Mercurial > repos > jjohnson > defuse
annotate defuse.xml @ 5:3bd1087db05e draft
Add dependecies for bowtie, blat, and faToTwoBit
author | Jim Johnson <jj@umn.edu> |
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date | Fri, 04 Jan 2013 15:01:19 -0600 |
parents | 679a5c7b1294 |
children | 6e30713cefb0 |
rev | line source |
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deFuse version 0.5.0 - Use tool_dependencies.xml
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1 <tool id="defuse" name="DeFuse" version="1.5"> |
1 | 2 <description>identify fusion transcripts</description> |
3 <requirements> | |
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4 <requirement type="package" version="0.5.0">defuse</requirement> |
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5 <requirement type="package" version="0.12.7">bowtie</requirement> |
3bd1087db05e
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6 <requirement type="package" version="34x10">blat</requirement> |
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7 <requirement type="package" version="34x10">fatotwobit</requirement> |
1 | 8 </requirements> |
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DeFuse - Allow user to save the workspace, create an html file with links to the files in the workspace.
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9 <command interpreter="command"> /bin/bash $shscript </command> |
1 | 10 <inputs> |
11 <param name="left_pairendreads" type="data" format="fastq" label="left part of read pairs" help="The left and right reads pairs must be in the same order, and not have any unpaired reads. (FASTQ interlacer will pair reads and remove the unpaired. FASTQ de-interlacer will separate the result into left and right reads.)"/> | |
12 <param name="right_pairendreads" type="data" format="fastq" label="right part of read pairs" help="In the same order as the left reads"/> | |
13 <conditional name="refGenomeSource"> | |
14 <param name="genomeSource" type="select" label="Will you select a built-in DeFuse Reference Dataset, or supply a configuration from your history" help=""> | |
15 <option value="indexed">Use a built-in DeFuse Reference Dataset</option> | |
16 <option value="history">Use a configuration from your history that specifies the DeFuse Reference Dataset</option> | |
17 </param> | |
18 <when value="indexed"> | |
19 <param name="index" type="select" label="Select a Reference Dataset" help="if your genome of interest is not listed - contact Galaxy team"> | |
20 <options from_file="defuse.loc"> | |
21 <column name="name" index="1"/> | |
22 <column name="value" index="2"/> | |
23 <filter type="sort_by" column="0" /> | |
24 <validator type="no_options" message="No indexes are available" /> | |
25 </options> | |
26 </param> | |
27 <conditional name="defuse_param"> | |
28 <param name="settings" type="select" label="Defuse parameter settings" help=""> | |
29 <option value="preSet">Default settings</option> | |
30 <option value="full">Full parameter list</option> | |
31 </param> | |
32 <when value="preSet" /> | |
33 <when value="full"> | |
34 <param name="max_insert_size" type="integer" value="500" optional="true" label="Bowtie max_insert_size" /> | |
35 <param name="dna_concordant_length" type="integer" value="2000" optional="true" label="Minimum gene fusion range dna_concordant_length" /> | |
36 <param name="discord_read_trim" type="integer" value="50" optional="true" label="Trim length for discordant reads discord_read_trim" help="(split reads are not trimmed)" /> | |
37 <param name="clustering_precision" type="float" value=".95" optional="true" label="Filter clustering_precision"> | |
38 <validator type="in_range" message="Choose a value between .1 and 1.0" min=".1" max="1"/> | |
39 </param> | |
40 <param name="span_count_threshold" type="integer" value="5" optional="true" label="Filter span_count_threshold" /> | |
41 <param name="split_count_threshold" type="integer" value="3" optional="true" label="Filter split_count_threshold" /> | |
42 <param name="percent_identity_threshold" type="float" value=".90" optional="true" label="Filter percent_identity_threshold"> | |
43 <validator type="in_range" message="Choose a value between .1 and 1.0" min=".1" max="1"/> | |
44 </param> | |
45 <param name="max_dist_pos" type="integer" value="600" optional="true" label="Filter max_dist_pos" /> | |
46 <param name="num_dist_genes" type="integer" value="500" optional="true" label="Filter num_dist_genes" /> | |
47 <param name="split_min_anchor" type="integer" value="4" optional="true" label="Filter split_min_anchor" /> | |
48 <param name="max_concordant_ratio" type="float" value="0.1" optional="true" label="Filter max_concordant_ratio"> | |
49 <validator type="in_range" message="Choose a value between 0.0 and 1.0" min="0" max="1"/> | |
50 </param> | |
51 <param name="splice_bias" type="integer" value="10" optional="true" label="Filter splice_bias" /> | |
52 <param name="probability_threshold" type="float" value="0.50" optional="true" label="Filter probability_threshold"> | |
53 <validator type="in_range" message="Choose a value between 0.0 and 1.0" min="0" max="1"/> | |
54 </param> | |
55 <param name="covariance_sampling_density" type="float" value="0.01" optional="true" label="covariance_sampling_density"> | |
56 <help>Position density when calculating covariance</help> | |
57 <validator type="in_range" message="Choose a value between 0.0 and 1.0" min="0" max="1"/> | |
58 </param> | |
59 <param name="denovo_assembly" type="select" label="denovo_assembly" help=""> | |
60 <option value="">Use Default</option> | |
61 <option value="no">no</option> | |
62 <option value="yes">yes</option> | |
63 </param> | |
64 <!-- | |
65 <param name="positive_controls" type="data" format="txt" optional=true label="Defuse positive_controls" help=""/> | |
66 --> | |
67 </when> <!-- full --> | |
68 </conditional> <!-- defuse_param --> | |
69 </when> | |
70 <when value="history"> | |
71 <param name="config" type="data" format="txt" label="Defuse Config file" help=""/> | |
72 </when> <!-- history --> | |
73 </conditional> <!-- refGenomeSource --> | |
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DeFuse - Allow user to save the workspace, create an html file with links to the files in the workspace.
