Uncoupling of sgRNAs from their associated barcodes during PCR amplification of combinatorial CRISPR screens.

PLoS One
Authors
Keywords
Abstract

Many implementations of pooled screens in mammalian cells rely on linking an element of interest to a barcode, with the latter subsequently quantitated by next generation sequencing. However, substantial uncoupling between these paired elements during lentiviral production has been reported, especially as the distance between elements increases. We detail that PCR amplification is another major source of uncoupling, and becomes more pronounced with increased amounts of DNA template molecules and PCR cycles. To lessen uncoupling in systems that use paired elements for detection, we recommend minimizing the distance between elements, using low and equal template DNA inputs for plasmid and genomic DNA during PCR, and minimizing the number of PCR cycles. We also present a vector design for conducting combinatorial CRISPR screens that enables accurate barcode-based detection with a single short sequencing read and minimal uncoupling.

Year of Publication
2018
Journal
PLoS One
Volume
13
Issue
5
Pages
e0197547
Date Published
2018
ISSN
1932-6203
DOI
10.1371/journal.pone.0197547
PubMed ID
29799876
PubMed Central ID
PMC5969736
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