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Method number: ID-191 Matrix: Bulk
Collection Procedure
Collect approximately 1 to 2 grams of each type of
material and place into separate 20 mL scintillation vials.
Analytical Procedure
A portion of each separate phase is analyzed by gross
examination, phase-polar examination, and central stop dispersion
microscopy.
Commercial manufacturers and products mentioned in this
method are for descriptive use only and do not constitute endorsements by
USDOL-OSHA. Similar products from other sources may be substituted.
1. Introduction
This method describes the collection and analysis of
asbestos bulk materials by light microscopy techniques including
phase-polar illumination and central-stop dispersion microscopy. Some
terms unique to asbestos analysis are defined below:
Amphibole: A family of minerals whose crystals are formed
by long, thin units which have two thin ribbons of double chain silicate
with a brucite ribbon in between. The shape of each unit is similar to an
"I beam". Minerals important in asbestos analysis include
cummingtonite-grunerite, crocidolite, tremolite-actinolite and
anthophyllite.
Asbestos: A term for naturally occurring fibrous minerals.
Asbestos includes chrysotile, cummingtonite-grunerite asbestos (amosite),
anthophyllite asbestos, tremolite asbestos, crocidolite, actinolite
asbestos and any of these minerals which have been chemically treated or
altered. The precise chemical formulation of each species varies with the
location from which it was mined. Nominal compositions are listed: Chrysotile......................................... Mg(3)Si(2)O(5)(OH)(4)
Crocidolite (Riebeckite asbestos)
.............................. Na(2)Fe(3)(2)+Fe(2)(3)+Si(8)O(22)(OH)(2)
Cummingtonite-Grunerite asbestos (Amosite)
........................................... (Mg,Fe)(7)Si(8)O(22)(OH)(2)
Tremolite-Actinolite asbestos
...................................... Ca(2)(Mg,Fe)(5)Si(8)O(22)(OH)(2)
Anthophyllite asbestos....................... (Mg,Fe)(7)Si(8)O(22)(OH)(2)
Asbestos Fiber: A fiber of asbestos meeting the criteria
for a fiber. (See section 3.5.)
Aspect Ratio: The ratio of the length of a fiber to its
diameter usually defined as "length : width", e.g. 3:1.
Brucite: A sheet mineral with the composition
Mg(OH)(2).
Central Stop Dispersion Staining (microscope): This is a
dark field microscope technique that images particles using only light
refracted by the particle, excluding light that travels through the
particle unrefracted. This is usually accomplished with a McCrone
objective or other arrangement which places a circular stop with apparent
aperture equal to the objective aperture in the back focal plane of the
microscope.
Cleavage Fragments: Mineral particles formed by the
comminution of minerals, especially those characterized by relatively
parallel sides and moderate aspect ratio.
Differential Counting: The term applied to the practice of
excluding certain kinds of fibers from a phase contrast asbestos count
because they are not asbestos.
Fiber: A particle longer than or equal to 5 um with a
length to width ratio greater than or equal to 3:1. This may include
cleavage fragments. (see section 3.5 of this appendix).
Phase Contrast: Contrast obtained in the microscope by
causing light scattered by small particles to destructively interfere with
unscattered light, thereby enhancing the visibility of very small
particles and particles with very low intrinsic contrast.
Phase Contrast Microscope: A microscope configured with a
phase mask pair to create phase contrast. The technique which uses this is
called Phase Contrast Microscopy (PCM).
Phase-Polar Analysis: This is the use of polarized light
in a phase contrast microscope. It is used to see the same size fibers
that are visible in air filter analysis. Although fibers finer than 1 um
are visible, analysis of these is inferred from analysis of larger bundles
that are usually present.
Phase-Polar Microscope: The phase-polar microscope is a
phase contrast microscope which has an analyzer, a polarizer, a first
order red plate and a rotating phase condenser all in place so that the
polarized light image is enhanced by phase contrast.
Sealing Encapsulant: This is a product which can be
applied, preferably by spraying, onto an asbestos surface which will seal
the surface so that fibers cannot be released.
Serpentine: A mineral family consisting of minerals with
the general composition Mg(3)(Si(2)O(5)(OH)(4) having the magnesium in
brucite layer over a silicate layer. Minerals important in asbestos
analysis included in this family are chrysotile, lizardite,
antigorite.
1.1. History
Light microscopy has been used for well over 100 years for
the determination of mineral species. This analysis is carried out using
specialized polarizing microscopes as well as bright field microscopes.
The identification of minerals is an on-going process with many new
minerals described each year. The first recorded use of asbestos was in
Finland about 2500 B.C. where the material was used in the mud wattle for
the wooden huts the people lived in as well as strengthening for pottery.
Adverse health aspects of the mineral were noted nearly 2000 years ago
when Pliny the Younger wrote about the poor health of slaves in the
asbestos mines. Although known to be injurious for centuries, the first
modern references to its toxicity were by the British Labor Inspectorate
when it banned asbestos dust from the workplace in 1898. Asbestosis cases
were described in the literature after the turn of the century. Cancer was
first suspected in the mid 1930's and a causal link to mesothelioma was
made in 1965. Because of the public concern for worker and public safety
with the use of this material, several different types of analysis were
applied to the determination of asbestos content. Light microscopy
requires a great deal of experience and craft. Attempts were made to apply
less subjective methods to the analysis. X-ray diffraction was partially
successful in determining the mineral types but was unable to separate out
the fibrous portions from the non-fibrous portions. Also, the minimum
detection limit for asbestos analysis by X-ray diffraction (XRD) is about
1%. Differential Thermal Analysis (DTA) was no more successful. These
provide useful corroborating information when the presence of asbestos has
been shown by microscopy; however, neither can determine the difference
between fibrous and non-fibrous minerals when both habits are present. The
same is true of Infrared Absorption (IR).