Jim Johnson <jj@umn.edu>
parents:
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74 <param name="keep_output" type="boolean" checked="true" truevalue="yes" falsevalue="no" label="Save DeFuse working directory files"/> |
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75 <param name="do_get_reads" type="boolean" checked="true" truevalue="yes" falsevalue="no" label="Run get_reads on each cluster"/> |
1 | 76 </inputs> |
77 <configfiles> | |
78 <configfile name="defuse_config"> | |
79 #import ast | |
80 #if $refGenomeSource.genomeSource == "history": | |
81 #include raw $refGenomeSource.config.__str__ | |
82 #else | |
83 #set $ref_dict = dict($ast.literal_eval($refGenomeSource.index.value)) | |
84 # | |
85 # Configuration file for defuse | |
86 # | |
87 # At a minimum, change all values enclused by [] | |
88 # | |
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Changes for defuse-0.4.3, modifications for non-human genomes no longer required, defuse.xml searches for location of scripts/defuse.pl
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89 |
1 | 90 # Directory where the defuse code was unpacked |
91 ## Default location in the tool/defuse directory | |
92 # source_directory = ${__root_dir__}/tools/defuse | |
93 source_directory = #slurp | |
94 #try | |
95 $ref_dict['source_directory'] | |
96 #except | |
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97 __DEFUSE_PATH__ |
1 | 98 #end try |
99 | |
100 # Directory where you want your dataset | |
101 dataset_directory = #slurp | |
102 #try | |
103 $ref_dict['dataset_directory'] | |
104 #except | |
105 /project/db/genomes/Hsapiens/hg19/defuse | |
106 #end try | |
107 | |
108 # Input genome and gene models | |
109 gene_models = #slurp | |
110 #try | |
111 $ref_dict['gene_models'] | |
112 #except | |
113 \$(dataset_directory)/Homo_sapiens.GRCh37.62.gtf | |
114 #end try | |
115 genome_fasta = #slurp | |
116 #try | |
117 $ref_dict['genome_fasta'] | |
118 #except | |
119 \$(dataset_directory)/Homo_sapiens.GRCh37.62.dna.chromosome.fa | |
120 #end try | |
121 | |
122 # Repeat table from ucsc genome browser | |
123 repeats_filename = #slurp | |
124 #try | |
125 $ref_dict['repeats_filename'] | |
126 #except | |
127 \$(dataset_directory)/rmsk.txt | |
128 #end try | |
129 | |
130 # EST info downloaded from ucsc genome browser | |
131 est_fasta = #slurp | |
132 #try | |
133 $ref_dict['est_fasta'] | |
134 #except | |
135 \$(dataset_directory)/est.fa | |
136 #end try | |
137 est_alignments = #slurp | |
138 #try | |
139 $ref_dict['est_alignments'] | |
140 #except | |
141 \$(dataset_directory)/intronEst.txt | |
142 #end try | |
143 | |
144 # Unigene clusters downloaded from ncbi | |
145 unigene_fasta = #slurp | |
146 #try | |
147 $ref_dict['unigene_fasta'] | |
148 #except | |
149 \$(dataset_directory)/Hs.seq.uniq | |
150 #end try | |
151 | |
152 # Paths to external tools | |
153 bowtie_bin = #slurp | |
154 #try | |
155 $ref_dict['bowtie_bin'] | |
156 #except | |
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157 __BOWTIE_BIN__ |
1 | 158 #end try |
159 bowtie_build_bin = #slurp | |
160 #try | |
161 $ref_dict['bowtie_build_bin'] | |
162 #except | |
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163 __BOWTIE_BUILD_BIN__ |
1 | 164 #end try |
165 blat_bin = #slurp | |
166 #try | |
167 $ref_dict['blat_bin'] | |
168 #except | |
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169 __BLAT_BIN__ |
1 | 170 #end try |
171 fatotwobit_bin = #slurp | |
172 #try | |
173 $ref_dict['fatotwobit_bin'] | |
174 #except | |
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175 __FATOTWOBIT_BIN__ |
1 | 176 #end try |
177 r_bin = #slurp | |
178 #try | |
179 $ref_dict['r_bin'] | |
180 #except | |
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181 __R_BIN__ |
1 | 182 #end try |
183 rscript_bin = #slurp | |
184 #try | |
185 $ref_dict['rscript_bin'] | |
186 #except | |
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187 __RSCRIPT_BIN__ |
1 | 188 #end try |
189 | |
190 #raw | |
191 # Dataset files | |
192 dataset_prefix = $(dataset_directory)/defuse | |
193 chromosome_prefix = $(dataset_prefix).dna.chromosomes | |
194 exons_fasta = $(dataset_prefix).exons.fa | |
195 cds_fasta = $(dataset_prefix).cds.fa | |
196 cdna_regions = $(dataset_prefix).cdna.regions | |
197 cdna_fasta = $(dataset_prefix).cdna.fa | |
198 reference_fasta = $(dataset_prefix).reference.fa | |
199 rrna_fasta = $(dataset_prefix).rrna.fa | |
200 ig_gene_list = $(dataset_prefix).ig.gene.list | |
201 repeats_regions = $(dataset_directory)/repeats.regions | |
202 est_split_fasta1 = $(dataset_directory)/est.1.fa | |
203 est_split_fasta2 = $(dataset_directory)/est.2.fa | |
204 est_split_fasta3 = $(dataset_directory)/est.3.fa | |
205 est_split_fasta4 = $(dataset_directory)/est.4.fa | |
206 est_split_fasta5 = $(dataset_directory)/est.5.fa | |
207 est_split_fasta6 = $(dataset_directory)/est.6.fa | |
208 est_split_fasta7 = $(dataset_directory)/est.7.fa | |
209 est_split_fasta8 = $(dataset_directory)/est.8.fa | |
210 est_split_fasta9 = $(dataset_directory)/est.9.fa | |
211 | |
212 # Fasta files with bowtie indices for prefiltering reads for concordantly mapping pairs | |
213 prefilter1 = $(unigene_fasta) | |
214 | |
215 # deFuse scripts and tools | |
216 scripts_directory = $(source_directory)/scripts | |
217 tools_directory = $(source_directory)/tools | |
218 data_directory = $(source_directory)/data | |
219 #end raw | |
220 | |
221 # Path to samtools, 0.1.8 is compiled for you, use other versions at your own risk | |
222 samtools_bin = #slurp | |
223 #try | |
224 $ref_dict['samtools_bin'] | |
