a EPA
United States
Environmental Protection
Agency
Office of Chemical Safety
and Pollution Prevention , '' —71
(7101) January 2012
Ecological Effects
Test Guidelines
OCSPP 850.2000:
Background
and Special
Considerations-
Tests with Terrestrial
Wildlife
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NOTICE
This guideline is one of a series of test guidelines established by the United States
Environmental Protection Agency's Office of Chemical Safety and Pollution Prevention
(OCSPP) for use in testing pesticides and chemical substances to develop data for
submission to the Agency under the Toxic Substances Control Act (TSCA) (15 U.S.C. 2601,
et seq.), the Federal Insecticide, Fungicide and Rodenticide Act (FIFRA) (7 U.S.C. 136, et
seq.), and section 408 of the Federal Food, Drug and Cosmetic (FFDCA) (21 U.S.C. 346a).
Prior to April 22, 2010, OCSPP was known as the Office of Prevention, Pesticides and Toxic
Substances (OPPTS). To distinguish these guidelines from guidelines issued by other
organizations, the numbering convention adopted in 1994 specifically included OPPTS as
part of the guideline's number. Any test guidelines developed after April 22, 2010 will use
the new acronym (OCSPP) in their title.
The OCSPP harmonized test guidelines serve as a compendium of accepted scientific
methodologies and protocols that are intended to provide data to inform regulatory decisions
under TSCA, FIFRA, and/or FFDCA. This document provides guidance for conducting the
test, and is also used by EPA, the public, and the companies that are subject to data
submission requirements under TSCA, FIFRA, and/or the FFDCA. As a guidance document,
these guidelines are not binding on either EPA or any outside parties, and the EPA may
depart from the guidelines where circumstances warrant and without prior notice. At places
in this guidance, the Agency uses the word "should." In this guidance, the use of "should"
with regard to an action means that the action is recommended rather than mandatory. The
procedures contained in this guideline are strongly recommended for generating the data
that are the subject of the guideline, but EPA recognizes that departures may be appropriate
in specific situations. You may propose alternatives to the recommendations described in
these guidelines, and the Agency will assess them for appropriateness on a case-by-case
basis.
For additional information about these test guidelines and to access these guidelines
electronically, please go to http://www.epa.gov/ocspp and select "Test Methods &
Guidelines" on the left side navigation menu. You may also access the guidelines in
http://www.requlations.qov grouped by Series under Docket ID #s: EPA-HQ-OPPT-2009-
0150 through EPA-HQ-OPPT-2009-0159, and EPA-HQ-OPPT-2009-0576.
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OCSPP 850.2000: Background and special considerations: tests with terrestrial
wildlife.
(a) Scope—
(1) Applicability. This guideline is intended to be used to help develop data to submit to EPA
under the Toxic Substances Control Act (TSCA) (15 U.S.C. 2601, et seq.), the Federal
Insecticide, Fungicide, and Rodenticide Act (FIFRA) (7 U.S.C. 136, et seq.), and the Federal
Food, Drug, and Cosmetic Act (FFDCA) (21 U.S.C. 346a).
(2) Background. This guideline provides general information applicable to conducting OCSPP
Series 850, Group B toxicity tests with terrestrial wildlife species. The source materials used in
developing this harmonized OCSPP guideline are: OPP 70-1 General Information, OPP 70-2
Definitions, OPP 70-3 General Test Standards, OPP 70-4 Reporting and Evaluation of Data
(Pesticide Assessment Guidelines Subdivision E—Hazard Evaluation: Wildlife and Aquatic
Organisms); the Pesticide Reregi strati on Rejection Rate Analysis Ecological Effects report and
the background materials in the OCSPP Series 850, Group B specific guidelines.
(3) General
(i) The OCSPP Series 850, Group B provides guidelines applicable to conducting
laboratory and field toxicity tests with terrestrial species, including birds and mammals.
Field tests are designed on a case-by-case basis. The guidelines in OCSPP Series 850,
Group B are applicable to evaluating the hazards and risks of industrial chemicals and
pesticides to terrestrial wildlife exposed directly or indirectly. Data concerning the
effects of pesticides on terrestrial wildlife are used in ecological risk assessment of
pesticides (40 CFR part 158, paragraph (k)(29) of this guideline). These data are also of
use in assessments of potential off-target injury to endangered and threatened wildlife
species listed by the Fish and Wildlife Service, Department of Interior, and when toxicity
concerns arise from incidents or during Special Review. These data are used for both
deterministic and probabilistic risk assessments.
(ii) Information is provided on the design and conduct of tests with terrestrial wildlife,
emphasizing the importance of adequately characterizing the test substance, use of
suitable experimental design, and establishing the physical and chemical conditions of the
test system in order to provide a scientifically sound understanding of how the test
substance behaves under test conditions. Also considered are the factors that can affect
the test outcome and interpretation of test results. This general information is primarily
applicable to the guidelines for laboratory toxicity tests, since field tests are designed on a
case-by-case basis. However, the OCSPP 850.2000 guideline lists critical quality
assurance and reporting standards common to all the guidelines in the OCSPP Series 850,
Group B guidelines.
(iii) The OCSPP Series 850, Group B guidelines have generally been validated in formal
round-robin tests or through repeated use.
(iv) Each submitted study should meet the data quality objectives for which the test is
designed. Test validity elements critical to determining the scientific soundness and
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acceptability of the study have been listed for each guideline in the OCSPP Series 850,
Group B.
(v) The guidelines contained in OCSPP Series 850, Group B recommend specific
procedures to be used in almost all circumstances to result in a satisfactory study result,
but also provide general guidance that allows for some latitude, based upon study-
specific circumstances. It is recognized that certain problems, some of which are
unavoidable, may arise both before and during testing and provisions have thus been
made in the guidelines for dealing with those that are commonly encountered. These
guidelines provide for exceptions, while at the same time maintaining a high level of
scientifically sound, state-of-the-art guidance so that following this guidance will provide
ecological effect information that is scientifically defensible for its intended use, while
also taking into consideration the chemistry and environmental fate of the test substance.
For a satisfactory test, the experimental design, execution of the experiments,
classification of the organism, sampling, measurement, and data analysis should be
accomplished by use of sound scientific techniques recognized by the scientific
community. Uniformity of procedures, materials, and reporting should be maintained
throughout the toxicity evaluation process. Refinements of procedures to increase their
accuracy and effectiveness are encouraged. When such refinements include major
modifications of any test procedure, the Agency should be consulted before
implementation. Also when in doubt, users of these guidelines should consult with the
appropriate regulatory authorities for clarification or additional information before
proceeding. All references supplied with respect to protocols or other test standards are
provided as recommendations.
(vi) For pesticides, a tiered testing approach given in 40 CFR 158.243 and 40 CFR
158.630 for terrestrial wildlife provides for greater efficiency of testing resources while
assuring data development as warranted to meet the objectives of a hazard and risk
assessment. To reduce or eliminate unnecessary toxicity testing for regulatory decision
making the specific test requirements for pesticides in 40 CFR part 158 depend upon the
use pattern of the pesticide and the potential for exposure of wildlife. In addition, there is
a hierarchal or tier system which progresses from basic laboratory tests to applied field
tests, where the results of each tier of tests should be evaluated to determine the potential
of the pesticide to cause adverse effects, and to determine whether further testing is
warranted to meet the objectives of the hazard or risk assessment (40 CFR part 202).