When electron microscopy was applied to asbestos analysis,
hundreds of fibers were discovered present too small to be visible in any
light microscope. There are two different types of electron microscope
used for asbestos analysis: Scanning Electron Microscope (SEM) and
Transmission Electron Microscope (TEM). Scanning Electron Microscopy is
useful in identifying minerals. The SEM can provide two of the three
pieces of information required to identify fibers by electron microscopy:
morphology and chemistry. The third is structure as determined by Selected
Area Electron Diffraction -- SAED which is performed in the TEM. Although
the resolution of the SEM is sufficient for very fine fibers to be seen,
accuracy of chemical analysis that can be performed on the fibers varies
with fiber diameter in fibers of less than 0.2 um diameter. The TEM is a
powerful tool to identify fibers too small to be resolved by light
microscopy and should be used in conjunction with this method when
necessary. The TEM can provide all three pieces of information required
for fiber identification. Most fibers thicker than 1 um can adequately be
defined in the light microscope. The light microscope remains as the best
instrument for the determination of mineral type. This is because the
minerals under investigation were first described analytically with the
light microscope. It is inexpensive and gives positive identification for
most samples analyzed. Further, when optical techniques are inadequate,
there is ample indication that alternative techniques should be used for
complete identification of the sample.
1.2. Principle
Minerals consist of atoms that may be arranged in random
order or in a regular arrangement. Amorphous materials have atoms in
random order while crystalline materials have long range order. Many
materials are transparent to light, at least for small particles or for
thin sections. The properties of these materials can be investigated by
the effect that the material has on light passing through it. The six
asbestos minerals are all crystalline with particular properties that have
been identified and cataloged. These six minerals are anisotropic. They
have a regular array of atoms, but the arrangement is not the same in all
directions. Each major direction of the crystal presents a different
regularity. Light photons traveling in each of these main directions will
encounter different electrical neighborhoods, affecting the path and time
of travel. The techniques outlined in this method use the fact that light
traveling through fibers or crystals in different directions will behave
differently, but predictably. The behavior of the light as it travels
through a crystal can be measured and compared with known or determined
values to identify the mineral species. Usually, Polarized Light
Microscopy (PLM) is performed with strain-free objectives on a
bright-field microscope platform. This would limit the resolution of the
microscope to about 0.4 um. Because OSHA requires the counting and
identification of fibers visible in phase contrast, the phase contrast
platform is used to visualize the fibers with the polarizing elements
added into the light path. Polarized light methods cannot identify fibers
finer than about 1 um in diameter even though they are visible. The finest
fibers are usually identified by inference from the presence of larger,
identifiable fiber bundles. When fibers are present, but not identifiable
by light microscopy, use either SEM or TEM to determine the fiber
identity.
1.3. Advantages and Disadvantages
The advantages of light microcopy are:
(a) Basic identification of the materials was first
performed by light microscopy and gross analysis. This provides a large
base of published information against which to check analysis and
analytical technique.
(b) The analysis is specific to fibers. The minerals
present can exist in asbestiform, fibrous, prismatic, or massive varieties
all at the same time. Therefore, bulk methods of analysis such as X-ray
diffraction, IR analysis, DTA, etc. are inappropriate where the material
is not known to be fibrous.
(c) The analysis is quick, requires little preparation
time, and can be performed on-site if a suitably equipped microscope is
available.
The disadvantages are:
(a) Even using phase-polar illumination, not all the
fibers present may be seen. This is a problem for very low asbestos
concentrations where agglomerations or large bundles of fibers may not be
present to allow identification by inference.
(b) The method requires a great degree of sophistication
on the part of the microscopist. An analyst is only as useful as his
mental catalog of images. Therefore, a microscopist's accuracy is enhanced
by experience. The mineralogical training of the analyst is very
important. It is the basis on which subjective decisions are made.
(c) The method uses only a tiny amount of material for
analysis. This may lead to sampling bias and false results (high or low).
This is especially true if the sample is severely inhomogeneous.
(d) Fibers may be bound in a matrix and not
distinguishable as fibers so identification cannot be made.
1.4. Method Performance
1.4.1. This method can be used for determination of
asbestos content from 0 to 100% asbestos. The detection limit has not been
adequately determined, although for selected samples, the limit is very
low, depending on the number of particles examined. For mostly
homogeneous, finely divided samples, with no difficult fibrous
interferences, the detection limit is below 1%. For inhomogeneous samples
(most samples), the detection limit remains undefined. NIST has conducted
proficiency testing of laboratories on a national scale. Although each
round is reported statistically with an average, control limits, etc., the
results indicate a difficulty in establishing precision especially in the
low concentration range. It is suspected that there is significant bias in
the low range especially near 1%. EPA tried to remedy this by requiring a
mandatory point counting scheme for samples less than 10%. The point
counting procedure is tedious, and may introduce significant biases of its
own. It has not been incorporated into this method.
1.4.2. The precision and accuracy of the quantitation
tests performed in this method are unknown. Concentrations are easier to
determine in commercial products where asbestos was deliberately added
because the amount is usually more than a few percent. An analyst's
results can be "calibrated" against the known amounts added by the
manufacturer. For geological samples, the degree of homogeneity affects
the precision.
