PCR primers
While there are a number of ways to obtain
a set of PCR primers to amplify your GOI, sometimes, you might just need to
customize your own to zero in on a particular region to specifically amplify a
transcript variant. The following method is a timeless protocol for those who
like to design their own primers.
Preparation
First, you will need the cDNA sequence of
your GOI. The sequence should ideally have the intron-exon boundaries clearly
marked. For this I recommend getting the cDNA sequence from Ensembl as they have
an option that allows users to mark the exons using an alternating color
scheme (see below).
 |
| Screen capture of the exon sequences from the ABCA1 transcript variant 1 from Ensembl |
Alternatively, you could just get the cDNA
sequence and mark out the intron-exon boundaries yourself.
Ideally, you will want your primers to
cover an intron-exon boundary. Crossing an intron-exon boundary will ensure
that your primers are annealing to and only amplifying from your cDNA template
rather than gDNA contamination. If your primers can anneal to both cDNA and gDNA,
on an agarose gel, the gDNA will either give you a higher MW band, become a
smear, or be the exact same size as your cDNA PCR product. Either way, gDNA
contamination will affect quantification and subsequent analyses.
Primer
design:
* You will want your primers to
be ~20 nucleotides long and to have ~50% GC.
* Do not have strings of >3
nucleotides of any kind (e.g. AAAAA or GGG or TTTT or CCCCC).
* At the 5’ end, start with A or
T nucleotides; at the 3’ end, have G or C nucleotides as the last 3 nucleotides.
This will give a stronger bond to the 3’ end; you do not want the 5’ end to
have too tight a bond.
* Aim for a product size of
~200bp.
* When ordering, standard desalt
purification is fine for PCR and cloning.
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