225 #except | |
226 \$(source_directory)/external/samtools-0.1.8/samtools | |
227 #end try | |
228 | |
229 # Bowtie parameters | |
230 bowtie_threads = #slurp | |
231 #try | |
232 $ref_dict['bowtie_threads'] | |
233 #except | |
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234 4 |
1 | 235 #end try |
236 bowtie_quals = #slurp | |
237 #try | |
238 $ref_dict['bowtie_quals'] | |
239 #except | |
240 --phred33-quals | |
241 #end try | |
242 max_insert_size = #slurp | |
243 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.max_insert_size.__str__ != "": | |
244 $refGenomeSource.defuse_param.max_insert_size | |
245 #else | |
246 #try | |
247 $ref_dict['max_insert_size'] | |
248 #except | |
249 500 | |
250 #end try | |
251 #end if | |
252 | |
253 # Parameters for building the dataset | |
254 chromosomes = #slurp | |
255 #try | |
256 $ref_dict.chromosomes | |
257 #except | |
258 1,2,3,4,5,6,7,8,9,10,11,12,13,14,15,16,17,18,19,20,21,22,X,Y,MT | |
259 #end try | |
260 mt_chromosome = #slurp | |
261 #try | |
262 $ref_dict['mt_chromosome'] | |
263 #except | |
264 MT | |
265 #end try | |
266 gene_sources = #slurp | |
267 #try | |
268 $ref_dict['gene_sources'] | |
269 #except | |
270 IG_C_gene,IG_D_gene,IG_J_gene,IG_V_gene,processed_transcript,protein_coding | |
271 #end try | |
272 ig_gene_sources = #slurp | |
273 #try | |
274 $ref_dict['ig_gene_sources'] | |
275 #except | |
276 IG_C_gene,IG_D_gene,IG_J_gene,IG_V_gene,IG_pseudogene | |
277 #end try | |
278 rrna_gene_sources = #slurp | |
279 #try | |
280 $ref_dict['rrna_gene_sources'] | |
281 #except | |
282 Mt_rRNA,rRNA,rRNA_pseudogene | |
283 #end try | |
284 | |
285 # Blat sequences per job | |
286 num_blat_sequences = #slurp | |
287 #try | |
288 $ref_dict['num_blat_sequences'] | |
289 #except | |
290 10000 | |
291 #end try | |
292 | |
293 # Minimum gene fusion range | |
294 dna_concordant_length = #slurp | |
295 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.dna_concordant_length.__str__ != "": | |
296 $refGenomeSource.defuse_param.dna_concordant_length | |
297 #else | |
298 #try | |
299 $ref_dict['dna_concordant_length'] | |
300 #except | |
301 2000 | |
302 #end try | |
303 #end if | |
304 | |
305 # Trim length for discordant reads (split reads are not trimmed) | |
306 discord_read_trim = #slurp | |
307 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.discord_read_trim.__str__ != "": | |
308 $refGenomeSource.defuse_param.discord_read_trim | |
309 #else | |
310 #try | |
311 $ref_dict['discord_read_trim'] | |
312 #except | |
313 50 | |
314 #end try | |
315 #end if | |
316 | |
317 # Filtering parameters | |
318 clustering_precision = #slurp | |
319 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.clustering_precision.__str__ != "" | |
320 $refGenomeSource.defuse_param.clustering_precision | |
321 #else | |
322 #try | |
323 $ref_dict['clustering_precision'] | |
324 #except | |
325 0.95 | |
326 #end try | |
327 #end if | |
328 span_count_threshold = #slurp | |
329 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.span_count_threshold.__str__ != "" | |
330 $refGenomeSource.defuse_param.span_count_threshold | |
331 #else | |
332 #try | |
333 $ref_dict['span_count_threshold'] | |
334 #except | |
335 5 | |
336 #end try | |
337 #end if | |
338 split_count_threshold = #slurp | |
339 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.split_count_threshold.__str__ != "" | |
340 $refGenomeSource.defuse_param.split_count_threshold | |
341 #else | |
342 #try | |
343 $ref_dict['split_count_threshold'] | |
344 #except | |
345 3 | |
346 #end try | |
347 #end if | |
348 percent_identity_threshold = #slurp | |
349 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.percent_identity_threshold.__str__ != "" | |
350 $refGenomeSource.defuse_param.percent_identity_threshold | |
351 #else | |
352 #try | |
353 $ref_dict['percent_identity_threshold'] | |
354 #except | |
355 0.90 | |
356 #end try | |
357 #end if | |
358 max_dist_pos = #slurp | |
359 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.max_dist_pos.__str__ != "" | |
360 $refGenomeSource.defuse_param.max_dist_pos | |
361 #else | |
362 #try | |
363 $ref_dict['max_dist_pos'] | |
364 #except | |
365 600 | |
366 #end try | |
367 #end if | |
368 num_dist_genes = #slurp | |
369 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.num_dist_genes.__str__ != "" | |
370 $refGenomeSource.defuse_param.num_dist_genes | |
371 #else | |
372 #try | |
373 $ref_dict['num_dist_genes'] | |
374 #except | |
375 500 | |
376 #end try | |
377 #end if | |
378 split_min_anchor = #slurp | |
379 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.split_min_anchor.__str__ != "" | |
380 $refGenomeSource.defuse_param.split_min_anchor | |
381 #else | |
382 #try | |
383 $ref_dict['split_min_anchor'] | |
384 #except | |
385 4 | |
386 #end try | |
387 #end if | |
388 max_concordant_ratio = #slurp | |
389 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.max_concordant_ratio.__str__ != "" | |
390 $refGenomeSource.defuse_param.max_concordant_ratio | |
391 #else | |
392 #try | |
393 $ref_dict['max_concordant_ratio'] | |
394 #except | |
395 0.1 | |
396 #end try | |
397 #end if | |
398 splice_bias = #slurp | |
399 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.splice_bias.__str__ != "" | |
400 $refGenomeSource.defuse_param.splice_bias | |
401 #else | |
402 #try | |
403 $ref_dict['splice_bias'] | |
404 #except | |
405 10 | |
406 #end try | |
407 #end if | |
408 denovo_assembly = #slurp | |
409 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.denovo_assembly.__str__ != "" | |
410 $refGenomeSource.defuse_param.denovo_assembly | |