Tests in the lower tiers (Tier I and Tier II) are designed to screen test substances to
determine the potential to cause adverse effects on survival and reproduction. For
pesticides, a Tier I test, referred to as a limit test in these Group B guidelines, tests a
single concentration and compares effects observed with appropriate controls. Tier II
testing for pesticides (multiple-concentration definitive test in these Group B guidelines)
provides for generation of dose-response curves for test substances which are known
toxicants or which in Tier I testing demonstrated toxicity. The wild mammal toxicity test
described in OCSPP 850.2400 and the field study described in OCSPP 850.2500 are
considered Tier III, and are designed on a case-by-case basis to further refine and
characterize the estimate of risks to terrestrial wildlife.
(vii) Data on toxicity to terrestrial wildlife may also be used to evaluate the potential
hazard and risk of industrial chemicals. Terrestrial wildlife toxicity data are requested
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when the pattern of production, use, or disposal indicates exposure to terrestrial wildlife.
This testing is part of the Tier I (base set) suite of tests in the OPPT testing scheme
developed for determining environmental effects (see the references in paragraphs
(k)(12), 00(13), (k)(18), (k)(19), (k)(31), and (k)(32) of this guideline for further details).
This testing scheme is deterministic for the most part, flexible, sequential, consistent,
iterative, transparent, discriminatory of the extent of toxicity, and applicable to all types
of chemicals.
(viii) For industrial chemicals, toxicity to birds may not be known or suspected, in
contrast to pesticides where it may be established that the substance is or could be toxic
to terrestrial wildlife. Thus, for industrial chemicals the maximum amount of toxicity test
information should be obtained from the initial or lower tier test, Avian Acute Oral
Toxicity Test (the OCSPP 850.2100 guideline). In contrast to pesticides, the toxicity of
industrial chemicals to terrestrial wildlife is generally uncharacterized. Thus, range-
finding tests, a preliminary step to define dose-response testing, are more commonly
conducted than limit or maximum challenge tests that use only one test concentration.
For non-toxic or low toxicity chemicals (based on the results of the OCSPP 850.2100
test) it is likely that no further higher tier testing (OCSPP 850.2200 guideline (Avian
Dietary Toxicity Test) or OCSPP 850.2300 guideline (Avian Reproduction Test), or
both) would be supported or recommended. For industrial chemicals, the base set Tier I
tests and requirement to proceed from one tier to the next are referenced in paragraphs
(k)(12), (k)(13), (k)(18), (k)(19), (k)(31), and (k)(32) of this guideline.
(ix) While performing field tests, all necessary measures should be taken to ensure that
nontarget plants and animals, especially endangered or threatened species, will not be
adversely affected either by direct hazard or by impact on food supply or food chain.
(b) Definitions. Terms used in the OCSPP Series 850, Group B guidelines have the meanings
set forth in Section 3 FIFRA regulations at 40 CFR 152.3 (Pesticide Registration and
Classification Procedures); 40 CFR part 158.300 (Product Chemistry Definitions); 40 CFR part
160 (Good Laboratory Practice Standards); and in TSCA Section 3 regulations 40 CFR part 792
(Good Laboratory Practice Standards); and the Agency's "Terms of Environment, Glossary,
Abbreviations and Acronyms" (see paragraph (k)(23) of this guideline). The definitions in this
section apply to the OCSPP Series 850 Group B test guidelines and where applicable, the
individual test guidelines contain additional or test-specific definitions.
Acclimation is the physiological or behavioral adaptation by test animals to one or more new
environmental conditions and basal diet associated with the test procedure.
Active Ingredient (a.i.) is any substance (or group of structurally similar substances if specified
by the Agency) that will prevent, destroy, repel or mitigate any pest, or that functions as a plant
regulator, desiccant, or defoliant within the meaning of FIFRA (40 CFR 152.3).
Acute toxicity is the discernible adverse effects (lethal or sublethal) induced in an organism
within a short exposure period (usually not constituting a substantial portion of the total life
cycle or life span, e.g. days).
Acute toxicity test is a comparative study in which organisms are subjected to a severe, short-
term stimulus (test substance). The organisms, exposed to different concentrations of the test
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substance (except in a limit test), are observed for a short period usually not constituting a
substantial portion of the total life cycle or life span. Acute exposure typically includes a lethal
biological response of relatively quick progression.
Adjuvant is a subsidiary ingredient or additive in a mixture which modifies, enhances or prolongs
by physical action the activity of the active ingredient(s). Examples of agricultural chemical
adjuvants include but are not limited to surfactants, crop oils, anti-foaming agents, buffering
compounds, drift control agents, compatibility agents, stickers and spreaders.
Basal diet is the food or diet as it is prepared or received from the supplier, without the addition
of any vehicle, diluent or test substance.
Chronic toxicity test is a comparative study in which organisms are exposed to different
concentrations of the test substance generally for a relatively long period that constitutes a
substantial, nearly complete, or complete portion of the total life cycle or life span. Chronic
exposure typically induces a sublethal biological response of relatively slow progression, or
which is cumulative in nature. For some chemicals with certain modes-of-action, shorter-term
exposure may result in chronic or latent effects, and continued or cumulative exposure is
therefore not necessary.
Concentration-response curve is the graphical and mathematical relationship between the
concentration of a test substance and a specific biological response produced from toxicity tests
when response (e.g., proportion or percent mortality) values are plotted against concentration of
test substance for a given exposure duration. This is also referred to as the dose-response curve
or concentration-effect curve.
Control refers to test organisms exposed to test conditions and test matrix (capsule, diet, gavage)
in the absence of any introduced test substance as part of the test design for the purpose of
establishing a basis of comparison with a test substance for known chemical or biological
measurements.
Effect Concentration (EC50) is the experimentally derived concentration of test substance
in the diet that would be expected to affect 50 percent of a test population of test animals which
is exposed exclusively to the treated diet under specified exposure conditions.
Formulation, as used within these guidelines, is a packaged end-use product (e.g., dust, wettable
powder, emulsifiable concentrate, ultra low volume, etc} of the test substance and may contain
one or more active ingredients and one or more inert ingredients.
Hatch refers to eggs or young birds that are the same age and that are derived from the same
adult breeding population, where the adults are of the same strain and stock.
Holding refers to the period from the time test organisms are received in the laboratory until they
are used in testing or begin acclimation to test conditions. Holding conditions may include
quarantine, lower temperatures to minimize disease, or other conditions that are different from
test conditions. Where holding conditions are different from test conditions, the test organisms
should be acclimated to test conditions prior to testing not to stress the organisms.
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Inert ingredient is any substance (or group of structurally similar substances if designated by the
Agency), other than an active ingredient, which is intentionally included in a pesticide product
(40 CFR 152.3).
Inhibition Concentration (1C50) is the experimentally derived concentration of test substance in
the diet that would be expected to inhibit 50 percent of a test population of test animals which is
exposed exclusively to the treated diet under specified exposure conditions.
