The ORFhunteR package is R and C++ library for an automatic determination and annotation of open reading frames (ORFs) in a large set of RNA molecules. It efficiently implements the machine learning model based on vectorization of nucleotide sequences and the random forest classification algorithm. The ORFhunteR package consists of a set of functions written in the R language in conjunction with C++. The efficiency of the package was confirmed by the examples of the analysis of RNA molecules from the NCBI RefSeq and Ensembl databases. The package can be used in basic and applied biomedical research related to the study of the transcriptome of normal as well as pathological (for example, cancerous) human cells.
ORFhunteR 1.12.0
This document describes the usage of the functions integrated in the package and is meant to be a reference document for the end user.
The ORFhunteR package is considered stable and will undergo few changes from now on. Please, report potential bugs and incompatibilities to bioinformatics.rfct.bio.bsu@gmail.com.
The usage of the package functions for an automatic determination and annotation of open reading frames (ORFs) is shown for an example set of 50 mRNA molecules loaded from the Ensembl. The path to the data set trans_sequences.fasta
is available as
trans <- system.file("extdata", "Set.trans_sequences.fasta",
package = "ORFhunteR")
Load the package with the following command:
if (!requireNamespace("BiocManager", quietly = TRUE)) {
install.packages("BiocManager")
}
BiocManager::install("ORFhunteR")
library('ORFhunteR')
#> Loading required package: Biostrings
#> Loading required package: BiocGenerics
#>
#> Attaching package: 'BiocGenerics'
#> The following objects are masked from 'package:stats':
#>
#> IQR, mad, sd, var, xtabs
#> The following objects are masked from 'package:base':
#>
#> anyDuplicated, aperm, append, as.data.frame, basename, cbind,
#> colnames, dirname, do.call, duplicated, eval, evalq, Filter, Find,
#> get, grep, grepl, intersect, is.unsorted, lapply, Map, mapply,
#> match, mget, order, paste, pmax, pmax.int, pmin, pmin.int,
#> Position, rank, rbind, Reduce, rownames, sapply, setdiff, table,
#> tapply, union, unique, unsplit, which.max, which.min
#> Loading required package: S4Vectors
#> Loading required package: stats4
#>
#> Attaching package: 'S4Vectors'
#> The following object is masked from 'package:utils':
#>
#> findMatches
#> The following objects are masked from 'package:base':
#>
#> expand.grid, I, unname
#> Loading required package: IRanges
#> Loading required package: XVector
#> Loading required package: GenomeInfoDb
#>
#> Attaching package: 'Biostrings'
#> The following object is masked from 'package:base':
#>
#> strsplit
#> Loading required package: rtracklayer
#> Loading required package: GenomicRanges
#> Loading required package: Peptides
The most important data sets are available with package as an external data. Furthermore, a number of additional data used in this vignette can be downloaded from our SST Center server.
You can load the data file of the mRNA molecules with the following command:
seq.set <- loadTrExper(tr = trans)
where the function argument tr
is a character string giving the name of file with transcripts of interest. Allowed file formats are fasta
or fa
. Alternative formats are gtf
or gff
. With gtf
or gff
formats, additional argument genome should be specified. This argument gives the name of pre-installed BSgenome data package with full genome sequences. Default value is BSgenome.Hsapiens.UCSC.hg38
.
Irrespective used format of input file, the function loadTrExper
returns a list of loaded transcript sequences. Each element of this list is character string of nucleotides sequence.
All possible in-frame ORF candidates in a sequence of interest can be determined by function findORFs
:
x <- "AAAATGGCTGCGTAATGCAAAATGGCTGCGAATGCAAAATGGCTGCGAATGCCGGCACGTTGCTACGT"
orf <- findORFs(x, codStart="ATG")
where the function argument x
is a character string giving the nucleotide sequence of interest. In current implementation, the function findORFs
scans the sequence for all sub-sequences that start with ATG start codon and end in-frame with a stop codon.
