Trinity
Contents
- 1 Introduction
- 2 Version 2.3.2, full help file
- 2.1 Obligatory options
- 2.2 Misc
- 2.3 Inchworm and K-mer counting-related options
- 2.4 Chrysalis-related options
- 2.5 Butterfly-related options
- 2.6 Butterfly Java and parallel execution settings
- 2.7 Quality Trimming Options
- 2.8 In silico Read Normalization Options
- 2.9 Genome-guided de novo assembly
- 2.10 Trinity phase 2 (parallel assembly of read clusters) Options
- 2.11 A typical Trinity command might be
Introduction
The widely established tool for transcriptome assembly. It consists of three main components (which is how it got its name) although a fourth one, Jellyfish, is also included in the following list because it's important, thogh not written by the Trinity team:
- Jelly fish
- Inchworm
- Chrysalis
- Butterfly
This list follws the sequence of operations.
Version 2.3.2, full help file
This is an editted version. With the module loaded, type
Trinity --show-full-usage-info
For the raw version.
Obligatory options
- --seqType <string>, what type of reads the inputs are: ('fa' or 'fq')
- --max_memory <string>, suggested max memory to use by Trinity where limiting can be enabled. (jellyfish, sorting, etc) in Gb of RAM, ie. '--max_memory 10G'
- --left <string> :left reads, one or more file names (separated by commas, no spaces)
- --right <string> :right reads, one or more file names (separated by commas, no spaces)
- --single <string> (obviously neither obligatory nor necessary if paired reads are being input). Ssingle reads, one or more file names, comma-delimited (note, if single file contains pairs, can use flag: --run_as_paired )
Or,
- --samples_file <string> tab-delimited text file indicating biological replicate relationships. For example:
cond_A cond_A_rep1 A_rep1_left.fq A_rep1_right.fq cond_A cond_A_rep2 A_rep2_left.fq A_rep2_right.fq cond_B cond_B_rep1 B_rep1_left.fq B_rep1_right.fq cond_B cond_B_rep2 B_rep2_left.fq B_rep2_right.fq
(if single-end instead of paired-end, then leave the 4th column above empty)
Misc
- --SS_lib_type <string> Strand-specific RNA-Seq read orientation. If paired: RF or FR. If single: F or R. For dUTP method = RF.
- --CPU <int>, number of CPUs to use, default: 2
- --min_contig_length <int>, minimum assembled contig length to report (default=200)
- --long_reads <string>, fasta file containing error-corrected or circular consensus (CCS) pac bio reads (Note: experimental parameter, this functionality continues to be under development)
- --genome_guided_bam <string>, genome guided mode, provide path to coordinate-sorted bam file (see genome-guided param section below)
- --jaccard_clip, set if you have paired reads and you expect high gene density with UTR overlap (use FASTQ input file format for reads). Note that this is an expensive operation, so avoid using it unless necessary due to finding excessive fusion transcripts without it.)
- --trimmomatic, run Trimmomatic to quality trim reads (see option --quality_trimming_params).
- --no_normalize_reads, a major change in version 2.3.2, because normalization is now the default. Defaults to max. read coverage of 50. See option --normalize_max_read_cov' below.
- --no_distributed_trinity_exec, do not run Trinity phase 2 (assembly of partitioned reads), and stop after generating command list.
- --output <string>, name of directory for output (will be created if it doesn't already exist). Default is your current working directory
- --full_cleanup, only retain the Trinity fasta file, rename as ${output_dir}.Trinity.fasta
- --cite, show the Trinity literature citation
- --verbose, provide additional job status info during the run.
- --version, reports Trinity version (Trinity-v2.3.2) and exits.
- --show_full_usage_info, show more options for running Trinity (expert usage).
- --KMER_SIZE <int>, kmer length to use (default: 25) max=32
- --prep, only prepare files (high I/O usage) and stop before kmer counting.
- --no_cleanup, retain all intermediate input files.
- --no_version_check, dont run a network check to determine if software updates are available.
- --min_kmer_cov <int>, min count for K-mers to be assembled by Inchworm (default: 1)
- --inchworm_cpu <int>, number of CPUs to use for Inchworm (only!), default is min(6, --CPU option)
- --no_run_inchworm, stop after running jellyfish, before inchworm. (phase 1, read clustering only)
- --max_reads_per_graph <int> :maximum number of reads to anchor within
- a single graph (default: 200000)
- --min_glue <int> :min number of reads needed to glue two inchworm contigs
- together. (default: 2)
- --no_bowtie :dont run bowtie to use pair info in chrysalis clustering.
