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**ajthomas** · 10-22-2013, 03:32 AM

No, you don't want to do paired-end sequencing for this. If I understand right, you will be amplifying these genes and then sequencing the amplicons, right? If so, just use the Lib-A adapters, rather than Lib-L, and you will get sequences from both ends. You won't sequence any individual bead from both ends, as you would with Illumina sequencing, but you will sequence some molecules from one end and others from the other end. After sequencing you will assemble the forward and reverse reads into full length sequences.

**chwang** · 10-22-2013, 08:22 AM

Hi. Thanks for the response. Could you explain how it would be possible to determine which forward and reverse sequences to stitch together? ...How to determine that both ends were sequence from the same DNA molecule? Because is I'm using the functional gene primers onto an environmental sample, not bacterial isolates.

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