Lethal concentration, median (LCso) is the experimentally derived concentration of the test
substance in the diet that would be expected to result in mortality of 50 percent (50%) of a
population of test animals which is exposed exclusively to the treated diet under specified
exposure conditions.
Lethal dose, median (LDso) is the experimentally derived dose of the test substance that would be
expected to result in mortality of 50% of a population of test animals which is treated with a
single oral dose under specified exposure conditions.
Limit of detection (LOD) is the analytic level below which the qualitative presence of the
material is uncertain. This is typically defined by the lowest concentration producing a signal
two standard deviations above the background noise from a matrix blank sample.
Limit of quantification (LOQ) is the analytic level below which the quantitative amount of the
material is uncertain. This is typically defined by the lowest concentration of fortified matrix
successfully analyzed.
Limit test is a toxicity test performed with a single test substance concentration or dose and a
control to establish that the value for the measurement endpoint of concern (e.g., LCso, LDso) is
greater than the test substance concentration or dose (limit concentration or dose, respectively).
Lowest observed effect concentration (LOEC) is the lowest concentration of a test substance to
which organisms are exposed under specified exposure conditions that causes a statistically
significant adverse effect as compared to the control(s). Throughout these guidelines, the terms
LOEC and lowest observed adverse effect concentration (LOAEC) have the same meaning.
Lowest observed effect level (LOEL) is the lowest dose level of a test substance to which
organisms are exposed under specified test conditions that causes a statistically significant
adverse effect as compared to the control(s). Throughout these guidelines, the terms LOEL and
lowest observed adverse effect level (LOAEL) have the same meaning.
Maximum acceptable toxicant concentration (MATC) is the highest concentration at which a test
substance can be present and not be toxic to the test organism. The MATC lies within the range
between the LOEC and NOEC. Operationally, for industrial chemicals, the MATC is defined as
the geometric mean of these values. The MATC is also referred to (in the Pre-Manufacture
Notification (PMN) program of OPPT) as the chronic value or chronic no-effect-concentration
(NEC).
Measured concentration is an analytically derived quantitative measure which lies above the
method detection limit.
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Measurement endpoint is a quantitative measurable response to a stressor that is used to infer a
measure of protection or evaluate risk to valued environmental entities. Examples of
measurement endpoints include, but are not limited to, mortality (e.g., LD50; NOEL), body
weight (e.g., NOEL), number of eggs (e.g., NOEL), etc. Each test-specific guideline identifies
the measurement endpoint(s) to be determined by the proscribed study. The term "measurement
endpoint" is used synonymously with the term "measures of effect".
Method detection limit (MDL) is operationally defined as the concentration of constituent that,
when processed through the complete method, produces a signal with 99% probability that it is
different from the blank. It is computed as the standard deviation multiplied by the Student's t
constant corresponding to the appropriate degrees of freedom (n-1). Thus, for seven spiked
samples prepared at the hypothetical LOQ, the MDL is 3.143 times the standard deviation of the
mean of the seven replicate measurements.
No observed effect concentration (NOEC) is the highest concentration of a test substance to
which organisms are exposed under specified exposure conditions that does not cause a
statistically significant adverse effect as compared to the control(s). The NOEC is the test
concentration immediately below the LOEC and can only be defined in the presence of the
LOEC. Throughout these guidelines, the terms NOEC and no observed adverse effect
concentration (NOAEC) have the same meaning.
No observed effect level (NOEL) is the highest dose level of a test substance to which organisms
are exposed under specified exposure conditions that does not cause a statistically significant
adverse effect as compared to the control(s). The NOEL is the test dosage immediately below
the LOEL and can only be defined in the presence of the LOEL. Throughout these guidelines,
the terms NOEL and no observed adverse effect level (NOAEL) have the same meaning.
Reagent water is water that has been prepared by deionization, glass distillation, or reverse
osmosis.
Replicate is the experimental unit within a toxicity test. It is the smallest physical entity to which
treatments can be independently assigned.
Subchronic toxicity test is a comparative study with terrestrial organisms that has characteristics
of both acute and chronic toxicity tests, but with more of the latter. Organisms are subjected to a
stimulus (test substance), of a longer duration than an acute test, but of a shorter duration than a
chronic test. Subchronic exposure typically induces a lethal or sublethal biological response of
relatively moderate progression for periods that constitute a portion of the total life cycle or life
span.
Test substance refers to the specific form of a chemical substance or mixture being evaluated
(e.g., pesticide active ingredient or formulation, or industrial chemical).
Treatment group refers to the set of replicates that receive the same amount (if any) of the test
substance; controls are treatment groups that receive none of the test substance.
Vehicle is any agent which facilitates the mixture, dispersion, or solubilization of a test substance
with a carrier (e.g., diet, capsule or gavage solution, drinking water) used to expose the test
organisms (40 CFR 160.3, 40 CFR 792.3).
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(c) Apparatus, facilities and equipment—
(1) Laboratory facilities and equipment. The type of facilities and equipment for conducting
the toxicity tests with the organisms in this group of guidelines varies depending upon the nature
of the test and the organism. In general the laboratory toxicity tests with terrestrial wildlife use
normal laboratory glassware, supplies and equipment as well as equipment for housing animals
and controlling temperature, humidity and lighting. Enclosures for animals should be large
enough to permit normal behavior and movement. Housing and maintenance conditions should
be in accordance with acceptable animal husbandry practices (e.g., United States Department of
Agriculture Animal Care Regulations). Construction materials and equipment that are toxic,
may affect toxicity, or that may sorb test substances should not be used. Pens should be
constructed of galvanized metal, stainless steel, or perfluorocarbon plastic (e.g. Teflon). Wire
mesh should be used for floors and external walls; solid sheeting should be used for common
walls and ceilings. See test-specific OCSPP Series 850, Group B guidelines for identification of
any atypical facility, equipment, or supplies used in the test.
(2) Maintenance and reliability. All equipment used in conducting the test, including
equipment used to prepare and administer the test substance, and equipment to maintain and
record environmental conditions, should be of such design and capacity that tests involving this
equipment can be conducted in a reliable and scientific manner. Equipment should be inspected,
cleaned, and maintained regularly, and be properly calibrated.
(3) Permits. Experimental use permits may be required for the terrestrial testing of pesticides
under field conditions. Recommend consulting with the Agency prior to conducting a field test
to identify what, if any, federal permits are required
(d) Experimental design and data analysis—
(1) Design elements. Elements of experimental design such as the number of test treatments,
progression factor between treatment levels, number of replicates, and number of organisms per
replicate and per treatment are based upon the purpose of the test, variability expected in
response measurements, and the type of statistical procedures that will be used to evaluate the
results. See the test-specific guidelines for specific information relating to these aspects of test
design. General principles of test design are set forth in this guideline. General guidance on the
statistical analysis of laboratory ecotoxicity tests can be found in the references in paragraphs
(k)(l), (k)(2), (k)(15), (k)(16), (k)(17), (k)(26), (k)(27) and (k)(28) of this guideline.
(2) Calculation of endpoints—
(i) Background.
