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ASTM E1619-11(2016)

(Test Method)

Standard Test Method for Chronic Oral Toxicity Study in Rats

Standard Test Method for Chronic Oral Toxicity Study in Rats

SIGNIFICANCE AND USE
5.1 This test method should generate data to identify the majority of chronic effects and shall serve to define long-term dose response relationships. In addition the test should allow for the detection of general toxic effects including neurological, physiological, biochemical, and hematological effects and exposure-related morphological (pathology) effects.  
5.2 This test method should provide information on target organs, the possibilities of accumulation, and may be used for establishing safety criteria for human exposure. It provides information on potential health hazards likely to arise from repeated exposure over a long period of time.
SCOPE
1.1 This test method covers a long-term study to determine the effects of a substance in a mammalian species such as the rat following prolonged and repeated oral exposure. Under the conditions of the chronic toxicity test, effects that require a long latency period or that are cumulative should become manifest.  
1.2 This test method assumes that the user is knowledgeable in mammalian toxicology and related pertinent areas, and relies heavily on the judgment of the evaluator.  
1.3 The values stated in SI units are to be regarded as the standard. The inch-pound units given in parentheses are for information only.  
1.4 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 and health practices and determine the applicability of regulatory limitations prior to use. For specific hazard statements, see Section 6.

General Information

Status
Published
Publication Date
31-Jan-2016
ICS
11.100.30 - Analysis of blood and urine
Technical Committee
E50 - Environmental Assessment, Risk Management and Corrective Action
Drafting Committee
E50.47 - Biological Effects and Environmental Fate
Current Stage
Ref Project

Relations

Replaces
ASTM E1619-11 - Standard Test Method for Chronic Oral Toxicity Study in Rats
Effective Date
01-Feb-2016
Refers
ASTM E609-16 - Standard Terminology Relating to Pesticides
Effective Date
15-Sep-2016
Refers
ASTM E609-15a - Standard Terminology Relating to Pesticides
Effective Date
01-May-2015
Refers
ASTM E609-15 - Standard Terminology Relating to Pesticides
Effective Date
01-Jan-2015
Refers
ASTM E609-10 - Standard Terminology Relating to Pesticides
Effective Date
01-Mar-2010
Refers
ASTM E943-08 - Standard Terminology Relating to Biological Effects and Environmental Fate
Effective Date
01-Mar-2008
Refers
ASTM E609-05 - Standard Terminology Relating to Pesticides
Effective Date
01-Apr-2005
Refers
ASTM E609-04 - Standard Terminology Relating to Pesticides
Effective Date
01-Nov-2004
Refers
ASTM E609-03a - Standard Terminology Relating to Pesticides
Effective Date
01-Oct-2003
Refers
ASTM E609-02a - Standard Terminology Relating to Pesticides
Effective Date
10-Oct-2002
Refers
ASTM E609-03 - Standard Terminology Relating to Pesticides
Effective Date
10-Oct-2002
Refers
ASTM E609-00 - Standard Terminology Relating to Pesticides
Effective Date
10-Apr-2001
Refers
ASTM E609-02 - Standard Terminology Relating to Pesticides
Effective Date
10-Apr-2001
Refers
ASTM E609-81(1997)e1 - Standard Terminology Relating to Pesticides
Effective Date
10-Apr-2001

