I recently prepared a library using the Multiplexed Shotgun Sequencing protocol (citation below) and sent the library off for sequencing on Illumina HiSeq. The library that I submitted was supposed to be at 10 nM in Qiagen EB buffer supplemented with 0.1% Tween 20. I received word that the library had failed to cluster on the flowcell.
After reviewing my notes, I noticed a large mistake...I added about ~100x too much Tween 20. The final solution was 10% instead of 0.1%. I have a feeling that this is probably what prevented clustering on the flowcell, but I can't find any conclusive info. Does anyone know if excess Tween 20 would interfere with HiSeq?
Thanks
Andolfatto, P., D. Davison, D. Erezyilmaz, T. T. Hu, J. Mast, T. Sunayama-Morita, and D. L. Stern. Multiplexed shotgun genotyping for rapid and efficient genetic mapping. Genome Research 21:610-617.
After reviewing my notes, I noticed a large mistake...I added about ~100x too much Tween 20. The final solution was 10% instead of 0.1%. I have a feeling that this is probably what prevented clustering on the flowcell, but I can't find any conclusive info. Does anyone know if excess Tween 20 would interfere with HiSeq?
Thanks
Andolfatto, P., D. Davison, D. Erezyilmaz, T. T. Hu, J. Mast, T. Sunayama-Morita, and D. L. Stern. Multiplexed shotgun genotyping for rapid and efficient genetic mapping. Genome Research 21:610-617.
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