The function findORFs returns a matrix with start and stop positions in RNA molecule, length and sequence of identified variants of ORFs. In fact, the predominant amount of identified ORF candidates are short pseudo-ORFs (see below), as demonstrated in Figure 1.
Figure 1. Distribution of the length of ORF candidates from lncRNAs and mRNAs and length of true ORFs derived from NCBI RefSeq annotations of human genes. This figure is based on NCBI RefSeq release 109 (GRCh38.p12 human genome assembly).
#Vectorization of the sequence features of ORFs
The function vectorizeORFs
extracts and vectorizes the sequences features of ORFs:
feats <- vectorizeORFs(x=DNAStringSet(x="ATGGGCCTCA"))
where the function argument x
is a DNAStringSet object with ORF sequence.
For each ORF, the function vectorizeORFs
calculates 104 sequence features: frequency of mono-, di- and trinucleotides (84 features in total), parameters of the Bao model representing the local frequency entropy values of sequences (12 features in total) (Bao J. et al., 2014), correlation factors of nucleotides and length of ORF (8 features in total). As was shown in numerous studies, these features are informative for classification of coding and non-coding RNA molecules. This function returns the object of class data.frame with ORF vectorized into sequence features.
#Calculation of the classification model
The function classifyORFsCandidates
builds a randomForest classifier for the ORF candidates:
## The files with sequences can be downloaded from SST Center server at www.sstcenter.com/download/ORFhunteR
fileORFLncRNAs <- "http://www.sstcenter.com/download/ORFhunteR/NCBI_RefSeq_release_109_GRCh38.p12_ORF_candidates_sequences_lncRNAs.fasta.gz"
ORFLncRNAs <- loadTrExper(tr = fileORFLncRNAs)
fileORFmRNAs <- "http://www.sstcenter.com/download/ORFhunteR/NCBI_RefSeq_release_109_GRCh38.p12_ORFs_true_sequences_mRNAs.fasta.gz"
ORFmRNAs <- loadTrExper(tr = fileORFmRNAs)
## Make the train dataset from N pseudo- and N real ORFs.
N <- 1000
ORFLncRNAs <- ORFLncRNAs[1:N]
ORFmRNAs <- ORFmRNAs[1:N]
## Calculate the classification model for the open reading frame.
clt <- classifyORFsCandidates(ORFLncRNAs = ORFLncRNAs,
ORFmRNAs = ORFmRNAs,
pLearn = 0.75,
nTrees = 500,
modelRF = NULL,
workDir = NULL,
showAccuracy = TRUE)
where the function argument ORFLncRNAs
is the object of the class list of pseudo-ORFs, ORFmRNAs
is the object of the class list of coding true ORFs, pLearn
is a threshold, in fractions of one, for random selecting the train set of ORFs (the rest amount, or 1-pLearn, is thus left for the test set of ORFs; default value is 0.75), nTrees
is a number of trees to grow (this should not be set to too small a number, to ensure that every input row gets predicted at least a few times; default value is 500), modelRF
is character string, giving the name of RDS-file to store the classification model (NULL is by default), and workDir
is character string giving the path to and the name of the work directory (NULL is by default that means the current working directory). Here and below, pseudo-ORFs are nucleotide sequences of long non-coding RNA molecules that beginning with ATG start codon and ending in-frame with one of the stop codons, but these sequences are not translated into proteins. We also use this term for non-coding mRNA-derived nucleotide sequences (usually short) with features of ORFs.
