A randomized multiplex CRISPRi-Seq approach for the identification of critical combinations of genes
Identifying virulence-critical genes from pathogens is often limited by functional redundancy. To rapidly interrogate the contributions of combinations of genes to a biological outcome, we have developed a mu ltiplex, r andomized C RISPR i nterference s equencing (MuRCiS) approach. At its center is...
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Veröffentlicht in: | eLife 2023-12, Vol.12 |
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Format: | Artikel |
Sprache: | eng |
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Zusammenfassung: | Identifying virulence-critical genes from pathogens is often limited by functional redundancy. To rapidly interrogate the contributions of combinations of genes to a biological outcome, we have developed a
mu
ltiplex,
r
andomized
C
RISPR
i
nterference
s
equencing (MuRCiS) approach. At its center is a new method for the randomized self-assembly of CRISPR arrays from synthetic oligonucleotide pairs. When paired with PacBio long-read sequencing, MuRCiS allowed for near-comprehensive interrogation of all pairwise combinations of a group of 44
Legionella pneumophila
virulence genes encoding highly conserved transmembrane proteins for their role in pathogenesis. Both amoeba and human macrophages were challenged with
L. pneumophila
bearing the pooled CRISPR array libraries, leading to the identification of several new virulence-critical combinations of genes.
lpg2888
and
lpg3000
were particularly fascinating for their apparent redundant functions during
L. pneumophila
human macrophage infection, while
lpg3000
alone was essential for
L. pneumophila
virulence in the amoeban host
Acanthamoeba castellanii
. Thus, MuRCiS provides a method for rapid genetic examination of even large groups of redundant genes, setting the stage for application of this technology to a variety of biological contexts and organisms. |
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ISSN: | 2050-084X 2050-084X |
DOI: | 10.7554/eLife.86903.3 |