MAKER has many FAILED
0
0
Entering edit mode
7 weeks ago
sansan96 ▴ 130

Hi everyone,

I'm trying to annotate a rather large plant genome (4Gb) but I've had problems with the first round of maker. I initially identified repeats in my genome with EarlGrey, a pipeline that runs RepeatModeler and RepeatMasker internally, which allowed me to obtain a softmask genome, as well as a series of files that allowed me to obtain a gff of repeats:

plant_primary_round3_sort.fasta.prep.cat.gz
plant_primary_round3_sort.fasta.prep.masked
plant_primary_round3_sort.fasta.prep.out
plant_primary_round3_sort.fasta.prep.tbl
...
plant_primary_round3_sort.fasta.prep.out.complex.gff3
plant_primary_round3_sort.fasta.prep.out.complex.reformat.gff3
plant_primary_round3_sort.fasta.prep.out.gff3

In my first round I am using my no-softmask genome, the gff file of repeats, proteins and a Trinity assembly, however I am getting many FAILED:

*I don't know if it could be because of my gff file of repeats.


scaffold_1      plant_round1_normal_datastore/49/CD/scaffold_1/    STARTED
scaffold_1      plant_round1_normal_datastore/49/CD/scaffold_1/    FINISHED
scaffold_2      plant_round1_normal_datastore/87/E3/scaffold_2/    STARTED
scaffold_2      plant_round1_normal_datastore/87/E3/scaffold_2/    FINISHED
scaffold_3      plant_round1_normal_datastore/47/19/scaffold_3/    STARTED
scaffold_3      plant_round1_normal_datastore/47/19/scaffold_3/    FINISHED
....
scaffold_9      plant_round1_normal_datastore/F3/F3/scaffold_9/    STARTED
scaffold_9      plant_round1_normal_datastore/F3/F3/scaffold_9/    FAILED
scaffold_10     plant_round1_normal_datastore/C3/86/scaffold_10/   STARTED
scaffold_10     plant_round1_normal_datastore/C3/86/scaffold_10/   FAILED
....
scaffold_4000     plant_round1_normal_datastore/3A/5C/scaffold_13/   STARTED
scaffold_4000     plant_round1_normal_datastore/3A/5C/scaffold_13/   FAILED

Could someone help me with this problem or perhaps suggest another way to annotate with maker? Maybe with the softmask genome.

My maker_opts.ctl (round1) is:

#-----Genome (these are always required)
genome=/primary/Acam_primary_round3_sort.fasta #genome sequence (fasta file or fasta embeded in GFF3 file)
organism_type=eukaryotic #eukaryotic or prokaryotic. Default is eukaryotic

#-----Re-annotation Using MAKER Derived GFF3
maker_gff= #MAKER derived GFF3 file
est_pass=0 #use ESTs in maker_gff: 1 = yes, 0 = no
altest_pass=0 #use alternate organism ESTs in maker_gff: 1 = yes, 0 = no
protein_pass=0 #use protein alignments in maker_gff: 1 = yes, 0 = no
rm_pass=0 #use repeats in maker_gff: 1 = yes, 0 = no
model_pass=0 #use gene models in maker_gff: 1 = yes, 0 = no
pred_pass=0 #use ab-initio predictions in maker_gff: 1 = yes, 0 = no
other_pass=0 #passthrough anyything else in maker_gff: 1 = yes, 0 = no

#-----EST Evidence (for best results provide a file for at least one)
est=/primary/anotacion_plant/maker_anotacion/evidence/Trinity_90.fasta #set of ESTs or assembled mRNA-seq in fasta format
altest= #EST/cDNA sequence file in fasta format from an alternate organism
est_gff= #aligned ESTs or mRNA-seq from an external GFF3 file
altest_gff= #aligned ESTs from a closly relate species in GFF3 format

#-----Protein Homology Evidence (for best results provide a file for at least one)
protein=/primary/anotacion_plant/maker_anotacion/evidence/Viridiplantae.fa  #protein sequence file in fasta format (i.e. from mutiple oransisms)
protein_gff=  #aligned protein homology evidence from an external GFF3 file

