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602panel_test
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602panel_test
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s1_noUMI_clean_align_FFPE_20230529.pbs

s1_noUMI_clean_align_FFPE_20230529.pbs 2.7 KB
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  1. 

  2. 

  3. #!/bin/sh
    4. 

  4. #PBS -N align_noUMI
    5. 

  5. #PBS -j oe
    6. 

  6. #PBS -l ncpus=20
    7. 

  7. #PBS -l nodes=1
    8. 

  8. #PBS -l mem=20G
    9. 

  9. 

  10. #inputpath=$1
    11. 

  11. #sample=$2
    12. 

  12. source  /home/liuxiangqiong/miniconda3/bin/activate base
    13. 

  13. hg19=/cgdata/Database/GATK/b37/human_g1k_v37_decoy.fasta
    14. 

  14. target=/cgdata/liuxiangqiong/work62pancancer/Client/v0/script/refdata/NanOnco_Plus_Panel_v2.0_Covered_b37_cg.parY2X.sort.bed
    15. 

  15. #################################################################################1.trim#########################################################
    16. 

  16. runstart="`date '+%F%n%T'`"
    17. 

  17. echo ${sample} "start at" $runstart
    18. 

  18. echo "#--------------------------------------STEP1.clean the raw data--------------------------------------#"
    19. 

  19. starttime="`date '+%Y%m%d%H%M%S'`"
    20. 

  20. #fastp -i ${inputpath}/${sample}_R1.fastq.gz -I ${inputpath}/${sample}_R2.fastq.gz  -o ${inputpath}/${sample}_clean_R1.fq.gz -O ${inputpath}/${sample}_clean_R2.fq.gz -c -l 50 -q 20 --umi --umi_loc read1 --umi_len 8 -j ${inputpath}/${sample}.fastp.json -h ${inputpath}/${sample}.fastp.html
    21. 

  21. 

  22. fastp -i ${inputpath}/${sample}_R1.fastq.gz -I ${inputpath}/${sample}_R2.fastq.gz  -o ${inputpath}/${sample}_clean_R1.fq.gz -O ${inputpath}/${sample}_clean_R2.fq.gz -c -l 50 -q 20  -j ${inputpath}/${sample}.fastp.json -h ${inputpath}/${sample}.fastp.html
    23. 

  23. 

  24. echo "#--------------------------------------STEP1.clean the raw data finished!---------------#"
    25. 

  25. #################################################################################2.mapping#########################################################
    26. 

  26. #2.1.speedseq align
    27. 

  27. echo "#--------------------------------------STEP2.align to refdata--------------------------------------#"
    28. 

  28. speedseq align -t 40  -o ${bam_dir}/${sample}_clean -R "@RG\tID:${sample}\tSM:${sample}\tLB:${sample}" ${hg19} ${inputpath}/${sample}_clean_R1.fq.gz ${inputpath}/${sample}_clean_R2.fq.gz
    29. 

  29. echo "#--------------------------------------STEP2.align to refdata finished!--------------------------------------#"
    30. 

  30. rm -rf ${bam_dir}/${sample}_clean.splitters.bam
    31. 

  31. rm -rf ${bam_dir}/${sample}_clean.splitters.bam.bai
    32. 

  32. rm -rf ${bam_dir}/${sample}_clean.discordants.bam
    33. 

  33. rm -rf ${bam_dir}/${sample}_clean.discordants.bam.bai
    34. 

  34. endtime="`date '+%Y%m%d%H%M%S'`"
    35. 

  35. echo "step1 run " $[$endtime-$starttime]"s">${inputpath}/${sample}_mapping.log
    36. 

  36. echo "${sample} mapping finish!" >>${inputpath}/${sample}_mapping.log
    37. 

  37. 

  38. echo "#--------------------------------------STEP3.qualimap--------------------------------------#"
    39. 

  39. ourputdir=${inputpath}/9Ontarget
    40. 

  40. samtools flagstat ${bam_dir}/${sample}_clean.bam > ${ourputdir}/${sample}_clean.abra2.flagstat
    41. 

  41. #cd ${ourputdir}
    42. 

  42. #qualimap bamqc -bam  ${bam_dir}/${sample}_clean.bam  -c --java-mem-size=40G -gff ${target}
    43. 

  43. #去掉dup
    44. 

  44. qualimap bamqc -bam  ${bam_dir}/${sample}_clean.bam  -c -sd --java-mem-size=40G -gff ${target}
    45.