Mercurial > repos > iuc > brew3r_r
view test-data/generate_test.R @ 0:928a52b5c938 draft
planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/brew3r_r commit 3e3c47b732510a9ef0b2864b284aa14308e75ab0
author | iuc |
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date | Tue, 11 Jun 2024 08:26:37 +0000 |
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children | d3b0390f325f |
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library(GenomicRanges) input_to_overlap_case1_2_3_4_6_7_8 <- GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = 3, end = 25 ), strand = "+", gene_id = "geneA", transcript_id = "transcriptA", type = "exon", exon_id = "exonA" ) big_gr <- NULL for (i in c(1:5, 7:10)) { temp.gr <- input_to_overlap_case1_2_3_4_6_7_8 temp.gr <- shift(temp.gr, 100 * (i - 1)) temp.gr$gene_id <- paste0("gene", LETTERS[i]) temp.gr$transcript_id <- paste0("transcript", LETTERS[i]) temp.gr$exon_id <- paste0("exon", LETTERS[i]) temp.gr$exon_number <- 1 big_gr <- c(big_gr, temp.gr) } input_to_overlap_case5_9 <- GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(1, 33, 45, 72), end = c(25, 40, 60, 75) ), strand = "+", gene_id = "geneA", transcript_id = "transcriptA", type = "exon", exon_id = c("exonA", "exonB", "exonC", "exonD") ) for (i in c(6, 11)) { temp.gr <- input_to_overlap_case5_9 temp.gr <- shift(temp.gr, 100 * (i - 1)) temp.gr$gene_id <- paste0("gene", LETTERS[i]) temp.gr$transcript_id <- paste0("transcript", LETTERS[i]) temp.gr$exon_id <- paste0("exon", LETTERS[i], letters[1:4]) temp.gr$exon_number <- 1:4 big_gr <- c(big_gr, temp.gr) } big_gr <- unlist(as(big_gr, "GRangesList")) input_gr <- c( # 1 GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 20), end = c(10, 30) ), strand = "+", gene_id = c("gene11", "gene12"), transcript_id = c("transcript11", "transcript12"), type = "exon", exon_id = c("exon11", "exon12") ), # 2 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 20), end = c(10, 25) ), strand = "+", gene_id = c("gene21", "gene22"), transcript_id = c("transcript21", "transcript22"), type = "exon", exon_id = c("exon21", "exon22") ), 100 ), # 3_5 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 20), end = c(10, 22) ), strand = "+", gene_id = c("gene31", "gene32"), transcript_id = c("transcript31", "transcript32"), type = "exon", exon_id = c("exon31", "exon32") ), 200 ), # 4 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 5), end = c(10, 22) ), strand = "+", gene_id = c("gene41", "gene42"), transcript_id = c("transcript41", "transcript42"), type = "exon", exon_id = c("exon41", "exon42") ), 300 ), # 4bis shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 5), end = c(10, 25) ), strand = "+", gene_id = c("gene51", "gene52"), transcript_id = c("transcript51", "transcript52"), type = "exon", exon_id = c("exon51", "exon52") ), 400 ), # 3_5 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 20), end = c(10, 22) ), strand = "+", gene_id = c("gene61", "gene62"), transcript_id = c("transcript61", "transcript62"), type = "exon", exon_id = c("exon61", "exon62") ), 500 ), # 6 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(1, 1, 30), end = c(10, 10, 40) ), strand = "+", gene_id = "gene71", transcript_id = c("transcript71", "transcript72", "transcript72"), type = "exon", exon_id = c("exon71", "exon71", "exon72") ), 600 ), # 6bis shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(1, 1, 30), end = c(10, 10, 40) ), strand = "+", gene_id = c("gene81", "gene82", "gene82"), transcript_id = c("transcript81", "transcript82", "transcript82"), type = "exon", exon_id = c("exon81", "exon82", "exon83") ), 700 ), # 7 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(1, 1, 30), end = c(8, 10, 40) ), strand = "+", gene_id = "gene1", transcript_id = c("transcript91", "transcript92", "transcript92"), type = "exon", exon_id = c("exon91", "exon92", "exon93") ), 800 ), # 8 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(1, 1, 30), end = c(8, 10, 40) ), strand = "+", gene_id = c("gene101", "gene102", "gene102"), transcript_id = c("transcript101", "transcript102", "transcript102"), type = "exon", exon_id = c("exon101", "exon102", "exon103") ), 900 ), # 9 shift( GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(5, 55), end = c(10, 70) ), strand = "+", gene_id = c("gene111", "gene112"), transcript_id = c("transcript111", "transcript112"), type = "exon", exon_id = c("exon111", "exon112") ), 1000 ) ) ## Add convergent genes overlapping a unstranded input_gr <- c( input_gr, GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = c(1100, 1110), end = c(1105, 1120) ), strand = c("+", "-"), gene_id = c("gene121", "gene122"), transcript_id = c("transcript121", "transcript122"), type = "exon", exon_id = c("exon121", "exon122") ) ) big_gr <- c( big_gr, GenomicRanges::GRanges( seqnames = "chr1", ranges = IRanges::IRanges( start = 1103, end = 1113 ), strand = "*", gene_id = "geneL", transcript_id = "transcriptL", type = "exon", exon_id = "exonL" ) ) input_gr$gene_name <- input_gr$gene_id input_gr$gene_name[input_gr$gene_id == "gene111"] <- "Gm001" library(BREW3R.r) new.gr <- extend_granges(input_gr, big_gr) library("rtracklayer") export.gff(input_gr, "input.gtf") export.gff(big_gr, "second_input.gtf") export.gff(sort(new.gr, ignore.strand = TRUE), "output.gtf")