Bio-Rad Model 785 Vacuum Blotter User Manual

2. There are three transfer procedures listed: the Standard Transfer Procedure, the

Rapid Transfer Procedure, and the RNA Transfer Procedure. The Standard Transfer
Procedure is for detection of single copy gene in genomic DNA. The Rapid Transfer
Procedure is for fast identification of DNA inserts from various cloned vectors.

Standard Procedure:

1. Depurinate the gel in 0.25 N HCl for 15 minutes in a tray. Cover the gel with 0.25 N

HCl and shake gently.

2. Remove the 0.25 N HCl solution. Rinse the gel twice with deionized distilled water.

3. Denature the gel in 0.5 N NaOH for 30 minutes. Cover the gel with 0.5 N NaOH and

shake gently.

4. Transfer the gel in 10x SSC for 90 minutes at 5 inches Hg. Follow the instructions in

Section 3.4 for the transfer procedures.

Rapid Transfer Procedure:

1. Depurinate the gel in 0.25 N HCl for 15 minutes in a tray. Cover the gel with 0.25 N

HCl and shake gently.

2. Remove the 0.25 N HCl solution. Rinse the gel twice with deionized distilled water.

3. Immediately, transfer in 0.5 N NaOH, 0.6 N NaCl for 90 minutes at 5 inches Hg.

Follow the instructions in Section 3.4 for the transfer procedures.

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Fig. 3.2. Exploded view of vacuum transfer set-up.

Sealing frame

Agarose gel

Window gasket

Nylon membrane

Filter paper

Porous vacuum plate