I. Via random hexamers

1. Solutions:

10X hexa nt mix*:
500 mM Tris-Cl pH 7.2
100 mM MgCl₂
1 mM dithioerythritol (DTE)
2 mg/ml BSA
62.5 A260 units/ml (1.56 mg/ml) random hexanucleotides

10x dig/dNTP mix*:
1 mM dATP
1 mM dCTP
1 mM dGTP
0.65 mM dTTP
0.35 mM alkali-labile digoxigenin (dig)-UTP (B-Mann cat# 1573152 or 1573179)

*supplied in the dig DNA labelling kit; also can order all tubes separately, i.e. without enzyme.

2. Reaction:

a. Heat at 100 deg C for 10' to denature: 15 µl (50-250ng) DNA (in TE or ddH₂O)

b. Cool quickly on ice (1-2')

c. Add:
2 µl 10X hexa nt mix
2 µl 10X dig/dNTP mix
1 µl Klenow* (5u/µl)

d. Incubate at 37 deg C >1 hr. (up to 20 hr)
e. Increase volume to 50 µl then add 5 µl 0.4 M EDTA pH 8
f. Purify through a G-50 spin column.

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II. Via PCR

1. Solutions:

10X PCR buffer:
100 mM Tris-Cl, pH 8.3
500 mM KCl

10X dig mix:
2 mM dATP
2 mM dCTP
2 mM dGTP
1.3 mM dTTP
0.7 mM alkali-labile dig-11-dUTP (B-Mann cat# 1573152 or 1573179)

2. Reaction:

10X PCR buffer 5 µl
25 mM MgCl₂ 3 µl
10X dig mix 5 µl
20 pmol oligo 1
20 pmol oligo 2
Template
Taq 1 µl
Water up to 50 µl

3. PCR:

94 deg C - 5 min
Then 35 cycles of:
94 deg C - 30 sec
50 deg C - 1 min
70 deg C - 2 min

4. To purify, spin through a G-50 column or gel-isolate fragment (depending on the purity of the amplification).

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