Skip to content

LiYingshu/Decode-seq

BranchesTags
 
 

Folders and files

NameName
Last commit message
Last commit date

Latest commit

 

History

3 Commits
LICENSE
LICENSE
 
 
README.md
README.md
 
 

Repository files navigation

Decode-seq

Description

The Decode-seq data analysis pipeline contains 3 python scripts: decode_barcode.py, decode_gene.py, decode_quant.py. We need to run these three scripts in sequential order on the input fastq files and the output is the count based quantification matrix, which is ready for downstream analysis by edgeR or DEseq2.

  • decode_barcode.py: take Read1 as the input, generate a barcode table (read name, USI, and UMI).
  • decode_gene.py: take Read2 as the input, generate a gene table (read name, transcript).
  • decode_quant.py: take two tables as the input, generate the count matrix (transcript X sample).

Dependencies

Usage

decode_barcode.py -i|--input <input> -u|--usi <usifile> [-q|--qscutoff <int>] [-b|--boundary GGG] [-c|--countonly]

decode_gene.py -f|--fastq <input> -d|--outdir <outdir> [-x|--STARIDX <STARIDX>] [-g|--gtf gtf] [-t|--thread threads] [-b|--bam bam]

decode_quant.py -g|--genetable <gene_table> -b|--barcodetable <barcode_table> -u|--usi <usifile>

Arguments

decode_barcode.py

  • -i,--input Read1 fastq file
  • -u,--usi A plain text file caontaining 2 columns: USI name and 6bp sequence.
  • -q,--qscutoff Minimum sequencing quality score of 1-6bp of Read1 (the USI position). Default 20
  • -b,--boundary 3-6 base between UMI sequence and cDNA sequence, usually three Guanines. Default GGG
  • -c,--countonly Only output the barcode filter summary in the standard output. Default output barcode sequence, cDNA sequence and barcode filter summary to standard output

decode_gene.py

  • Note: take either '-f-d[-x-g-t]' (run star then process bam) or '-b' (process bam directly) as the input
  • -f, --fastq Read2 fastq file
  • -d, --outdir Run star directory
  • -x, --STARIDX Reference genome STAR index
  • -g, --gtf <file.gtf> Reference genome annotation
  • -t, --thread Number of threads to use for STAR mapping. Default 1.
  • -b, --bam <file.bam> STAR output bam file, default file name is Aligned.toTranscriptome.out.bam. This bam output requires the parameter --quantMode TranscriptomeSAM GeneCounts when running STAR.

decode_quant.py

  • -g, --genetable <gene_table> output of decode_barcode.py
  • -b, --barcodetable <barcode_table> output of decode_gene.py
  • -u, --usi A plain text file containing 2 columns: USI name and 6bp sequence.

Examples

decode_barcode.py  -i sample_R1.fq -u usi.txt > sample.barcode.tab

decode_gene.py     -f sample_R2.fq -d star_output_dir -t 30 -x star_index -g annotation.gtf > sample.gene.tab

decode_quant.py    -b sample.barcode.tab -g sample.gene.tab -u usi.txt > sample.quant.tab

About

Analysis pipeline for Decode-seq

Resources

Readme

License

GPL-3.0 license
Activity

Stars

0 stars

Watchers

0 watching

Forks

0 forks
Report repository

Releases

No releases published

Packages

No packages published