diff --git a/workflows/transcriptomics/rnaseq-sr/rnaseq-sr.ga b/workflows/transcriptomics/rnaseq-sr/rnaseq-sr.ga index 2bf8cd853..bd159c3f9 100644 --- a/workflows/transcriptomics/rnaseq-sr/rnaseq-sr.ga +++ b/workflows/transcriptomics/rnaseq-sr/rnaseq-sr.ga @@ -1,6 +1,6 @@ { "a_galaxy_workflow": "true", - "annotation": "This workflow takes as input a list of single-read fastqs. Adapters and bad quality bases are removed with cutadapt. Reads are mapped with STAR with ENCODE parameters and genes are counted simultaneously. The counts are reprocess to be similar to HTSeq-count output. FPKM are computed with cufflinks. Coverage (per million mapped reads) are computed with bedtools on uniquely mapped reads.", + "annotation": "This workflow takes as input a list of single-reads fastqs. Adapters and bad quality bases are removed with cutadapt. 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107.63336181640625, + "top": 522.134886401586 }, "tool_id": null, "tool_state": "{\"restrictOnConnections\": true, \"parameter_type\": \"text\", \"optional\": false}", @@ -110,8 +110,8 @@ "name": "Input dataset", "outputs": [], "position": { - "left": 50.60003662109375, - "top": 508.15479689456936 + "left": 125.60003662109375, + "top": 606.751585620336 }, "tool_id": null, "tool_state": "{\"optional\": false, \"tag\": \"\"}", @@ -137,8 +137,8 @@ "name": "Input parameter", "outputs": [], "position": { - "left": 81.25, - "top": 568.5214961133194 + "left": 156.25, + "top": 667.118284839086 }, "tool_id": null, "tool_state": "{\"restrictions\": [\"stranded - forward\", \"stranded - reverse\", \"unstranded\"], \"parameter_type\": \"text\", \"optional\": false}", @@ -149,37 +149,10 @@ "workflow_outputs": [] }, "5": { - "annotation": "Whether coverage should be for forward and reverse separated", - "content_id": null, - "errors": null, - "id": 5, - "input_connections": {}, - "inputs": [ - { - 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