Question

How to specify Illumina Single End data in the MaSuRCA Assembler config file

1

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10.5 years ago

ajaybioinfo ▴ 80

Dear All,

Hi I am new to MaSuRCA and want to perform a hybrid denovo assembly of a plant genome.

I have successfully completed the assembly on the provided test data set.

But here i Have 2 paired end run of illumina and 3 run of Illumina Single end. In the tutorial it is clearly mention how to specify the Paired - End data but it is not mention how to specify Single end Illumina data in the config file.

Can anyone one guide to specify the single end illumina data in the configuration file

Thanks a lot

next-gen Assembly • 5.7k views

ADD COMMENT • link updated 3.2 years ago by Ram 44k • written 10.5 years ago by ajaybioinfo ▴ 80

0

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Dear Sukhdeep,

Sorry for late reply I have tried your suggested option but it doesnt work. it is giving below error:

Command:

/root/Desktop/DesktopBKP/MaSuRCA-2.2.2/bin/./masurca 2as-config-file1-25-4.txt

Error:

missing forward file for PE library H3 at /root/Desktop/DesktopBKP/MaSuRCA-2.2.2/bin/./masurca line 305, <FILE> line 16)

My Configuration File

PARAMETERS
CA_PARAMETERS= ovlMerSize=30 cgwErrorRate=0.25 merylMemory=8192 ovlMemory=4GB
KMER_COUNT_THRESHOLD = 1
GRAPH_KMER_SIZE=auto
USE_LINKING_MATES=0
NUM_THREADS= 64
DO_HOMOPOLYMER_TRIM=1
JF_SIZE=50000000000
END

DATA
PE= GA 525 60 /nrcpb1/ajay/wheat-genome2as-2014/illumina/raw-masurca/2AS_GA_s_1_1_sequence.fastq /nrcpb1/ajay/wheat-genome2as-2014/illumina/raw-masurca/2AS_GA_s_1_2_sequence.fastq
PE= H1 525 60 /nrcpb1/ajay/wheat-genome2as-2014/illumina/raw-masurca/2AS_HS_s_1_1_sequence.fastq /nrcpb1/ajay/wheat-genome2as-2014/illumina/raw-masurca/2AS_HS_s_1_2_sequence.fastq
PE= H2 525 60 /nrcpb1/ajay/wheat-genome2as-2014/illumina/raw-masurca/2AS_HS_s_2_1_sequence.fastq /nrcpb1/ajay/wheat-genome2as-2014/illumina/raw-masurca/2AS_HS_s_2_2_sequence.fastq

PE= H3 525 60 /nrcpb1/ajay/wheat-genome2as-2014/illumina/s_2_2_sequence.fastq # (Illumina Single End file 1)
PE= H4 525 60 /nrcpb1/ajay/wheat-genome2as-2014/illumina/s_3_2_sequence.fastq # (Illumina Single End file 2)

OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/G73MYLX.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/G7DSIN1.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/G7QNE8J.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/G7SIGDD.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/G92D85N.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/HD4EOM.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/HDJUW5E.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/HDRDHMJ.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/HDWU88M.frg
OTHER=/nrcpb1/ajay/wheat-genome2as-2014/454-CABOG/HG1SIK2.frg

END

please tell me where I am wrong in the configuration file I am using MaSuRCA2.2.2, I have tried 2.2.1 also but getting same error

Is MaSuRCA is supporting illumina single end data?

Thanks

ADD REPLY • link updated 4.9 years ago by Ram 44k • written 10.5 years ago by ajaybioinfo ▴ 80

Ram · Answer 1 · 2014-05-17

2

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10.5 years ago

Sukhi Singh 11k

Just specifying one file should work and replacing pe by se.

DATA 
 PE= pe avg_read_length std_dev /FULL_PATH/paired_read1.fastq /FULL_PATH/paired_read2.fastq 
 PE= se avg_read_length std_dev /FULL_PATH/single_read.fastq
 END

 PARAMETERS
 GRAPH_KMER_SIZE= kmer_size
 USE_LINKING_MATES=1   #1 for using Illumina reads
 JF_SIZE= int          #jellyfish hash size - 10x the genome
 END

Reference: http://compgenomics2014.biology.gatech.edu/index.php/Genome_Assembly_Group

ADD COMMENT • link updated 4.9 years ago by Ram 44k • written 10.5 years ago by Sukhi Singh 11k

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Dear Sukhdeep

Thanks for your suggestion it worked now and i am able to get the assemble.sh file from configuration file.

one more thing I am not giving the exact path of the SE fastq file thats why it is not creating the assemble.sh script. Once again thanks for your support

Cheers

ADD REPLY • link updated 4.9 years ago by Ram 44k • written 10.5 years ago by ajaybioinfo ▴ 80

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I don't understand your configuration. We cannot use 2 libraries of SE ?

ADD REPLY • link 8.0 years ago by Picasa ▴ 650

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This have not worked for me (version 11152016).

Also, believe that two numbers after tag of the library are not avg/std_dev _read_length but average/std dev fragment length (i.e. the distance of the pair end reads).

ADD REPLY • link 8.0 years ago by kamiljaron ▴ 230