411 #else | |
412 #try | |
413 $ref_dict['denovo_assembly'] | |
414 #except | |
415 no | |
416 #end try | |
417 #end if | |
418 probability_threshold = #slurp | |
419 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.probability_threshold.__str__ != "" | |
420 $refGenomeSource.defuse_param.probability_threshold | |
421 #else | |
422 #try | |
423 $ref_dict['probability_threshold'] | |
424 #except | |
425 0.50 | |
426 #end try | |
427 #end if | |
428 positive_controls = \$(data_directory)/controls.txt | |
429 | |
430 # Position density when calculating covariance | |
431 covariance_sampling_density = #slurp | |
432 #if $refGenomeSource.defuse_param.settings == "full" and $refGenomeSource.defuse_param.covariance_sampling_density.__str__ != "" | |
433 $refGenomeSource.defuse_param.covariance_sampling_density | |
434 #else | |
435 #try | |
436 $ref_dict['covariance_sampling_density'] | |
437 #except | |
438 0.01 | |
439 #end try | |
440 #end if | |
441 | |
442 | |
443 # Number of reads for each job in split | |
444 reads_per_job = 1000000 | |
445 | |
446 # Number of regions for each breakpoint sequence job in split | |
447 regions_per_job = 20 | |
448 | |
449 #raw | |
450 # If you have command line 'mail' and wish to be notified | |
451 # mailto = andrew.mcpherson@gmail.com | |
452 | |
453 # Remove temp files | |
454 remove_job_files = yes | |
455 remove_job_temp_files = yes | |
456 | |
457 # Converting to fastq | |
458 # Fastq converter config format 1 for reads stored in separate files for each end | |
459 # data_lane_rexex_N is a perl regex which stores the lane id in $1 | |
460 # data_end_regex_N is a perl regex which stores the end, 1 or 2, in $1 | |
461 # data_compress_regex_N is a perl regex which stores the compression extension in $1 | |
462 # data_convert_N is the associated conversion utility that takes data at stdin and outputs fastq at stdout | |
463 # Fastq converter config format 2 for reads stored in separate files for each end | |
464 # data_lane_regex_N is a perl regex which stores the lane id in $1 | |
465 # data_compress_regex_N is a perl regex which stores the compression extension in $1 | |
466 # data_end1_converter_N is the associated conversion utility that takes data at stdin and outputs fastq for end 1 at stdout | |
467 # data_end2_converter_N is the associated conversion utility that takes data at stdin and outputs fastq for end 2 at stdout | |
468 | |
469 data_lane_regex_1 = ^(.+)_[12]_export\.txt.*$ | |
470 data_end_regex_1 = ^.+_([12])_export\.txt.*$ | |
471 data_compress_regex_1 = ^.+_[12]_export\.txt(.*)$ | |
472 data_converter_1 = $(scripts_directory)/fq_all2std.pl export2std | |
473 | |
474 data_lane_regex_2 = ^(.+)_[12]_concat_qseq\.txt.*$ | |
475 data_end_regex_2 = ^.+_([12])_concat_qseq\.txt.*$ | |
476 data_compress_regex_2 = ^.+_[12]_concat_qseq\.txt(.*)$ | |
477 data_converter_2 = $(scripts_directory)/qseq2fastq.pl | |
478 | |
479 data_lane_regex_3 = ^(.+)\.bam.*$ | |
480 data_compress_regex_3 = ^.+\.bam(.*)$ | |
481 data_end1_converter_3 = samtools view - | filter_sam_mate.pl 1 | sam_to_fastq.pl | |
482 data_end2_converter_3 = samtools view - | filter_sam_mate.pl 2 | sam_to_fastq.pl | |
483 | |
484 data_lane_regex_4 = ^(.+).[12].fastq.*$ | |
485 data_end_regex_4 = ^.+.([12]).fastq.*$ | |
486 data_compress_regex_4 = ^.+.[12].fastq(.*)$ | |
487 data_converter_4 = cat | |
488 #end raw | |
489 | |
490 #end if | |
491 | |
492 </configfile> | |
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493 <configfile name="shscript"> |
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494 #!/bin/bash |
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495 ## define some things for cheetah proccessing |
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496 #set $ds = chr(36) |
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497 #set $amp = chr(38) |
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498 #set $gt = chr(62) |
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499 #set $lt = chr(60) |
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500 #set $echo_cmd = 'echo' |
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501 ## Find the defuse.pl in the galaxy tool path |
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502 #import Cheetah.FileUtils |
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503 ## declare a bash function for converting a results tsv into html with links to the get_reads output files |
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504 results2html() { |
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505 rlts=${ds}1 |
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506 rslt_name=`basename ${ds}rlts` |
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507 html=${ds}2 |
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508 echo '${lt}html${gt}${lt}head${gt}${lt}title${gt}Defuse '${ds}rslt_name'${lt}/title${gt}${lt}/head${gt}${lt}body${gt}' ${gt} ${ds}html |
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509 echo '${lt}h2${gt}Defuse '${ds}rslt_name'${lt}/h2${gt}${lt}table${gt}' ${gt}${gt} ${ds}html |
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510 if [ -z "${ds}3" ] |
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511 then |
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512 awk '${ds}1 ~ /cluster_id/{printf("${lt}tr${gt}");for (i = 1; i ${lt}= NF; i++) {printf("${lt}th${gt}%s${lt}/th${gt}", ${ds}i);}; printf("${lt}/tr${gt}\n");}\ |
