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Hi All,
I have heard that sanger/dye termination sequencing is more accurate than illumina/solexa DNA cluster-based sequencing. I have been reading about both methods and am trying to identify the key point(s) in the illumina/solexa process in which additional error is introduced and accuracy diverges from the sanger method. I read that it is because illumina/solexa sequencing ‘requires PCR amplification’ of DNA clusters.
Is cluster amplification the main error-introducing step?
Why is this step necessary for the process to work, i.e. why can’t the incorporated nucleotide signal be captured while only a single molecule is being synthesized?
Thank you!
kateveronica
I have heard that sanger/dye termination sequencing is more accurate than illumina/solexa DNA cluster-based sequencing. I have been reading about both methods and am trying to identify the key point(s) in the illumina/solexa process in which additional error is introduced and accuracy diverges from the sanger method. I read that it is because illumina/solexa sequencing ‘requires PCR amplification’ of DNA clusters.
Is cluster amplification the main error-introducing step?
Why is this step necessary for the process to work, i.e. why can’t the incorporated nucleotide signal be captured while only a single molecule is being synthesized?
Thank you!
kateveronica
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