1.4.3. The performance of the method is analyst dependent.
The analyst must choose carefully and not necessarily randomly the
portions for analysis to assure that detection of asbestos occurs when it
is present. For this reason, the analyst must have adequate training in
sample preparation, and experience in the location and identification of
asbestos in samples. This is usually accomplished through substantial
on-the-job training as well as formal education in mineralogy and
microscopy.
1.5. Interferences
Any material which is long, thin, and small enough to be
viewed under the microscope can be considered an interference for
asbestos. There are literally hundreds of interferences in workplaces. The
techniques described in this method are normally sufficient to eliminate
the interferences. An analyst's success in eliminating the interferences
depends on proper training.
Asbestos minerals belong to two mineral families: the
serpentines and the amphiboles. In the serpentine family, the only common
fibrous mineral is chrysotile. Occasionally, the mineral antigorite occurs
in a fibril habit with morphology similar to the amphiboles. The amphibole
minerals consist of a score of different minerals of which only five are
regulated by federal standard: amosite, crocidolite, anthophyllite
asbestos, tremolite asbestos and actinolite asbestos. These are the only
amphibole minerals that have been commercially exploited for their fibrous
properties; however, the rest can and do occur occasionally in asbestiform
habit.
In addition to the related mineral interferences, other
minerals common in building material may present a problem for some
microscopists: gypsum, anhydrite, brucite, quartz fibers, talc fibers or
ribbons, wollastonite, perlite, attapulgite, etc. Other fibrous materials
commonly present in workplaces are: fiberglass, mineral wool, ceramic
wool, refractory ceramic fibers, kevlar, nomex, synthetic fibers, graphite
or carbon fibers, cellulose (paper or wood) fibers, metal fibers, etc.
Matrix embedding material can sometimes be a negative
interference. The analyst may not be able to easily extract the fibers
from the matrix in order to use the method. Where possible, remove the
matrix before the analysis, taking careful note of the loss of weight.
Some common matrix materials are: vinyl, rubber, tar, paint, plant fiber,
cement, and epoxy. A further negative interference is that the asbestos
fibers themselves may be either too small to be seen in Phase contrast
Microscopy (PCM) or of a very low fibrous quality, having the appearance
of plant fibers. The analyst's ability to deal with these materials
increases with experience.
1.6. Uses and Occupational Exposure
Asbestos is ubiquitous in the environment. More than 40%
of the land area of the United States is composed of minerals which may
contain asbestos. Fortunately, the actual formation of great amounts of
asbestos is relatively rare. Nonetheless, there are locations in which
environmental exposure can be severe such as in the Serpentine Hills of
California.
There are thousands of uses for asbestos in industry and
the home. Asbestos abatement workers are the most current segment of the
population to have occupational exposure to great amounts of asbestos. If
the material is undisturbed, there is no exposure. Exposure occurs when
the asbestos-containing material is abraded or otherwise disturbed during
maintenance operations or some other activity. Approximately 95% of the
asbestos in place in the United States is chrysotile.
Amosite and crocidolite make up nearly all the difference.
Tremolite and anthophyllite make up a very small percentage. Tremolite is
found in extremely small amounts in certain chrysotile deposits.
Actinolite exposure is probably greatest from environmental sources, but
has been identified in vermiculite containing, sprayed-on insulating
materials which may have been certified as asbestos-free.
1.7. Physical and Chemical Properties
The nominal chemical compositions for the asbestos
minerals were given in Section 1. Compared to cleavage fragments of the
same minerals, asbestiform fibers possess a high tensile strength along
the fiber axis. They are chemically inert, non-combustible, and heat
resistant. Except for chrysotile, they are insoluble in Hydrochloric acid
(HCl). Chrysotile is slightly soluble in HCl. Asbestos has high electrical
resistance and good sound absorbing characteristics. It can be woven into
cables, fabrics or other textiles, or matted into papers, felts, and
mats.
1.8. Toxicology (This Section is for Information Only and
Should Not Be Taken as OSHA Policy)
Possible physiologic results of respiratory exposure to
asbestos are mesothelioma of the pleura or peritoneum, interstitial
fibrosis, asbestosis, pneumoconiosis, or respiratory cancer. The possible
consequences of asbestos exposure are detailed in the NIOSH Criteria
Document or in the OSHA Asbestos Standards 29 CFR 1910.1001 and 29 CFR
1926.1101 and 29 CFR 1915.1001.
2. Sampling Procedure
2.1. Equipment for Sampling
(a) Tube or cork borer sampling device
(b) Knife
(c) 20 mL scintillation vial or similar vial
(d) Sealing encapsulant
2.2. Safety Precautions
Asbestos is a known carcinogen. Take care when sampling.
While in an asbestos-containing atmosphere, a properly selected and
fit-tested respirator should be worn. Take samples in a manner to cause
the least amount of dust. Follow these general guidelines:
(a) Do not make unnecessary dust.
(b) Take only a small amount (1 to 2 g).
(c) Tightly close the sample container.
(d) Use encapsulant to seal the spot where the sample was
taken, if necessary.
2.3. Sampling Procedure
Samples of any suspect material should be taken from an
inconspicuous place. Where the material is to remain, seal the sampling
wound with an encapsulant to eliminate the potential for exposure from the
sample site. Microscopy requires only a few milligrams of material. The
amount that will fill a 20 mL scintillation vial is more than adequate. Be
sure to collect samples from all layers and phases of material. If
possible, make separate samples of each different phase of the material.
