Bio-Rad Rotofor® and Mini Rotofor Cells User Manual

Refractionation

Rotofor fractions 4,5 and 6 were collected, pooled, and refractionated in the

Rotofor cell without additional ampholytes. The total protein load was 50 mil-
ligrams. Upon refractionation, an overall 1000-fold purification of Apo J and the
unknown protein was obtained in Rotofor fraction 11. See Figure 2b.

Fig. 2. Analysis of Rotofor fractions by 2-D gel electrophoresis. 2a) Initial Rotofor fractionation
provided enrichment for the proteins of interest in Rotofor fraction 5, shown here. 2b) Refractionation of
Rotofor fraction 5 shown here resulted in 1000-fold purification of Apo J and the unknown 49 kd protein
by comparison to the starting sample in Figure 1. Analytical 2-D gels were silver stained.

Preparative SDS-PAGE

For preparative gel electrophoresis, the discontinuous buffer system of

Laemmli was used

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. The total acrylamide concentration (%T) of the separating gel

was optimized at 12%.

The sample (Rotofor fraction 11) contained approximately 2.5 mg of total protein
dissolved in 2.0 ml of sample buffer (see Table 1). After a 5 minute incubation at
95°C, the sample was loaded onto the Prep cell and the gel run for 16 hours.
Running buffer was pumped through the elution chamber at a rate of 0.5 ml per
minute.

Table 1. Model 491 Prep cell running conditions

Resolving gel:

12% acrylamide/ 2.6% C (PDA crosslinker)

Resolving gel length: 8 cm in 37 mm gel tube

Resolving gel buffer: Tris-HCl (0.375 M) pH 8.8

Stacking gel:

4% T/2.6% C (PDA crosslinker)

Stacking gel buffer:

Tris-HCl (125 mM) pH 6.5

Running buffer:

Tris-Glycine-SDS (25 mM-192mM-0.1%)

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