chenqingwang
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lncRNAseq
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From fastq to lncRNA profile.
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lncRNAseq/workflow.wdl

108 行
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原始文件 永久链接 Blame 文件历史 

  1. import "./tasks/fastp.wdl" as fastp

  2. import "./tasks/hisat2.wdl" as hisat2

  3. import "./tasks/samtools.wdl" as samtools

  4. import "./tasks/featureCounts.wdl" as featureCounts

  5. 

  6. 

  7. workflow {{ project_name }} {

  8.     String sample_id

  9.     File read1

  10.     File read2

  11.     String adapter_sequence

  12.     String adapter_sequence_r2

  13.     String fastp_docker

  14.     String fastp_cluster

  15.     String umi_loc	

  16.     Int trim_front1

  17.     Int trim_tail1

  18.     Int max_len1

  19.     Int trim_front2

  20.     Int trim_tail2

  21.     Int max_len2

  22.     Int disable_adapter_trimming

  23.     Int length_required

  24.     Int umi_len

  25.     Int UMI

  26.     Int qualified_quality_phred

  27.     Int length_required1

  28.     Int disable_quality_filtering

  29.     File idx

  30.     String idx_prefix

  31.     String pen_intronlen

  32.     String hisat2_docker

  33.     String hisat2_cluster	

  34.     Int pen_cansplice

  35.     Int pen_noncansplice

  36.     Int min_intronlen

  37.     Int max_intronlen

  38.     Int maxins

  39.     Int minins	

  40.     String ins_size = sample_id + ".ins_size"

  41.     String samtools_docker

  42.     String samtools_cluster	

  43.     Int insert_size	

  44.     File lnc_gtf_file

  45.     String subread_docker

  46.     String subread_cluster	

  47. 

  48. 	call fastp.fastp as fastp {

  49. 		input: 

  50. 		sample_id = sample_id,

  51. 		read1 = read1, 

  52. 		read2 = read2,

  53. 		docker = fastp_docker,

  54. 		cluster = fastp_cluster,

  55. 		adapter_sequence = adapter_sequence,

  56. 		adapter_sequence_r2 = adapter_sequence_r2,

  57. 		umi_loc = umi_loc,

  58. 		trim_front1 = trim_front1,

  59. 		trim_tail1 = trim_tail1, 

  60. 		max_len1 = max_len1,

  61. 		trim_front2 = trim_front2,

  62. 		trim_tail2 = trim_tail2,

  63. 		max_len2 = max_len2,

  64. 		disable_adapter_trimming = disable_adapter_trimming,

  65. 		length_required = length_required,

  66. 		umi_len = umi_len,

  67. 		UMI = UMI,

  68. 		qualified_quality_phred = qualified_quality_phred,

  69. 		length_required1 = length_required1,

  70. 		disable_quality_filtering = disable_quality_filtering

  71. 	}

  72. 

  73. 	call hisat2.hisat2 as hisat2 {

  74. 		input: 

  75. 		sample_id = sample_id,

  76. 		idx = idx, 

  77. 		idx_prefix = idx_prefix, 

  78. 		Trim_R1 = fastp.Trim_R1, 

  79. 		Trim_R2 = fastp.Trim_R2,

  80. 		docker = hisat2_docker,

  81. 		cluster = hisat2_cluster,

  82. 		pen_intronlen = pen_intronlen,

  83. 		pen_cansplice = pen_cansplice,

  84. 		pen_noncansplice = pen_noncansplice,

  85. 		min_intronlen = min_intronlen,

  86. 		max_intronlen = max_intronlen,

  87. 		maxins = maxins,

  88. 		minins = minins

  89. 	}

  90. 

  91. 	call samtools.samtools as samtools {

  92. 		input: 

  93. 		sample_id = sample_id,

  94. 		sam = hisat2.sam,

  95. 		docker = samtools_docker,

  96. 		cluster = samtools_cluster,

  97. 		insert_size = insert_size

  98. 	}

  99. 

  100. 	call featureCounts.featureCounts as featureCounts {

  101. 		input: 

  102. 		sample_id = sample_id,

  103. 		bam_file = samtools.out_bam,

  104. 		lnc_gtf_file = lnc_gtf_file,

  105. 		docker = subread_docker,

  106. 		cluster = subread_cluster

  107. 	}

  108. }