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Labeling oligonucleotides with 32P ATP

2024-10-09 DNA 加入收藏
Wear gloves throughout and work in radiation area. Monitor area before and after

Wear gloves throughout and work in radiation area. Monitor area before and after use.

Mix the following in an eppendorf tube:

1. 0.5 microgram oligonucleotide dissolved in H2O.

2. 3 microliters 10x kinase buffer.

3. 2 microliters 32 P ATP from ICN (>5000 ci/mmole).

4. H2O so that the final volume is 30 microliters.

Add 25 units T4 polynucleotide kinase and incubate 60 min at 37 ℃.

Purify labeled Oligonucleotide away from unincorporated ATP

Currently, we use mini Quick Spin Oligo Columns (#1 814 397) from Roche to purify the labeled oligonucleotide.

Prepare the column according to the manufactuer's instructions by centrifugation of the resuspended matrix for 1 min @ 1000 x g.

insert column into a new eppendorf tube and add oligo labeling reaction, adding slowly to center of column. Centrifuge 1000 x g for 4 min.

Recover purified labeled oligo. For most applications, add 70 microliters TE to the 30 microliters recovered for a total of 100 microliters.

Quantitate radioactive incorporation by counting 1 microliter of a 1/10 diluted sample. Expect between 20 -100 million cpm total.

10x Kinase Buffer

0.5 M Tris pH 7.6

0.1 M MgCl2

50 mM DTT


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