Generating single cell-derived knockout clones in mammalian cells with CRISPR/Cas9

Giuliano, Christopher J.; Lin, Andy; Sheltzer, Jason M.

doi:10.7287/peerj.preprints.27511v1

Cited by 14 publications

(16 citation statements)

References 44 publications

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“…No. 108099) using a BsmBI digestion as previously described (Giuliano et al, 2019). Plasmids were transformed in Stbl3 E. coli (Thermo Fisher; Cat.…”

Section: Crispri Plasmid Construction and Virus Generationmentioning

confidence: 99%

“…In addition to the C604W and S611G alterations, multiple silent mutations were included in the donor oligo to prevent re-cutting following template-mediated repair (Table S1A). Guide RNAs were cloned into the Lenti-Cas9-gRNA-GFP vector (Addgene # 124770) as previously described (Giuliano et al, 2019). To perform CRISPR-mediated HDR, 2mg of Mps1 gRNA plasmid was transfected along with 100 pmol of ssODN into Cas9-expressing cell lines using Lipofectamine 3000 (Thermo Fischer Scientific, Cat.…”

Section: Quantification Of Micronucleimentioning

confidence: 99%

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Single-Chromosomal Gains Can Function as Metastasis Suppressors and Promoters in Colon Cancer

et al. 2020

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“…No. 108099) using a BsmBI digestion as previously described (Giuliano et al, 2019). Plasmids were transformed in Stbl3 E. coli (Thermo Fisher; Cat.…”

Section: Crispri Plasmid Construction and Virus Generationmentioning

confidence: 99%

Section: Quantification Of Micronucleimentioning

confidence: 99%

Single-Chromosomal Gains Can Function as Metastasis Suppressors and Promoters in Colon Cancer

et al. 2020

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“…In a final step, we asked how differences in editing efficiency, the number of sgRNAs per gene, and potential clonality effects might affect the determination of gene essentiality. We were especially interested in differences in gene essentiality between the Cas9 bulk cell line and the two Cas9 single-cell clones, since the generation of single-cell clones from bulk populations forces cells to go through a genetic bottleneck, which might favor certain genetic alterations [ 44 ] and thus dependencies. Therefore, we used BAGEL [ 32 ] to analyze depleted genes in each HAP1 cell line using the combined HD CRISPR library (8 sgRNAs per gene) and the individual sub-libraries A and B.…”

Section: Resultsmentioning

confidence: 99%

Genome-scale CRISPR screening at high sensitivity with an empirically designed sgRNA library

et al. 2020

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Background In recent years, large-scale genetic screens using the CRISPR/Cas9 system have emerged as scalable approaches able to interrogate gene function with unprecedented efficiency and specificity in various biological contexts. By this means, functional dependencies on both the protein-coding and noncoding genome of numerous cell types in different organisms have been interrogated. However, screening designs vary greatly and criteria for optimal experimental implementation and library composition are still emerging. Given their broad utility in functionally annotating genomes, the application and interpretation of genome-scale CRISPR screens would greatly benefit from consistent and optimal design criteria. Results We report advantages of conducting viability screens in selected Cas9 single-cell clones in contrast to Cas9 bulk populations. We further systematically analyzed published CRISPR screens in human cells to identify single-guide (sg) RNAs with consistent high on-target and low off-target activity. Selected guides were collected in a novel genome-scale sgRNA library, which efficiently identifies core and context-dependent essential genes. Conclusion We show how empirically designed libraries in combination with an optimized experimental design increase the dynamic range in gene essentiality screens at reduced library coverage.

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“…We provide a brief overview of lentivirus production below. Our lab has made available a more detailed protocol for this process, which can be found in Giuliano et al (2019). iii.…”

Section: Materials and Reagentsmentioning

confidence: 99%

A CRISPR Competition Assay to Identify Cancer Genetic Dependencies

Girish¹,

Sheltzer²

2020

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The CRISPR/Cas9 system is a powerful tool for genome editing, wherein the RNA-guided nuclease Cas9 can be directed to introduce double-stranded breaks (DSBs) at a targeted locus. In mammalian cells, these DSBs are typically repaired through error-prone processes, resulting in insertions or deletions (indels) at the targeted locus. Researchers can use these Cas9-mediated lesions to probe the consequences of loss-of-function perturbations in genes of interest. Here, we describe an optimized protocol to identify specific genes required for cancer cell fitness through a CRISPR-mediated cellular competition assay. Identifying these genetic dependencies is of utmost importance, as they provide potential targets for anti-cancer drug development. This protocol provides researchers with a robust and scalable approach to investigate gene dependencies in a variety of cell lines and cancer types and to validate the results of high-throughput or whole-genome screens.

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Generating single cell-derived knockout clones in mammalian cells with CRISPR/Cas9

Cited by 14 publications

References 44 publications

Single-Chromosomal Gains Can Function as Metastasis Suppressors and Promoters in Colon Cancer

Single-Chromosomal Gains Can Function as Metastasis Suppressors and Promoters in Colon Cancer

Genome-scale CRISPR screening at high sensitivity with an empirically designed sgRNA library

A CRISPR Competition Assay to Identify Cancer Genetic Dependencies

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