Dear all,

I have two queries regarding the structural variation identification using whole genome sequencing in human.

If you can suggest, to identify structural variation (SV) like balanced chromosomal abnormalities (BCA) what technology would be the best or good to use in whole genome sequencing (WGS): Illumina 2 x 300 bp read length technology (fragment analysis) or mate-pair technology . What would be the difference between these two technologies (advantages/disadvantages). If Illumina 300 bp read length technology would be good enough to serve the purpose here instead of mate-pair. Also cost wise which will be effective?

Also if there is any recommended/standard best practices guidelines/pipelines for BCA breakpoint identification and/or any other SV identification analysis. How to analyze the data?

Thanks & regards, Aneek

Detecting large-scale copy-neutral events purely from short read sequencing data is difficult. Your entire signal is in the breakpoints so the strength of that signal is depend on the mappable coverage you have across the breakpoints. Events in extremely repetitive sequence (eg centromeres) are unlikely to be found by either short or long read sequencing. In such cases you'd have better luck with karyotyping (eg FISH).

As for your question, it depends on your library fragment size. If you do 2x300bp sequencing with a mean library fragment size of 500bp, your signal will be much weaker than the same sequencing on a library with 1,000bp fragments. Mate-pair libraries have much longer fragment lengths, thus will require lower coverage for the same signal strength. If you don't need an exact breakpoint reconstruction, then you get more value per sequenced base by sequencing shorter reads (since more fragments span the breakpoint) but if you need exact breakpoint sequence reconstruction, then sequencing longer reads is preferable due to the better mapability of the longer reads.

any recommended/standard best practices guidelines/pipelines for BCA breakpoint identification and/or any other SV identification analysis. How to analyze the data?

SV calling is still well behind SNV and small indel calling both in terms both specificity and sensitivity and hasn't yet matured to the point where you can swap out callers and get results that are mostly the same. For the 2x300bp data, I would recommend GRIDSS as the SV caller, and StructuralVariantAnnotation for downstream analysis, but LUMPY and manta are other good options. For mate-pair, you will have a smaller selection of tools as most SV callers don't support mate-pair libraries. As you're looking for large-scale event, you can't filter on event size so you're going to get a lot of false positive calls due to sequence homology.

Are you open to alternate approaches? Molecular barcoding approaches such as the 10X Genomics Chromium are showing some really impressive early results (eg http://biorxiv.org/content/early/2016/09/10/074518) but the analysis techniques are immature.

@d-cameron

Hi,

Thank you very much for the useful information. As you said I think 2 x 300 bp read length in larger fragments/inserts (1-2Kb) would be ideal for SV identification. As we are not very expert in data analysis, mate-pair analysis may not be suitable due to limited proper tools availability. Please correct me if I am wrong.

10X Genomics Chromium is an advanced newly arrived technology and not affordable for our laboratory at present.

For analysis there is python based software named SVfinder. Details can be found in this link: https://github.com/cauyrd/SVfinder I have found it very easy to use but not sure about the specificity. It would helpful to know your opinion about the program.

Another thing I would like to ask, where can I get Illumina paired-end raw fastq files for whole genomes sequencing where short read length + larger fragments technology was used for SV identification?

Thanks & regards, Aneek