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Instructions for Sephadex Media
Sephadex is a beaded gel prepared by crosslinking dextran with epichlorohydrin. Its main application is group separations of low and high molecular weight molecules. Desalting is the most common use. Desalting with Sephadex is superior to dialysis because of the considerable time savings, the low dilution factor (which can be as low as 1.4:1), and the high activity recoveries even with very small amounts of sample. Sephadex G-25 is available prepacked in PD-10 columns, which are ideal for rapid, routine work.
Related applications include buffer exchange and the removal of small molecules during the preparation of large biomolecules, such as ampholytes, detergents, radioactive or fluorescent labels, and phenol (during DNA purification).
| Gel Type | Fractionation Range, Globular Proteins (D) | Fractionation Range, Dextrans (D) | Approx. Bed Volume (mL swelled per g dry) | Approx. Dry Bead Diameter (µm) | Approx. Maximum Operating Pressure (bar) |
| G-10 | ≤700 | ≤700 | 2–3 | 40–120 | * |
| G-15 | ≤1500 | ≤1500 | 2.5–3.5 | 40–120 | * |
| G-25 Superfine Fine Medium Coarse | 1000–5000 (all grades) | 100–5000 (all grades) | 4–6 (all grades) | 20–50 20–80 50–150 100–300 | * |
| G-50 Superfine Fine Medium Coarse | 1500–30000 (all grades) | 500–10000 (all grades) | 9–11 (all grades) | 20–50 20–80 50–150 100–300 | * |
| G-75 G-75 Superfine | 3000–80000 3000–70000 | 1000–50000 1000–50000 | 12–15 12–15 | 40–120 20–50 | 0.16 0.16 |
| G-100 G-100 Superfine | 4000–150000 4000–100000 | 1000–100000 1000–100000 | 15–20 15–20 | 40–120 20–50 | 0.096 0.096 |
| G-150 ** G-150 Superfine | 5000–300000 5000–150000 | 1000–150000 1000–150000 | 20–30 18–22 | 40–120 20–50 | 0.036 0.036 |
| G-200 ** G-200 Superfine | 5000–600000 5000–250000 | 1000–200000 1000–200000 | 30–40 20–25 | 40–120 20–50 | 0.016 0.016 |
* The beads behave as rigid spheres and therefore obey Darcy's Law: the flow rate is proportional to the pressure drop over the bed and inversely proportional to the bed height.
** Sephadex G150, G150SF, G200 & G200SF are discontinued products.
Swelling
Sephadex is supplied as a dry powder, and must be allowed to swell in excess buffer before use. Filter all buffers through a 0.22-µm filter to help prevent microbial growth.
1. Weigh out the appropriate amount of dry Sephadex for the required bed volume of your column (Table 1). If packing at the maximum pressure for the gel, choose the lowest bed volume factor (mL/g) for calculating the amount of dry Sephadex.
2. Add enough buffer to equal the total volume of the column plus 30%. Swelling times for the different types of Sephadex are given in Table 2. The process is accelerated by using a boiling water bath.
3. After swelling is complete, decant the supernatant.
4. Add buffer to make a 75% suspension.
5. Degas the suspension before packing.
1. Pour the entire slurry into the column in one portion, taking care not to trap air bubbles.
2. Start the gravity flow to initiate packing.
Good packing is essential to obtain good resolution. Ideally, the column should be packed at the highest pressure possible without deforming the beads.
For Sephadex G-10–G-50, the beads behave as rigid spheres. The pressure tolerance of the column is the limiting factor: pack at the maximum pressure specified for your column.
For the softer gels, Sephadex G-75–G-200, more care must be taken to avoid compressing the gel. Do not increase the pressure beyond the values given in Table 1.
With wider columns, slightly reduced maximum operating pressures must be used. Flow rate is inversely proportional to bed height: increasing the bed height will decrease the flow rate, but does not affect the maximum operating pressure.
1. Using a reservoir if necessary, pour the entire slurry into the column in one portion.
2. Start the pump to initiate packing.
3. Once all the gel has sedimented into the column, remove the reservoir.
4. Insert an adaptor and pack at the maximum operating pressure of the gel.
5. Once the gel is thoroughly packed into the column, adjust the flow adaptor to the surface of the gel bed.
6. Pass a further 2–3 column volumes of the buffer to be used in the separation. This stabilizes and equilibrates the bed.
7. Readjust the flow adaptor to the surface of the gel bed.
1. Wash with two column volumes of 0.2 M NaOH or a solution of a nonionic detergent. Washing the more porous Sephadex types (G-50–G-200) with NaOH should be done outside the column because the gel will swell.
2. Reequilibrate the gel with 2–3 column volumes of buffer before your next experiment. When necessary, the gel can be removed from the column and sterilized by autoclaving at 120 °C, pH 7.
Store unused gel dry at 2–8 °C.
Store used gel at 2–8 °C in 20% ethanol or in a solution of a microbial growth inhibitor such as 0.002% Hibitane/chlorhexidine or 0.02% sodium azide.
sephadex G-25凝膠過濾填料
sephadex G-25凝膠過濾填料
