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**r.rosati** · 05-10-2018, 11:53 AM

Ciao Isabella!
Some troubleshooting information can be obtained from the report.
How did the consensus keys look?
Were the test fragments OK (according to the % 50AQ17 and histogram)?
If you want, share the PDF run report, it'd be easier to troubleshoot.

**ferjusa** · 05-21-2018, 11:36 AM

Ciaooooo!
Here I attached the PDF run report...horrible!

Could the problem be the dilution factor of my library (64 barcodes) before the emulsion pcr? or maybe the chip loading?

Please help!

Grazie mille

Attached Files

Auto_user_SN2-73-HCV_04.05.18_282.pdf (611.3 KB, 60 views)

**r.rosati** · 05-21-2018, 02:11 PM

Ciao Isabella!
I see that the consensus key is very low... I would think that you had an issue with either the polymerase or the sequencing primer... or with the run itself.
You do have a huge % of "no template" ISPs and very low policlonality. You mention the dilution factor of your libraries, do you suspect having used too few DNA at the emulsion PCR step? But then you should have likely removed the empty beads at the ES purification step, having very few ISP left, and you'd see a lot of test fragment ISPs in the run. (Do you by chance save those 2ul of ISPs for the Ion Sphere Quality Control Kit on the Qubit?)

**r.rosati** · 05-21-2018, 02:19 PM

P.S.: There's a useful document from the now-defunct IonCommunity called "How to assess a PGM sequencing run report". Do you have it? I don't know where Thermo would be storing it nowadays, if it wasn't lost forever in the pyre.

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