The function classifyORFsCandidates
returns an object of class randomForest (Liaw A. et al., 2002) that can be used for subsequent automatic determination of ORFs in experimental RNA molecules of interest. In addition, the function automatically saves the RDS file of the classification model modelRF
into the directory workDir
and generates:
i) the randomForest type plots: the sorted variable importance, the error rates, and the dotchart of variable importance as measured by a classification model;
ii) the evaluation estimates of the classification model on the train and test datasets: the confusion matrix and the measures of Accuracy, Precision, Recall, and the Score F1, calculated as
Accuracy \[Accuracy = \frac{TP + TN}{TP + TN + FP + FN}\] Precision \[Precision = \frac{TP}{TP + FP}\] Recall \[Recall = \frac{TP}{TP + FN}\] The Score F1 \[The Score F1 = \frac{2 * TP}{2 * TP + FP + FN}\]
where TP – true positive (the positive class is predicted as the positive class number); FN – false negative (the positive class is predicted as the negative class number); FP – false positive (the negative class is predicted as the positive class number); TN – true negative (the negative class is predicted as the negative class number).
With calculated classification model, identification of the true ORFs among ORF candidates extracted from RNA molecules of interest can be done using function predictORF
:
model <- "http://www.sstcenter.com/download/ORFhunteR/classRFmodel_1.rds"
ORFs <- predictORF(tr = trans,
model= model,
prThr = 0)
where the function argument tr
is a character string giving the name of file with transcripts of interest, model
is a character string giving the connection or full path to the file from which the classification model is read, and argument prThr
is probability threshold for the “winning” class of ORFs (default value is 0). Allowed file formats for transcripts of interest are fasta
or fa
. Alternative formats are gtf
or gff
. With gtf
or gff
formats, additional argument genome
should be specified. This argument gives the name of pre-installed BSgenome data package with full genome sequences. Default value is “BSgenome.Hsapiens.UCSC.hg38”.
The function predictORF
returns an object of class data.frame with five fields:
head(ORFs)
#> transcript_id start end length prob
#> 1 ENST00000235453 279 1469 1191 1.000
#> 2 ENST00000246505 36 1397 1362 1.000
#> 3 ENST00000258105 21 359 339 0.948
#> 4 ENST00000278833 542 1597 1056 1.000
#> 5 ENST00000285021 216 3038 2823 1.000
#> 6 ENST00000302797 219 1187 969 1.000
The function predictORF
selects only one ORF candidate per RNA molecule that was assigned with maximal value of prob
field. In fact, 91.9% of ORFs that were identified in mRNA molecules (Ensembl release 97, GRCh38.p12 human reference genome assembly) demonstrates probability 0.9 (Figure 2).
Figure 2. Empirical cumulative distribution (a) and frequency (b) of probability values for ORFs that were identified in Ensembl human mRNA molecules.
At the same time, distribution of probability values for ORF candidates from long non-coding RNA molecules is completely differ (Figure 3). This difference between two classes of RNA molecules makes it possible to set a probability threshold prThr that discriminates pseudo- and true ORFs.
Figure 3. Boxplot demonstrating the distribution of probability values for ORFs that were identified in human mRNAs and lncRNAs (Ensembl release 97, GRCh38.p12 human reference genome assembly).
The sequences of identified can be extracted with function getSeqORFs
:
orfs_path <- system.file("extdata",
"Set.trans_ORFs.coordinates.txt",
package="ORFhunteR")
tr_path <- system.file("extdata",
"Set.trans_sequences.fasta",
package="ORFhunteR")
seq_orfs <- getSeqORFs(orfs = orfs_path,
tr = tr_path,
genome="BSgenome.Hsapiens.UCSC.hg38",
workDir=NULL)
This function needs the name of tab-delimited TXT file with coordinates of ORFs (as generated by function predictORF
) and the name of file with transcripts of interest. The last file must include the transcripts for which the ORFs were identified and listed in above file with coordinates of ORFs. Allowed file formats for transcripts of interest are fasta
or fa
. Alternative formats are gtf
or gff
. With gtf
or gff
formats, additional argument genome
should be specified. This argument gives the name of pre-installed BSgenome data package with full genome sequences. Default value is BSgenome.Hsapiens.UCSC.hg38
.
