Hi everyone!
I'm new with RNA-seq analysis..
Wich would be the best tool to do a de novo assembly of RNA-seq Illumina PE reads (2x100 bp) with a 32 Gb RAM server?
Thanks in advance!
MF
Hi Stephen!
Thank you so much for your quick answer!
For Trinity I found a Jellyfish memory parameter which I was already using, I couldn't find any other for memory adjustment.
Is there another one for this purpose? I have 196 Mi PE reads.
Thanks!
MF
check all paramters by only using the --show_full_usage parameter. You can specify butterfly usage. Also, as Matt suggests, use the in silico normalization parameter which will reduce your number of reads given a sequencing depth coverage threshold (default 50x). Also, make sure you QC your reads: trim barcodes/adapters left over from sequencing, and low quality bases. You can use the trimmomatic parameter to trim your reads if you don't have a program of choice. Sickle is also a good one if you want to run it prior to Trinity.
For Trinity, the only way to adjust is using the -JM setting, which you have already discovered. This only effects memory usage in 1 stage of the assembly, so not exactly sufficient. Depending on the number of reads you have, you may want to use digital normalization. You could also increase the --min_kmer_cov to 2, but this will almost always result in a more fragmented assembly.
Use of this site constitutes acceptance of our User Agreement and Privacy Policy.
version 2.3.6
There's plenty out there: Trinity, Oases, Trans-Abyss, Cufflinks; to name a few. It depends what your end goal is. How many reads in your files? I don't have much experience with the others, but I know for Trinity, you can adjust the memory usage on the command line. I ran a SE assembly that had approx. 60 million reads on a workstation with 12Gb RAM.