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ASTM E1619-11(2016) - Standard Test Method for Chronic Oral Toxicity Study in RatsASTM E1619-11(2016) - Standard Test Method for Chronic Oral Toxicity Study in Rats
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ASTM E1619-11(2016) - Standard Test Method for Chronic Oral Toxicity Study in Rats
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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.
Designation: E1619 − 11 (Reapproved 2016)
Standard Test Method for
Chronic Oral Toxicity Study in Rats
This standard is issued under the fixed designation E1619; the number immediately following the designation indicates the year of
original adoption or, in the case of revision, the year of last revision. A number in parentheses indicates the year of last reapproval. A
superscript epsilon (´) indicates an editorial change since the last revision or reapproval.
1. Scope Administration, Part 58, Good Laboratory Practice for
Nonclinical Studies
1.1 This test method covers a long-term study to determine
Title 40, CFR, Toxic Substance ControlAct, Part 792, Good
the effects of a substance in a mammalian species such as the
Laboratory Practice Standards
rat following prolonged and repeated oral exposure. Under the
Title 40, CFR, Environmental Protection Agency, Part 798,
conditions of the chronic toxicity test, effects that require a
Health Effects Testing Guidelines, Subpart D, Chronic
long latency period or that are cumulative should become
Exposure, Chronic Toxicity
manifest.
1.2 This test method assumes that the user is knowledgeable
3. Terminology
inmammaliantoxicologyandrelatedpertinentareas,andrelies
3.1 Definitions—See Terminology E609 and Terminology
heavily on the judgment of the evaluator.
E943.
1.3 The values stated in SI units are to be regarded as the
3.2 Definitions of Terms Specific to This Standard:
standard. The inch-pound units given in parentheses are for
3.2.1 chronic toxicity, n—the adverse effects occurring as a
information only.
result of the daily exposure of mammalian species to a test
1.4 This standard does not purport to address all of the
substance by diet, water, capsule, or gavage for a one-year
safety concerns, if any, associated with its use. It is the
period.
responsibility of the user of this standard to establish appro-
3.2.2 concentration, n—the weight of test substance per unit
priate safety and health practices and determine the applica-
weight of the diet (expressed as milligrams per kilogram of
bility of regulatory limitations prior to use. For specific hazard
diet). The weight of test substance per volume of H O
statements, see Section 6.
(expressed as milligrams per millilitre of water), or at a
constant rate in the diet (expressed as parts per million).
2. Referenced Documents
2 3.2.3 feed effıciency, n—this value is a measure of the
2.1 ASTM Standards:
efficiency with which the animals convert food to body weight.
E609 Terminology Relating to Pesticides
The calculation is the total body weight gain per total food
E943 Terminology Relating to Biological Effects and Envi-
consumed.
ronmental Fate
3 3.2.4 gavage, n—forced feeding, as by tube that is passed
2.2 Federal Standards:
down the throat to the stomach.
Title 40, Code of Federal Regulations (CFR), Environmental
3.2.5 test substance, n—pesticide or other material
Protection Agency, Subchapter E, Pesticide Programs:
Part 160, Good Laboratory Practice Standards (element, chemical compound, formulation, known mixture)
administered orally for the purpose of determining chronic
Title21, CodeofFederalRegulations(CFR).FoodandDrug
toxicity.
4. Summary of Test Method
This test method is under the jurisdiction of ASTM Committee E50 on
Environmental Assessment, Risk Management and Corrective Action and is the
4.1 One mammalian species, a rodent, is required; the rat is
direct responsibility of Subcommittee E50.47 on Biological Effects and Environ-
the preferred rodent. Forty rats (twenty females and twenty
mental Fate.
Current edition approved Feb. 1, 2016. Published May 2016. Originally
males) are used at each of the five dose levels (control-, low-,
approved in 1994. Last previous edition approved in 2011 as E1619 – 11. DOI:
two intermediate levels-, and high-dosage groups). If it is
10.1520/E1619-11R16.
determined that an interim sacrifice is necessary, the number
For referenced ASTM standards, visit the ASTM website, www.astm.org, or
contact ASTM Customer Service at service@astm.org. For Annual Book of ASTM
Standards volume information, refer to the standard’s Document Summary page on
the ASTM website.
3 4
Available from U.S. Government Publishing Office, 732 N. Capitol St., NW, Benitz, K. F., “Measurement of Chronic Toxicity,” Methods of Toxicology, ed.
Washington DC 20401-0001, http://www.gpo.gov. G. E. Paget, Blackwell Scientific Publications, Oxford, England, 1970, pp. 32-131.
Copyright © ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959. United States
E1619 − 11 (2016)
should be increased by the number of animals scheduled to be lines suggested by the Institute of Laboratory Resources or
sacrificed during the course of the study (see CFR, Title 40, facilities that have been approved by such organizations as the
Part 798). American Association for Accreditation of Laboratory Animal
Care (AAALAC).
4.2 The high-dose level in rats should elicit some signs of
toxicity without causing excessive lethality. The lowest dosage 7.2 Environment—House test and control animals in cages
level should be one that does not induce any evidence of designed to hold laboratory animals. Provide for appropriate
toxicity. This level should be higher (if possible) than that water and food consumption. Maintain all animals in a
expected for human exposure. The intermediate-dosage level temperature-, humidity-, and light-controlled room. The con-
should produce a minimal observable effect. Where ditions should be 18 to 26°C (64.4 to 78.8°F) for temperature,
appropriate, a vehicle control (the volume of which corre- 40 to 70 % for humidity, and a 12-h light, 12-h dark lighting
sponds to the volume of vehicle at the highest exposure level) cycle.
should be used.The selection of test substance dosages may be
estimated from a preliminary 14-day range finding study. 8. Test Animals
4.3 Daily observations of all individual animals for signs of
8.1 Perform the test with one mammalian species; the rat is
toxicity and mortality are recorded. the preferred rodent species. If another mammalian species is
used, justification or reasoning for the selection must be
4.4 Afteroneyear,priortonecropsy,urine,hematology,and
recorded.
blood samples are collected for analysis and then test animals
are sacrificed.
8.2 Obtain rats three weeks post-weaning. The Sprague-
Dawley (COBS/CD) rat is an example of a strain frequently
4.5 Data collected from treatment and control groups are
used. The females should be nulliparious and nonpregnant.
compared statistically to detect changes in food or water
Acclimate the animals for a period of no less than seven days.
consumption, or both, body weights, organ-to-body weight,
Dosing of rats should begin ideally before six weeks old, but
and organ-to-brain weight ratios, hematology, and clinical
no later than eight weeks of age.
blood and urine values. Histopathological examinations are
also performed on selected tissues. 8.3 All animals for a given test must come from one source
and strain and be approximately the same age to minimize