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513 ${ds}1 ~ /[1-9][0-9]*/{printf("${lt}tr${gt}");for (i = 1; i ${lt}= NF; i++) {printf("${lt}td${gt}%s${lt}/td${gt}", ${ds}i);}; printf("${lt}/tr${gt}\n");}' ${ds}rlts ${gt}${gt} ${ds}html |
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514 echo '${lt}/table${gt}' ${gt}${gt} ${ds}html |
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515 echo '${lt}/body${gt}${lt}/html${gt}' ${gt}${gt} ${ds}html |
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516 else |
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517 export _EFP=${ds}3 |
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518 mkdir -p ${ds}_EFP |
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519 awk '${ds}1 ~ /cluster_id/{printf("${lt}tr${gt}");for (i = 1; i ${lt}= NF; i++) {printf("${lt}th${gt}%s${lt}/th${gt}", ${ds}i);}; printf("${lt}/tr${gt}\n");}\ |
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520 ${ds}1 ~ /[1-9][0-9]*/{fn="cluster_"${ds}1"_reads.txt"; \ |
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521 printf("${lt}tr${gt}${lt}td${gt}${lt}a href=\"%s\"${gt}%s${lt}/a${gt}${lt}/td${gt}",fn, ${ds}1);for (i = 2; i ${lt}= NF; i++) {printf("${lt}td${gt}%s${lt}/td${gt}", ${ds}i);}; printf("${lt}/tr${gt}\n");}' ${ds}rlts ${gt}${gt} ${ds}html |
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522 echo '${lt}/table${gt}' ${gt}${gt} ${ds}html |
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523 echo '${lt}/body${gt}${lt}/html${gt}' ${gt}${gt} ${ds}html |
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524 for i in `awk '${ds}1 ~ /[1-9][0-9]*/{print ${ds}1}' ${ds}rlts`; |
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525 do fn=cluster_${ds}{i}_reads.txt; |
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526 pn=${ds}_EFP/${ds}fn; |
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527 perl \${DEFUSE_PATH}/scripts/get_reads.pl -c $defuse_config -o output_dir -i ${ds}i ${gt} ${ds}pn; |
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528 done |
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529 fi |
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530 } |
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531 ## substitute pathnames into config file |
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532 if `grep __DEFUSE_PATH__ $defuse_config ${gt} /dev/null`;then sed -i'.tmp' "s#__DEFUSE_PATH__#\${DEFUSE_PATH}#" $defuse_config; fi |
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533 if `grep __SAMTOOLS_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} SAMTOOLS_BIN=`which samtools`;then sed -i'.tmp' "s#__SAMTOOLS_BIN__#\${SAMTOOLS_BIN}#" $defuse_config; fi |
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534 if `grep __BOWTIE_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} BOWTIE_BIN=`which bowtie`;then sed -i'.tmp' "s#__BOWTIE_BIN__#\${BOWTIE_BIN}#" $defuse_config; fi |
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535 if `grep __BOWTIE_BUILD_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} BOWTIE_BUILD_BIN=`which bowtie-build`;then sed -i'.tmp' "s#__BOWTIE_BUILD_BIN__#\${BOWTIE_BUILD_BIN}#" $defuse_config; fi |
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536 if `grep __BLAT_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} BLAT_BIN=`which blat`;then sed -i'.tmp' "s#__BLAT_BIN__#\${BLAT_BIN}#" $defuse_config; fi |
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537 if `grep __FATOTWOBIT_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} FATOTWOBIT_BIN=`which faToTwoBit`;then sed -i'.tmp' "s#__FATOTWOBIT_BIN__#\${FATOTWOBIT_BIN}#" $defuse_config; fi |
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538 if `grep __R_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} R_BIN=`which R`;then sed -i'.tmp' "s#__R_BIN__#\${R_BIN}#" $defuse_config; fi |
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539 if `grep __RSCRIPT_BIN__ $defuse_config ${gt} /dev/null` ${amp}${amp} RSCRIPT_BIN=`which Rscript`;then sed -i'.tmp' "s#__RSCRIPT_BIN__#\${RSCRIPT_BIN}#" $defuse_config; fi |
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540 |
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541 |
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542 ## copy config to output |
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543 cp $defuse_config $config_txt |
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544 ## make a data_dir and ln -s the input fastq |
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545 mkdir -p data_dir |
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546 ln -s $left_pairendreads data_dir/reads_1.fastq |
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547 ln -s $right_pairendreads data_dir/reads_2.fastq |
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548 ## ln to output_dir in from_work_dir |
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549 #if $defuse_out.__str__ != 'None': |
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550 mkdir -p $defuse_out.extra_files_path |
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551 ln -s $defuse_out.extra_files_path output_dir |
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552 #else |
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553 mkdir -p output_dir |
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554 #end if |
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555 ## run defuse.pl |
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556 perl \${DEFUSE_PATH}/scripts/defuse.pl -c $defuse_config -d data_dir -o output_dir -p 8 |
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557 ## copy primary results to output datasets |