(A) Data generated in ecotoxicity tests with terrestrial animals may be of three
types:
(1) Quantal (dichotomous), where the variable has only two mutually exclusive
outcomes (e.g., dead or alive)—note that quantal data are a special case of
discrete data;
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(2) Discrete, where there is a finite number of values possible or there is a space
on the number line between two possible values (e.g., number of young
produced); or
(3) Continuous, where the variable can assume a continuum of possible outcomes
(e.g., height and weight).
(B) These data may be analyzed using regression-based techniques or hypothesis-
testing procedures depending on the objectives and endpoints of a specific test
guideline. Traditionally, the results of acute toxicity tests have been expressed as
point estimates (e.g., LCso or LDso for lethality, or ECso or ICso for other effects),
while the results of chronic tests have been expressed as the results of hypothesis-
testing procedures to determine the NOEC and LOEC (or NOEL and LOEL).
Regarding terminology, the term ICX is more appropriately used for continuous
endpoints, rather than ECX. For information on the advantages and disadvantages
of these approaches, see the references in paragraphs (k)(5), (k)(8), (k)(16),
(k)(17) and (k)(20) of this guideline. Specific test guideline objectives, either
point estimate or hypothesis-based endpoints or both, are identified in each
specific test guideline.
(ii) Point estimates and concentration-response or dose-response tests. This type of
toxicity test is designed to allow calculation of a concentration- or dose-response curve
(mathematical model) and to estimate one or more specific points (point estimates) on the
curve, such as an LDso. Because of the normal variation in sensitivity of individuals
within a group of test organisms, a measure of the degree of certainty in the model
parameters and the point estimate value(s) should be determined.
(A) No single statistical technique is appropriate for all data sets, and the
assumptions and requirements of each method should be known before using (see
paragraphs (k)(l), (k)(4), (k)(6), (k)(7), (k)(9), (k)(10), (k)(ll), (k)(14), (k)(20),
and (k)(30) of this guideline). Not all methods suitable for continuous data are
appropriate for quantal data (see paragraphs (k)(4) and (k)(14) of this guideline).
For point estimate tests, regression-based methods (e.g., probit) that model the
full concentration- or dose-response relationship and provide error estimates of
the model parameters and point estimate(s) are desired. The regression model
used to fit data should be recorded, and the error estimates of the model
parameters (e.g., standard error of slope and intercept), and goodness-of-fit should
be calculated and recorded. For a point estimate (e.g., LCso or LDso) the 95%
confidence limits and standard error are calculated and recorded. If data do not fit
a regression-based model, other point estimator methods (e.g., binomial, moving
average, trimmed Spearman-Karber, linear interpolation (e.g., Boostrap ICp)) are
available (see paragraphs (k)(24), (k)(27) and (k)(28) of this guideline). Which of
these other methods is selected is dependent upon the shape of the concentration-
response curve, the number of treatments with partial mortalities (i.e., where
mortality is greater than 0% but less than 100%), the magnitude of these
mortalities, and the number of replicates. The method used to estimate the
endpoint and, if applicable, the 95% confidence limits for the point estimate
should be recorded.
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(B) Dose-response models are good estimating tools only for the range of doses
used to fit them; therefore, endpoints that are extrapolated beyond the range of the
doses tested would be considered to be of lower confidence or potentially, of such
low confidence that they would not be appropriate to estimate.
(iii) Hypothesis-based methods—
(A) Multiple-concentration or dose-definitive tests. In this type of test, the
purpose is to determine if the biological response to a treatment level differs from
the response of a control. Hypothesis testing-based endpoints, expressed as the
NOEC and LOEC (or NOEL and LOEL), are calculated by determining
statistically significant differences from the control. The null hypothesis is that
no difference exists among the mean (or median if nonparametric) control and
treatment responses. The alternative hypothesis is that the treatment(s) results in
an adverse biological effect relative to the control sample. Parametric and
nonparametric analysis of variance (ANOVA) tests and multiple-comparison tests
are often appropriate for continuous data and for count data and may be
appropriate for some categorical data (rank, order, score). Contingency table tests
are usually appropriate for categorical data. Parametric tests are based on normal
distribution theory and assume that the data within treatments are a random
sample from an approximately normal distribution and that the error variance is
constant among treatments. These assumptions should be examined using
appropriate tests, and data transformations (see paragraph (d)(2)(iv)(A) of this
guideline) or non-parametric techniques should be used where the assumptions
are not met. Where possible multiple comparison tests that restrict the number of
comparisons made should be used. Generally, the more powerful multiple-
comparison tests are those which assume a concentration- or dose-response
relationship in the data. When the assumption of a monotonic dose-response
holds, Williams' and Jonckheere's test, respectively, are examples of parametric
and nonparametric tests that can be used. When the assumption of a monotonic
dose-response fails, Dunnett's t-test and either Steel's many-one rank test or the
Wilcoxon rank sum test with Bonferroni adjustment, respectively, are examples of
parametric and nonparametric multiple comparison tests requiring no assumption
about the dose-response but which restrict comparisons of the treatments to a
control. A measure of the sensitivity of the test, such as the minimum significant
difference (parametric tests), should be calculated. Alternatively, a calculation of
the number of replicates necessary to achieve data quality objectives given the
actual measured test responses and variability should be made. At a minimum,
the percent reduction from the control for each treatment should be calculated.
(B) Types of decisions and errors.
(1) Table 1 presents the two possible outcomes and decisions that can be reached
in the statistical hypothesis tests discussed in paragraph (d)(3)(ii)(A) of this
guideline:
(a) There is no difference among the mean control and treatment responses; or
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(b) There is a difference among the mean control and treatment responses
(concerned with direction, where response is adverse relative to the control).
(2) Statistical tests of hypothesis can be designed to control for the chances of
making incorrect decisions. The types of incorrect and correct decisions that can
be made in a hypothesis-based test and the probability of making these decisions
are represented in Table 1. For multiple comparison tests the Type I error rate is
controlled to account for multiple test comparisons.
Table 1.—Types of Errors and the Probabilities of Making Correct and Incorrect
Decisions Based on the Results of Testing
Test Decision Outcome:
Treatment Response > Control Response
Treatment Response < Control Response
Actual (or True) Condition:
Treatment Response >
Control Response
Correct Decision
probability = 1- alpha (a)
Type I error (False positive)
probability = a
Treatment Response < Control
Response
Type II error (False negative)
probability = beta (p)
Correct Decision
probability (Power of test) = 1-p
(C) Power of the test. Power of the test versus percent reduction in treatment
response relative to the control mean at various coefficients of variation is
provided in the reference in paragraph (k)(24) of this guideline. Examples are
specifically given for 5 and 8 replicates for a one-tailed test alpha (a) of 0.05 and
0.10. Effects on the number of replicates at various coefficients of variation are
also provided in the reference in paragraph (k)(24) of this guideline for various
low a and beta (P) values (i.e., a + P = 0.25). See also the references in
paragraphs (k)(9) and (k)(25) of this guideline.
(D) Limit test. In a limit test it is only necessary to ascertain that: a fixed
standard (such as the LDso or LCso for acute oral and subchronic dietary,
respectively) is greater than a given threshold; and/or the response at the limit
dose or concentration does not differ from the control response. Only one
treatment, the limit dose or concentration, and the appropriate control(s) are
tested. This is referred to as a limit test or maximum challenge concentration test.
