2023
DOI: 10.1021/acssynbio.2c00595
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New Target Gene Screening Using Shortened and Random sgRNA Libraries in Microbial CRISPR Interference

Abstract: CRISPR interference (CRISPRi) screening has been used for identification of target genes related to specific phenotypes using single-molecular guide RNA (sgRNA) libraries. In CRISPRi screening, the sizes of random sgRNA libraries contained with the original target recognition sequences are large (∼10 12 ). Here, we demonstrated that the length of the target recognition sequence (TRS) can be shortened in sgRNAs from the original 20 nucleotides (N 20 ) to 9 nucleotides (N 9 ) that is still sufficient for dCas9 t… Show more

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Cited by 5 publications
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“…In some CRISPR systems, catalytically inactive Cas proteins are fused to effector domains or repressive elements. These effector molecules enable more precise and robust gene regulation by modulating chromatin structure or interacting with the transcription machinery [14,47,48]. By enabling the selective and reversible induction or downregulation of particular genes, CRISPRi facilitates a more exhaustive examination of gene function and the repercussions of alterations in gene expression.…”
Section: Crispr-interference (Crispri)mentioning
confidence: 99%
“…In some CRISPR systems, catalytically inactive Cas proteins are fused to effector domains or repressive elements. These effector molecules enable more precise and robust gene regulation by modulating chromatin structure or interacting with the transcription machinery [14,47,48]. By enabling the selective and reversible induction or downregulation of particular genes, CRISPRi facilitates a more exhaustive examination of gene function and the repercussions of alterations in gene expression.…”
Section: Crispr-interference (Crispri)mentioning
confidence: 99%