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§797.1050 Algal acute toxicity test.
(a) Purpose. The guideline in this section is intended for use in developing data on the acute toxicity of chemical substances and mixtures ("chemicals") subject to environmental effects test regulations under the Toxic Substances Control Act (TSCA) (Pub. L. 94-469, 90 Stat. 2003, 15 U.S.C. 2601 et seq.). This guideline prescribes test procedures and conditions using freshwater and marine algae to develop data on the phytotoxicity of chemicals. The United States Environmental Protection Agency (U.S. EPA) will use data from these tests in assessing the hazard of a chemical to the environment.
(b) Definitions. The definitions in section 3 of the Toxic Substances Control Act (TSCA) and the definitions in part 792 -- Good Laboratory Practice Standards of this chapter apply to this test guideline. The following definitions also apply to this guideline:
(1) Algicidal means having the property of killing algae.
(2) Algistatic means having the property of inhibiting algal growth.
(3) ECx means the experimentally derived chemical concentration that is calculated to effect X percent of the test criterion.
(4) Growth means a relative measure of the viability of an algal population based on the number and/or weight of algal cells per volume of nutrient medium or test solution in a specified period of time.
(5) Static system means a test container in which the test solution is not renewed during the period of the test.
(c) Test procedures -- (1) Summary of the test. (i) In preparation for the test, fill test containers with appropriate volumes of nutrient medium and/or test solution. Start the test by introducing algae into the test and control containers in the growth chambers. Environmental conditions within the growth chambers are established at predetermined limits.
(ii) At the end of 96 hours enumerate the algal cells in all containers to
determine inhibition or stimulation of growth in test containers compared to
controls. Use data to define the concentration-response curve, and calculate the
EC (2) [Reserved]
(3) Range-finding test. (i) A range-finding test should be conducted
to determine:
(A) If definitive testing is necessary.
(B) Test chemical concentrations for the definitive test.
(ii) Algae are exposed to a widely spaced (e.g., log interval) chemical
concentration series. The lowest value in the series, exclusive of controls,
should be at the chemical's detection limit. The upper value, for water soluble
compounds, should be the saturation concentration. No replicates are required;
and nominal concentrations of the chemical are acceptable unless definitive
testing is not required.
(iii) The test is performed once for each of the recommended algal species or
selected alternates. Test chambers should contain equal volumes of test solution
and approximately 1×104 Selenastrum cells/ml or 7.7×10
4 Skeletonema cells/ml of test solution. The algae should be
exposed to each concentration of test chemical for up to 96 hours. The exposure
period may be shortened if data suitable for the purposes of the range-finding
test can be obtained in less time.
(iv) Definitive testing is not necessary if the highest chemical
concentration tested (water saturation concentration or 1000 mg/l) results in
less than a 50 percent reduction in growth or if the lowest concentration tested
(analytical detection limit) results in greater than a 50 percent reduction in
growth.
(4) Definitive test. (i) The purpose of the definitive test is to
determine the concentration response curves, the EC (ii) Algae should be exposed to five or more concentrations of the test
chemical in a geometric series in which the ratio is between 1.5 and 2.0 (e.g.,
2, 4, 8, 16, 32, and 64 mg/l). Algae shall be placed in a minimum of three
replicate test containers for each concentration of test chemical and control.
More than three replicates may be required to provide sufficient quantities of
test solution for determination of test substance concentration at the end of
the test. Each test chamber should contain equal volumes of test solution and
approximately 1×104 Selenastrum cells/ml or 7.7×104
Skeletonema cells/ml of test solution. The chemical concentrations should
result in greater than 90 percent of algal growth being inhibited or stimulated
at the highest concentrations of test substance compared to controls.
(iii) Every test shall include a control consisting of the same nutrient
medium, conditions, procedures, and algae from the same culture, except that
none of the test substance is added. If a carrier is present in any of the test
chambers, a separate carrier control is required.
(iv) The test begins when algae from 5- to 10-day-old stock cultures are
placed in the test chambers containing test solutions having the appropriate
concentrations of the test substance. Algal growth in controls should reach the
logarithmic growth phase by 96 hours. If logarithmic growth cannot be
demonstrated, the test shall be repeated. At the end of 24, 48, 72, and 96 hours
the algal growth response (number or weight of algal cells/ml) in all test
containers and controls shall be determined by an indirect (spectrophotometry,
electronic cell counters, dry weight, etc.) or a direct (actual microscopic cell
count) method. Indirect methods shall be calibrated by a direct microscopic
count. The percentage inhibition or stimulation of growth for each
concentration, EC (v) At the end of the definitive test, the following additional analyses of
algal growth response shall be performed:
(A) Determine whether the altered growth response between controls and test
algae was due to a change in relative cell numbers, cell sizes or both. Also
note any unusual cell shapes, color differences, flocculations, adherence of
algae to test containers, or aggregation of algal cells.