This will aid in determining the actual hazard. DO NOT USE ENVELOPES,
PLASTIC OR PAPER BAGS OF ANY KIND TO COLLECT SAMPLES. The use of plastic
bags presents a contamination hazard to laboratory personnel and to other
samples. When these containers are opened, a bellows effect blows fibers
out of the container onto everything, including the person opening the
container.
If a cork-borer type sampler is available, push the tube
through the material all the way, so that all layers of material are
sampled. Some samplers are intended to be disposable. These should be
capped and sent to the laboratory. If a non-disposable cork borer is used,
empty the contents into a scintillation vial and send to the laboratory.
Vigorously and completely clean the cork borer between samples.
2.4 Shipment
Samples packed in glass vials must not touch or they might
break in shipment.
(a) Seal the samples with a sample seal over the end to
guard against tampering and to identify the sample.
(b) Package the bulk samples in separate packages from the
air samples. They may cross-contaminate each other and will invalidate the
results of the air samples.
(c) Include identifying paperwork with the samples, but
not in contact with the suspected asbestos.
(d) To maintain sample accountability, ship the samples by
certified mail, overnight express, or hand carry them to the
laboratory.
3. Analysis
The analysis of asbestos samples can be divided into two
major parts: sample preparation and microscopy. Because of the different
asbestos uses that may be encountered by the analyst, each sample may need
different preparation steps. The choices are outlined below. There are
several different tests that are performed to identify the asbestos
species and determine the percentage. They will be explained below.
3.1. Safety
(a) Do not create unnecessary dust. Handle the samples in
HEPA-filter equipped hoods. If samples are received in bags, envelopes or
other inappropriate container, open them only in a hood having a face
velocity at or greater than 100 fpm. Transfer a small amount to a
scintillation vial and only handle the smaller amount.
(b) Open samples in a hood, never in the open lab
area.
(c) Index of refraction oils can be toxic. Take care not
to get this material on the skin. Wash immediately with soap and water if
this happens.
(d) Samples that have been heated in the muffle furnace or
the drying oven may be hot. Handle them with tongs until they are cool
enough to handle.
(e) Some of the solvents used, such as THF
(tetrahydrofuran), are toxic and should only be handled in an appropriate
fume hood and according to instructions given in the Material Safety Data
Sheet (MSDS).
3.2. Equipment
(a) Phase contrast microscope with 10x, 16x and 40x
objectives, 10x wide-field eyepieces, G-22 Walton-Beckett graticule,
Whipple disk, polarizer, analyzer and first order red or gypsum plate, 100
Watt illuminator, rotating position condenser with oversize phase rings,
central stop dispersion objective, Kohler illumination and a rotating
mechanical stage.
(b) Stereo microscope with reflected light illumination,
transmitted light illumination, polarizer, analyzer and first order red or
gypsum plate, and rotating stage.
(c) Negative pressure hood for the stereo microscope
(d) Muffle furnace capable of 600 deg. C
(e) Drying oven capable of 50 -- 150 deg. C
(f) Aluminum specimen pans
(g) Tongs for handling samples in the furnace
(h) High dispersion index of refraction oils (Special for
dispersion staining.) n = 1.550
n = 1.585
n = 1.590
n = 1.605
n = 1.620
n = 1.670
n = 1.680
n = 1.690
(i) A set of index of refraction oils from about n = 1.350
to n = 2.000 in n = 0.005 increments. (Standard for Becke line
analysis.)
(j) Glass slides with painted or frosted ends 1 x 3 inches
1mm thick, precleaned.
(k) Cover Slips 22 x 22 mm, #1 1/2
(l) Paper clips or dissection needles
(m) Hand grinder
(n) Scalpel with both #10 and #11 blades
(o) 0.1 molar HCl
(p) Decalcifying solution (Baxter Scientific Products)
Ethylenediaminetetraacetic Acid, Tetrasodium................................................... 0.7 g/l
Sodium Potassium Tartrate................................ 8.0 mg/liter
Hydrochloric Acid........................................ 99.2 g/liter
Sodium Tartrate.......................................... 0.14 g/liter
(q) Tetrahydrofuran (THF)
(r) Hotplate capable of 60 deg. C
(s) Balance
(t) Hacksaw blade
(u) Ruby mortar and pestle
3.3. Sample Pre-Preparation
Sample preparation begins with pre-preparation which may
include chemical reduction of the matrix, heating the sample to dryness or
heating in the muffle furnace. The end result is a sample which has been
reduced to a powder that is sufficiently fine to fit under the cover slip.
Analyze different phases of samples separately, e.g., tile and the tile
mastic should be analyzed separately as the mastic may contain asbestos
while the tile may not.
(a) Wet samples
Samples with a high water content will not give the proper
dispersion colors and must be dried prior to sample mounting. Remove the
lid of the scintillation vial, place the bottle in the drying oven and
heat at 100 deg. C to dryness (usually about 2 h). Samples which are not
submitted to the lab in glass must be removed and placed in glass vials or
aluminum weighing pans before placing them in the drying oven.
(b) Samples With Organic Interference -- Muffle
Furnace
These may include samples with tar as a matrix, vinyl
asbestos tile, or any other organic that can be reduced by heating. Remove
the sample from the vial and weigh in a balance to determine the weight of
the submitted portion. Place the sample in a muffle furnace at 500 deg. C
for 1 to 2 h or until all obvious organic material has been removed.
Retrieve, cool and weigh again to determine the weight loss on ignition.
This is necessary to determine the asbestos content of the submitted
sample, because the analyst will be looking at a reduced sample.
