SOAPdenovo2

Where:

Run SOAPdenovo2 in the same folder as your DNA-seq reads. (Use File --> OpenDir to open a new window in your reads folder.)

Input:

Input files selected in the blreads table are ignored! Specify your read files in Libraries:

Libraries
- SOAPdenovo2 asks the user to specify one or more libraries of read files and parameters to use with those read files. For example, reads with 300 nt inserts would be in one library, and reads with a 400 nt inserts must be in a different library.

The Parameters tab allows you to specify up to 4 pairs of reads for the first library. The additionalLIBS tab lets you specify up to three libraries, each with four sets of read files. For each library, all reads in the library will be processed with the following parameters:
Paired-end vs. single end reads - For single end reads, choose a Left pair read file and leave the Right filename blank.

For each library, don't forget to click "Yes" on the first line to add that library to the input.

Output:
The default "../reads.trimmed.corrected.SOAPdenovo2" means that output files will be written to a folder in the parent folder (..)  called SOAPdenovo2.

The most useful human-readable output files:

soapdenovo2.log - Detailed progress on the assembly.

<prefix>.scaffStatistics - Statistics on contigs and scaffolds, including numbers such as N50, base composition etc.