(B) In test concentrations where growth is maximally inhibited, algistatic
effects may be differentiated from algicidal effects by the following two
methods for Skeletonema and by the second method for Selenastrum.
(1) Add 0.5 ml of a 0.1 percent solution (weight/volume) of Evans blue
stain to a 1 milliliter aliquot of algae from a control container and to a 1
milliliter aliquot of algae from the test container having the lowest
concentration of test chemical which completely inhibited algal growth (if algal
growth was not completely inhibited, select an aliquot of algae for staining
from the test container having the highest concentration of test chemical which
inhibited algal growth). Wait 10 to 30 minutes, examine microscopically, and
determine the percent of the cells which stain blue (indicating cell mortality).
A staining control shall be performed concurrently using heat-killed or
formaldehyde-preserved algal cells; 100 percent of these cells shall stain blue.
(2) Remove 0.5 ml aliquots of test solution containing
growth-inhibited algae from each replicate test container having the
concentration of test substance evaluated in paragraph (c)(4)(v)(B)(1) of
this section. Combine these aliquots into a new test container and add a
sufficient volume of fresh nutrient medium to dilute the test chemical to a
concentration which does not affect growth. Incubate this subculture under the
environmental conditions used in the definitive test for a period of up to 9
days, and observe for algal growth to determine if the algistatic effect noted
after the 96-hour test is reversible. This subculture test may be discontinued
as soon as growth occurs.
(5) [Reserved]
(6) Analytical measurements -- (i) Chemical. (A) Glass
distilled or deionized water shall be used in the preparation of the nutrient
medium. The pH of the test solution shall be measured in the control and test
containers at the beginning and at the end of the definitive test. The
concentration of test chemical in the test containers shall be determined at the
beginning and end of the definitive test by standard analytical methods which
have been validated prior to the test. An analytical method is unacceptable if
likely degradation products of the chemical, such as hydrolysis and oxidation
products, give positive or negative interference.
(B) At the end of the test and after aliquots have been removed for algal
growth-response determinations, microscopic examination, mortal staining, or
subculturing, the replicate test containers for each chemical concentration may
be pooled into one sample. An aliquot of the pooled sample may then be taken and
the concentration of test chemical determined. In addition, the concentration of
test chemical associated with the algae alone should be determined. Separate and
concentrate the algal cells from the test solution by centrifuging or filtering
the remaining pooled sample and measure the test substance concentration in the
algal-cell concentrate.
(ii) Numerical. Algal growth response (as percent of inhibition or
stimulation in the test solutions compared to the controls) is calculated at the
end of the test. Mean and standard deviation should be calculated and plotted
for each treatment and control. Appropriate statistical analyses should provide
a goodness-of-fit determination for the concentration response curves. The
concentration response curves are plotted using the mean measured test solution
concentrations obtained at the end of the test.
(d) Test conditions -- (1) Test species. Species of algae
recommended as test organisms for this test are the freshwater green alga,
Selenastrum capricornutum, and the marine diatom, Skeletonema
costatum. Algae to be used in acute toxicity tests may be initially obtained
from commercial sources and subsequently cultured using sterile technique.
Toxicity testing shall not be performed until algal cultures are shown to be
actively growing (i.e., capable of logarithmic growth within the test period) in
at least 2 subcultures lasting 7 days each prior to the start of the definitive
test. All algae used for a particular test shall be from the same source and the
same stock culture. Test algae shall not have been used in a previous test,
either in a treatment or a control.
(2) Facilities -- (i) General. (A) Facilities needed to perform
this test include: a growth chamber or a controlled environment room that can
hold the test containers and will maintain the air temperature, lighting
intensity and photoperiod specified in this test guideline; apparatus for
culturing and enumerating algae; a source of distilled and/or deionized water;
and apparatus for carrying out analyses of the test chemical.
(B) Disposal facilities should be adequate to accommodate spent glassware,
algae and test solutions at the end of the test and any bench covering, lab
clothing, or other contaminated materials.
(ii) Test containers. Erlenmeyer flasks should be used for test
containers. The flasks may be of any volume between 125 and 500 ml as long as
the same size is used throughout a test and the test solution volume does not
exceed 50 percent of the flask volume.
(iii) Cleaning and sterilization. New test containers may contain
substances which inhibit growth of algae. They shall therefore be cleaned
thoroughly and used several times to culture algae before being used in toxicity
testing. All glassware used in algal culturing or testing shall be cleaned and
sterilized prior to use according to standard good laboratory practices.
