PCR protocol

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2019.7.25

PCR reaction
Protocol for 50µl reaction - adjust amounts if necessary, for a 20µl reaction use the same volumes of primer and dNTP-mix, but adjust the volume of water and 10x buffer, for a 100µl reaction use twice the volume of everything. This protocol is for with 10x buffer with added MgCl2, if this is not included add it to a concentration of 1.5 mM or other concentration found to be optimal.

In a 200µl PCR tube take 5µl 10X PCR buffer (from enzyme kit).
Add 1µl dNTP-mix.
Add 1µl of 10 pmoles/µl solution of Forward primer.
Add 1µl of 10 pmoles/µl solution of Reverse primer.
Add 1µl template DNA, or a tiny bit of colony on agar-plate picked with a tooth-pick.
Add 40.5µl (or 41.5µl if using a colony pick) dH2O.
Add 0.5µl Taq DNA polymerase (5U/µl).
Mix gently by pipetting.
Place in PCR machine, and close hot-lid (if the machine does not have a hot-lid add a couple of drops of mineral oil on top of reaction to prevent evaporation.
Perform PCR with a suitable program for the template, primers, and thermal cycler:

Agarose gel for analysis of PCR products
Protocol for 60 ml gel - adjust amounts if necessary.

5 minutes at 95°C (especially important if using colony pick or unopened cells af any form)
30 times:
30 seconds at 95°C (depending on PCR machine)
30 seconds at 50°C (adjust according to annealing temperatures of primers)
30 seconds at 72°C (long PCR products (>1kb) require longer)
6 minutes at 72°C

Solutions

dNTP-mix for PCR
10µl 100mM dATP, 10µl 100mM dCTP, 10µl 100mM dGTP, 10µl 100mM dTTP, 60µl DEPC-treated dH2O
6X loading buffer for agarose gel
25µl 1% (w/v) bromo-phenol blue, 25µl 1% (w/v) xylene-cyanol FF, 30µl 100% glycerol, 20µl dH2O

protocol

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