide for Developing Conceptual Site Models for Contaminated Sites; E1848-96(2003) Standard Guide for Selecting and Using Ecological Endpoints for Contaminated Sites; E2020-99a Standard Guide for Data and Information Options for Conducting an Ecological Risk Assessment at Contaminated Sites; E2205/E2205M-02 Standard Guide for Risk-Based Corrective Action for Protection of Ecological resources; E1739-95(2002) Standard Guide for Risk-Based Corrective Action Applied at Petroleum Release Sites]. Specialized cases for reporting data have also been standardized [E1849-96(2002) Standard Guide for Fish and Wildlife Incident Monitoring and Reporting] as have sampling procedures to characterize vegetation [E1923-97(2003) Standard Guide for Sampling Terrestrial and Wetlands Vegetation].  
1.2 Most states have enacted laws modeled after the federal acts and follow similar procedures. Typically, estimates of likely exposure levels to constituents of potential concern (CoPC) are compared to toxicity benchmark values or concentration-response profiles to establish the magnitude of risk posed by the CoPC and to inform risk managers considering potential mitigation/remediation options. The likelihood of exposure is influenced greatly by the foraging behavior and residence time of the animals of interest in the areas containing significant concentrations of the CoPC. Foraging behavior and residence time of the animals are related to landscape features (vegetation and physiognomy) that comprise suitable habitat for the species. This guide presents a framework for incorporating habitat quality into the calculation of exposure levels for use in EcoRAs.  
1.3 This guide is intended only as a framework for using measures of habitat quality in species specific habitat suitability models to assist with the calculation of exposure levels in EcoRA. Information from published Habitat Suitability Index (HSI) models (5) is used in this guide. The user should become familiar with the strengths and limitations of any particular HSI model used in order to characterize uncertainty in the exposure assessment (5-7). For species that do not have published habitat suitability models, the user may elect to develop broad categorical descriptions of habitat quality for use in estimating exposure.

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ASTM
ASTM D6152/D6152M-12(2024)(Specification)
Standard Specification for SEBS-Modified Mopping Asphalt Used in Roofing

ABSTRACT
This specification covers SEBS (styrene-ethylenebutylene-styrene)-modified mopping asphalt intended for use in built-up roof construction, construction of some modified bitumen systems, construction of bituminous vapor retarder systems, and for adhering insulation boards used in various types of roofing systems. This specification is intended as a material specification and issues regarding the suitability of specific roof constructions or application techniques are beyond its scope. The specified tests and property values are intended to establish minimum properties. In place system design criteria or performance attributes are factors beyond the scope of this specification. The base asphalt shall be prepared from crude petroleum and the SEBS-modified asphalt shall incorporate sufficient SEBS as the primary polymeric modifier. The SEBS modified asphalt shall be homogeneous and free of water and shall conform to the prescribed physical properties including (1) softening point before and after heat exposure, (2) softening point change, (3) flash point, (4) penetration before and after heat exposure, (5) penetration change, (6) solubility in trichloroethylene, (7) tensile elongation, (8) elastic recovery, and (9) low temperature flexibility. The sampling and test methods to determine compliance with the specified physical properties, as well as the evaluation for stability during heat exposure are detailed.
SCOPE
1.1 This specification covers SEBS (styrene-ethylene-butylene-styrene)-modified asphalt intended for use in built-up roof construction, construction of some modified bitumen systems, construction of bituminous vapor retarder systems, and for adhering insulation boards used in various types of roof systems.  
1.2 This specification is intended as a material specification. Issues regarding the suitability of specific roof constructions or application techniques are beyond its scope.  
1.3 The specified tests and property values used to characterize SEBS-modified asphalt are intended to establish minimum properties. In-place system design criteria or performance attributes are factors beyond the scope of this specification.  
1.4 The values stated in either SI units or inch-pound units are to be regarded separately as standard. The values stated in each system may not be exact equivalents; therefore, each system shall be used independently of the other. Combining values from the two systems may result in nonconformance with the standard.  
1.5 This standard does not purport to address the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health, and environmental practices and determine the applicability of regulatory limitations prior to use.  
1.6 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

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