CRISPR-Based Approaches for Gene Regulation in Non-Model Bacteria

Call, Stephanie N.; Andrews, Lauren B.

doi:10.3389/fgeed.2022.892304

“…Our results here suggest that dCas13 mediated activation (tlCRISPRa) could offer advantages over DNA-targeting dCas9 (txCRISPRa) by enabling control of individual genes in multi-gene operons. txCRISPRa is also subject to relatively stringent target requirements that have limited its generalizability to arbitrary gene targets (19, 58, 59). If tlCRISPRa with dCas13 is subject to less stringent or even simply different target requirements, it will expand the range of accessible gene targets in bacteria.…”

Section: Discussionmentioning

confidence: 99%

CRISPR-Cas tools for simultaneous transcription & translation control in bacteria

Cardiff,

Faulkner,

Beall

et al. 2023

Preprint

0

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Robust control over gene translation at arbitrary mRNA targets is an outstanding challenge in microbial synthetic biology. The development of tools that can regulate translation will greatly expand our ability to precisely control genes across the genome. InE. coli, most genes are contained in multi-gene operons, which are subject to polar effects where targeting one gene for repression leads to silencing of both genes. These effects pose a challenge for independently regulating individual genes in multi-gene operons. Here, we use CRISPR-dCas13 to address this challenge. We find that dCas13-mediated repression exhibits up to 6-fold lower polar effects compared to dCas9. We then show that we can selectively activate single genes in a synthetic multi-gene operon by coupling dCas9 transcriptional activation of an operon with dCas13 translational repression of individual genes within the operon. We also show that dCas13 and dCas9 can be multiplexed for improved biosynthesis of a medically-relevant human milk oligosaccharide. Taken together, our findings suggest that combining transcriptional and translational control can access effects that are difficult to achieve with either mode independently. These combined tools for gene regulation will expand our abilities to precisely engineer bacteria for biotechnology and perform systematic genetic screens.Graphical Abstract

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“…The study of plasmid-encoded functions in bacteria other than the Lyme disease spirochetes can therefore be facilitated by implementation of a Cas9-mediated plasmid curation protocol. Translation of this approach across bacterial phyla is likely feasible, as demonstrated by the successful broad implementation of CRISPR-based methods of gene regulation [ 76 ].…”

Section: Discussionmentioning

confidence: 99%

Cas9-mediated endogenous plasmid loss in Borrelia burgdorferi

Takacs

¹

,

Nakajima

²

,

Haber

³

et al. 2022

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The spirochete Borrelia burgdorferi, which causes Lyme disease, has the most segmented genome among known bacteria. In addition to a linear chromosome, the B. burgdorferi genome contains over 20 linear and circular endogenous plasmids. While many of these plasmids are dispensable under in vitro culture conditions, they are maintained during the natural life cycle of the pathogen. Plasmid-encoded functions are required for colonization of the tick vector, transmission to the vertebrate host, and evasion of host immune defenses. Different Borrelia strains can vary substantially in the type of plasmids they carry. The gene composition within the same type of plasmid can also differ from strain to strain, impeding the inference of plasmid function from one strain to another. To facilitate the investigation of the role of specific B. burgdorferi plasmids, we developed a Cas9-based approach that targets a plasmid for removal. As a proof-of-principle, we showed that targeting wild-type Cas9 to several loci on the endogenous plasmids lp25 or lp28-1 of the B. burgdorferi type strain B31 results in sgRNA-specific plasmid loss even when homologous sequences (i.e., potential sequence donors for DNA recombination) are present nearby. Cas9 nickase versions, Cas9D10A or Cas9H840A, also cause plasmid loss, though not as robustly. Thus, sgRNA-directed Cas9 DNA cleavage provides a highly efficient way to eliminate B. burgdorferi endogenous plasmids that are non-essential in axenic culture.

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“…The study of plasmid-encoded functions in bacteria other than the Lyme disease spirochetes can therefore be facilitated by implementation of a Cas9-mediated plasmid curation protocol. Translation of this approach across bacterial phyla is likely feasible, as demonstrated by the successful broad implementation of CRISPR-based methods of gene regulation [66].…”

Section: Discussionmentioning

confidence: 99%

Cas9-mediated endogenous plasmid loss in Borrelia burgdorferi

Takacs

¹

,

Nakajima

²

,

Haber

³

et al. 2022

Preprint

0

View full text Add to dashboard Cite

The spirochete Borrelia burgdorferi, which causes Lyme disease, has the most segmented genome among known bacteria. In addition to a linear chromosome, the B. burgdorferi genome contains over 20 linear and circular endogenous plasmids. While many of these plasmids are dispensable under in vitro culture conditions, they are maintained during the natural life cycle of the pathogen. Plasmid-encoded functions are required for colonization of the tick vector, transmission to the vertebrate host, and evasion of host immune defenses. Different Borrelia strains can vary substantially in the type of plasmids they carry. The gene composition within the same type of plasmid can also differ from strain to strain, impeding the inference of plasmid function from one strain to another. To facilitate the investigation of the role of specific B. burgdorferi plasmids, we developed a Cas9-based approach that targets a plasmid for removal. As a proof-of-principle, we showed that targeting wild-type Cas9 to several loci on the endogenous plasmids lp25 or lp28-1 of the B. burgdorferi type strain B31 results in sgRNA-specific plasmid loss even when homologous sequences (i.e., potential sequence donors for DNA recombination) are present nearby. Cas9 nickase versions, Cas9D10A or Cas9H840A, also cause plasmid loss, though not as robustly. Thus, sgRNA-directed Cas9 DNA cleavage provides a highly efficient way to eliminate B. burgdorferi endogenous plasmids that are non-essential in axenic culture.

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CRISPR-Based Approaches for Gene Regulation in Non-Model Bacteria

Cited by 23 publications

References 227 publications

CRISPR-Cas tools for simultaneous transcription & translation control in bacteria

CRISPR-Cas tools for simultaneous transcription & translation control in bacteria

Cas9-mediated endogenous plasmid loss in Borrelia burgdorferi

Cas9-mediated endogenous plasmid loss in Borrelia burgdorferi

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