Primer design: Difference between revisions
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Primers are [[Watson-Crick base pairing|Watson-Crick]] complimentary short [[Nucleotide|nucleotide]] sequences used to initiate [[DNA|DNA]] replication and amplification through [[PCR|PCR]] or to identify target sequences within DNA: | Primers are [[Watson-Crick base pairing|Watson-Crick]] complimentary short [[Nucleotide|nucleotide]] sequences used to initiate [[DNA|DNA]] replication and amplification through [[PCR|PCR]] or to identify target sequences within DNA: | ||
*Ideally primers should be 18-20 base pairs in length, this is so that they are unique enough to anneal to the DNA at the flanking sequences of the | *Ideally primers should be 18-20 base pairs in length, this is so that they are unique enough to anneal to the DNA at the flanking sequences of the fragment/gene we wish to amplify or isolate and so that they anneal to the DNA after it has been melted before the rest of the strands re-anneal. they are also kept at this length to ensure that they do not "mis-prime" if 1 out of the 20 bases does not bind then polymerase will not be able to synthesize new DNA." | ||
*Primers also cannot be | *Primers also cannot be complementary to each other, if so these form "primer dimers". this is when they anneal and are amplified instead of the intended DNA sample. | ||
*Primers can also contain "dangling ends" these are restriction endonuclease sites at the outside edges of the primers that enable the DNA to be amplified to be inserted into a [[Plasmid|plasmid]] or [[Genome|genome]] cut by the same [[ | *Primers can also contain "dangling ends" these are restriction endonuclease sites at the outside edges of the primers that enable the DNA to be amplified to be inserted into a [[Plasmid|plasmid]] or [[Genome|genome]] cut by the same [[Restriction Endonuclease|restriction endonuclease]]. | ||
*[[ | *[[DNA bases|Bases]] [[Thymine|T]] and [[Adenine|A]] should be avoided at the 3' end of the primer (as this is where polymerase binds) as they are more likely to mispair. [[Guanine|G]] and [[Cytosine|C]] are much more stable. | ||
*Primers can be modified to contain | *Primers can be modified to contain fluorophores so that when they bind to target sequences of DNA we can visualize and isolate them etc. | ||
See also: | See also: | ||
[[PCR|PCR ]] | [[PCR|PCR ]] | ||
[[Recombinant DNA Technology|Recombinant DNA technology]] | |||
Latest revision as of 20:20, 4 December 2017
Primers are Watson-Crick complimentary short nucleotide sequences used to initiate DNA replication and amplification through PCR or to identify target sequences within DNA:
- Ideally primers should be 18-20 base pairs in length, this is so that they are unique enough to anneal to the DNA at the flanking sequences of the fragment/gene we wish to amplify or isolate and so that they anneal to the DNA after it has been melted before the rest of the strands re-anneal. they are also kept at this length to ensure that they do not "mis-prime" if 1 out of the 20 bases does not bind then polymerase will not be able to synthesize new DNA."
- Primers also cannot be complementary to each other, if so these form "primer dimers". this is when they anneal and are amplified instead of the intended DNA sample.
- Primers can also contain "dangling ends" these are restriction endonuclease sites at the outside edges of the primers that enable the DNA to be amplified to be inserted into a plasmid or genome cut by the same restriction endonuclease.
- Bases T and A should be avoided at the 3' end of the primer (as this is where polymerase binds) as they are more likely to mispair. G and C are much more stable.
- Primers can be modified to contain fluorophores so that when they bind to target sequences of DNA we can visualize and isolate them etc.
See also: