Seqanswers Leaderboard Ad

**Chipper** · 05-28-2014, 06:54 AM

Originally posted by Fernas View Post

Hi all,

My question is about processing RNASeq data in order to extract the normal gene expression count matrix:

if two reads are mapped uniquely to the same genome position and both of them have identical alignment region. Shall we count them as 2 reads or simply 1.

If you say that we count them as 2 reads, then my question: why in Chipseq processing, we count these 2 reads as only 1 to remove the PCR bias problem which may cause such duplicates.

De-duplication would not let you analyze highly expressed transcripts which will need to have many identical reads. If you think your RNA-seq sample has a high PCR duplication rate it is better to downsample it.

**Fernas** · 05-28-2014, 07:03 AM

Thanks @chipper.
But I am still wondering why in Chipseq processing steps, we remove duplicates, however, in RNASeq we keep them.

Topics	Statistics	Last Post
Cancer Metastasis: A Deep Dive into Cellular Plasticity by seqadmin Started by seqadmin, 04-11-2024, 12:08 PM	0 responses 51 views 0 likes	Last Post by seqadmin 04-11-2024, 12:08 PM
Proteogenomic Profiles Offer New Clues in Prostate Cancer by seqadmin Started by seqadmin, 04-10-2024, 10:19 PM	0 responses 50 views 0 likes	Last Post by seqadmin 04-10-2024, 10:19 PM
Novel Diagnostic Assay Enhances Ovarian Cancer Detection by seqadmin Started by seqadmin, 04-10-2024, 09:21 AM	0 responses 44 views 0 likes	Last Post by seqadmin 04-10-2024, 09:21 AM
Evolutionary Dynamics of Centromeres: A Comparative Genomic Analysis by seqadmin Started by seqadmin, 04-04-2024, 09:00 AM	0 responses 55 views 0 likes	Last Post by seqadmin 04-04-2024, 09:00 AM

Seqanswers Leaderboard Ad

Announcement

RNASeq: Multiple identical uniquely mapped reads

Comment

Comment

Latest Articles

ad_right_rmr

News