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558 if [ -e output_dir/log/defuse.log ]; then cp output_dir/log/defuse.log $defuse_log; fi |
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559 if [ -e output_dir/results.tsv ]; then cp output_dir/results.tsv $results_tsv; fi |
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560 if [ -e output_dir/results.filtered.tsv ]; then cp output_dir/results.filtered.tsv $results_filtered_tsv; fi |
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561 if [ -e output_dir/results.classify.tsv ]; then cp output_dir/results.classify.tsv $results_classify_tsv; fi |
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562 ## create html with links for output_dir |
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563 #if $defuse_out.__str__ != 'None': |
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564 if [ -e $defuse_out ] |
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565 then |
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566 echo '${lt}html${gt}${lt}head${gt}${lt}title${gt}Defuse Output${lt}/title${gt}${lt}/head${gt}${lt}body${gt}' ${gt} $defuse_out |
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567 echo '${lt}h2${gt}Defuse Output Files${lt}/h2${gt}${lt}ul${gt}' ${gt}${gt} $defuse_out |
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568 pushd $defuse_out.extra_files_path |
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569 for f in `find -L . -maxdepth 1 -type f`; |
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570 do fn=`basename ${ds}f`; echo '${lt}li${gt}${lt}a href="'${ds}fn'"${gt}'${ds}fn'${lt}/a${gt}${lt}/li${gt}' ${gt}${gt} $defuse_out; |
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571 done |
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572 popd |
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573 echo '${lt}/ul${gt}' ${gt}${gt} $defuse_out |
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574 echo '${lt}/body${gt}${lt}/html${gt}' ${gt}${gt} $defuse_out |
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575 fi |
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576 #end if |
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577 ## run get_reads.pl on each cluster |
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578 #if $fusion_reads.__str__ != 'None': |
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579 if [ -e output_dir/results.filtered.tsv -a -e $fusion_reads ] |
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580 then |
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581 mkdir -p $fusion_reads.extra_files_path |
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582 results2html output_dir/results.filtered.tsv $fusion_reads $fusion_reads.extra_files_path |
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583 fi |
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584 #end if |
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585 </configfile> |
1 | 586 </configfiles> |
587 <outputs> | |
588 <data format="txt" name="config_txt" label="${tool.name} on ${on_string}: config.txt"/> | |
3
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589 <data format="txt" name="defuse_log" label="${tool.name} on ${on_string}: defuse.log" /> |
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590 <data format="html" name="defuse_out" label="${tool.name} on ${on_string}: defuse_output"> |
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591 <filter>keep_output == True</filter> |
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592 </data> |
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593 <data format="html" name="fusion_reads" label="${tool.name} on ${on_string}: fusion_reads"> |
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594 <filter>do_get_reads == True</filter> |
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595 </data> |
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596 <data format="tabular" name="results_tsv" label="${tool.name} on ${on_string}: results.tsv" /> |
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597 <data format="tabular" name="results_filtered_tsv" label="${tool.name} on ${on_string}: results.filtered.tsv" /> |
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598 <data format="tabular" name="results_classify_tsv" label="${tool.name} on ${on_string}: results.classify.tsv" /> |
1 | 599 </outputs> |
600 <tests> | |
601 </tests> | |
602 <help> | |
603 **DeFuse** | |
604 | |
605 DeFuse_ is a software package for gene fusion discovery using RNA-Seq data. The software uses clusters of discordant paired end alignments to inform a split read alignment analysis for finding fusion boundaries. The software also employs a number of heuristic filters in an attempt to reduce the number of false positives and produces a fully annotated output for each predicted fusion. | |
606 | |
607 Journal reference: http://www.ploscompbiol.org/article/info%3Adoi%2F10.1371%2Fjournal.pcbi.1001138 | |
608 | |
609 .. _DeFuse: http://sourceforge.net/apps/mediawiki/defuse/index.php?title=Main_Page | |
610 | |
611 ------ | |
612 | |
613 **Inputs** | |
614 | |
615 DeFuse requires 2 fastq files for paried reads, one with the left mate of the paired reads, and a second fastq with the the right mate of the paired reads (**with reads in the same order as in the first fastq dataset**). | |
616 | |
617 If your fastq files have reads in different orders or include unpaired reads, you can preprocess them with **FASTQ interlacer** to create a single interlaced fastq dataset with only the paired reads and input that to **FASTQ de-interlacer** to separate the reads into a left fastq and right fastq. | |