(1) Fixed standard. For a fixed standard limit test, the null hypothesis is that the
estimated limit treatment parameter (e.g., percent survival or average weight gain)
is greater than or equal to the fixed threshold value (e.g., 50% survival). The
alternative hypothesis is that the estimated limit parameter is less than the fixed
threshold value (e.g., 50% survival) (Concerned with direction, where response
is inhibition relative to the control switch hypotheses around.) Examples of
statistical approaches are one sample binomial tests or one sample t-tests.
(2) Difference between two means (or medians). For testing if the treatment
level affects the test organism, the null hypothesis is that the treatment mean (or
median) response is equal to the control response mean (or median) level and the
alternative hypothesis is that the treatment mean response differs from the control
response. The direction of the alternative hypothesis depends on what is
considered an adverse direction for the specific response being evaluated, such as
decreased number of eggs laid, decreased proportion of uncracked eggs,
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decreased number of surviving 14 day old chicks as compared to the control
response. Examples of parametric and nonparametric two-group comparison tests
are Student's t-test and Wilcoxon rank sum test, respectively.
(iv) Transformations, outliers, and non-detects—
(A) Transformations. Transforma-tion of data (e.g., square root, log, arcsine-
square root) may be useful for a number of statistical analysis purposes. The two
main reasons are to satisfy assumptions for statistical testing and to derive a linear
relationship between two variables, so that linear regression analysis can be
applied. Added benefits include consolidating data that may be spread out or that
have several extreme values (see reference in paragraph (k)(25) of this guideline).
Once the data have been transformed, all statistical analyses are performed on the
transformed data.
(B) Outliers. Outliers are measurements that are extremely large or small relative
to the rest of the data and, therefore, are suspected of misrepresenting the
population from which they were collected. Unless there is a known documented
reason for the outlier(s), such as measurement system problems or instrument
breakdown, the statistical analyses performed should at a minimum include
results using the full data set (i.e., the suspected outlier(s) are not discarded).
Outliers should not be discarded based on a statistical outlier test (see reference in
paragraph (k)(25) of this guideline). The analyst may conduct all statistical
analysis of the data with both a full and truncated (presumed outliers are
discarded) data set, however, so that the effect of the presumed outlier(s) on the
conclusion may be assessed.
(C) Nondetects. Data generated from chemical analysis that falls below the LOD
of the analytical procedure are generally described as not detected, or nondetects,
(rather than as zero or not present) and the appropriate LOD should be reported.
There are a variety of ways to evaluate data that include both detected and non-
detected values (see reference in paragraph (k)(25) of this guideline). However,
for a satisfactory test in a number of the Group B guidelines, test substance
concentrations should not be below the LOD (see specific OCSPP Series 850,
Group B guidelines), except in controls.
(3) Selection of test treatments—
(i) Point estimate and concentration-response or dose-response test. Toxicity tests
where the objective is the concentration- or dose-response curve (mathematical model)
and a specific point(s) on the curve (e.g.., LD50), usually consist of a control treatment and
at least five test treatments which should bracket the specific point response of concern
for the test. To obtain a reasonably precise estimate of the LCso or LDso using probit
analysis, for example, one or more treatments should kill between, but not include, 0 and
50% of the test organisms and one or more treatments should kill between, but not
include, 50 and 100% of the test organisms. The spacing between test treatment levels
(doses or concentrations) depends upon the expected slope of the concentration- or dose-
response curve, information about which can be gained during a range-finding test. The
test treatment levels (doses or concentrations) are usually selected in a geometric series in
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which the ratio is between 1.5 and 3.2. When the objective of the test is to determine a
regression-based estimate and sampling size constraints apply, the use of more treatment
levels is preferable to the use of more replicates. The inclusion of additional treatment
levels rather than additional replicates results in better characterization of the overall
concentration- or dose-response relationship.
(ii) Hypothesis-based test—
(A) Multiple-concentration or -dose definitive test. Each test usually consists
of a control treatment and at least five test treatments which span the expected
environmental concentrations and where at least the lowest treatment level is the
NOEC (or NOEL). The test treatments are usually selected in a geometric series
in which the ratio is between 1.5 and 3.2. A key assumption is that the response
data is monotonic with increasing concentration or dose (i.e.., the degree of
biological effect increases as concentration or dose increases) or that there is a
threshold response such that a NOEC (or NOEL) for a given biological response
should not occur at a treatment concentration or dose higher than one found to be
statistically different from the control for the given biological response. If these
assumptions do not hold, it is recommended that additional concentrations or
doses be included to better characterize the relationship of the biological response
with exposure concentration or dose. If high variability in a given response
measurement is expected, increasing the number of replicates is recommended.
(B) Limit test. A limit test consists of a single treatment level and the appropriate
control. Individual OCSPP Series 850 Group B guidelines identify the
concentration or dose that satisfies the limit treatment level test for that guideline.
(4) Randomization. For test results to be satisfactory test treatments should be randomly
assigned to individual test containers and the test containers randomly assigned to locations.
Randomized block designs may be used. For test results to be satisfactory, test organisms should
ideally be randomly assigned to the test containers; where this is not practical impartial
assignment can be used (with the exception of assignment intentionally according to sex). (Note:
random assignment as used here implies a mathematically-based unbiased assignment method
and impartial assignment implies a non mathematically-based unbiased assignment procedure.)
All test containers should be treated as similarly as possible to eliminate potential bias in test
results. The methods used to randomize treatments among test containers and test containers
among locations should be recorded, as well as methods of impartial organism assignment to test
containers.
(5) Number of replicates. The number of replicate test containers for a given treatment is
dependent upon the objective of the test. Except for field tests which are designed on a case-by-
case basis, the minimum number of replicates for a given test is described in each individual
OCSPP Series 850 Group B guideline.
(i) Regression-based test. When the objective of the test is to determine a regression-
based estimate and sample size constraints apply, the inclusion of additional
concentrations rather than additional replicates results in better characterization of the
overall concentration-response relationship. The objective of some OCSPP Group B
guideline tests includes determination of both a regression-based point estimate (e.g.,
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and a hypothesis-based endpoint (e.g., NOEC) in which case the minimum number
of replicates will be determined by the hypothesis-based method.
(ii) Hypothesis-based test. For hypothesis-based tests, the determination of the test-
specific number of replicates depends upon the objectives of the test, the statistical
method(s) that may be used, the coefficient of variation, the size of effect to be detected,
and the acceptable error rate. (Note: several of the recommended non-parametric
multiple-comparison tests can not be performed without at least a minimum of four
replicates.) Individual testing facilities should consider variability observed in their
laboratory and adjust the number of replicates upward where the minimum replication
number identified in a test specific guideline is not sufficient to provide the statistical
power to detect adverse effects to the test organisms or, if appropriate, identify and
correct any environmental, handling, and culturing conditions, etc. that are resulting in
the high variability.
(e) Test substance characterization—
(1) Background information on the test substance. The information in paragraphs (e)(l)(i)
through (e)(l)(vi) of this guideline should be known about the test substance prior to testing:
(i) Chemical name; CAS number; molecular structure; source; lot or batch number; purity
or percent active ingredient (a.i.); identities and concentrations of major ingredients and
major impurities; radiolabeling if any, location of label(s), and radiopurity; date of most
recent assay and expiration date for sample.
