Difference between revisions of "Template:Team:Groningen/CONTENT/EXPERIMENTS/PCR ferritin construct (fr1)"
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|title=00:00, 31 Augustus 2015 - 00:00, 31 Augustus 2015 | |title=00:00, 31 Augustus 2015 - 00:00, 31 Augustus 2015 | ||
|executor=Harm Ruesink | |executor=Harm Ruesink | ||
| − | |content=<div class="text">Ferritin was ordered with sequence with prefix and suffix primers from IDT. PCR was performed ( | + | |content=<div class="text">Ferritin was ordered with sequence with prefix and suffix primers from IDT. PCR was performed (Figure 1) using NEB Q5 High-Fidelity 2X Master Mix with the prefix and suffix primers.</div> |
<div class="object data" id="tbl1"> | <div class="object data" id="tbl1"> | ||
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<div class="caption">PCR components.</div> | <div class="caption">PCR components.</div> | ||
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<div class="text">The following thermocycle was used for the PCR.</div> | <div class="text">The following thermocycle was used for the PCR.</div> | ||
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<div class="caption">PCR Thermocycle.</div> | <div class="caption">PCR Thermocycle.</div> | ||
| + | </div> | ||
<div class="text">The PCR prduct was loaded on a 1% agarose gel with DNA stain G (1:50000) and run for 1 hour on 100 V.</div> | <div class="text">The PCR prduct was loaded on a 1% agarose gel with DNA stain G (1:50000) and run for 1 hour on 100 V.</div> | ||
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| − | <div class="text"> | + | <div class="text">A band of approximately 1600 bp was visible on the gel. This corresponds to the size of ferritin.</div> |
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Latest revision as of 21:40, 21 November 2015
00:00, 31 Augustus 2015 - 00:00, 31 Augustus 2015
Ferritin was ordered with sequence with prefix and suffix primers from IDT. PCR was performed (Figure 1) using NEB Q5 High-Fidelity 2X Master Mix with the prefix and suffix primers.
Primer
Sequence
prefix
CAGGCAGTTGAATTCGCGGCCGCTTCTAGA
suffix
CTTGAGCTCCTGCAGCGGCCGCTACTAGTA
Primers for ferritin PCR.
The following PCR mix was prepared.
Compound
Amount
Q5 polymerase
9 µL
Template DNA (Ferritin IDT)
1 µL
Each primer
0.3 µL
\( \mathrm{H_2O}\)
9 µL
PCR components.
The following thermocycle was used for the PCR.
#
Step
Temperature
Time
1
Initial denaturation
98 °C
5:00
2
Denaturation
98 °C
0:30
3
Annealing
60 °C
0:30
4
Extension
72 °C
1:30
5
Go back to step 2 (30x)
6
Final extension
72 °C
10:00
PCR Thermocycle.
The PCR prduct was loaded on a 1% agarose gel with DNA stain G (1:50000) and run for 1 hour on 100 V.
Sample:
1 µL DNA (ferritin).
1 µL 6x buffer.
4 µL \( \mathrm{H_2O}\).
Ladder:
2 µL Thermo Scientific GeneRuler 1kb DNA ladder, ready to use.
A band of approximately 1600 bp was visible on the gel. This corresponds to the size of ferritin.