618 | |
619 DeFuse uses a Reference Dataset to search for gene fusions. The Reference Dataset is generated from the following sources in DeFuse_Version_0.4_: | |
620 - genome_fasta from Ensembl | |
621 - gene_models from Ensembl | |
622 - repeats_filename from UCSC RepeatMasker rmsk.txt | |
623 - est_fasta from UCSC | |
624 - est_alignments from UCSC intronEst.txt | |
625 - unigene_fasta from NCBI | |
626 | |
627 .. _DeFuse_Version_0.4: http://sourceforge.net/apps/mediawiki/defuse/index.php?title=DeFuse_Version_0.4.2 | |
628 | |
629 ------ | |
630 | |
631 **Outputs** | |
632 | |
633 The galaxy history will contain 5 outputs: the config.txt file that provides DeFuse with its parameters, the defuse.log which details what DeFuse has done and can be useful in determining any errors, and the 3 results files that defuse generates. | |
634 | |
635 DeFuse generates 3 results files: results.txt, results.filtered.txt, and results.classify.txt. All three files have the same format, though results.classify.txt has a probability column from the application of the classifier to results.txt, and results.filtered.txt has been filtered according to the threshold probability as set in config.txt. | |
636 | |
637 The file format is tab delimited with one prediction per line, and the following fields per prediction (not necessarily in this order): | |
638 | |
639 - **Identification** | |
640 - cluster_id : random identifier assigned to each prediction | |
641 - library_name : library name given on the command line of defuse | |
642 - gene1 : ensembl id of gene 1 | |
643 - gene2 : ensembl id of gene 2 | |
644 - gene_name1 : name of gene 1 | |
645 - gene_name2 : name of gene 2 | |
646 - **Evidence** | |
647 - break_predict : breakpoint prediction method, denovo or splitr, that is considered most reliable | |
648 - concordant_ratio : proportion of spanning reads considered concordant by blat | |
649 - denovo_min_count : minimum kmer count across denovo assembled sequence | |
650 - denovo_sequence : fusion sequence predicted by debruijn based denovo sequence assembly | |
651 - denovo_span_pvalue : p-value, lower values are evidence the prediction is a false positive | |
652 - gene_align_strand1 : alignment strand for spanning read alignments to gene 1 | |
653 - gene_align_strand2 : alignment strand for spanning read alignments to gene 2 | |
654 - min_map_count : minimum of the number of genomic mappings for each spanning read | |
655 - max_map_count : maximum of the number of genomic mappings for each spanning read | |
656 - mean_map_count : average of the number of genomic mappings for each spanning read | |
657 - num_multi_map : number of spanning reads that map to more than one genomic location | |
658 - span_count : number of spanning reads supporting the fusion | |
659 - span_coverage1 : coverage of spanning reads aligned to gene 1 as a proportion of expected coverage | |
660 - span_coverage2 : coverage of spanning reads aligned to gene 2 as a proportion of expected coverage | |
661 - span_coverage_min : minimum of span_coverage1 and span_coverage2 | |
662 - span_coverage_max : maximum of span_coverage1 and span_coverage2 | |
663 - splitr_count : number of split reads supporting the prediction | |
664 - splitr_min_pvalue : p-value, lower values are evidence the prediction is a false positive | |
665 - splitr_pos_pvalue : p-value, lower values are evidence the prediction is a false positive | |
666 - splitr_sequence : fusion sequence predicted by split reads | |
667 - splitr_span_pvalue : p-value, lower values are evidence the prediction is a false positive | |
668 - **Annotation** | |
669 - adjacent : fusion between adjacent genes | |
670 - altsplice : fusion likely the product of alternative splicing between adjacent genes | |
671 - break_adj_entropy1 : di-nucleotide entropy of the 40 nucleotides adjacent to the fusion splice in gene 1 | |
672 - break_adj_entropy2 : di-nucleotide entropy of the 40 nucleotides adjacent to the fusion splice in gene 2 | |
673 - break_adj_entropy_min : minimum of break_adj_entropy1 and break_adj_entropy2 | |
674 - breakpoint_homology : number of nucleotides at the fusion splice that align equally well to gene 1 or gene 2 | |
675 - breakseqs_estislands_percident : maximum percent identity of fusion sequence alignments to est islands | |
676 - cdna_breakseqs_percident : maximum percent identity of fusion sequence alignments to cdna | |
677 - deletion : fusion produced by a genomic deletion | |
678 - est_breakseqs_percident : maximum percent identity of fusion sequence alignments to est | |
679 - eversion : fusion produced by a genomic eversion | |
680 - exonboundaries : fusion splice at exon boundaries | |
681 - expression1 : expression of gene 1 as number of concordant pairs aligned to exons | |
682 - expression2 : expression of gene 2 as number of concordant pairs aligned to exons | |
683 - gene_chromosome1 : chromosome of gene 1 | |
684 - gene_chromosome2 : chromosome of gene 2 | |
685 - gene_end1 : end position for gene 1 | |
686 - gene_end2 : end position for gene 2 | |
687 - gene_location1 : location of breakpoint in gene 1 | |
688 - gene_location2 : location of breakpoint in gene 2 | |
689 - gene_start1 : start of gene 1 | |
690 - gene_start2 : start of gene 2 | |
691 - gene_strand1 : strand of gene 1 | |
692 - gene_strand2 : strand of gene 2 | |
693 - genome_breakseqs_percident : maximum percent identity of fusion sequence alignments to genome | |
