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§798.6400 Neuropathology.
(a) Purpose. The techniques in this guideline are designed to develop data on morphologic changes in the nervous system for chemical substances and mixtures subject to such testing under the Toxic Substances Control Act. The data will detect and characterize morphologic changes, if and when they occur, and determine a no-effect level for such changes. Neuropathological evaluation should be complemented by other neurotoxicity studies, e.g. behavioral and neurophysiological studies. Neuropathological evaluation may be done following acute, subchronic or chronic exposure.
(b) Definition. Neurotoxicity or a neurotoxic effect is an adverse change in the structure or function of the nervous system following exposure to a chemical agent.
(c) Principle of the test method. The test substance is administered to several groups of experimental animals, one dose being used per group. The animals are sacrificed and tissues in the nervous system are examined grossly and prepared for microscopic examination. Starting with the highest dosage level, tissues are examined under the light microscope for morphologic changes, until a no effect level is determined. In cases where light microscopy has revealed neuropathology, the no effect level may be confirmed by electron microscopy.
(d) Test procedure -- (1) Animal selection -- (i) Species and strain. Testing shall be performed in the species being used in other tests for neurotoxicity. This will generally be the laboratory rat. The choice of species shall take into consideration such factors as the comparative metabolism of the chemical and species sensitivity to the toxic effects of the test substance, as evidenced by the results of other studies, the potential for combined studies, and the availability of other toxicity data for the species.
(ii) Age. Animals shall be young adults (150-200 gm for rats) at the start of exposure.
(iii) Sex. Both sexes shall be used unless it is demonstrated that one sex is refractory to the effects.
(2) Number of animals. A minimum of six animals per group shall be used. The tissues from each animal shall be examined separately. It is recomse (iv)mended that ten animals per group be used.
(3) Control groups. (i) A concurrent control group(s) is (are) required. This group must be an untreated control group or, if a vehicle is used in administering the test substance, a vehicle control group. If the vehicle used has a known or potential toxic property, both untreated and vehicle control groups are required.
(ii) A satellite group of animals may be treated with the high level for 90 days and observed for reversibility, persistence, or delayed occurrence of toxic effects for a post-treatment period of appropriate length; normally not less than 28 days.
(4) Dose levels and dose selection. At least 3 doses, equally spaced
on a log scale (e.g., (i) The highest dose shall produce (A) clear behavioral effects or (B)
life-threatening toxicity.
(ii) The data from the lower doses must show either (A) graded dose-dependent
effects at two dose levels or (B) no effects at two dose levels, respectively.
(5) Duration of testing. The exposure duration will be specified in
the test rule. This will generally be 90 days exposure.
(6) Route of administration. The test substance shall be administered
by a route specified in the test rule. This will generally be the route most
closely approximating the route of human exposure. The exposure protocol shall
conform to that outlined in the appropriate acute or subchronic toxicity
guideline.
(7) Combined protocol. The tests described herein may be combined with
any other toxicity study, as long as none of the requirements of either are
violated by the combination.
(8) Study conduct -- (i) Observation of animals. All
toxicological (e.g., weight loss) and neurological signs (e.g., motor
disturbance) shall be recorded frequently enough to observe any abnormality, and
not less than weekly.
(ii) Sacrifice of animals -- (A) General. The goal of the
techniques outlined for sacrifice of animals and preparation of tissues is
preservation of tissues morphology to simulate the living state of the cell.
(B) Perfusion technique. Animals shall be perfused in situ by a
generally recognized technique. For fixation suitable for light or electronic
microscopy, saline solution followed by buffered 2.5 percent glutaraldehyde or
buffered 4.0 percent paraformaldehyde, is recommended. While some minor
modifications or variations in procedures are used in different laboratories, a
detailed and standard procedure for vascular perfusion may be found in the text
by Zeman and Innes (1963) under paragraph (f)(7) of this section, Hayat (1970)
under paragraph (f)(3) of this section, and by Spencer and Schaumburg (1980)
under paragraph (f)(6) of this section. A more sophisticated technique is
described by Palay and Chan-Palay (1974) under paragraph (f)(4) of this section.
(C) Removal of brain and cord. After perfusion, the bonystructure
(cranium and vertebral column) shall be exposed. Animals shall then be stored in
fixative-filled bags at 4 °C for 8-12 hours. The cranium and vertebral column
shall be removed carefully by trained technicians without physical damage of the
brain and cord. Detailed dissection procedures may be found in the text by Palay
and Chan-Palay (1974) under paragraph (f)(4) of this section. After removal,
simple measurement of the size (length and width) and weight of the whole brain
(cerebrum, cerebellum, pons-medulla) shall be made. Any abnormal coloration or
discoloration of the brain and cord shall also be noted and recorded.