5. Significance and Use
variability. Test animals may be obtained from commercial
sourcesorrearedinlaboratorycolonies,buttheymustnothave
5.1 This test method should generate data to identify the
been used in a previous test. Animals should be healthy and
majority of chronic effects and shall serve to define long-term
disease free and those that are deformed, injured, emaciated or
dose response relationships. In addition the test should allow
phenotypically different from normal animals must not be used
for the detection of general toxic effects including
as test subjects.
neurological, physiological, biochemical, and hematological
effectsandexposure-relatedmorphological(pathology)effects.
9. Diets
5.2 This test method should provide information on target
9.1 The preferred administration of test substance is incor-
organs, the possibilities of accumulation, and may be used for
porated into a diet. However, the test substance may be
establishing safety criteria for human exposure. It provides
administered dissolved in drinking water or a solvent, or given
information on potential health hazards likely to arise from
by gavage or capsule for a period of at least twelve months.
repeated exposure over a long period of time.
The choice of route of administration depends upon the
physical and chemical characteristics of the test substance.
6. Hazards
9.1.1 If the test substance is administered by gavage, a five-
6.1 Minimize contact with all test substances and solutions
day/week dosing regimen is acceptable.
with appropriate protective clothing, gloves, eye protection,
9.1.2 When necessary, dissolve or suspend the test sub-
etc. The use of fume hoods and increased ventilation in test
stance in a suitable solvent. If a vehicle or diluent is needed, it
rooms is necessary when handling volatile substances. Infor-
should not elicit toxic effects itself nor substantially alter the
mation concerning acute mammalian toxicity and special
chemical or toxicological properties of the test substance.
handling procedures should be known before this test method
9.2 Formulate diets in accordance with the nutrient require-
is used.
ments of the test species. Any unmedicated commercial diet
6.2 Dispose excess test substance, solutions, diets, excreta,
thatmeetstheminimumnutritionalstandardsofthetestspecies
and treated animals with consideration for health and environ-
is acceptable.
mental safety, and in accordance with all federal, state, and
local regulations.
10. Range-Finding Study
7. Facilities 10.1 Previous data or a range-finding study should be
used/conducted to assist in the selection of the appropriate
7.1 No precise physical requirements concerning facilities
doses for the chronic study.
are set forth. However, the animal facility shall meet the
established standard(s) that may be required by law or regula- 10.2 Use groups of six male and six female rats between six
tions. It is desirable that the animal facilities meet the guide- and eight weeks of age. Randomize, number, and place all
E1619 − 11 (2016)
animals in appropriate cages for a five-day acclimation period.
K = dosage of substance that is desired and is expressed as
During this period, all rats will receive rodent diet minus the
grams of test substance/kilogram of body weight/day,
test substance. Dietary levels of the test substance to be
G = amount of food consumed/day over a one-week period
administered may approximate the acute oral LD dosages
and is expressed as grams of food consumed per
and fractions thereof (such as 1X, 0.5X, 0.25X, 0.125X,
kilogram of body weight/day.
0.0625X,0.03125XoftheLD ).Oneadditionalgroupofeach
Record food consumption (and water if necessary) through-
sex will serve as a solvent or untreated control.
out the study.
10.3 It is strongly recommended that a dietary group be
11.5.2 An alternative to this test method would be to
removed from testing for humane purposes when food con-
determine the concentration of test substance in the feed prior
sumption is markedly reduced. If consumption as compared to
to study initiation and then have it remain constant throughout
controls or acclimation period values, or both, is reduced by
the study.
more than 90 %, continued exposure will result in mortality of
11.6 Observations—Make observations of each animal at
test animals in that group.
least once per day, with appropriate actions taken to minimize
10.4 Base the no-effect and effect levels on the following
loss of animals to the study (for example, necropsy or
parameters: body weight, organ-to-body weight ratios,
refrigeration of animals found dead and isolation or sacrifice of
hematology, clinical chemistry, gross necropsy, and food or
weak or moribund animals).
water consumption, or both, if necessary. Histology on a
11.6.1 Recordsignsoftoxicity(bydosagegroupandsex)as
limited selection of organs may be necessary in some in-
they are observed, including time of onset, degree, and
stances.
duration.These signs include, but are not limitedto, changes in
10.5 If a lethal dose is not found, set the highest dietary
skin and fur, eyes and mucous membranes, and also
dosage at 1000 mg/kg, since dosage below this value is
respiratory, circulatory, autonomic and central nervous
assumed to be nontoxic.
systems, somatomotor activity, and unusual behavior patterns.
11.6.2 Weighallanimalsatleastonceperweek,onthesame
11. Procedure
day of each week and record weights.
11.1 Select four dosage levels (low, two intermediate
11.6.3 Record temperature and humidity continually
concentrations, and high) plus an untreated or solvent control.
throughout the study.
Dose all animals by the same method during the entire
11.6.4 At the end of the one year, sacrifice all surviving
experimental period.
animals.
11.2 Randomize, number, and assign at least 40 rats (20
11.7 Clinical Examinations—Make the following clinical
females and 20 males) to each dosage group. If additional
examinations on at least five of each sex in each group of rats.
sacrifices are planned, increase the number of animals by the
number scheduled to be sacrificed during the course of the 11.7.1 Urinalysis—Perform urinalysis at the termination of
study.
the testing period. Place randomly selected animals in from
each group and from each sex in metabolism cages for urine
11.3 Administer the test substance (if in the diet or drinking
collection.Evaluateeachurinesampleindividuallyandinclude
water) ad libitum throughout the study and depending on the
the following measurements: specific gravity, pH, protein,
stability of the test material replace at least weekly.
glucose, ketones, bilirubins, urobilinogen, as well as micro-
11.4 Perform chemical analysis of test mixtures (depending
scopic examination of formed elements.
on stability of test substance) at least once on each new batch
11.7.2 Hematology—Make the following hematology deter-
of test food or water prepared.
minations at least twice during the test period on all groups of
11.5 Diet Preparation—Calculate test substance food mix-
animals including concurrent controls (at six months into the
tures for the first two weeks using the mean body weights and
study and just prior to the terminal sacrifice at the end of the
mean food consumption weights computed during the accli-
study) as follows: hematocrit, hemoglobin concentration,
mation period. Thereafter, prepare the mixtures from the mean
erythrocyte count, total and differential leukocyte counts, and a
body weights and mean food c
...