- --no_run_chrysalis :stop after running inchworm, before chrysalis. (phase 1, read clustering only)
- --bfly_opts <string>, additional parameters to pass through to butterfly see butterfly options:
java -jar Butterfly.jar
(note: only for expert or experimental use. Commonly used parameters are exposed through this Trinity menu here).
== Butterfly read-pair grouping settings (used to define 'pair paths'):
- --group_pairs_distance <int> :maximum length expected between fragment pairs (default: 500)
- (reads outside this distance are treated as single-end)
- Butterfly default reconstruction mode settings. (no CuffFly or PasaFly custom settings are currently available).
- --path_reinforcement_distance <int> :minimum overlap of reads with growing transcript
- path (default: PE: 75, SE: 25)
- Set to 1 for the most lenient path extension requirements.
- Butterfly transcript reduction settings:
- --no_path_merging : all final transcript candidates are output (including SNP variations, however, some SNPs may be unphased)
- By default, alternative transcript candidates are merged (in reality, discarded) if they are found to be too similar, according to the following logic:
- (identity=(numberOfMatches/shorterLen) > 95.0% or if we have <= 2 mismatches) and if we have internal gap lengths <= 10
- with parameters as:
- --min_per_id_same_path <int> default: 98 min percent identity for two paths to be merged into single paths
- --max_diffs_same_path <int> default: 2 max allowed differences encountered between path sequences to combine them
- --max_internal_gap_same_path <int> default: 10 maximum number of internal consecutive gap characters allowed for paths to be merged into single paths.
- If, in a comparison between two alternative transcripts, they are found too similar, the transcript with the greatest cumulative
- compatible read (pair-path) support is retained, and the other is discarded.
Butterfly Java and parallel execution settings
- --bflyHeapSpaceMax <string>, java max heap space setting for butterfly (default: 4G this yields command
java -Xmx4G -jar Butterfly.jar ... $bfly_opts
- --bflyHeapSpaceInit <string>, java initial hap space settings for butterfly (default: 1G) this yields command
java -Xms1G -jar Butterfly.jar ... $bfly_opts
- --bflyGCThreads <int>, threads for garbage collection (default: 2))
- --bflyCPU <int>, CPUs to use (default will be normal number of CPUs; e.g., 2)
- --bflyCalculateCPU, Calculate CPUs based on 80% of max_memory divided by maxbflyHeapSpaceMax
- --bfly_jar <string>, /path/to/Butterfly.jar, otherwise default Trinity-installed version is used.
Quality Trimming Options
- --quality_trimming_params <string> defaults to: "ILLUMINACLIP:/usr/local/Modules/modulefiles/tools/trinity/2.3.2/trinity-plugins/Trimmomatic/adapters/TruSeq3-PE.fa:2:30:10 SLIDINGWINDOW:4:5 LEADING:5 TRAILING:5 MINLEN:25"
In silico Read Normalization Options
- --normalize_max_read_cov <int> defaults to 50
- --normalize_by_read_set run normalization separate for each pair of fastq files,
- then one final normalization that combines the individual normalized reads.
- Consider using this if RAM limitations are a consideration.
Genome-guided de novo assembly
- * required:
- --genome_guided_max_intron <int> :maximum allowed intron length (also maximum fragment span on genome)
- * optional:
- --genome_guided_min_coverage <int> :minimum read coverage for identifying and expressed region of the genome. (default: 1)
- --genome_guided_min_reads_per_partition <int> :default min of 10 reads per partition
Trinity phase 2 (parallel assembly of read clusters) Options
- --grid_exec <string>, your command-line utility for submitting jobs to the grid. This should be a command line tool that accepts a single parameter:
${your_submission_tool} /path/to/file/containing/commands.txt and this submission tool should exit(0) upon successful completion of all commands.
- --grid_node_CPU <int> number of threads for each parallel process to leverage. (default: 1)
- --grid_node_max_memory <string> max memory targeted for each grid node. (default: 1G)
- The --grid_node_CPU and --grid_node_max_memory are applied as
- the --CPU and --max_memory parameters for the Trinity jobs run in
- Trinity Phase 2 (assembly of read clusters)
A typical Trinity command might be
Trinity --seqType fq --max_memory 50G --left reads_1.fq --right reads_2.fq --CPU 6
and for Genome-guided Trinity:
Trinity --genome_guided_bam rnaseq_alignments.csorted.bam --max_memory 50G --genome_guided_max_intron 10000 --CPU 6
- see:
/usr/local/Modules/modulefiles/tools/trinity/2.3.2/sample_data/test_Trinity_Assembly/ for sample data and 'runMe.sh' for example Trinity execution