(D) Sampling. Unless a given test rule specifies otherwise,
cross-sections of the following areas shall be examined: The forebrain, the
center of the cerebrum, the midbrain, the cerebellum and pons, and the medulla
oblongata; the spinal cord at cervical and lumbar swelling (C (iii) Specimen storage. Tissue samples from both the central and
peripheral nervous system shall be further immersion fixed and stored in
appropriate fixative (e.g., 10 percent buffered formalin for light microscopy;
2.5 percent buffered gluteraldehyde or 4.0 percent buffered paraformaldehyde for
electron microscopy) for future examination. The volume of fixative versus the
volume of tissues in a specimen jar shall be no less than 25:1. All stored
tissues shall be washed with buffer for at least 2 hours prior to further tissue
processing.
(iv) Histopathology examination. (A) Fixation. Tissue specimens
stored in 10 percent buffered formalin may be used for this purpose. All tissues
must be immersion fixed in fixative for at least 48 hours prior to further
tissue processing.
(B) Dehydration. All tissue specimens shall be washed for at least 1
hour with water or buffer, prior to dehydration. (A longer washing time is
needed if the specimens have been stored in fixative for a prolonged period of
time.) Dehydration can be performed with increasing concentration of graded
ethanols up to absolute alcohol.
(C) Clearing and embedding. After dehydration, tissue specimens shall
be cleared with xylene and embedded in paraffin or paraplast. Multiple tissue
specimens (e.g. brain, cord, ganglia) may be embedded together in one single
block for sectioning. All tissue blocks shall be labelled showing at least the
experiment number, animal number, and specimens embedded.
(D) Sectioning. Tissue sections, 5 to 6 microns in thickness, shall be
prepared from the tissue blocks and mounted on standard glass slides. It is
recommended that several additional sections be made from each block at this
time for possible future needs for special stainings. All tissue blocks and
slides shall be filed and stored in properly labeled files or boxes.
(E) Histopathological techniques. Although the information available
for a given chemical substance may dictate test-rule specific changes, the
following general testing sequence is proposed for gathering histopathological
data:
(1) General staining. A general staining procedure shall be
performed on all tissue specimens in the highest treatment group. Hematoxylin
and eosin (H&E) shall be used for this purpose. The staining shall be
differentiated properly to achieve bluish nuclei with pinkish background.
(2) Special stains. Based on the results of the general
staining, selected sites and cellular components shall be further evaluated by
the use of specific techniques. If H&E screening does not provide such
information, a battery of stains shall be used to assess the following
components in all appropriate required samples: neuronal body (e.g.. Einarson's
gallocyanin), axon (e.g., Bodian), myelin sheath (e.g.. Kluver's Luxol Fast
Blue) and neurofibrils (e.g.. Bielchosky). In addition, peripheral nerve fiber
teasing shall be used. Detailed staining methodology is available in standard
histotechnological manuals such as AFIP (1968) under paragraph (f)(1) of this
section, Ralis et al. (1973) under paragraph (f)(5) of this section, and Chang
(1979) under paragraph (f)(2) of this section. The nerve fiber teasing technique
is discussed in Spencer and Schaumberg (1980) under paragraph (f)(6) of this
section. A section of normal tissue shall be included in each staining to assure
that adequate staining has occurred. Any changes shall be noted and
representative photographs shall be taken. If a lesion(s) is observed, the
special techniques shall be repeated in the next lower treatment group until no
further lesion is detectable.
(3) Alternative technique. If the anatomical locus of expected
neuro-pathology is well-defined, epoxy-embedded sections stained with toluidine
blue may be used for small sized tissue samples. This technique obviates the
need for special stains for cellular components. Detailed methodology is
available in Spencer and Schaumberg (1980) under paragraph (f)(6) of this
section.
(4) Electron microscopy. Based on the results of light
microscopic evaluation, specific tissue sites which reveal a lesion(s) shall be
further evaluated by electron microscopy in the highest treatment group which
does not reveal any light microscopic lesion. If a lesion is observed, the next
lower treatment group shall be evaluated until no significant lesion is found.
Detailed methodology is available in Hayat (1970) under paragraph (f)(3) of this
section.
