Team I Gene Prediction Group

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Team members: Genevieve Brandt, Victoria Caban, Yuntian He, Junyu Li, Yiqiuyi Liu, Yihao Ou, Wenyi Qiu, Casey Smith, Mohit Thakur, Stephen Wist, Qinyu Yue

Introduction

Data

We were given de Novo assemblies of 258 isolates of Klebsiella spp..

Background

Our overarching goal is to understand what causes heteroresistance in Klebsiella spp. At this step, our objective was, given assembled genomes, to predict genes for Klebsiella that could later be annotated to understand functionality.

Gene Prediction

Gene prediction is the process of identifying the specific regions of genomic DNA that encode for genes. After sequencing and assembly, gene prediction is one of the first steps in understanding the genome of a species. In the past, confirming that the gene prediction is accurate demanded in vivo experimentation through gene knockout and other assays. Today, bioinformatics research has made it possible to predict the function of a gene based on its sequence alone. There are two general methods to do this: homology-based tools and ab-initio tools.

There is a big difference between prokaryotic and eukaryotic gene prediction. For eukaryotes, genes may be separated by introns, which makes it challenging to find the whole genomic sequence. Promoter sequences are more complex and less well understood in eukaryotes as well. In prokaryotes, the promoter regions are well understood, which is useful when using ab initio tools, since these tools search for signs of specific signs of protein coding genes. In prokaryotic genomes there are also contiguous open reading frames (ORFs) - when paired with the high amount of stop codons in prokaryotes this can indicate, with high probability, a gene being present. Our challenge when looking at ORFs is that every gene is a ORF, but not every ORF is a gene.

Methods

Pipeline (general workflow)

Homology-Based Methods

BLAST

One sequence by itself is not informative; it must be analyzed by comparative methods against existing sequence databases to develop hypothesis concerning relatives and function. BLAST(Basic Local Alignment Search Tool) is a widely used tool for similarity search, which adopts a Heuristic approach based on the Smith Waterman algorithm. BLAST provides not only the results of best local alignment, but various statistical significance as well.This algorithm compares a query sequence against reference sequence or specific database, such as nucleotide database. Because there are 258 assemblies that we are intending to BLAST, we chose to use local BLAST. The reference sequences we picked are the sequences which were used for gene assembly, the query sequences are the assembly results from Spades.

To run BLAST, we first need to create a database using the reference genome, then blast the query sequence against the database.

Commands:

makeblastdb -in reference.fasta -dbtype nucl -out db_name
blastn -db db_name -query assembly_result.fasta -outfmt 6 -out blast_result.gff

Ab-initio Methods

Ab-initio tools always predict genes based on the gene content and signal detection(e.g. start/stop codon; Ribosome Biding Site, RBS etc.). In another words, they predict genes by analyzing statistical features of genes first, then separate the coding sequences and non-coding sequences apart.

There are so many different algorithms among different ab-initio tools. For example, Dynamic programming gene finding, Hidden Markov Model, Interpolated Markov Model, Linear Discriminant Analysis and so on. By comparing the sensitive, PPV and running time, we chose some tools below to generate our final results.


Prodigal

Pros:

  • Straightforward installation and use
  • Accuracy: sensitivity - 94.7%, positive predictive value - 94.1%. Comparable to other tools
  • Speed: averaged 17 seconds/genome
  • Cons:

  • Fairly limited number of options
  • Parameters used:

  • mode: normal mode (DEFAULT-single genome, any number of sequences)
  • translation table: 4 (DEFAULT-standard bacteria, archaea) and 11 (DEFAULT-mycoplasma/spiroplasma)
  • gap mode: 0 (DEFAULT-partial genes run into gaps)
  • output format: gff (GFF format for the gene coordinates file)
  • rbs motif: (DEFAULT-looks for default Shine-Dalgarno motif)
  • Input: assembly file (.fna) Output: gene coordinates (.gff), nucleotide sequences (.fna), protein sequences (.fna) Command:

    prodigal -i input.fna -o output.gff -f gff -d nucleotide_seq.fna -a protein_seq.fna

    Reference: Hyatt, Doug, et al. "Prodigal: prokaryotic gene recognition and translation initiation site identification." BMC bioinformatics 11.1 (2010): 119.

    Genemark.hmm

    Before running GeneMark.hmm, it is necessary to got a mode file first. One way is to download the models from GeneMark website(http://opal.biology.gatech.edu/GeneMark/). Or you can generated them by GeneMarkS or GeneMark.