Note: Heating above 600 deg. C will cause the sample to
undergo a structural change which, given sufficient time, will convert the
chrysotile to forsterite. Heating even at lower temperatures for 1 to 2 h
may have a measurable effect on the optical properties of the minerals. If
the analyst is unsure of what to expect, a sample of standard asbestos
should be heated to the same temperature for the same length of time so
that it can be examined for the proper interpretation.
(c) Samples With Organic Interference -- THF
Vinyl asbestos tile is the most common material treated
with this solvent, although, substances containing tar will sometimes
yield to this treatment. Select a portion of the material and then grind
it up if possible. Weigh the sample and place it in a test tube. Add
sufficient THF to dissolve the organic matrix. This is usually about 4 to
5 mL. Remember, THF is highly flammable. Filter the remaining material
through a tared silver membrane, dry and weigh to determine how much is
left after the solvent extraction. Further process the sample to remove
carbonate or mount directly.
(d) Samples With Carbonate Interference
Carbonate material is often found on fibers and sometimes
must be removed in order to perform dispersion microscopy. Weigh out a
portion of the material and place it in a test tube. Add a sufficient
amount of 0.1 M HCl or decalcifying solution in the tube to react all the
carbonate as evidenced by gas formation; i.e., when the gas bubbles stop,
add a little more solution. If no more gas forms, the reaction is
complete. Filter the material out through a tared silver membrane, dry and
weigh to determine the weight lost.
3.4. Sample Preparation
Samples must be prepared so that accurate determination
can be made of the asbestos type and amount present. The following steps
are carried out in the low-flow hood (a low-flow hood has less than 50 fpm
flow):
(1) If the sample has large lumps, is hard, or cannot be
made to lie under a cover slip, the grain size must be reduced. Place a
small amount between two slides and grind the material between them or
grind a small amount in a clean mortar and pestle. The choice of whether
to use an alumina, ruby, or diamond mortar depends on the hardness of the
material. Impact damage can alter the asbestos mineral if too much
mechanical shock occurs. (Freezer mills can completely destroy the
observable crystallinity of asbestos and should not be used). For some
samples, a portion of material can be shaved off with a scalpel, ground
off with a hand grinder or hack saw blade.
The preparation tools should either be disposable or
cleaned thoroughly. Use vigorous scrubbing to loosen the fibers during the
washing. Rinse the implements with copious amounts of water and air-dry in
a dust-free environment.
(2) If the sample is powder or has been reduced as in (1)
above, it is ready to mount. Place a glass slide on a piece of optical
tissue and write the identification on the painted or frosted end. Place
two drops of index of refraction medium n = 1.550 on the slide. (The
medium n = 1.550 is chosen because it is the matching index for
chrysotile. Dip the end of a clean paper-clip or dissecting needle into
the droplet of refraction medium on the slide to moisten it. Then dip the
probe into the powder sample. Transfer what sticks on the probe to the
slide. The material on the end of the probe should have a diameter of
about 3 mm for a good mount. If the material is very fine, less sample may
be appropriate. For non-powder samples such as fiber mats, forceps should
be used to transfer a small amount of material to the slide. Stir the
material in the medium on the slide, spreading it out and making the
preparation as uniform as possible. Place a cover-slip on the preparation
by gently lowering onto the slide and allowing it to fall "trapdoor"
fashion on the preparation to push out any bubbles. Press gently on the
cover slip to even out the distribution of particulate on the slide. If
there is insufficient mounting oil on the slide, one or two drops may be
placed near the edge of the coverslip on the slide. Capillary action will
draw the necessary amount of liquid into the preparation. Remove excess
oil with the point of a laboratory wiper.
Treat at least two different areas of each phase in this
fashion. Choose representative areas of the sample. It may be useful to
select particular areas or fibers for analysis. This is useful to identify
asbestos in severely inhomogeneous samples.
When it is determined that amphiboles may be present,
repeat the above process using the appropriate high-dispersion oils until
an identification is made or all six asbestos minerals have been ruled
out. Note that percent determination must be done in the index medium
1.550 because amphiboles tend to disappear in their matching mediums.
3.5. Analytical Procedure
Note: This method presumes some knowledge of mineralogy
and optical petrography.
The analysis consists of three parts: The determination of
whether there is asbestos present, what type is present and the
determination of how much is present. The general flow of the analysis
is:
(1) Gross examination.
(2) Examination under polarized light on the stereo
microscope.
(3) Examination by phase-polar illumination on the
compound phase microscope.
(4) Determination of species by dispersion stain.
Examination by Becke line analysis may also be used; however, this is
usually more cumbersome for asbestos determination.
(5) Difficult samples may need to be analyzed by SEM or
TEM, or the results from those techniques combined with light microscopy
for a definitive identification. Identification of a particle as asbestos
requires that it be asbestiform. Description of particles should follow
the suggestion of Campbell. (Figure 1) (For Figure 1 of Asbestos Particles, Click Here)
For the purpose of regulation, the mineral must be one of
the six minerals covered and must be in the asbestos growth habit. Large
specimen samples of asbestos generally have the gross appearance of wood.
Fibers are easily parted from it. Asbestos fibers are very long compared
with their widths. The fibers have a very high tensile strength as
demonstrated by bending without breaking. Asbestos fibers exist in bundles
that are easily parted, show longitudinal fine structure and may be tufted
at the ends showing "bundle of sticks" morphology. In the microscope some
of these properties may not be observable. Amphiboles do not always show
striations along their length even when they are asbestos. Neither will
they always show tufting. They generally do not show a curved nature
except for very long fibers. Asbestos and asbestiform minerals are usually
characterized in groups by extremely high aspect ratios (greater than
100:1). While aspect ratio analysis is useful for characterizing
populations of fibers, it cannot be used to identify individual fibers of
intermediate to short aspect ratio. Observation of many fibers is often
necessary to determine whether a sample consists of "cleavage fragments"
or of asbestos fibers.
