We're just about to do some 454 sequencing and de novo assembly of bacterial genomes. We're considering using molecular markers to sequence multiple different genomes instead of the rubber gasket to divide the plate because using the gasket reduces the number of reads dramatically.
I understand that using the molecular markers may introduce bias in the sequencing but I don't fully understand this. What are the downsides of using a rubber gasket that we should be aware of?
I understand that using the molecular markers may introduce bias in the sequencing but I don't fully understand this. What are the downsides of using a rubber gasket that we should be aware of?
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