Difference between revisions of "Template:Team:Groningen/CONTENT/PROTOCOLS/PCR"
Line 61: | Line 61: | ||
<div class="record"> | <div class="record"> | ||
<div class="field fw3">Initial denaturation</div> | <div class="field fw3">Initial denaturation</div> | ||
− | <div class="field fw3"> | + | <div class="field fw3">98 °C</div> |
<div class="field fw7">30 s</div> | <div class="field fw7">30 s</div> | ||
<div class="field fw7">1</div> | <div class="field fw7">1</div> | ||
Line 67: | Line 67: | ||
<div class="record"> | <div class="record"> | ||
<div class="field fw3">Denaturation</div> | <div class="field fw3">Denaturation</div> | ||
− | <div class="field fw3"> | + | <div class="field fw3">98 °C</div> |
<div class="field fw7">5-10 s</div> | <div class="field fw7">5-10 s</div> | ||
<div class="field fw7">25-35</div> | <div class="field fw7">25-35</div> | ||
Line 80: | Line 80: | ||
<div class="record"> | <div class="record"> | ||
<div class="field fw3">Extension</div> | <div class="field fw3">Extension</div> | ||
− | <div class="field fw3"> | + | <div class="field fw3">72 °C</div> |
<div class="field fw7">15-30 s/kb</div> | <div class="field fw7">15-30 s/kb</div> | ||
<div class="field fw7">25-35</div> | <div class="field fw7">25-35</div> | ||
Line 94: | Line 94: | ||
<div class="record"> | <div class="record"> | ||
<div class="field fw3">Hold</div> | <div class="field fw3">Hold</div> | ||
− | <div class="field fw3"> | + | <div class="field fw3">4 °C</div> |
<div class="field fw7">Hold</div> | <div class="field fw7">Hold</div> | ||
<div class="field fw7">1</div> | <div class="field fw7">1</div> |
Revision as of 21:26, 21 August 2015
PCR mix
1. Create the following mix.
Ingredient
20 μl reaction
Final Concentration
\( \mathrm{H_2O}\)
Add to 20 μl
5x Phusion HF buffer*
4 μl
1x
10 mM dNTPs
0.4 μl
200 μM each
Forward primer**
X μl
0.5 μM
Template DNA
X μl
(DMSO***, optional)
(0.6 μl)
(3%)
Phusion DNA polymerase
0.2 μl
0.02 U/ μL
2. Gently vortex the samples and spin down.
3. Place the reactions in a thermal cycler. Perform PCR using recommended thermal cycling conditions.
Cycle Step
Temperature
Time
Cycle
Initial denaturation
98 °C
30 s
1
Denaturation
98 °C
5-10 s
25-35
Annealing
T m - 5°C
10-30 s
25-35
Extension
72 °C
15-30 s/kb
25-35
Final extension
72°C
5-10 min
1
Hold
4 °C
Hold
1