Most cleavage fragments of the asbestos minerals are
easily distinguishable from true asbestos fibers. This is because true
cleavage fragments usually have larger diameters than 1 um. Internal
structure of particles larger than this usually shows them to have no
internal fibrillar structure. In addition, cleavage fragments of the
monoclinic amphiboles show inclined extinction under crossed polars with
no compensator. Asbestos fibers usually show extinction at zero degrees or
ambiguous extinction if any at all. Morphologically, the larger cleavage
fragments are obvious by their blunt or stepped ends showing prismatic
habit. Also, they tend to be acicular rather than filiform.
Where the particles are less than 1 um in diameter and
have an aspect ratio greater than or equal to 3:1, it is recommended that
the sample be analyzed by SEM or TEM if there is any question whether the
fibers are cleavage fragments or asbestiform particles.
Care must be taken when analyzing by electron microscopy
because the interferences are different from those in light microscopy and
may structurally be very similar to asbestos. The classic interference is
between anthophyllite and biopyribole or intermediate fiber. Use the same
morphological clues for electron microscopy as are used for light
microscopy, e.g. fibril splitting, internal longitudinal striation,
fraying, curvature, etc.
(1) Gross examination:
Examine the sample, preferably in the glass vial.
Determine the presence of any obvious fibrous component. Estimate a
percentage based on previous experience and current observation. Determine
whether any pre-preparation is necessary. Determine the number of phases
present. This step may be carried out or augmented by observation at 6 to
40 x under a stereo microscope.
(2) After performing any necessary pre-preparation,
prepare slides of each phase as described above. Two preparations of the
same phase in the same index medium can be made side-by-side on the same
glass for convenience. Examine with the polarizing stereo microscope.
Estimate the percentage of asbestos based on the amount of birefringent
fiber present.
(3) Examine the slides on the phase-polar microscopes at
magnifications of 160 and 400 x . Note the morphology of the fibers. Long,
thin, very straight fibers with little curvature are indicative of fibers
from the amphibole family. Curved, wavy fibers are usually indicative of
chrysotile. Estimate the percentage of asbestos on the phase-polar
microscope under conditions of crossed polars and a gypsum plate. Fibers
smaller than 1.0 um in thickness must be identified by inference to the
presence of larger, identifiable fibers and morphology. If no larger
fibers are visible, electron microscopy should be performed. At this
point, only a tentative identification can be made. Full identification
must be made with dispersion microscopy. Details of the tests are included
in the appendices.
(4) Once fibers have been determined to be present, they
must be identified. Adjust the microscope for dispersion mode and observe
the fibers. The microscope has a rotating stage, one polarizing element,
and a system for generating dark-field dispersion microscopy (see Section
4.6. of this appendix). Align a fiber with its length parallel to the
polarizer and note the color of the Becke lines. Rotate the stage to bring
the fiber length perpendicular to the polarizer and note the color. Repeat
this process for every fiber or fiber bundle examined. The colors must be
consistent with the colors generated by standard asbestos reference
materials for a positive identification. In n = 1.550, amphiboles will
generally show a yellow to straw-yellow color indicating that the fiber
indices of refraction are higher than the liquid. If long, thin fibers are
noted and the colors are yellow, prepare further slides as above in the
suggested matching liquids listed below:
________________________________________________________________________
|
Type of asbestos | Index of refraction
_________________________________________|______________________________
|
Chrysotile...............................| n = 1.550.
Amosite..................................| n = 1.670 r 1.680.
Crocidolite..............................| n = 1.690.
Anthophyllite............................| n = 1.605 nd 1.620.
Tremolite................................| n = 1.605 and 1.620.
Actinolite...............................| n = 1.620.
_________________________________________|_______________________________
Where more than one liquid is suggested, the first is
preferred; however, in some cases this liquid will not give good
dispersion color. Take care to avoid interferences in the other liquid;
e.g., wollastonite in n = 1.620 will give the same colors as tremolite. In
n = 1.605 wollastonite will appear yellow in all directions. Wollastonite
may be determined under crossed polars as it will change from blue to
yellow as it is rotated along its fiber axis by tapping on the cover slip.
Asbestos minerals will not change in this way.
Determination of the angle of extinction may, when
present, aid in the determination of anthophyllite from tremolite. True
asbestos fibers usually have 0 deg. extinction or ambiguous extinction,
while cleavage fragments have more definite extinction.
Continue analysis until both preparations have been
examined and all present species of asbestos are identified. If there are
no fibers present, or there is less than 0.1% present, end the analysis
with the minimum number of slides (2).
(5) Some fibers have a coating on them which makes
dispersion microscopy very difficult or impossible. Becke line analysis or
electron microscopy may be performed in those cases. Determine the
percentage by light microscopy. TEM analysis tends to overestimate the
actual percentage present.
(6) Percentage determination is an estimate of occluded
area, tempered by gross observation. Gross observation information is used
to make sure that the high magnification microscopy does not greatly over-
or under-estimate the amount of fiber present. This part of the analysis
requires a great deal of experience. Satisfactory models for asbestos
content analysis have not yet been developed, although some models based
on metallurgical grain-size determination have found some utility.
Estimation is more easily handled in situations where the grain sizes
visible at about 160 x are about the same and the sample is relatively
homogeneous.
