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  • RSEM: differential expression of specific enzymes within transcriptome

    Hi
    I'm interested in specific proteolytic enzymes in transcriptomic data. I chose 3 different transcripts from de novo assembly and run RSEM analysis with pair-end data reads.
    First question: Is it Ok to run RSEM on such small set of reference sequences?

    Second question: How to deal with different length of reference sequences? In my case I had 980, 247 and 929 nucleotides. I run two analysis, one with original length of reference sequences, and second with trimmed sequences on 247 nucleotides for all sequences and I got different results.

    thanks in advance.

    Roman

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