    Pros:

  • easy to install and use
  • Accuracy: sensitivity - 93.11%, positive predictive value - 93.10%. Comparable to other tools
  • Speed: averaged 1.71 seconds/genome
  • Parameters used:

  • motif:1
  • Input: assembly file (.fna) Output: gene coordinates (.gff), nucleotide sequences (.fna), protein sequences (.fna) Command:

    gmhmmp -o <output.gff> -f G -m <model with its path> <input_file> 

    Reference: http://opal.biology.gatech.edu/GeneMark/background.html

    Lukashin, Alexander V., and Mark Borodovsky. "GeneMark. hmm: new solutions for gene finding." Nucleic acids research 26.4 (1998): 1107-1115.

    GLIMMER

    Run_glimmer.sh includes:

    1. Add GLIMMER executables to PATH
    2. Create output and log directories GFF/ and logs/
    3. GLIMMER calling, done through a pipeline script GLIMMER3 provides g3-from-scratch.csh
    4. Convert GLIMMER outputs to GFFs

    Parameters used: (default in g3-from-scratch.csh)

  • -o 50: max prediction overlap length
  • -g 110: min gene length
  • -t 30: max entropy distance score
  • -d 7 : depth of interpolated context model
  • -p 3: period of interpolated context model
  • -w 12: width of interpolated context model
  • Input: directory of assembly FASTA file(s) Output: Gene table (.predict and .detail) and byproducts (.icm, .train, .longorfs) Command:

     bash run_glimmer.sh [directory] 


    Reference: https://ccb.jhu.edu/software/glimmer/glim302notes.pdf

    ncRNA Methods

    Infernal

    There exists large varieties of ncRNA beyond tRNA and rRNA that are important for biological function. Infernal is a de novo ncRNA prediction tool that can predict diverse families of ncRNA. Infernal compares nucleotide sequences against profiles, structually annotated multiple sequence alignments of RNA, to predict RNA sequences. Its compares both primary and secondary structure to increase its accuracy. These profiles use position specific scoring to account the importatnce of each insertions, deletions, and substitutions. Structural annotations can identify key residues which are dependent on each other. These profiles are implemented by Infernal as covariance models (CM), a specialized version of hidden markov models [1].

    RFam is a database of RNA CMs information about RNA families [2]. The istR RNA CM was chosen based on its potential role in heteroresistance. The TisB-istR toxin-antitoxin system is induced by DNA damage and causes the cell to arrest growth rather than die [3]. This could be a cause of the ability of our heteroresistant and non-heteroresistant Klebsiella pneumoniae spp. To persist in environments it shouldn’t.

    Infernal is a suite of many executables to create, manipulate, and analyze using covariance models. For our purposes we only needed to use the `cmscan` program. This command searches query sequences against a covariance model database.

    Command:

    cmscan --tblout <path to write tblout file> <cm file> <input fasta> > <path to write cmscan output>

    Aragorn

    A homology non coding RNA prediction tool, his program quickly identifies tRNA and tmRNA genes. It uses heuristic algorithms to predict tRNA secondary structure, based on homology with recognized tRNA consensus sequences. This program outputs reports ofthe proposed tRNA secondary structure and, for tmRNA genes, the secondary structure of the tRNA domain, the tmRNA gene sequence, the tag peptide and a list of organisms with matching tmRNA peptide tags.

    Command:

    ./aragorn -t <input file> 


    RNAMMER

    RNAmmer is a widely used ribosomal RNA prediction tool, it accepts both Prokaryotic and Eukaryotic inputs and returns result in gff, fasta and html formats based on need.

     rnammer -S bac -m lsu,ssu,tsu -multi -gff output_file.gff -f output_file.fasta < input.fasta 

    Results

    Final Pipeline

    Gene Prediction

    Ab-initio

    Prodigal

    GeneMark HMM


    Non-coding RNA

    RNAmmer

    Infernal

    Aragorn

    References

    https://ghr.nlm.nih.gov/primer/basics/gene

    https://www.biostat.wisc.edu/bmi776/spring-15/lectures/IMMs.pdf

    http://ece.drexel.edu/gailr/ECE-S690-503/markov_models.ppt.pdf

    http://onlinelibrary.wiley.com/doi/10.1042/BC20070137/full#footer-citing

    https://iweb.langara.bc.ca/biology/mario/Biol2315notes/biol2315chap11.h