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  • chip-seq normalization when two sample total reads vary largely

    HI:

    i am new to chip-seq and I fellow tranditional way to analyze my data.
    I normalized my two chip-seq data by total reads. (I divided genome into 50bp bin), total reads here means reads after bowtie and filter out redundancy.
    I visualize it on IGV and found one sample is relative lower than the other on the genome-wide scale as well as some house keeping gene such as ACTB and GAPDH.

    My major concern is the total reads after filter out redundancy is quite difference: one is 9.5M and the other is 14M.

    My question is does the normalization by total reads could fail when two sample vary largely, and How?

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