View all of the area under the cover slip to make the
percentage determination. View the fields while moving the stage, paying
attention to the clumps of material. These are not usually the best areas
to perform dispersion microscopy because of the interference from other
materials. But, they are the areas most likely to represent the accurate
percentage in the sample. Small amounts of asbestos require slower
scanning and more frequent analysis of individual fields.
Report the area occluded by asbestos as the concentration.
This estimate does not generally take into consideration the difference in
density of the different species present in the sample. For most samples
this is adequate. Simulation studies with similar materials must be
carried out to apply microvisual estimation for that purpose and is beyond
the scope of this procedure.
(7) Where successive concentrations have been made by
chemical or physical means, the amount reported is the percentage of the
material in the "as submitted" or original state. The percentage
determined by microscopy is multiplied by the fractions remaining after
pre-preparation steps to give the percentage in the original sample. For
example:
Step 1. 60% remains after heating at 550 deg. C for 1
h.
Step 2. 30% of the residue of step 1 remains after
dissolution of carbonate in 0.1 m HCl.
Step 3. Microvisual estimation determines that 5% of the
sample is chrysotile asbestos. The reported result is:
R = (Microvisual result in percent) x (Fraction remaining after step 2)
x (Fraction remaining of original sample after step 1)
R = (5) x (.30) x (.60) = 0.9%
(8) Report the percent and type of asbestos present. For
samples where asbestos was identified, but is less than 1.0%, report
"Asbestos present, less than 1.0%." There must have been at least two
observed fibers or fiber bundles in the two preparations to be reported as
present. For samples where asbestos was not seen, report as "None
Detected."
4. Auxiliary Information
Because of the subjective nature of asbestos analysis,
certain concepts and procedures need to be discussed in more depth. This
information will help the analyst understand why some of the procedures
are carried out the way they are.
4.1. Light
Light is electromagnetic energy. It travels from its
source in packets called quanta. It is instructive to consider light as a
plane wave. The light has a direction of travel. Perpendicular to this and
mutually perpendicular to each other, are two vector components. One is
the magnetic vector and the other is the electric vector. We shall only be
concerned with the electric vector. In this description, the interaction
of the vector and the mineral will describe all the observable phenomena.
From a light source such a microscope illuminator, light travels in all
different direction from the filament.
In any given direction away from the filament, the
electric vector is perpendicular to the direction of travel of a light
ray. While perpendicular, its orientation is random about the travel axis.
If the electric vectors from all the light rays were lined up by passing
the light through a filter that would only let light rays with electric
vectors oriented in one direction pass, the light would then be
POLARIZED.
Polarized light interacts with matter in the direction of
the electric vector. This is the polarization direction. Using this
property it is possible to use polarized light to probe different
materials and identify them by how they interact with light.
The speed of light in a vacuum is a constant at about 2.99
x 10(8) m/s. When light travels in different materials such as air, water,
minerals or oil, it does not travel at this speed. It travels slower. This
slowing is a function of both the material through which the light is
traveling and the wavelength or frequency of the light. In general, the
more dense the material, the slower the light travels. Also, generally,
the higher the frequency, the slower the light will travel. The ratio of
the speed of light in a vacuum to that in a material is called the index
of refraction (n). It is usually measured at 589 nm (the sodium D line).
If white light (light containing all the visible wavelengths) travels
through a material, rays of longer wavelengths will travel faster than
those of shorter wavelengths, this separation is called dispersion.
Dispersion is used as an identifier of materials as described in Section
4.6.
4.2. Material Properties
Materials are either amorphous or crystalline. The
difference between these two descriptions depends on the positions of the
atoms in them. The atoms in amorphous materials are randomly arranged with
no long range order. An example of an amorphous material is glass. The
atoms in crystalline materials, on the other hand, are in regular arrays
and have long range order. Most of the atoms can be found in highly
predictable locations. Examples of crystalline material are salt, gold,
and the asbestos minerals.
It is beyond the scope of this method to describe the
different types of crystalline materials that can be found, or the full
description of the classes into which they can fall. However, some general
crystallography is provided below to give a foundation to the procedures
described.
With the exception of anthophyllite, all the asbestos
minerals belong to the monoclinic crystal type. The unit cell is the basic
repeating unit of the crystal and for monoclinic crystals can be described
as having three unequal sides, two 90 deg. angles and one angle not equal
to 90 deg.. The orthorhombic group, of which anthophyllite is a member has
three unequal sides and three 90 deg. angles. The unequal sides are a
consequence of the complexity of fitting the different atoms into the unit
cell. Although the atoms are in a regular array, that array is not
symmetrical in all directions. There is long range order in the three
major directions of the crystal. However, the order is different in each
of the three directions. This has the effect that the index of refraction
is different in each of the three directions. Using polarized light, we
can investigate the index of refraction in each of the directions and
identify the mineral or material under investigation. The indices alpha,
beta, and gamma are used to identify the lowest, middle, and highest index
of refraction respectively. The x direction, associated with alpha is
called the fast axis. Conversely, the z direction is associated with gamma
and is the slow direction. Crocidolite has alpha along the fiber length
making it "length-fast". The remainder of the asbestos minerals have the
gamma axis along the fiber length. They are called "length-slow". This
orientation to fiber length is used to aid in the identification of
asbestos.
4.3. Polarized Light Technique
Polarized light microscopy as described in this section
uses the phase-polar microscope described in Section 3.2. A phase contrast
microscope is fitted with two polarizing elements, one below and one above
the sample. The polarizers have their polarization directions at right
angles to each other. Depending on the tests performed, there may be a
compensator between these two polarizing elements. Light emerging from a
polarizing element has its electric vector pointing in the polarization
direction of the element. The light will not be subsequently transmitted
through a second element set at a right angle to the first element. Unless
the light is altered as it passes from one element to the other, there is
no transmission of light.