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4.2 The test article, reference materials, and controls are exposed to human plasma. The plasma is tested on a coagulation device. Each sample tube is assayed in duplicate. The results are reported as a percentage of the negative control.
SCOPE
1.1 This test method covers the screening of circulating blood-contacting device materials for their ability to induce blood coagulation via the intrinsic coagulation pathway. This assay should be part of the hemocompatibility evaluation for devices and materials contacting human blood, as per ANSI/AAMI/ISO 10993-4.  
1.2 All safety policies and practices shall be observed during the performance of this test method.  
1.3 All plasma and any materials that had contact with plasma will be bagged in a biohazard bag, properly labelled with the contents, and disposed of by appropriate means. The plasma should be handled at the Biosafety Level 2 as recommended in the Centers for Disease Control/National Institutes of Health Manual Biosafety in Microbiological Laboratories.  
1.4 The normal pooled human plasma must have tested negative for Hepatitis B (HBV) or Human Immunodeficiency (HIV) viruses. The plasmas should be treated like any patient plasma using standard precautions. The plasma should be handled at the Biosafety Level 2 as recommended in the Centers for Disease Control/National Institutes of Health Manual Biosafety in Microbiological Laboratories.  
1.5 The values stated in SI units are to be regarded as standard. No other units of measurement are included in this standard.  
1.6 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.  
1.7 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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ASTM
ASTM F1984-99(2018)(Practice)
Standard Practice for Testing for Whole Complement Activation in Serum by Solid Materials

