Seqanswers Leaderboard Ad

**sklages** · 06-19-2011, 02:38 AM

Just works like importing the qseq files (what you probably did import before as txt). Select to import fastq.

**atgc** · 06-19-2011, 08:45 AM

Thank you.

**boetsie** · 06-19-2011, 01:54 PM

First of all; probably the 'older' .txt format was also a .fastQ format. CASAVA spits out a .txt file, which is basically a .fastQ file.

Anyway; Best way to import Illumina Paired-end data is to go to 'File -> Import High-throughput sequencing data -> Illumina". Select here both paired-reads and choose your file format (.fastQ). See this link from CLC:

Home - QIAGEN Digital Insights

http://www.clcbio.com/index.php?id=1330&manual=Illumina_Genome_Analyzer_from_Illumina.html

Welcome to QIAGEN Digital Insights LabCorp uses QCI and HGMD to improve identification and interpretation of genetic variants within inhereited diseases.Read...

Illumina HiSeq data can be treated the same as Illumina Genome Analyzer data.

**atgc** · 06-19-2011, 07:57 PM

Initially the paired end read data that was given to me was two files/ sample - a forward and a reverse read. However this new data set includes 4 or more files / sample. I don't understand why this is.

**sklages** · 06-19-2011, 10:06 PM

Originally posted by atgc View Post

Initially the paired end read data that was given to me was two files/ sample - a forward and a reverse read. However this new data set includes 4 or more files / sample. I don't understand why this is.

If this data has been generated via CASAVA 1.8 then this is due to the fact that every fastq file generated has a constant number of sequences (except for the last one which holds the remainder), but at most 16mio. So one lane of HiSeq data is almost always splitted into more than one read (fastq) file.

E.g.

Code:

sample2_CGATGT_L003_R1_001.fastq.gz
sample2_CGATGT_L003_R2_001.fastq.gz
sample2_CGATGT_L003_R1_002.fastq.gz
sample2_CGATGT_L003_R2_002.fastq.gz
sample2_CGATGT_L003_R1_003.fastq.gz
sample2_CGATGT_L003_R2_003.fastq.gz

hth, Sven

**atgc** · 06-20-2011, 11:10 AM

That helps. Thanks.

**atgc** · 06-20-2011, 12:24 PM

I am getting an error when I import fastq reads into the CLC Genomics Workbench.

The message reads as follows:

"The data seems to be corrupt or originates from different sources since the input files contain different number of reads. The previous sequences have been properly saved but it is highly likely the import data is incomplete or defective. Please double-check the sources."

I have two forward and two reverse fastq files. I tried to import only one of each and I still get the error when importing.

Would anyone here know the source of this error or what it means.

Thanks for your help in advance.

Topics	Statistics	Last Post
Genomics-Driven Care in Neurodevelopmental Disorders Shows Promising Results by seqadmin Started by seqadmin, 01-09-2025, 04:04 PM	0 responses 439 views 0 likes	Last Post by seqadmin 01-09-2025, 04:04 PM
Study Questions Accuracy of Genetic Testing for Opioid Use Disorder Risk by seqadmin Started by seqadmin, 01-09-2025, 09:42 AM	0 responses 444 views 0 likes	Last Post by seqadmin 01-09-2025, 09:42 AM
New Algorithm Brings Precision and Scalability to Single-Cell RNA Analysis by seqadmin Started by seqadmin, 01-08-2025, 03:17 PM	0 responses 459 views 0 likes	Last Post by seqadmin 01-08-2025, 03:17 PM
Nanopores as Precision Diagnostic Tools in Molecular Biology by seqadmin Started by seqadmin, 01-03-2025, 11:18 AM	1 response 50 views 1 like	Last Post by Tonia 01-05-2025, 12:15 PM

Seqanswers Leaderboard Ad

Announcement

Mapping and base calling

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Latest Articles

ad_right_rmr

News