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**kcchan** · 10-12-2014, 07:54 PM

You can do a primer rehyb on your flow cell and restart the run. Call Illumina tech support and they can help you with that.

**nucacidhunter** · 10-12-2014, 09:19 PM

Other options are to let the run to continue and add the 9th base from the adapter to all indices or during demultiplexing mask the 9th base from your index reads.

**kcchan** · 10-12-2014, 11:31 PM

Originally posted by nucacidhunter View Post

Other options are to let the run to continue and add the 9th base from the adapter to all indices or during demultiplexing mask the 9th base from your index reads.

Unfortunately that won't help him with the 100bp index 2 read. After 8 bases you'll end up with a bunch of adapter sequence followed by read 1 all over again.

**nucacidhunter** · 10-13-2014, 12:32 AM

Unfortunately that won't help him with the 100bp index 2 read. After 8 bases you'll end up with a bunch of adapter sequence followed by read 1 all over again.

You are right. I thought it was read 2 not index 2.

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wrong run parameters. How can I change it after 1 cycle?

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