SIGNIFICANCE AND USE
5.1 Inappropriate activation of complement by blood-contacting medical devices may have serious acute or chronic effects on the host. This practice is useful as a simple, inexpensive screening method for determining functional whole complement activation by solid materials in vitro.  
5.2 This practice is composed of two parts. In Part A (Section 11), human serum is exposed to a solid material. Complement may be depleted by the classical or alternative pathways. In principle, nonspecific binding of certain complement components also may occur. The alternative pathway can deplete later acting components common to both pathways, that is components other than C1, C4, and C3 (1) .4 In Part B (Section 12), complement activity remaining in the serum after exposure to the test material is assayed by classical pathway-mediated lysis of sensitized RBC.  
5.3 Assessment of in vitro whole complement activation, as described here, provides one method for predicting potential complement activation by medical materials intended for clinical application in humans when the material contacts the blood. Other test methods for complement activation are available, including assays for specific complement components and their split products (see X1.3 and X1.4).  
5.4 This in vitro test method is suitable for adoption in specifications and standards for screening solid materials for use in the construction of medical devices intended to be implanted in the human body or placed in contact with human blood.
SCOPE
1.1 This practice provides a protocol for rapid,  in vitro screening for whole complement activating properties of solid materials used in the fabrication of medical devices that will contact blood.  
1.2 This practice is intended to evaluate the acute  in vitro whole complement activating properties of solid materials intended for use in contact with blood. For this practice, the words “serum” and “complement” are used interchangeably (most biological supply houses use these words synonymously in reference to serum used as a source of complement).  
1.3 This practice consists of two procedural parts. Procedure A describes exposure of solid materials to a standard lot of human serum, using a 0.1-mL serum/13 x 100-mm disposable test tube. Cellulose acetate powders and fibers are used as examples of test materials. Procedure B describes assaying the exposed serum for significant functional whole complement depletion as compared to control samples.  
1.4 This practice does not address function, elaboration, or depletion of individual complement components, nor does it address the use of plasma as a source of complement.  
1.5 This practice is one of several developed for the assessment of the biocompatibility of materials. Practice F748 may provide guidance for the selection of appropriate methods for testing materials for other aspects of biocompatibility.  
1.6 The values stated in SI units are to be regarded as standard. No other units of measurement are included in this standard.  
1.7 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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ASTM
ASTM F3209-16(Guide)
Standard Guide for Autologous Platelet-Rich Plasma for Use in Tissue Engineering and Cell Therapy

