Trinity

Where:

Run Trinity in the same folder as your RNA-seq reads. (Use File --> OpenDir to open a new window in your RNA-seq reads folder.)

Input:

RNAseq reads: Before opening this menu, select RNA-seq readfiles to be mapped to the genome. For paired-end reads, Trinity works with pairs of files. Files can be selected in pairs using File --> guesspairs.py.

Trinity does not allow combining paird-end and single read data! Before running Trinity, select ONLY paird-end, or ONLY single-end read files.


Resources 

maximum memory to use (Gb) - The Trinity Wiki FAQ suggests setting 1Gb RAM per million reads. "
The memory usage mostly depends on the complexity of the RNA-Seq data set, specifically on the number of unique k-mers. If you do not have access to a high-memory server, other freely available options are available."

Output:
The default "../reads.trimmed.corrected.Trinity" means that output files will be written to a folder in the parent folder (..)  called Trinity.

The progress of the assembly can be found in trinity.log.