Description

CHM13 PRO-seq and RNA-seq Bowtie2-F3852 alignments and Meryl unique k-mer filtering

Methods

The PRO-seq experiment was done on CHM13 cells and sequenced for 75bp single-ended reads.

The native RNA-seq libraries were done on CHM13 cells using oligodT during library prep and sequenced for 150bp paired-end reads.

Reads were trimmed and filtered before mapped with Bowtie2 -N 0 -k 100 and samtools filtered (F3852)

Mapped reads were then filtered through two different sets of genome-wide unique k-mers: 21mers, 51mers

Display Conventions and Configuration

Data access

Release history

1. 2020-09-22: CHM13 v1.0 release (chm13.draft_v1.0.fasta)

Contacts

• Savannah Hoyt <savannah.klein@uconn.edu>

Credits

Savannah Hoyt (PROseq library prep & sequencing; all mapping & filtering)

Rachel O'Neill

Megan Dennis (RNAseq library prep & sequencing)

Colin Shew (RNAseq library prep & sequencing)

Arang Rhie (Meryl software)