Truncated File: Trouble with SRA > Fastq > Sam

DPCook

Member

Join Date: Sep 2014
Posts: 10

Truncated File: Trouble with SRA > Fastq > Sam

12-10-2014, 10:49 AM

Hi everyone,

I know there have been several posts regarding truncated SAM files, but I'm having a difficult time finding a solution.

I've converted an SRA file to FASTQ with fastq-dump:

Code:

fastq-dump [SRA] [Output-prefix]

QC/Trimmed the FASTQ,

Bowtie to align (SAM output):

Code:

bowtie -n 2 -k 1 -l 40 --best -m 1 -S [genome] [FASTQ] [SAM output]

But when I try to convert sam to bam

Code:

$ samtools view -Sb [.SAM] > [.BAM]
[W::sam_read1] parse error at line 26
[main_samview] truncated file.

So I looked at line 26 and it does appear odd (bottom line):

Code:

@HD	VN:1.0	SO:unsorted
@SQ	SN:chr1	LN:197195432
@SQ	SN:chr2	LN:181748087
@SQ	SN:chr3	LN:159599783
@SQ	SN:chr4	LN:155630120
@SQ	SN:chr5	LN:152537259
@SQ	SN:chr6	LN:149517037
@SQ	SN:chr7	LN:152524553
@SQ	SN:chr8	LN:131738871
@SQ	SN:chr9	LN:124076172
@SQ	SN:chr10	LN:129993255
@SQ	SN:chr11	LN:121843856
@SQ	SN:chr12	LN:121257530
@SQ	SN:chr13	LN:120284312
@SQ	SN:chr14	LN:125194864
@SQ	SN:chr15	LN:103494974
@SQ	SN:chr16	LN:98319150
@SQ	SN:chr17	LN:95272651
@SQ	SN:chr18	LN:90772031
@SQ	SN:chr19	LN:61342430
@SQ	SN:chrX	LN:166650296
@SQ	SN:chrY	LN:15902555
@SQ	SN:chrM	LN:16299
@PG	ID:Bowtie	VN:1.1.1	CL:"bowtie --wrapper basic-0 -n 2 -k 1 -l 40 --best -m 1 -S /Users/DPC/Documents/Genome_Indexes/mm9.ebwt/mm9 /Volumes/My Passport/Hi-C/ChIP-seq-files/Ezh2/EZH2-trimmed.fastq /Volumes/My Passport/Hi-C/ChIP-seq-files/Ezh2/EZH2.sam"
EZH2-SRR579282.1	4	*	0	0	*	*	0	0	TAGTTTGATTCACCCAAGGGTGAATGGGGGAACAAGAAAG	F>BACFHAHIEHFGII@FHGEE;9CFAHH)8??FFH;BDH	XM:i:0
X¢˚˚p¢˚˚D@X¢˚˚p¢˚˚D@X¢˚˚p¢˚˚D@EZH2-SRR579282.5	4	*	0	0	*	*	0	0	GCTAAAACCATCCAGTGGAAGAAAAACAGCATTTTCAACA	HHHHIIIIIIHIIIHHHIEGHEGIIFIIGAGHIIGFGHII	XM:i:1

I'm not quite sure what's going on here. I've had it happen with a couple of SAM files generated from SRA > Fastq, so I'm thinking it may be coming from the fastq-dump step.

Any insight or help would be greatly appreciated,

David

Tags: fastq-dump, sam, sequencing, sra, truncated

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