(ii) Appropriate storage and handling conditions for the test substance to protect the
integrity of the test substance. (Note: health and safety precautions should also be
known. These considerations are beyond the scope of these guidelines and depend upon
the characteristics of the test substance).
(iii) Physical and chemical properties of the test substance, including solubility in water
and various solvents; vapor pressure; hydrolysis at various pH, etc. Of particular
relevance are rates for processes such as hydrolysis, photolysis, and volatilization.
(iv) Stability and solubility as relevant, under the test conditions (see paragraph (e)(2) of
this guideline).
(v) Physical and chemical properties and stability information for the analytical standard
(if applicable).
(vi) Analytical method for quantification of the test substance in the feed or dosing
solutions. Analyses are conducted with the specific media which will be used during the
test, i.e., under test conditions.
(2) Preliminary analyses.
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(i) The Agency recommends preliminary testing of the test substance. The information
about stability of the test substance should be developed under actual test conditions.
This information can be gained while doing the range-finding studies.
(ii) Information on the behavior of a test substance should be based on experiments which
are conducted under the same conditions as those occurring during the test. These
include but are not limited to:
(A) Test diet or dosing solution characteristics.
(B) Temperature, humidity, lighting.
(C) With test organisms in place (when practical).
(D) Use of the same test containers.
(iii) The tests in paragraphs (e)(2)(iii)(A) through (e)(2)(iii)(D) of this guideline should
be performed:
(A) Stability trials should be conducted under actual test conditions.
(B) If relevant, solubility trials should be conducted under test conditions.
(C) Chemical analysis methods as detailed in paragraph (g) of this guideline.
(D) Determination of storage stability of the test substance in the samples to be
collected for chemical analyses. This includes determining whether and how
samples can be stored for future analysis.
(3) Sample storage. If samples of the diet or other dosing preparation collected for chemical
analysis cannot be analyzed immediately, they should be handled and stored appropriately to
minimize loss of the test substance. Loss could be caused by such processes as microbial
degradation, hydrolysis, oxidation, photolysis, reduction, sorption, or volatilization. Stability
determination under storage conditions, whether it refers to storing the test substance before
testing or storing samples awaiting analysis, is required by GLP regulation. Test substance
stability under storage conditions should be documented.
(4) Stability. A test substance is considered to be stable under actual test conditions if, under
those conditions, it does not degrade, volatilize, dissipate, or otherwise decline to concentrations
less than 80% of the initial measured concentration during the study period.
(5) Analytical test substance determinations—
(i) Measurement at initiation and termination of testing.
(A) For stable test substances in the diet it is preferred that the concentration in the diet
be confirmed at the beginning and end of the longest exposure period in laboratory tests,
but minimally, analyses should be conducted at the initiation of exposure.
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(B) If the test substance is known to be unstable to the extent that 20% or more loss
occurs over the longest exposure period under test conditions, then a second series of
analyses of the same concentrations previously analyzed should be conducted with
samples taken at the end of the exposure period. If it is observed that the stability or
homogeneity of the test substance in the diet or dosing solutions cannot be maintained,
care should be taken in the interpretation of the results and a note made that the results
may not be reproducible.
(ii) Field tests. For field tests, media and frequency of testing depends on the objective
of the study, the stability and fate of the test substance, and is determined on a case-by-
case basis.
(6) Measured concentrations versus nominal concentrations. This section describes
acceptable limits of deviation of measured from nominal concentrations.
(i) Pesticides and other chemicals that are used at very low levels tend to have high
biological activity. For this reason, it is imperative that the toxicity data developed for
these test substances be accurate and scientifically defensible. Toxicity results should
also be precise (repeatable and reproducible).
(ii) Measured concentrations are used because:
(A) There are concerns that the actual concentrations to which the test organisms are
exposed may differ from "nominal." This variation may be due to chemical
characteristics, test conditions, or mechanical apparatus. Exposure estimates using
measured concentrations account for characteristics that make testing difficult (high
volatility, short half-life, etc). These characteristics are not a reason for developing
misleading toxicity values from laboratory tests.
(B) Measured concentrations confirm that the test system was designed appropriately and
is operating acceptably. Measurement of test concentrations is not performed solely to
determine if the technician knows how to prepare the dosing matrix once. Among other
things, this measurement also ensures that the dosing matrix was prepared correctly each
time. It corroborates the precision of the technician or mechanics of the test system.
(iii) If test levels are not measured, the nominal values are used to calculate the test
endpoints. If the test substance has degraded or has become unavailable because of
volatility, photodegradation, hydrolysis, etc., the test substance may be characterized as
less toxic than it actually is.
(iv) When a laboratory test design has been specifically modified to accommodate the
instability of test substance or other factors likely to cause variability in test
concentrations, and the design is judged adequate based on sufficient preliminary
information, the study will not be rejected solely on the grounds that measured
concentrations varied by more than 20% of the nominal concentration. (This assumes
that the preliminary stability tests were conducted under test conditions essentially
identical to the actual test conditions.) A change in measured test concentration of more
than 20% from the nominal concentration during the test will generally not result in
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rejection, provided that the conditions in paragraph (e)(6)(iv)(A) through (e)(6)(iv)(E) of
this guideline are met:
(A) A reasonable and scientific explanation is given, and the variability of results
produced by the chemical analysis method is adequately characterized.
(B) All test treatment levels exhibit a similar (but not necessarily identical) shift. If
concentrations at some treatment levels go up substantially (>20%) and test
concentrations at other treatment levels go down substantially (>20%), they will not be
considered to have exhibited a similar shift. The most important validity element is that
test levels not experience a shift in "order." That is, the highest test level should remain
the highest; the next should remain second, etc. If orders are shifted, the test may be
rejected, since regression analysis would not yield statistically sound median lethal
concentrations and confidence limits.
(C) The variability of the measured concentrations is acceptable.
(D) A statistically valid endpoint can be derived from the measured concentrations (e.g.,
either an LCso, LD50, etc., or that the LCso or LD50 is greater than the limit concentration).
(E) The preliminary stability information is provided with complete documentation and
description of methods used to derive such information.
(v) In some cases, high variability cannot be avoided because the test concentrations are
approaching the LOD or because of unavoidable binding of the test substance to the
chemical analysis apparatus. When the ratio of the highest concentration to the lowest
measured concentration is expected to vary by more than 1.5 the submitter is strongly
advised to justify an exception to this standard in advance of conducting the studies. This
exception justification should include:
(A) Documentation of the preliminary analyses indicating this problem.
(B) The specific steps that will be taken to reduce the variation.
(C) The fully developed chemical analysis method.
(D) The raw data, standards, quality control samples, and chromatograms from a
representative analysis using the method. For each chemistry method, identify the
method detection limit and limit of quantification.
(vi) The Agency will decide on each exception justification on a case-by-case basis.
However, if a series of tests are to be conducted with one chemical and it is anticipated
that these limits will be exceeded, one exception justification may cover more than one
study. The Agency will then exercise judgment in evaluating studies with test substances
that are difficult to measure.
(f) Preparation of test substance.