The output of function getSeqORFs
is a DNAStringSet object with sequences of ORFs:
head(seq_orfs)
#> DNAStringSet object of length 6:
#> width seq names
#> [1] 1191 ATGGCGGCAGCTCCACGGGAGGA...ATGATTATCCATTTTCTCAATAA ENST00000235453
#> [2] 1362 ATGGCGCACATTACCATTAACCA...CTCCCCTGTCCACGGTGTGTTGA ENST00000246505
#> [3] 339 ATGGCAGCTGCCTTGGCTCGGCT...CGGGCGCTGATACTGGTCGCTGA ENST00000258105
#> [4] 1056 ATGGCGCCGGTGTTGCCCCTGGT...AGGAGGATCTATCTGAGGCCTAG ENST00000278833
#> [5] 2823 ATGGCTCGGAAACGCGCGGCCGG...TGTTCCCATTTGAGCAGCTGTGA ENST00000285021
#> [6] 969 ATGGATCCAACCATCTCAACCTT...CGGGAAGCAGATTGGAGCAGTGA ENST00000302797
With identified ORFs, the PTCs can be inferred using function findPTCs
:
orfs_path <- system.file("extdata",
"Set.trans_ORFs.coordinates.txt",
package="ORFhunteR")
gtf_path <- system.file("extdata",
"Set.trans_sequences.gtf",
package="ORFhunteR")
ptcs <- findPTCs(orfs = orfs_path,
gtf = gtf_path,
workDir = NULL)
This function needs the name of tab-delimited TXT file with coordinates of ORFs (as generated by function predictORF
) and the name of file with structure of transcripts in format gtf
or gff
. The output of function findPTCs
is an object of class data.frame with field stop.status
:
head(ptcs)
#> transcript_id start end length prob stop.status
#> 1 ENST00000235453 279 1469 1191 1.000 mature
#> 2 ENST00000246505 36 1397 1362 1.000 mature
#> 3 ENST00000258105 21 359 339 0.904 premature
#> 4 ENST00000278833 542 1597 1056 1.000 mature
#> 5 ENST00000285021 216 3038 2823 1.000 mature
#> 6 ENST00000302797 219 1187 969 1.000 mature
In silico translation of identified ORFs can be done with function translateORFs
:
seq_orf_path <- system.file("extdata",
"Set.trans_ORFs.sequences.fasta",
package="ORFhunteR")
prot_seqs <- translateORFs(seqORFs=seq_orf_path)
This function accepts fasta
(or fa
) file with sequences of identified ORFs (as generated by function getSeqORFs
) and translates these sequences into strings of amino acids according to standard genetic code. The output of function translateORFs
is an AAStringSet object with amino acid sequences:
head(prot_seqs)
#> AAStringSet object of length 6:
#> width seq names
#> [1] 396 MAAAPREEKRWPQPVFSNPVVLW...EEITSGGFCGGKDKLQYDYPFSQ ENST00000235453
#> [2] 453 MAHITINQYLQQVYEAIDSRDGA...ISHQHQKLVVSKQNPFPPLSTVC ENST00000246505
#> [3] 112 MAAALARLGLRPVKQVRVQFCPF...FASHIRARDAAGSGDKPGADTGR ENST00000258105
#> [4] 351 MAPVLPLVLPLQPRIRLAQGLWL...ACRPAPEEAPPGEAPPKEDLSEA ENST00000278833
#> [5] 940 MARKRAAGGEPRGRELRSQKSKA...GGPKKTKREKKAAASHLFPFEQL ENST00000285021
#> [6] 322 MDPTISTLDTELTPINGTEETLC...EVDEGGGQLPEEILELSGSRLEQ ENST00000302797
If necessary, the coding of amino acid symbols can be switched from one-letter to three-letter using argument aaSymbol
of function.
