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A software for the multispecies design of CRISPR/Cas9 libraries

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DOI

#CRISPR Library Designer (CLD): a software for the multispecies design of sgRNA libraries

This version is deprecated:

Please see the dockerized version of cld that can be found here:

 cld docker on github

The Mac version 1.4.2 will not work anymore on recent MacOS.

CITATION

F. Heigwer*, T. Zhan*, M. Breinig, J. Winter, D. Brügemann, S. Leible, M. Boutros, CRISPR library designer (CLD): software for multispecies design of single guide RNA libraries, Genome Biol., 2016, DOI:10.1186/s13059-016-0915-2

ABSTRACT

Here we describe CRISPR library designer (CLD), an integrated bioinformatics application for the design of custom single guide RNA (sgRNA) libraries for all organisms with annotated genomes. CLD is suitable for the design of libraries using modified CRISPR enzymes and targeting non-coding regions. To demonstrate its utility, we perform a pooled screen for modulators of the TNF-related apoptosis inducing ligand (TRAIL) pathway using a custom library of 12,471 sgRNAs.

Quick-Start:

On Linux:

  1. If you haven't, install Xquartz from http://www.xquartz.org/

1.1 When logging in remotely: log into your remote server by ssh -X 2. Download CLD_GUI_Ubuntu.zip according to your Operating system and unzip it. 3. Double click on the application or open it by ./CLD in the Terminal. 4. Download the database for your organism of interest. 5. Enter its name in the reference organism field on the start page. 6. Enter a list of gene identifiers in the "Gene List" tab and go to the "Design Parameter" tab to set your parameters. 7. Go to the "Start Analysis" tab to start sgRNA search. 8. The results will be created in the selected output directory ("Input/Output" tab).

Command-Line-Start:

cld can be called either with “--version”, printing its version number and copyrights, “--help” printing a more elusive help documentation and with “--task”.

EXAMPLE to execute from the path containing all needed files:

cld --task=end_to_end --output-dir=. --parameter-file=./params.txt --gene-list=./gene_list.txt

cld can run 2 distinct tasks, database creation and library design.

Database creation is called using the “--task=make_database” command giving the organism name of interest, as it is denoted in ENSEMBLs ftp folder structure e.g. homo_sapiens, and the rsync url to the current ftp server of ENSEMBL, examples can be found when cld --help is called. After calling this function CLD will automatically download the latest toplevel FASTA, GFF and GTF files for the organism of interest and compile a database containing bowtie indexes, mygff files and reformatted sequence files. If not enough computing power is available to the user, these databases also might be downloaded from http://www.e-crisp.org/E-CRISP/CLD-DB/.

Library design can either be done in two steps: “cld --task=target_ident” and then “cld --task=library_assembly” if the user wants to separate the two steps for example in order to only identify target sites without compiling a clonable library. Else “cld --task=end_to_end” which automatically will perform the steps mentioned before and present the end-result in a user defined output folder. For reasons of manageability for high throughput design, output files are kept as simple and standardised as possible. However a genome wide library targeting the human genome quickly spans several GB depending on how strict the parameters are chosen. Since the end_to_end task takes most time we benchmarked its time consumption to be approximately 1 h wall-time for an 8-core cpu node.

For running cld from the command line the syntax as outlined in the MANUAL must be used.

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