4.4. Angle of Extinction
Crystals which have different crystal regularity in two or
three main directions are said to be anisotropic. They have a different
index of refraction in each of the main directions. When such a crystal is
inserted between the crossed polars, the field of view is no longer dark
but shows the crystal in color. The color depends on the properties of the
crystal. The light acts as if it travels through the crystal along the
optical axes. If a crystal optical axis were lined up along one of the
polarizing directions (either the polarizer or the analyzer) the light
would appear to travel only in that direction, and it would blink out or
go dark. The difference in degrees between the fiber direction and the
angle at which it blinks out is called the angle of extinction. When this
angle can be measured, it is useful in identifying the mineral. The
procedure for measuring the angle of extinction is to first identify the
polarization direction in the microscope. A commercial alignment slide can
be used to establish the polarization directions or use anthophyllite or
another suitable mineral. This mineral has a zero degree angle of
extinction and will go dark to extinction as it aligns with the
polarization directions. When a fiber of anthophyllite has gone to
extinction, align the eyepiece reticle or graticule with the fiber so that
there is a visual cue as to the direction of polarization in the field of
view. Tape or otherwise secure the eyepiece in this position so it will
not shift.
After the polarization direction has been identified in
the field of view, move the particle of interest to the center of the
field of view and align it with the polarization direction. For fibers,
align the fiber along this direction. Note the angular reading of the
rotating stage. Looking at the particle, rotate the stage until the fiber
goes dark or "blinks out". Again note the reading of the stage. The
difference in the first reading and the second is an angle of
extinction.
The angle measured may vary as the orientation of the
fiber changes about its long axis. Tables of mineralogical data usually
report the maximum angle of extinction. Asbestos forming minerals, when
they exhibit an angle of extinction, usually do show an angle of
extinction close to the reported maximum, or as appropriate depending on
the substitution chemistry.
4.5. Crossed Polars with Compensator
When the optical axes of a crystal are not lined up along
one of the polarizing directions (either the polarizer or the analyzer)
part of the light travels along one axis and part travels along the other
visible axis. This is characteristic of birefringent materials.
The color depends on the difference of the two visible
indices of refraction and the thickness of the crystal. The maximum
difference available is the difference between the alpha and the gamma
axes. This maximum difference is usually tabulated as the birefringence of
the crystal.
For this test, align the fiber at 45 deg. to the
polarization directions in order to maximize the contribution to each of
the optical axes. The colors seen are called retardation colors. They
arise from the recombination of light which has traveled through the two
separate directions of the crystal. One of the rays is retarded behind the
other since the light in that direction travels slower. On recombination,
some of the colors which make up white light are enhanced by constructive
interference and some are suppressed by destructive interference. The
result is a color dependent on the difference between the indices and the
thickness of the crystal. The proper colors, thicknesses, and retardations
are shown on a Michel-Levy chart. The three items, retardation, thickness
and birefringence are related by the following relationship: R = t(n(gamma) -- n(alpha))
R = retardation, t = crystal thickness in um, and
n(alpha, gamma) = indices of refraction.
Examination of the equation for asbestos minerals reveals
that the visible colors for almost all common asbestos minerals and fiber
sizes are shades of gray and black. The eye is relatively poor at
discriminating different shades of gray. It is very good at discriminating
different colors. In order to compensate for the low retardation, a
compensator is added to the light train between the polarization elements.
The compensator used for this test is a gypsum plate of known thickness
and birefringence. Such a compensator when oriented at 45 deg. to the
polarizer direction, provides a retardation of 530 nm of the 530 nm
wavelength color. This enhances the red color and gives the background a
characteristic red to red-magenta color. If this "full-wave" compensator
is in place when the asbestos preparation is inserted into the light
train, the colors seen on the fibers are quite different. Gypsum, like
asbestos has a fast axis and a slow axis. When a fiber is aligned with its
fast axis in the same direction as the fast axis of the gypsum plate, the
ray vibrating in the slow direction is retarded by both the asbestos and
the gypsum. This results in a higher retardation than would be present for
either of the two minerals. The color seen is a second order blue. When
the fiber is rotated 90 deg. using the rotating stage, the slow direction
of the fiber is now aligned with the fast direction of the gypsum and the
fast direction of the fiber is aligned with the slow direction of the
gypsum. Thus, one ray vibrates faster in the fast direction of the gypsum,
and slower in the slow direction of the fiber; the other ray will vibrate
slower in the slow direction of the gypsum and faster in the fast
direction of the fiber. In this case, the effect is subtractive and the
color seen is a first order yellow. As long as the fiber thickness does
not add appreciably to the color, the same basic colors will be seen for
all asbestos types except crocidolite. In crocidolite the colors will be
weaker, may be in the opposite directions, and will be altered by the blue
absorption color natural to crocidolite. Hundreds of other materials will
give the same colors as asbestos, and therefore, this test is not
definitive for asbestos. The test is useful in discriminating against
fiberglass or other amorphous fibers such as some synthetic fibers.
Certain synthetic fibers will show retardation colors different than
asbestos; however, there are some forms of polyethylene and aramid which
will show morphology and retardation colors similar to asbestos minerals.
This test must be supplemented with a positive identification test when
birefringent fibers are present which can not be excluded by morphology.
This test is relatively ineffective for use on fibers less than 1 um in
diameter. For positive co
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