Slide-A-Lyzer
2015-01-13azim58 - Slide-A-Lyzer
Slide-A-Lyzer
Slidalyzer or slide a lyzer
used for dialysis, sold from thermo scientific
http://www.piercenet.com/browse.cfm?fldID=E1D032C4-B084-2D48-7ECC-27D9E94B4
1F4
Instructions
http://www.piercenet.com/instructions/2162132.pdf
Typical dialysis buffer: PBS or TBS
Large flask
- large flask not contaminated with soap for use with dialysis last
A. Hydrate Membrane
- Remove the cassette from its protective pouch. To prevent membrane
touch the membrane with ungloved hands. The cassette may be placed
upright on the bottom end on a flat surface.
- Immerse cassette in dialysis buffer for 2 minutes to hydrate membrane
be necessary to hold the cassette under the surface for the hydration
step as the air inside the cassette may cause it to float sideways.
Note: Hydration increases membrane flexibility and allows it to adjust
more readily to the sample loading and removal of excess air.
- Remove cassette from buffer. To remove excess buffer, gently tap the
Do not blot the membrane.
B. Add Sample
Note: The minimum sample volume for the 3, 15, 30 and 70mL cassette is
approximately > ⅓ of the cassette’s maximum volume or leakage can
occur. For the 0.5mL cassette, the minimum sample volume is ≥ 250μL.
Caution: To avoid injury from the needle, do not remove the needle’s
plastic sheath until ready to use. The cassette is designed for 18 gauge,
1-inch beveled needles (21-gauge, 1-inch beveled needles also may be
used).
- Fill the syringe with the sample, leaving a small amount of air in the
- Penetrate the gasket through a syringe port at the cassette’s
the middle rather than the sides to avoid tearing the membrane.
Overextending the needle into the sample chamber may puncture the
membrane (Figure 2). Slowly extend the needle minimally into the cavity
so that the open end of the needle is barely visible (Figure 3).
- Inject approximately half of the sample. For samples with high protein
slowly.
- Withdraw some air from the cassette by pulling back on the syringe
- With the needle inserted into the cassette cavity, withdraw remaining
possible membrane surface area. Use caution to prevent the needle from
contacting the membrane. A small amount of air left inside the cassette
will not significantly affect dialysis efficiency.
- Remove needle from the cassette while retaining air in the syringe.
air. Place a mark on the cassette corner with a permanent marker to note
which needle port was used.
C. Dialyze Sample
- Float cassette vertically in the dialysis buffer and stir gently to
the stir bar.
- Dialyze for an amount of time sufficient to remove low molecular
dialysis procedure is as follows: dialyze for 2 hours at room temperature
or 4ºC; change the dialysis buffer and dialyze for another 2 hours;
change the dialysis buffer and dialyze overnight. Use the dialysis buffer
at a total of at least 300 times the sample volume throughout the course
of the dialysis procedure.
- May want to concentrate sample by adding BSA to surface of membrane. May
be repeated (possibly with fresh BSA as well) until you have the volume
desired).
D. Recover Sample
Note: Avoid penetrating guide ports more than once to prevent gasket
coring and subsequent sample loss.
- Penetrate gasket with the needle through an unused syringe guide port
volume to separate membranes, which prevents membrane needle puncture.
(Figure 4).
- With the needle in place, turn the unit so that needle is at the
collect near the port and withdraw sample into the syringe (Figure 5).