Dear guys We ave sequenced the whole genome of a plant species (about 700Mb) using two technologies and the data output as bellow:

Illumina: PE 2*150, insert size 330-550bp, random sharing total reads : 606 037 434 total bases: 91 511 652 534 (90Gb)

IonTorrent : single read, average lenght 125bp, enzymatique sharing, total reads : 247 000 000 total bases : ~ 20 000 000 000 (20Gb)

My questions are : can we perform a denovo assembly? have you a methodological proposal to optimise the assembly (combining these two data sets ? Which software you suggest to use? Thank you i advance for you help! have a nice day to all.

Soapdenovo2 would be useful for this as it allows simple use of different libraries (if you want to do this).

I don't think the Ion Torrent reads are going to help at all though, since they are a shorter read length and not paired end. To my knowledge they also contain a lot of indel errors, which are awful for assemblies.

Remember to trim your Illumina reads before assembling.

SOAPdenovo2 is a good choice. You can also try velvet and newbler which gives you option of considering reference genome as input and provides reference guided assembly

thankyou colindaven, I'll try with Soapdenovo. What about if I want to perform a denovo using a reference? thanks.

Thank you colindaven for your reactivity.