1 general troubleshooting – Bio-Rad Model 111 Mini IEF Cell User Manual

Section 7
Troubleshooting

7.1 General Troubleshooting

Problem

Cause

Solution

19

1. Excessive pooling

of water at the
cathode(-)
Agarose only.

2. Distortion in

gradient where
sample is applied.

3. Sample streaking.

4. pH gradient does

not cover
expected range.

a. Poor quality agarose.

b. Gel has not been sufficiently

blotted dry sufficiently
blotted dry prior to run.

a. Too much salt in sample.

b. Sample is applied too

near the anode.

c. Sample load excessive.

d. Sample precipitation.

a. Particles in sample.

b. Sample absorbed onto

applicator.

c. Precipitation at point of

application.

a. Focused too long or use of

excessive voltage.

b. Basic gels stored too

long.

c. Poor quality acrylamide

and Bis.

d. Old acrylamide and

Bis stock solutions.

a. Use Bio-Rad’s Zero - Mr Agrose

only

b. Blot all excess liquid from gel prior

to run.

a. Dialyze against ampholyte1%

glycine or water, or desalt with
Bio-Gel P-2 or P-6DG gel.

b. Apply elsewhere on plate,

minimum of 1 cm from anode.

c. Dilute sample.

d. Spin to remove insolubles or use

detergents.

a. Centrifuge sample before

application.

b. Change application method.

c. Try a different position.Use

additives (1% glycine,urea, non-
ionic detergents,amphoteric
detergents).

a. At recommended constant voltage,

proteins should be focused within
1.5 hours.

b. Use basic gels (pH>7)

immediately to prevent hydrolysis
of acrylamide to acrylic acid,
which causes
electroendosmosis.

c. Use highest quality acrylamide

and Bis to avoid polymerizing
acrylic acid into into the gel.

d. Prolonged storage of acrylamide

and Bis leads to acrylic acid
formation.