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1. As the primersequences for the in-gel PCR in the RNA seq protocoll are known, has anyone ever tried it with custom primers (e.g. own barcode sequences)?
2. Paired end sequencing allows me to sequence 35 bp from the other direction (P2 adaptor). From which point are these 35 bp counted? Because when you use a barcode (+ internal adaptor) and these 35 bp are counted from the P2 adaptor, you lose a lot of bp just for these two (barcode and internatl adaptor) sequences.
Thank you!
2. Paired end sequencing allows me to sequence 35 bp from the other direction (P2 adaptor). From which point are these 35 bp counted? Because when you use a barcode (+ internal adaptor) and these 35 bp are counted from the P2 adaptor, you lose a lot of bp just for these two (barcode and internatl adaptor) sequences.
Thank you!
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