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(1) The preferred choice for preparation of the test substance is to use reagent water (deionized,
distilled or reverse osmosis water), providing the test substance can be dissolved in water and
does not readily hydrolyze. If the test substance cannot be dissolved in reagent water, vehicles
are often used. If a vehicle, i.e. a solvent, is absolutely necessary to dissolve the test substance,
the amount used should not exceed the minimum volume necessary to dissolve or suspend the
test substance. If the test substance is a mixture, formulation or commercial product, none of the
ingredients is considered a vehicle unless an extra amount is used in its preparation for testing.
(i) Preferred vehicles include acetone, methylene chloride, table grade corn oil, propylene
glycol, gum arable (acacia), and 1% carboxymethylcellulose.
(ii) If a vehicle is used to prepare the test substance, a vehicle control is included in the
test. The same batch of vehicle used to prepare the test treatment doses or concentrations
is used in the vehicle control. For a valid test, the selected vehicle should not affect the
test organisms at the concentration used. A vehicle should not interfere with the
metabolism (degradation) of the test substance, alter the chemical properties of the test
substance, or produce physiological or toxic effects to test organisms.
(iii) Ideally, vehicle concentration should be kept constant in the vehicle control and all
test treatments. If the concentration of vehicle is not kept constant, the highest
concentration of vehicle used in any test treatment level should be used in the vehicle
control. The vehicle should not comprise more than 2% by weight of the treated diet.
(2) All techniques used in stock solution preparation of test substance (shaking, stirring,
sonication, heating, solvent, etc.) should be recorded. The appearance of the stock solution
should be observed and recorded.
(3) If the test substance is a formulated pesticide product, the test concentrations should be
expressed in terms of the concentration of a.i.
(g) Analytical methods and sampling for verification of exposure—
(1) Method validation.
(i) The analytical method used to measure the amount of test substance in the diet or
dosing solutions should be validated by appropriate laboratory practices before beginning
the definitive test. An analytical method is not acceptable if likely degradation products
of the test substance, such as hydrolysis and oxidation products, give positive or negative
interferences which cannot be systematically identified and mathematically corrected,
unless it is shown that such degradation products are not present during the test.
(ii) Method validation is conducted for the purpose of determining the linear range,
detection limit, accuracy and precision (repeatability and reproducibility) of the method
for analysis of the test substance under the conditions of the test. Thus, quality control
(fortification) samples should be prepared at concentrations spanning the range of
concentrations to be used in the definitive test, using the same procedures (vehicles, etc.)
and in the same matrix (feed, etc.) as will be used in the definitive test.
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(iii) The method validation should include a determination of linearity between detector
response and test substance concentration, the LOQ, the MDL, method accuracy (average
percent recovery) and precision (relative standard deviation). The method validation
should establish the acceptance criteria for the quality control (QC) samples that will be
prepared and analyzed during the test.
(2) Collection of samples. Samples should be collected in such a manner as to provide an
accurate representation of the matrix being sampled. Samples should be processed and analyzed
immediately, or handled and stored in a manner which minimizes loss of test substance through
microbial degradation, photodegradation, chemical reaction, volatilization, sorption or other
processes.
(3) Analysis of test samples. Concurrent with each analysis of test samples, quality control
(fortified) samples should be analyzed. QC samples are prepared by adding known amounts of
the test substance to the test matrix. Minimally, one QC sample should be at the low end of the
test concentration range and one QC sample at the high end. A control (zero-level fortification)
sample should also be included. To determine concordance with the provisions of paragraphs
(e)(4), (e)(6)(iv) and (e)(6)(v) test sample recoveries may be corrected for inherent method bias
as determined from the concurrent analysis of freshly fortified QC samples.
(h) Reference toxicants. Historically, reference toxicity testing has been thought to provide
three types of information relevant to the interpretation of toxicity test data: An indication of the
relative health of the organisms used in the test; A demonstration that the laboratory can perform
the test procedure in a reproducible manner over a period of time; and Information to indicate
whether the sensitivity of a particular strain or population in use at a laboratory is comparable to
that of those used in other facilities and how intra- and inter-laboratory sensitivity varies over
time. However, performance of control organisms over time may be a better indicator of success
in handling and testing of at least some organisms. Nonetheless, periodic reference toxicant
testing can provide an indication of the overall comparability of results within and among
laboratories. Although a positive control is not standard for each test, a quarterly or semiannual
positive control (on a guideline-specific basis) can serve as a means of detecting possible
interlaboratory or temporal variation. A reference toxicant might also be desirable when there is
any significant change in food, housing, source of test animals or in other test conditions.
Despite these potential uses of reference toxicants, alternative means of assessing organism
health, test reproducibility, and intra- and inter-laboratory variation should be considered in order
to minimize of the use of test animals.
(i) Monitoring of test conditions. Test conditions are specified in each test-specific guideline.
These conditions include environmental factors such as temperature, humidity, and lighting.
Methods used for monitoring test conditions should be in accordance with established methods
(e.g., those published by U.S. EPA, ASTM, APHA et al., etc.).
(1) Temperature. Preferably, temperature should be monitored continuously (recorded at least
hourly). Alternatively, the maximum and minimum should be measured daily (which is a
minimum of at least two measurements during each 24 hour period during the study).
Temperature measurements should be made in at least one representative location.
(2) Humidity. Where applicable, humidity should be monitored continuously in at least one
representative location.
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(3) Lighting. Guidance for lighting in laboratory toxicity tests can be found in the reference in
paragraph (k)(3) of this guideline.
(j) Reporting—
(1) Background information. In addition to the reporting requirements prescribed in the Good
Laboratory Practices Standards (40 CFR part 792 and 40 CFR part 160), the report should
include the information in paragraphs (j)0)(i) through (j)(l)(vi) in this guideline:
(i) Test facility (name and location), test dates, and personnel.
(ii) The name of the sponsor, study director, principal investigator, names of other
scientists or professionals, and the names of all supervisory personnel involved in the
study.
(iii) Raw data sufficient to allow independent confirmation the study authors' conclusions
should be presented with the study report. Raw data includes all measurements recorded
during the study including, but not limited to, effects (mortality, growth, etc.),
environmental conditions (temperature, etc.) and test substance concentration or dose
measured as specified and are used for the reconstruction and evaluation of the report of
that study. The absence of raw data may make the study incomplete and impossible to
review for scientific soundness and thus can lead to rejection of the study as scientifically
sound.
(iv) The signed and dated reports of each of the individual scientists or other
professionals involved in the study, including each person who, at the request or direction
of the testing facility or sponsor, conducted an analysis or evaluation of data or
specimens from the study after data generation was completed.
(v) The locations where all raw data and the final report are stored.
(vi) The statement prepared and signed by the quality assurance unit identifying whether
or not the study was conducted in compliance with Good Laboratory Practices Standards
(40 CFR part 792 or 40 CFR part 160). Alternatively the statement can indicate it was
conducted under OECD Principles of Good Laboratory Practice, in accordance with the
multilateral agreement with OECD member countries.
(2) Data elements. The test report should provide a complete and accurate description of test
procedures and evaluation of test results including but not limited to the material in paragraphs
(j)(2)(i) through (j)(2)(xiii) of this guideline:
(i) Objectives and procedures stated in the guideline, including any changes or deviations
or occurrences which may have influenced the results of the test.