694 - genomic_break_pos1 : genomic position in gene 1 of fusion splice / breakpoint | |
695 - genomic_break_pos2 : genomic position in gene 2 of fusion splice / breakpoint | |
696 - genomic_strand1 : genomic strand in gene 1 of fusion splice / breakpoint, retained sequence upstream on this strand, breakpoint is downstream | |
697 - genomic_strand2 : genomic strand in gene 2 of fusion splice / breakpoint, retained sequence upstream on this strand, breakpoint is downstream | |
698 - interchromosomal : fusion produced by an interchromosomal translocation | |
699 - interrupted_index1 : ratio of coverage before and after the fusion splice / breakpoint in gene 1 | |
700 - interrupted_index2 : ratio of coverage before and after the fusion splice / breakpoint in gene 2 | |
701 - inversion : fusion produced by genomic inversion | |
702 - orf : fusion combines genes in a way that preserves a reading frame | |
703 - probability : probability produced by classification using adaboost and example positives/negatives (only given in results.classified.txt) | |
704 - read_through : fusion involving adjacent potentially resulting from co-transcription rather than genome rearrangement | |
705 - repeat_proportion1 : proportion of the spanning reads in gene 1 that span a repeat region | |
706 - repeat_proportion2 : proportion of the spanning reads in gene 2 that span a repeat region | |
707 - max_repeat_proportion : max of repeat_proportion1 and repeat_proportion2 | |
708 - splice_score : number of nucleotides similar to GTAG at fusion splice | |
709 - num_splice_variants : number of potential splice variants for this gene pair | |
710 - splicing_index1 : number of concordant pairs in gene 1 spanning the fusion splice / breakpoint, divided by number of spanning reads supporting the fusion with gene 2 | |
711 - splicing_index2 : number of concordant pairs in gene 2 spanning the fusion splice / breakpoint, divided by number of spanning reads supporting the fusion with gene 1 | |
712 | |
713 | |
714 **Example** | |
715 | |
716 results.tsv:: | |
717 | |
718 cluster_id splitr_sequence splitr_count splitr_span_pvalue splitr_pos_pvalue splitr_min_pvalue adjacent altsplice break_adj_entropy1 break_adj_entropy2 break_adj_entropy_min break_predict breakpoint_homology breakseqs_estislands_percident cdna_breakseqs_percident concordant_ratio deletion est_breakseqs_percident eversion exonboundaries expression1 expression2 gene1 gene2 gene_align_strand1 gene_align_strand2 gene_chromosome1 gene_chromosome2 gene_end1 gene_end2 gene_location1 gene_location2 gene_name1 gene_name2 gene_start1 gene_start2 gene_strand1 gene_strand2 genome_breakseqs_percident genomic_break_pos1 genomic_break_pos2 genomic_strand1 genomic_strand2 interchromosomal interrupted_index1 interrupted_index2 inversion library_name max_map_count max_repeat_proportion mean_map_count min_map_count num_multi_map num_splice_variants orf read_through repeat_proportion1 repeat_proportion2 span_count span_coverage1 span_coverage2 span_coverage_max span_coverage_min splice_score splicing_index1 splicing_index2 | |
719 1169 GCTTACTGTATGCCAGGCCCCAGAGGGGCAACCACCCTCTAAAGAGAGCGGCTCCTGCCTCCCAGAAAGCTCACAGACTGTGGGAGGGAAACAGGCAGCAGGTGAAGATGCCAAATGCCAGGATATCTGCCCTGTCCTTGCTTGATGCAGCTGCTGGCTCCCACGTTCTCCCCAGAATCCCCTCACACTCCTGCTGTTTTCTCTGCAGGTTGGCAGAGCCCCATGAGGGCAGGGCAGCCACTTTGTTCTTGGGCGGCAAACCTCCCTGGGCGGCACGGAAACCACGGTGAGAAGGGGGCAGGTCGGGCACGTGCAGGGACCACGCTGCAGG|TGTACCCAACAGCTCCGAAGAGACAGCGACCATCGAGAACGGGCCATGATGACGATGGCGGTTTTGTCGAAAAGAAAAGGGGGAAATGTGGGGAAAAGCAAGAGAGATCAGATTGTTACTGTGTCTGTGTAGAAAGAAGTAGACATGGGAGACTCCATTTTGTTCTGTACTAAGAAAAATTCTTCTGCCTTGAGATTCGGTGACCCCACCCCCAACCCCGTGCTCTCTGAAACATGTGCTGTGTCCACTCAGGGTTGAATGGATTAAGGGCGGTGCGAGACGTGCTTT 2 0.000436307890680442 0.110748295953850 0.0880671602973091 N Y 3.19872427442695 3.48337348351473 3.19872427442695 splitr 0 0 0 0 Y 0 N N 0 0 ENSG00000105549 ENSG00000213753 + - 19 19 376013 59111168 intron upstream THEG AC016629.2 361750 59084870 - + 0 375099 386594 + - N 8.34107429512245 - N output_dir 82 0.677852348993289 40.6666666666667 1 11 1 N N 0.361271676300578 0.677852348993289 12 0.758602776578432 0.569678713445872 0.758602776578432 0.569678713445872 2 0.416666666666667 - | |
720 3596 TGGGGGTTGAGGCTTCTGTTCCCAGGTTCCATGACCTCAGAGGTGGCTGGTGAGGTTATGACCTTTGCCCTCCAGCCCTGGCTTAAAACCTCAGCCCTAGGACCTGGTTAAAGGAAGGGGAGATGGAGCTTTGCCCCGACCCCCCCCCGTTCCCCTCACCTGTCAGCCCGAGCTGGGCCAGGGCCCCTAGGTGGGGAACTGGGCCGGGGGGCGGGCACAAGCGGAGGTGGTGCCCCCAAAAGGGCTCCCGGTGGGGTCTTGCTGAGAAGGTGAGGGGTTCCCGGGGCCGCAGCAGGTGGTGGTGGAGGAGCCAAGCGGCTGTAGAGCAAGGGGTGAGCAGGTTCCAGACCGTAGAGGCGGGCAGCGGCCACGGCCCCGGGTCCAGTTAGCTCCTCACCCGCCTCATAGAAGCGGGGTGGCCTTGCCAGGCGTGGGGGTGCTGCC|TTCCTTGGATGTGGTAGCCGTTTCTCAGGCTCCCTCTCCGGAATCGAACCCTGATTCCCCGTCACCCGTGGTCACCATGGTAGGCACGGCGACTACCATCGAAAGTTGATAGGGCAGACGTTCGAATGGGTCGTCGCCGCCACGGGGGGCGTGCGATCAGCCCGAGGTTATCTAGAGTCACCAAAGCCGCCGGCGCCCGCCCCCCGGCCGGGGCCGGAGAGGGGCTGACCGGGTTGGTTTTGATCTGATAAATGCACGCATCCCCCCCGCGAAGGGGGTCAGCGCCCGTCGGCATGTATTAGCTCTAGAATTACCACAGTTATCCAAGTAGGAGAGGAGCGAGCGACCAAAGGAACCATAACTGATTTAATGAGCCATTCGCAGTTTCACTGTACCGGCCGTGCGTACTTAGACATGCATGGCTTAATCTTTGAGACAAGCATATGCTACTGGCAGG 250 7.00711162298275e-72 0.00912124762512338 0.00684237452309549 N N 3.31745197152461 3.47233119514066 3.31745197152461 splitr 7 0.0157657657657656 0 0 N 0.0135135135135136 N N 0 0 ENSG00000156860 ENSG00000212932 - + 16 21 30682131 48111157 coding upstream FBRS RPL23AP4 30670289 48110676 + + 0.0157657657657656 30680678 9827473 - + Y - - N output_dir 2 1 1.11111111111111 1 1 1 N N 0 1 9 0.325530693397641 0.296465452915709 0.325530693397641 0.296465452915709 2 - - | |
721 | |
722 </help> | |
723 </tool> |