RNA-Seq Analysis Service¶
Overview¶
The RNA-Seq Analysis Service provides services for aligning, assembling, and testing differential expression on RNA-Seq data. The service provides two recipes for processing RNA-Seq data: 1) Tuxedo, based on the tuxedo suite of tools (i.e., Bowtie, Cufflinks, Cuffdiff); and 2) and HISAT2 for host (human, etc.) reference genomes. The service provides SAM/BAM output for alignment, tab delimited files profiling expression levels, and differential expression test results between conditions. A tutorial for using the RNA-Seq Analysis Service is available here.
The RNA-Seq Service can be accessed from the Services Menu at the top of the BV-BRC website page and via the Command Line Interface (CLI).
See also¶
Using the RNA-Seq Analysis Service¶
The RNA-Seq Analysis submenu option under the Services main menu (Transcriptomics category) opens the RNA-Seq Analysis input form (shown below). Note: You must be logged into BV-BRC to use this service.
Options¶
Parameters¶
Strategy¶
This parameter governs the software used to align, assemble, quantify, and compare reads from different samples.
Tuxedo: Runs the tuxedo strategy using Bowtie2, Cufflinks, and CuffDiff to align, assemble, and compare samples respectively. This is a similar strategy as used by RNA-Rocket.
Host HISAT2: Runs HISAT2 for alignment against the selected host and then uses the remainder of the Tuxedo strategy using Cufflinks and CuffDiff to assemble and compare samples respectively.
Target Genome¶
The target genome to align the reads against. If this genome is a private genome, the search can be narrowed by clicking on the filter icon under the words Target Genome.
Output Folder¶
The workspace folder where results will be placed.
Output Name¶
Name used to uniquely identify results.
Paired read library¶
Read File 1 & 2¶
Many paired read libraries are given as file pairs, with each file containing half of each read pair. Paired read files are expected to be sorted such that each read in a pair occurs in the same Nth position as its mate in their respective files. These files are specified as READ FILE 1 and READ FILE 2. For a given file pair, the selection of which file is READ 1 and which is READ 2 does not matter. Click the arrow button (->) to move the files into the Selected Libraries to treat as a single RNA-Seq analysis. See “Selected Libraries” description below.
Condition¶
Dropdown list for selecting conditions to associate with the read files. Note: The conditions are defined by the user in the Groups/Conditions section of the form (see below). The group/condition specified will be used to determine contrasts in the differential expression portion of the analysis. Each group will be compared to every other group in all vs. all fashion. Reads assigned to the same group will be used as replicates.
Groups/Conditions¶
Turning on Groups/Conditions also turns on differential expression analysis. In this panel the user has the ability to specify conditions that can be assigned to read libraries. When this option is enabled each read library moved to the “Selected libraries” panel must have a group designation. Read libraries assigned to different groups will be compared for differential expression in all vs. all fashion. Two or more read libraries marked with the same group will be regarded as replicates.
Selected libraries¶
Read files placed here will contribute to a single RNA-Seq analysis. If the Groups/Conditions option is turned on, read files placed into this table under the same group will be considered replicates.
Contrasts¶
Contrasts specify which pairs of conditions to compare in differential expression analysis. The RockHopper strategy performs all vs all contrats by default, hence, no cotrasts need to be specified.
Output Results¶
The RNA-Seq Analysis Service generates several files that are deposited in the Private Workspace in the designated Output Folder. These include
diffexp - A Differential Expression Object created to represent a log-ratio comparison of expression values of genes between conditions as specified in the contrasts section of the RNA-Seq interface.
.bam - A binary version of a SAM file that describes the alignment andalignment quality of each read in a sample file
.bai - A binary index alignment file gives the byte range offset of particular sequence regions in the BAM file. This can be used to selectively load information for a particular region out of a BAM file.
.samstat.html - An HTML report summarizing the alignment quality of reads for a given sample. This includes MAPQ quality scores: MAPQ: MAPping Quality. It equals −10 log10 Pr{mapping position is wrong}, rounded to the nearest integer. A value 255 indicates that the mapping quality is not available.
.fastqc.html - An HTML report summarizing the Phred read base call quality scores in a read sample file. If base call quality is poor then alignments are likely to be as well.
genes.fpkm_tracking - This file contains the estimated gene-level expression values in the generic FPKM Tracking Format. Note, however, that as there is only one sample, the “q” format is not used.
isoforms.fpkm_tracking - This file contains the estimated isoform-level expression values in the generic FPKM Tracking Format. Note, however, that as there is only one sample, the “q” format is not used.
skipped.gtf - Dictated by -max-bundle-frags option, which sets the maximum number of fragments a locus may have before being skipped. Skipped loci are listed in skipped.gtf. Default: 1000000
transcripts.gtf - This GTF file contains Cufflinks’ assembled isoforms. The first 7 columns are standard GTF, and the last column contains attributes, some of which are also standardized (“gene_id”, and “transcript_id”). There one GTF record per row, and each record represents either a transcript or an exon within a transcript.
cds.diff - This tab-delimited file lists, for each gene, the amount of overloading detected among its coding sequences, i.e., how much differential CDS output exists between samples. Only genes producing two or more distinct CDS (i.e., multi-protein genes) are listed here.
cds_exp.diff - Coding sequence differential expression. Tests differences in the summed FPKM of transcripts sharing each p_id independent of tss_id.
gene_exp.diff - Gene-level differential expression. Tests differences in the summed FPKM of transcripts sharing each gene_id
gene_exp.gmx - This file, generated by BV-BRC, describes the different contrast comparisons between conditions in terms of log ratios.
promoters.diff - This tab-delimited file lists, for each gene, the amount of overloading detected among its primary transcripts, i.e., how much differential promoter use exists between samples. Only genes producing two or more distinct primary transcripts (i.e., multi-promoter genes) are listed here.
splicing.diff - This-tab delimited file lists, for each primary transcript, the amount of isoform switching detected among its isoforms, i.e., how much differential splicing exists between isoforms processed from a single primary transcript. Only primary transcripts from which two or more isoforms are spliced are listed in this file.
tss_group_exp.diff - Primary transcript differential expression. Tests differences in the summed FPKM of transcripts sharing each tss_id
tss_id - The ID of this transcript’s inferred start site as assigned by Cufflinks. Determines which primary transcript this processed transcript is believed to come from. Cuffcompare appends this attribute to every transcript reported in the .combined.gtf file.
p_id - The ID of the coding sequence this transcript contains as assigned by Cufflinks. This attribute is attached by Cuffcompare to the .combined.gtf records only when it is run with a reference annotation that include CDS records. Further, differential CDS analysis is only performed when all isoforms of a gene have p_id attributes, because neither Cufflinks nor Cuffcompare attempt to assign an open reading frame to transcripts.
Clicking the Browser icon at the top left displays the Genome Browser with the reference genome loaded.
RNA-seq analysis result tracks are available to add to the browser by clicking the associated track options in the upper left corner. Transcripts are displayed in gold with orientation arrows, and individual reads with the colors indicative of the orientation (blue is forward, red is reverse).
References¶
Kim, D., et al., TopHat2: accurate alignment of transcriptomes in the presence of insertions, deletions and gene fusions. Genome Biol, 2013. 14(4): p. R36.
Kim, D., B. Langmead, and S.L. Salzberg, HISAT: a fast spliced aligner with low memory requirements. Nat Methods, 2015. 12(4): p. 357-60.
McClure, R., et al., Computational analysis of bacterial RNA-Seq data. Nucleic Acids Res, 2013. 41(14): p. e140.