Nucleic acids (continued) – Bio-Rad Zeta-Probe Membranes User Manual

Problem

7. No autoradiograph signal

Solution

1. After transfer, stain the gel to check that

transfer was complete. If not, increase
transfer time and/or voltage of transfer,
or see solution to problem #1 above.

2. Be sure probe is denatured by boiling or

heating to 65°C for 5 min in 50%
formamide prior to hybridization.

25

Problem

4. Localized

high

background

observed on autoradiograph

5. Lane background or extra bands

6. Low autoradiograph signal

Solution

1. Make sure the membrane is free-floating

within the plastic bag during hybridiza-
tion. Membrane/bag contact during
hybridization can cause background.
Add more hybridization solution.

2. Make sure not to pinch the membrane

when sealing the plastic bag prior to
hybridization.

3. Be sure no bubbles exist in the

hybridization bag.

1. Indicates contaminated template. Make

sure the probe is synthesized with the
pure template of choice.

This problem may occur when total genomic
DNA is probed for single-copy or low copy
number genes.

1. Incorporate 10% dextran sulfate in the

hybridization mixture. This polymer effec-
tively reduces the solvent volume, there-
by increasing the concentration of the
solutes and enhancing hybridization.
Refer to Section 4.3.

2. Increase exposure time to increase sig-

nal-to-noise ratio.

3. Increase sample load on the gel.

4. If low signal is accompanied by low

background, probe concentration can
be increased 2- to 4-fold.

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Nucleic Acids (Continued)

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