(iv) Conditioning. Test containers should be conditioned by a rinse
with the appropriate test solutions prior to the start of the test. Decant and
add fresh test solutions after an appropriate conditioning period for the test
chemical.
(v) Nutrient medium. (A) Formulation and sterilization of nutrient
medium used for algal culture and preparation of test solutions should conform
to those currently recommended by the U.S. EPA for freshwater and marine algal
bioassays. No chelating agents are to be included in the nutrient medium used
for test solution preparation. Nutrient medium should be freshly prepared for
algal testing and may be dispensed in appropriate volumes in test containers and
sterilized by autoclaving or filtration. The pH of the nutrient medium shall be
7.5 (±0.1) for Selenastrum and 8.1 (±0.1) for Skeletonema at the
start of the test and may be adjusted prior to test chemical addition with 0.1N
NaOH or HC1.
(B) Dilution water used for preparation of nutrient medium and test solutions
should be filtered, deionized or glass distilled. Saltwater for marine algal
nutrient medium and test solutions should be prepared by adding a commercial,
synthetic, sea salt formulation or a modified synthetic seawater formulation to
distilled/deionized water to a concentration of 30 parts per thousand.
(vi) Carriers. Nutrient medium shall be used in making stock solutions
of the test chemical. If a carrier other than nutrient medium is absolutely
necessary to dissolve the chemical, the volume used shall not exceed the minimum
volume necessary to dissolve or suspend the chemical in the test solution.
(3) Test parameters. (i) The test temperature shall be 24 °C for
Selenastrum and 20 °C for Skeletonema. Excursions from the test
temperature shall be no greater than ±2 °C. Temperature should be recorded
hourly during the test.
(ii) Test chambers containing Selenastrum shall be illuminated
continuously and those containing Skeletonema shall be provided a 14-hour
light and 10-hour dark photoperiod with a 30 minute transition period under
fluorescent lamps providing 300 ± 25 uEin/m 2 sec (approximately 400
ft-c) measured adjacent to the test chambers at the level of test solution.
(iii) Stock algal cultures should be shaken twice daily by hand. Test
containers shall be placed on a rotary shaking apparatus and oscillated at
approximately 100 cycles/minute for Selenastrum and at approximately 60
cycles/minute for Skeletonema during the test. The rate of oscillation
should be determined at least once daily during testing.
(iv) The pH of nutrient medium in which algae are subcultured shall be 7.5
(±0.1) for Selenastrum and 8.1 (±0.1) for Skeletonema, and is not
adjusted after the addition of the algae. The pH of all test solutions shall be
measured at the beginning and end of the test.
(v) Light intensity shall be monitored at least daily during the test at the
level of the test solution.
(e) Reporting. The sponsor shall submit to the EPA all data developed
by the test that are suggestive or predictive of acute phytotoxicity. In
addition to the general reporting requirements prescribed in part 792 -- Good
Laboratory Practice Standards of this Chapter, the following shall be
reported:
(1) Detailed information about the test organisms, including the scientific
name, method of verification, and source.
(2) A description of the test chambers and containers, the volumes of
solution in the containers, the way the test was begun (e.g., conditioning, test
substance additions, etc.), the number of replicates, the temperature, the
lighting, and method of incubation, oscillation rates, and type of apparatus.
(3) The concentration of the test chemical in the control and in each
treatment at the end of the test and the pH of the solutions.
(4) The number of algal cells per milliliter in each treatment and control
and the method used to derive these values at the beginning, 24, 48, and 72
hours, and end of the test; the percentage of inhibition or stimulation of
growth relative to controls; and other adverse effect in the control and in each
treatment.
(5) The 96-hour EC (6) Methods and data records of all chemical analyses of water quality and
test substance concentrations, including method validations and reagent blanks.
(7) The results of any optional analyses such as: Microscopic appearance of
algae, size or color changes, percent mortality of cells and the fate of
subcultured cells, the concentration of test substance associated with algae and
test solution supernate or filtrate.
(8) If the range-finding test showed that the highest concentration of the
chemical tested (not less than 1000 mg/l or saturation concentration) had no
effect on the algae, report the results and concentration and a statement that
the chemical is of minimum phytotoxic concern.
(9) If the range-finding test showed greater than a 50 percent inhibition of
algal growth at a test concentration below the analytical detection limit,
report the results, concentration, and a statement that the chemical is
phytotoxic below the analytical detection limit.
[50 FR 39321, Sept. 27, 1985, as amended at 52 FR 19058, May 20,
1987]
