How
to prepare samples using freeze-substitution without an expensive
machine.
This method has been
used successfully in our laboratory since 1994. The protocol
assumes all users will be familiar with routine TEM preparation
methods. An important application of this method was made by
Dr. A. Whitney who
used it to examine MDCK cells grown on filters.
- Aldehyde Fixation
- Fix cells or tissues
in buffered aldehyde solution. We use either 4% formaldehyde
(made up from paraformaldehyde) or a mixture of 4% formaldehyde
and 0.2% gluteraldeyhde, buffered in 100mM phosphate buffer.
Fixation times vary but routinely we use 1 hr. Whole organs
are best fixed by perfusiing the with fixative.
- Cryoprotection
- Incubate fixed
material in 2.3M sucrose. This cryoprotection method is also
used for material that is to be frozen for cryosectioning.
Small pieces of the material are left for 1 hour to infiltrate.
- Freezing
- Mount the small,
cryoprotected sample pieces onto metal pins and immerse in
liquid nitrogen. The pins are useful for manipulating the
frozen samples during the early stages of the protocol and
ensure the sample is submerged during freezing.
- Substitution
- Quickly transfer
the samples into glass vials of methanol on a bed of dry ice
in a styrofoam box. Alternatively, the vials can be left in
a REVCO freezer. Seal vials well and leave for 8 - 48 hours.
Smaller samples will substitute faster than larger samples.
Increased contrast can be achieved if 1% uranyl acetate or
osmium tetroxide is added to the substitution mix. These heavy
metals do not interfere with resin polymerization. Dry acetone
can be used as a substitution medium instead of methanol.
However, it is important for the acetone to be dry.
- Washing
- Wash in fresh
changes of substitution medium prior to embedding in resin.
Usually 2 - 3 changes over a few hours is sufficient.
- Embedding in resin
(using Lowicryl HM20)
|
Time |
MeOH:resin |
|
1 hr. |
1:1 |
|
1 hr. |
1:2 |
|
1 hr. |
pure resin |
|
overnight. |
pure resin |
- Resin polymerization
- Remove sample
pieces from the glass vials and place in precooled BEEM capsules
or small Eppendorf tubes containing fresh HM20 Lowicryl resin.
Keep the tubes on dry ice and seal them as soon as the sample
pieces have been added. Place only one sample per tube. Arrange
the tubes on a rack in a styrofoam box, covered on the inside
with aluminum foil, and pack with dry ice. Cover the tubes
with a triangular shaped cardboard box that has been covered
with aluminum foil. Place a UV light above the box and leave
for up to 3 days to polymerize. The resin polymerizes in indirect
360 nm UV light. Too rapid polymerization will result in shrinkage
of the block and uneven polymerization. Once the blocks have
hardened, polymerization can continue at room teperatures
using direct sunlight or the UV light used to sterilize cell
culture hoods
- Sectioning
- Lowicryl resins
do not crosslink well at tissue-resin borders. It is important,
when trimming the block, to make sure the sample is not dislodged.
The best way to trim the block is by using either a glass
knife or one of the trimming devices currently available (supplied
by Diatome US or Harris Diamond Co.). Once the block is trimmed,
it is fairly easy to section using routine sectioning methods.
Diamond knives are recommended. The HM20 resin will not change
shape if water is splashed onto the block. Sections can be
picked up from the water surface with metal specimen grids.
The sections are now ready to be labeled with affinity
markers.
|