The package ORFhunteR includes function annotateORFs
for basic annotation of identified ORFs. This function works according to following syntax:
orfs_path <- system.file("extdata",
"Set.trans_ORFs.coordinates.txt",
package="ORFhunteR")
tr_path <- system.file("extdata",
"Set.trans_sequences.fasta",
package="ORFhunteR")
gtf_path <- system.file("extdata",
"Set.trans_sequences.gtf",
package="ORFhunteR")
prts_path <- system.file("extdata",
"Set.trans_proteins.sequences.fasta",
package="ORFhunteR")
anno_orfs <- annotateORFs(orfs = orfs_path,
tr = tr_path,
gtf = gtf_path,
prts = prts_path,
workDir = NULL)
The function annotateORFs
needs five arguments. The argument orfs
is the name of tab-delimited TXT file with coordinates of ORFs (as generated by function predictORF). The argument tr
is a character string giving the name of file with transcripts of interest. This file must include the transcripts for which the ORFs were identified and listed in above file with coordinates of ORFs. Allowed file formats for transcripts of interest are fasta
or fa
. The argument gtf
is the name of file with structure of transcripts in format gtf
or gff.
The argument prts
is a character string giving the name of fasta
file with sequences of in silico translated proteins encoded by identified ORFs (as generated by function translateORFs
). The last argument workDir
is a character string giving the path to and name of work directory (NULL by default that mean the current working directory).
The function annotateORFs
returns an object of class data.frame. This object includes information on each analysed transcript: transcript ID, length of 5’UTRs, type of start codon, start coordinate of ORF, stop coordinate of ORF, type of stop codon, PTC status of stop codon, length of ORF, length of 3’UTRs, molecular weight of in silico translated protein, isoelectic point of a protein sequence and potential protein interaction index.
head(anno_orfs)
#> transcript_id f_utr.length start.codon orf.start orf.stop stop.codon
#> 1 ENST00000235453 278 ATG 279 1469 TAA
#> 2 ENST00000246505 35 ATG 36 1397 TGA
#> 3 ENST00000258105 20 ATG 21 359 TGA
#> 4 ENST00000278833 541 ATG 542 1597 TAG
#> 5 ENST00000285021 215 ATG 216 3038 TGA
#> 6 ENST00000302797 218 ATG 219 1187 TGA
#> stop.status orf.length t_utr.length MW pI indexPPI
#> 1 mature 1191 726 44.90 6.59 1.25
#> 2 mature 1362 389 52.10 8.61 1.19
#> 3 premature 339 137 12.11 8.98 1.96
#> 4 mature 1056 281 37.21 5.97 0.46
#> 5 mature 2823 794 105.95 9.30 2.60
#> 6 mature 969 3 36.25 7.57 0.13
If you use the ORFhunteR package for a scientific work, then please cite (Yatskou M. M. et al., 2019) and (Skakun V. V. et al., 2020).
Bao J., Yuan R., Bao Z. An improved alignment-free model for DNA sequence similarity metric. // BMC Bioinformatics. – 2014. – Vol. 15. – P. 321. doi: 10.1186/1471-2105-15-321
Liaw A., Wiener M. Classification and regression by randomForest. // R News. – 2002. – Vol. 2. – P. 18-22.
ORFhunteR: an accurate approach for the automatic identification and annotation of open reading frames in human mRNA molecules. Vasily V. Grinev, Mikalai M. Yatskou, Victor V. Skakun, Maryna K. Chepeleva, Petr V. Nazarov. bioRxiv 2021.02.05.429963; doi: https://doi.org/10.1101/2021.02.05.429963
Skakun V. V., Yatskou M. M., Nazarov P. V., Grinev V. V. ORFhunteR software package for automatic detection of open reading frames in human RNA molecules. // Computer Technology and Data Analysis (CTDA’2020): materials of the II International Scientific and Practical Conference, Minsk, 23-24 April 2020 / Editorial board: Skakun V. V. (editor-in-chief) [and others]. – Minsk: BSU, 2020. pp. 20-24.
Yatskou M. M., Skakun V. V., Grinev V. V. Development of a computational approach for automatic determination of open reading frames in human RNA molecules. // Quantum electronics: materials of the XII International Scientific and Technical Conference, Minsk, 18-22 November 2019 / Editorial board: Kugeiko M. M. [and others]. – Minsk: RIVSH, 2019. pp. 279-281.