SIGNIFICANCE AND USE
4.1 Autologous PRP and platelet gels are utilized in a wide range of orthopedic, sports medicine, regenerative medicine, and surgical applications (3-5). PRP and platelet gels are layered, sprayed, injected, molded, or packed, alone or in combination with graft material or TEMPs, into a variety of anatomical sites, tissues, and voids (3, 6). These platelet concentrates can provide an assortment of bioactive molecules, cells, and physical properties that are potentially attractive for promoting healing and other cell therapy applications (7). Unfortunately, the term “platelet-rich plasma” or “PRP,” which is ubiquitous in early and contemporary medical literature related to a variety of platelet concentrates, only unambiguously denotes one critical parameter of a platelet suspension—increased platelet concentration. Without further context, this common description of PRP offers no information about other important physical and cellular aspects of platelet concentrations. As scientific and clinical understanding of PRP and other cellular therapies increases standardization of nomenclature and terminology is critical for defining key properties, standardizing processing parameters and techniques, and developing repeatable assays for quality assurance and scientific evaluation (5, 8-13). This guide outlines basic guidelines to describe key properties of unique PRP and platelet gel formulations in a standardized fashion. Reliable, standardized descriptions can provide valuable context to PRP end users, such as clinicians seeking a PRP or platelet gel with certain biological attributes or scientific investigators seeking to duplicate a published formulation or to correlate a given PRP or platelet gel feature to other biological properties or outcomes.
SCOPE
1.1 This guide defines terminology and identifies key fundamental properties of autologous platelet-rich plasma (PRP) and PRP-derived platelet gels intended to be used for tissue engineered medical products (TEMPS) or for cell therapy applications. This guide provides a common nomenclature and basis for describing notable properties and processing parameters for PRP and platelet gels that may have utility for manufacturers, researchers, and clinicians. Further discussion is also provided on certain aspects of PRP processing techniques, characterization, and quality assurance and how those considerations may impact key properties. The PRP characteristics outlined in this guide were selected based n a review of contemporary scientific and clinical literature but do not necessarily represent a comprehensive inventory; other significant unidentified properties may exist or be revealed by future scientific evaluation. This guide provides general recommendations for how to identify and cite relevant characteristics of PRP, based on broad utility; however, users of this standard should consult referenced documents for further information on the relative import or significance of any particular PRP characteristic in a particular context.  
1.2 The scope of this guide is confined to aspects of PRP and platelet gels derived and processed from autologous human peripheral blood. Platelet-rich plasma, as defined within the scope of this standard, may include leukocytes.  
1.3 The scope of this document is limited to guidance for PRP and platelet gels that are intended to be used for TEMPS or for cell therapy applications. Processing of PRP, other platelet concentrates or other blood components for direct intravenous transfusion is outside the scope of this guide. Apheresis platelets and other platelet concentrates utilized in transfusion medicine are outside the scope of this document. Production of PRP or platelet gels for diagnostic or research applications unrelated to PRP intended for TEMPS or cell therapy is also outside the scope of this guide. Fibrin gels devoid of platelets are also excluded from discussion within this document.  
1.4 This standar...

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