GE RPN1607 Label Maker User Manual


 
12
Protocol
2. Place the required tubes from
the Megaprime system, with
the exception of the enzyme,
at room temperature to
thaw. Leave the enzyme at
-15°C to -30°C until required,
and return immediately after
use.
3. Place 25 ng of template DNA
into a microcentrifuge tube
and to it add 5 µl of primers
and the appropriate volume
of water to give a total
volume of 50 µl in the final
Megaprime reaction.
Denature by heating to
95–100°C for 5 minutes
in a boiling water bath.
4. Spin briefly in a microcentrifuge
to bring the contents to the
bottom of the tube.
5. Keeping the tube at room
temperature, add the
nucleotides and reaction
buffer (RPN 1604/5) or the
labelling buffer (RPN 1606/7)
followed by the radiolabelled
dNTP(s) and enzyme as
follows:
Notes
3. When labelling DNA in low
melting point agarose, first
place the tube containing the
stock DNA in a boiling water
bath for 30 seconds to melt
the agarose before removing
the required volume. The
volume of low melting point
agarose DNA should not
exceed 25 µl in a 50 µl reaction.
5. The reaction volume may be
scaled up or down if more or
less than 25 ng of DNA is to
be labelled.