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**kcchan** · 03-10-2013, 07:36 PM

It may have something to do with RTA not getting enough data to perform basecalling. The first 12 bases are used to calculate the color matrix and phasing/prephasing values, and 25 are needed for quality scoring.

Just curious, may I ask why this run is designed to be in this asymmetric manner?

**sunleaf** · 03-10-2013, 07:57 PM

Thanks for your answer. That's what I suspected too. We are developing our own assay and 14 cycle is all we needed for that end. I'll contact Illumina to see if I can salvage the data and run 25 cycles in the future.

**kcchan** · 03-10-2013, 08:56 PM

You can check the error logs in MSR and see what's going on. I would guess that BCL files were never generated from read 1 and all you had were CIF intensity files. You might be able to use offline basecaller to get the basecalls out of it, but I've never tried it in such a situation. Illumina tech support may be your best bet in this case. Good luck and let us know how things turn out!

**sunleaf** · 03-11-2013, 09:04 AM

Just talked with a very helpful Illumina tech support. Yes, we can use CASAVA to demultiplex the other end with --usebasemask option and designated 14 bases, and the sample sheet should be made for Hiseq instead of Miseq. That's just too much trouble to go through for our repeated runs. I think it would just be easier to run read1 for 25 cycles.

**kmcarr** · 03-11-2013, 11:28 AM

Originally posted by sunleaf View Post

Just talked with a very helpful Illumina tech support. Yes, we can use CASAVA to demultiplex the other end with --usebasemask option and designated 14 bases, and the sample sheet should be made for Hiseq instead of Miseq. That's just too much trouble to go through for our repeated runs. I think it would just be easier to run read1 for 25 cycles.

If you are using a 50 cycle kit make sure that the total number of cycles doesn't exceed the capacity of the kit. Officially a 50 cycle kit has sufficient reagents for 76 cycles; we have safely done 78 cycles. If you increase read 1 to 25 cycles without changing the other settings you cycle total will be 81 (25|6|50).

**kcchan** · 03-11-2013, 12:52 PM

Good point kmcarr. It's never good to run out of reagents since it can suck air into the lines. I believe the scan mix is usually the first to run out.

It may be a good idea to re-think the library design a bit. You can squeeze the indices inline at the start of read 1 to lengthen the read, but unfortunately I don't think the MiSeq has an easy way to demultiplex inline barcodes, so you're stuck with CASAVA if you want to go that route.

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