#-----Repeat Masking (leave values blank to skip repeat masking)
model_org=simple #select a model organism for RepBase masking in RepeatMasker
rmlib= #provide an organism specific repeat library in fasta format for RepeatMasker
repeat_protein=/data/software/maker-2.31/maker/data/te_proteins.fasta #provide a fasta file of transposable element proteins for RepeatRunner
rm_gff=/EarlGrey/Acam_primary_round3_sort.fasta.prep.out.complex.reformat.gff3 #pre-identified repeat elements from an external GFF3 file
prok_rm=0 #forces MAKER to repeatmask prokaryotes (no reason to change this), 1 = yes, 0 = no
softmask=1 #use soft-masking rather than hard-masking in BLAST (i.e. seg and dust filtering)

#-----Gene Prediction
snaphmm= #SNAP HMM file
gmhmm= #GeneMark HMM file
augustus_species= #Augustus gene prediction species model
fgenesh_par_file= #FGENESH parameter file
pred_gff= #ab-initio predictions from an external GFF3 file
model_gff= #annotated gene models from an external GFF3 file (annotation pass-through)
est2genome=1 #infer gene predictions directly from ESTs, 1 = yes, 0 = no
protein2genome=1 #infer predictions from protein homology, 1 = yes, 0 = no
trna=0 #find tRNAs with tRNAscan, 1 = yes, 0 = no
snoscan_rrna= #rRNA file to have Snoscan find snoRNAs
unmask=0 #also run ab-initio prediction programs on unmasked sequence, 1 = yes, 0 = no

#-----Other Annotation Feature Types (features MAKER doesn't recognize)
other_gff= #extra features to pass-through to final MAKER generated GFF3 file

#-----External Application Behavior Options
alt_peptide=C #amino acid used to replace non-standard amino acids in BLAST databases
cpus=1 #max number of cpus to use in BLAST and RepeatMasker (not for MPI, leave 1 when using MPI)

#-----MAKER Behavior Options
max_dna_len=100000 #length for dividing up contigs into chunks (increases/decreases memory usage)
min_contig=1 #skip genome contigs below this length (under 10kb are often useless)

pred_flank=200 #flank for extending evidence clusters sent to gene predictors
pred_stats=0 #report AED and QI statistics for all predictions as well as models
AED_threshold=1 #Maximum Annotation Edit Distance allowed (bound by 0 and 1)
min_protein=0 #require at least this many amino acids in predicted proteins
alt_splice=0 #Take extra steps to try and find alternative splicing, 1 = yes, 0 = no
always_complete=0 #extra steps to force start and stop codons, 1 = yes, 0 = no
map_forward=0 #map names and attributes forward from old GFF3 genes, 1 = yes, 0 = no
keep_preds=0 #Concordance threshold to add unsupported gene prediction (bound by 0 and 1)

split_hit=10000 #length for the splitting of hits (expected max intron size for evidence alignments)
single_exon=0 #consider single exon EST evidence when generating annotations, 1 = yes, 0 = no
single_length=250 #min length required for single exon ESTs if 'single_exon is enabled'
correct_est_fusion=0 #limits use of ESTs in annotation to avoid fusion genes

tries=2 #number of times to try a contig if there is a failure for some reason
clean_try=0 #remove all data from previous run before retrying, 1 = yes, 0 = no
clean_up=0 #removes theVoid directory with individual analysis files, 1 = yes, 0 = no
TMP=/scratch #specify a directory other than the system default temporary directory for temporary files

Thank so much.

genome softmask MAKER annotation • 442 views
ADD COMMENT
1
Entering edit mode

Is there any additional information in logs? Are those contigs large and are failing because of memory availability?

ADD REPLY
0
Entering edit mode

Hi GenoMax

It finishes but does not throw any error, I even increased the ram memory but I still have no success, do you recommend another way with maker?

ADD REPLY
0
Entering edit mode

This may sound stupid but let us go in the other direction. Have the contigs been filtered and QC'ed (for minimum length/content e.g. no poly-G's etc)?

ADD REPLY

Login before adding your answer.

Traffic: 1953 users visited in the last hour
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6