Bio-Rad Model 785 Vacuum Blotter User Manual

5.2 Southern Hybridization Troubleshooting

The performance of the vacuum transfer will reflect in Southern hybridization

results. The table below summarizes the problems, the probable causes, and the
solutions. The term “signal” refers to the band on the Southern hybridization
autoradiograph. Refer to the Zeta-Probe

®

GT manual also for specific troubleshooting.

Solutions/

Condition

Probable Causes

Preventions

1. No signal/

• Insufficient DNA loaded.

• Load between 5-10 µg

weak signal.

of DNA.

• Poor or no DNA trans-

• Stain gel after it is trans-

ferred.

ferred. Have positive
control lane. Both pre-
cautions are for checking
if DNA has transferred.

•

32

P-labeled probe is

• Make sure probe concen-

faulty.

trations and specific
activity is correct.

• Prolonged vacuum

• Vacuum transfer no longer

transfer.

than 90 minutes.

• Nylon membrane was

• Bake membrane in 80

not baked.

degree oven for 30
minutes.

2. Partial signal.

• Porous membrane is

• Use new porous gel

clotted.with agarose

support or clean the

or salt at signal.

clotted spot.

3. High background.

• Uncleaned probe.

• Remove all radio-isotopic

nucleotides in labeling
reaction. Can use Bio-Rad
P-30 desalting column.

• Dirty nylon membrane.

• Soak nylon membrane

in 2x SSC for 5 minutes
before air drying.

• Hybridization conditions. • For Zeta-Probe membrane

use hybridization buffer
with 7% SDS + 0.5 M
NaH

2

PO

4

pH 7.2 + 1 mM

EDTA.

• Check hybridization

temperature.

10