(ii) Identification of the test substance (including source, lot or batch number, and purity)
and known physical and chemical properties that are pertinent to the test. As relevant,
solubility and stability of the test substance under the test conditions, and stability of the
test substance under storage conditions if stored prior to analysis. It should be reported if
a formulation is being tested. Where appropriate a cross-reference to OCSPP Series 830
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(Product Properties Test Guidelines) guideline study results can be used to report this
data.
(iii) Methods of preparation of the test substance and the concentrations or doses used in
definitive testing. If vehicles are used, the name and source of the vehicle, the nominal
concentration of the test substance in the vehicle, and the vehicle concentration(s) and
dosage used in the test.
(iv) Information about the test organisms.
(v) A description of the test system used in definitive and any preliminary testing. This
includes a description of the test chambers, method of test substance introduction,
number of organisms per chamber, number of replicates per treatment, all environmental
parameters, description of any feeding during the test (if applicable), including type of
food, source, amount given and frequency.
(vi) Document and submit to the Agency the preliminary test results for review with the
study to which they apply.
(vii) Results of measurements of test substance. All analytical procedures and results
should be described. Report all chemistry methods used in preliminary trials, in range-
finding tests, in establishing percent purity of batches of test substance, or in measuring
concentrations in feed, dosing solutions, or animals. Include in the documentation a
complete description of the method so that a bench chemist can independently determine
what equipment to use and perform the analysis. Also include the raw data, standards,
quality control samples, and chromatograms from samples taken during either definitive
or range-finding tests, not of standard or samples from recovery tests. For a satisfactory
test, the accuracy of the method, LOD, MDL, and LOQ should be given.
(viii) Any difficulties in maintaining constant test substance concentrations should also
be reported. If it is observed that the stability or homogeneity of the test substance
cannot be maintained, care should be taken in the interpretation of the results, and note
made that the results may not be reproducible.
(ix) Methods, frequency, and results of environmental monitoring performed during the
study (temperature, lighting, etc) and other records of test conditions.
(x) Biological observations should be reported in sufficient detail to allow complete
independent evaluation of the results (see specific test guidelines in this group for a
description of what should be reported).
(xi) All data developed during the study that is suggestive or predictive of toxic effects
and all concomitant gross toxicological manifestations.
(xii) Calculated endpoints and a description of all statistical methods, including: software
used, handling of outlier data points, handling of non-detect or zero values, tests to
validate the assumptions of the analyses, level of significance, any data transformations,
for hypothesis tests a measure of the sensitivity of the test (either the minimum
significant difference or the percent change from the control that this minimum difference
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represents). Raw data should be reported to allow independent verification of statistical
procedures.
(xiii) Methods used for test chamber and treatment randomization as well as methods for
impartial assignment of test organisms to test chambers.
(k) References. The references in this paragraph should be consulted for additional background
material on this test guideline.
(1) American Public Health Association, American Water Works Association, Water
Environment Federation, 1998. Standard Methods for the Examination of Water and
Wastewater, 20* edition. Part 8010, Toxicity: Introduction.
(2) American Society for Testing and Materials, 2003. ASTM E 1847-96. Standard practice for
statistical analysis of toxicity tests conducted under ASTM guidelines. In: Annual Book of
ASTM Standards, Vol. 11.06, West Conshohocken, PA. Current edition approved December 10,
1996; Reapproved 2003.
(3) American Society for Testing and Materials, 2002. ASTM E 1733-95. Standard guide for
the use of lighting in laboratory testing. In: Annual Book of ASTM Standards, Vol. 11.06, West
Conshohocken, PA. Current edition approved September 10, 1995; Reapproved 2002.
(4) Bruce, R.D. and DJ. Versteeg, 1992. A statistical procedure for modeling continuous
toxicity data. Environmental Toxicology and Chemistry 11: 1485-1491.
(5) Chapman, G.A., B.S. Anderson, AJ. Bailer, R.B. Baird, R. Berger, D.T. Burton, D.L.
Denton, W.L. Goodfellow, M. A. Heber, L.L. McDonald, T. J. Norberg-King and P. J. Ruffier,
1996. Methods and appropriate endpoints. In Whole Effluent Toxicity Testing, D.R. Grothe,
K.L. Dickson and D.K. Reed-Judkins, eds., SETAC Press, Pensacola, FL.
(6) Daum, R.J., 1970. Revision of two computer programs for probit analysis. Bulletin of the
Entomological Society of America 16:10-15.
(7) Daum, RJ. and W. Killcreas, 1966. Two computer programs for probit analysis. Bulletin of
the Entomological Society of America 12:365-369.
(8) deBruijn, J.H.M. and M. Hof, 1997. How to measure no effect. Part IV: How acceptable is
the ECX from an environmental policy point of view? Environmetrics 8:263-267.
(9) Fairweather, P.G., 1991. Statistical power and design requirements for environmental
monitoring. Australian Journal Marine Freshwater Research 42:555-567.
(10) Finney, D.J., 1971. Probit Analysis 3rd ed., Cambridge: London and New York.
(11) Litchfield, J.T., Jr. and F. Wilcoxon, 1949. A simplified method of evaluating dose-effect
experiments. Journal of Pharmacological Experimental Therapy 96:99-133.
(12) Nabholz, J.V., 1991. Environmental hazard and risk assessment under the Toxic Substances
Control Act. Science of the Total Environment, 109/110: 649-665.
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(13) Nabholz, J.V., P. Miller and M. Zeeman, 1993. Environmental risk assessment of new
chemicals under the Toxic Substances Control Act (TSCA) Section 5, In Environmental
Toxicology and Risk Assessment, Landis, W.G., Hughes, J.S., and Lewis, M.A., eds., ASTM
STP 1179, American Society for Testing and Materials, Philadelphia, PA, pp. 40 -55.
(14) Nyholm, N., P.S. Sorenson, K.O. Kusk, and E.R. Christensen, 1992. Statistical treatment of
data from microbial toxicity tests. Environmental Toxicology and Chemistry 11:157-167.
(15) Organization for Economic Co-operation and Development, 1998. Report of the OECD
Workshop on Statistical Analysis of Aquatic Toxicity Data. OECD Series on Testing and
Assessment, No. 10. ENV/MC/CHEM(98)18.
(16) Organization for Economic Co-Operation and Development. 2006. Current Approaches in
the Statistical Analysis of Ecotoxicity Data: A Guidance to Application. OECD Series on
Testing and Assessment, No. 54. ENV/JM/MONO(2006)18.
(17) Pack, S., 1993. A review of statistical data analysis and experimental design in OECD
aquatic toxicology test guidelines. Report to OECD. Paris.
(18) Smrchek, J.C., R. Clements, R. Morcock, and W. Rabert, 1993. Assessing ecological
hazard under TSCA: methods and evaluation of data, In Environmental Toxicology and Risk
Assessment, Landis, W.G., Hughes, J.S., and Lewis, M.A., eds., ASTM STP 1179, American
Society for Testing and Materials, Philadelphia, PA, pp. 22-39.
(19) Smrchek, J.C. and M.G. Zeeman, 1998. Assessing risks to ecological systems from
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