(F) Examination -- (1) General. All stained microscopic
slides shall be examined with a standard research microscope. Examples of
cellular alterations (e.g., neuronal vacuolation, degeneration, and necrosis)
and tissue changes (e.g., gliosis, leukocytic infiltration, and cystic
formation) shall be recorded and photographed.
(2) Electron microscopy. Since the size of the tissue samples
that can be examined is very small, at least 3 to 4 tissue blocks from each
sampling site must be examined. Tissue sections must be examined with a
transmission electron microscope. Three main categories of structural changes
must be considered:
(i) Neuronal body. The shape and position of the nucleus and
nucleolus as well as any change in the chromatin patterns shall be noted. Within
the neuronal cytoplasm, cytoplasmic organelles such as mitochondria, lysosomes,
neurotubules, neurofilaments, microfilaments, endoplasmic reticulum and
polyribosomes (Nissl substance), Golgi complex, and secretory granules shall be
examined.
(ii) Neuronal processes. The structural integrity or
alterations of dendrites, axons (myelinated and unmyelinated), myelin sheaths,
and synapses shall be noted.
(iii) Supporting cells. Attention must also be paid to the
number and structural integrity of the neuroglial elements (oligodendrocytes,
astrocytes, and microglia) of the central nervous system, and the Schwann cells,
satellite cells, and capsule cells of the peripheral nervous system. Any changes
in the endothelial cells and ependymal lining cells shall also be noted whenever
possible. The nature, severity, and frequency of each type of lesion in each
specimen must be recorded. Representative lesions must be photographed and
labeled appropriately.
(e) Data collection, reporting, and evaluation. In addition to
information meeting the requirements stated under 40 CFR part 792 subpart J, the
following specific information shall be reported:
(1) Description of test system and test methods. A description of the
general design of the experiment shall be provided. This shall include a short
justification explaining any decisions where professional judgment is involved
such as fixation technique and choice of stains.
(2) Results. All observations shall be recorded and arranged by test
groups. This data may be presented in the following recommended format:
(i) Description of signs and lesions for each animal. For each animal,
data must be submitted showing its identification (animal number, treatment,
dose, duration), neurologic signs, location(s) nature of, frequency, and
severity of lesion(s). A commonly-used scale such as 1+, 2+, 3+, and 4+ for
degree of severity ranging from very slight to extensive may be used. Any
diagnoses derived from neurologic signs and lesions including naturally
occurring diseases or conditions, should also be recorded.
(ii) Counts and incidence of lesions, by test group. Data shall be
tabulated to show:
(A) The number of animals used in each group, the number of animals
displaying specific neurologic signs, and the number of animals in which any
lesion was found;
(B) The number of animals affected by each different type of lesion, the
average grade of each type of lesion, and the frequency of each different type
and/or location of lesion.
(iii) Evaluation of data. (A) An evaluation of the data based on gross
necropsy findings and microscopic pathology observations shall be made and
supplied. The evaluation shall include the relationship, if any, between the
animal's exposure to the test substance and the frequency and severity of the
lesions observed.
(B) The evaluation of dose-response, if existent, for various groups shall be
given, and a description of statistical method must be presented. The evaluation
of neuropathology data should include, where applicable, an assessment in
conjunction with other neurotoxicity studies performed (eg.
electrophysiological, behavioral, neurochemical).
(f) References. For additional background information on this test
guideline the following references should be consulted:
(1) AFIP. Manual of Histologic Staining Methods. (New York:
McGraw-Hill (1968).
(2) Chang, L.W. A Color Atlas and Manual for Applied Histochemistry.
(Springfield, IL: Charles C. Thomas, 1979).
(3) Hayat, M.A. "Vol. 1. Biological applications," Principles and
techniques of electron microscopy. (New York: Van Nostrand Reinhold, 1970)
(4) Palay S.L., Chan-Palay, V. Cerebellar Cortex: Cytology and
Organization. (New York: Springer-Verlag, 1974).
(5) Ralis, H.M., Beesley, R.A., Ralis, Z.A. Techniques in
Neurohistology. (London: Butterworths, 1973).
(6) Spencer, P.S., Schaumburg, H.H. (eds). Experimental and Clinical
Neurotoxicology. (Baltimore: Williams and Wilkins, 1980).
(7) Zeman, W., JRM Innes, J.R.M. Craigie's Neuroanatomy of the Rat.
(New York: Academic, 1963).
[50 FR 39397, Sept. 27, 1985, as amended at 52 FR 19082, May 20,
1987]
