Review
doi: 10.1038/nrm3860.
RNAi screening comes of age: improved techniques and complementary approaches
Affiliations
- PMID: 25145850
- PMCID: PMC4204798
- DOI: 10.1038/nrm3860
Item in Clipboard
Review
RNAi screening comes of age: improved techniques and complementary approaches
Nat Rev Mol Cell Biol.
2014 Sep.
Abstract
Gene silencing through sequence-specific _targeting of mRNAs by RNAi has enabled genome-wide functional screens in cultured cells and in vivo in model organisms. These screens have resulted in the identification of new cellular pathways and potential drug _targets. Considerable progress has been made to improve the quality of RNAi screen data through the development of new experimental and bioinformatics approaches. The recent availability of genome-editing strategies, such as the CRISPR (clustered regularly interspaced short palindromic repeats)-Cas9 system, when combined with RNAi, could lead to further improvements in screen data quality and follow-up experiments, thus promoting our understanding of gene function and gene regulatory networks.
Conflict of interest statement
Figures
RNAi reagents can be introduced into cells through different routes: siRNAs or endoribonuclease-prepared siRNAs (esiRNAs) can be transfected into mammalian (and other) cells; short hairpin RNAs (shRNAs) can be virally transduced into mammalian (and other) cells; double-stranded RNAs (dsRNAs) in solution can be applied to Drosophila melanogaster cells resulting in their uptake; dsRNAs (D. melanogaster or C. elegans) or shRNAs (D. melanogaster or mice) can be expressed from transgenic constructs; dsRNAs can be microinjected (C. elegans, D. melanogaster and some non-model insects); and Escherichia coli expressing dsRNAs can be fed to living animals (C. elegans or Planaria). Once in the cells, reagents such as dsRNAs are recognized by DICER (not shown), which processes them into siRNAs of 21–23 nucleotides in length. The synthetic or endogenously processed siRNA molecules are then incorporated into the RNA-induced silencing complex (RISC) and mediate gene silencing through _target mRNA cleavage (if perfect sequence complementarity exists between the _target mRNA and the siRNA) or translational interference (if the complementarity is partial; not shown).
a | RNA-induced silencing complex (RISC)-incorporated siRNAs mediate _target mRNA cleavage upon perfect sequence complementarity in either the coding region or the 3′ untranslated region (UTR) of the mRNA (depending on the siRNA design). For the siRNA shown, the 5′ seed region is in green, the middle region is in yellow and the 3′ end is in orange. b | Testing for potential off-_target effects of a given siRNA can be carried out using the C911 method. siRNA bases 9–11 are mutated while the seed region (bases 2–8) remains intact. This maintains off-_target interactions mediated by seed region matches but perturbs on-_target silencing. c | On-_target specificity by phenotypic rescue can be demonstrated by the co-expression of RNAi-resistant versions of the _target mRNA. Synonymous mutations in the siRNA-_targeted region of the mRNA can be introduced to prevent RISC-mediated silencing while preserving function. Alternatively, a homologous gene from a related species that has sufficient sequence divergence in the siRNA _targeting region to be RNAi resistant, but also sufficient similarity to elicit function, can be used to test on-_target specificity of the RNAi construct.
A number of points of intersection exist between RNAi screening (or other types of large-scale screening, such as overexpression of open reading frame (ORF) clones, or microRNA (miRNA) mimics or inhibitors (BOX 2)) and genome-engineering technologies (step 1) such as TAL effector nucleases (TALENs) and the CRISPR (clustered regularly interspaced short palindromic repeats)– Cas9 systems (highlighted in blue). Genome engineering can be used to create robust, well-controlled assays (step 2) in cell lines and model organisms by introducing various mutations such as gene knockouts, diseaseassociated mutations and knock-in of selectable markers or in-frame fusions or reporter genes. CRISPR–Cas9-mediated knockouts (step 3) in mouse or human cells have been reported as an effective method for pooled-format screens. These can be performed in parallel to RNAi screens, followed by comparison of results from the two types of screens. Independently of the screening approach, genome engineering can be used to modify cells or organisms for follow-up studies of specific gene candidates (step 4). In this case, the CRISPR–Cas9 system or TALENs can be used to knock out genes identified in RNAi screens, with a concordance of the knockdown and knockout phenotypes providing a high degree of confidence in the results. They can also be used to create other types of modifications useful for follow-up studies, for example, transcriptional upregulation or downregulation, using modified forms of Cas9, or introducing fluorescence tags or reporters using a knock-in approach.
Similar articles
-
RNA Interference in the Age of CRISPR: Will CRISPR Interfere with RNAi?Int J Mol Sci. 2016 Feb 26;17(3):291. doi: 10.3390/ijms17030291. Int J Mol Sci. 2016. PMID: 26927085 Free PMC article. Review.
-
High-throughput RNAi screening to dissect cellular pathways: a how-to guide.Biotechnol J. 2010 Apr;5(4):368-76. doi: 10.1002/biot.200900277. Biotechnol J. 2010. PMID: 20349460
-
RNAi/CRISPR Screens: from a Pool to a Valid Hit.Trends Biotechnol. 2019 Jan;37(1):38-55. doi: 10.1016/j.tibtech.2018.08.002. Epub 2018 Aug 31. Trends Biotechnol. 2019. PMID: 30177380 Review.
-
High-throughput functional genomics using CRISPR-Cas9.Nat Rev Genet. 2015 May;16(5):299-311. doi: 10.1038/nrg3899. Epub 2015 Apr 9. Nat Rev Genet. 2015. PMID: 25854182 Free PMC article. Review.
-
A Perspective on the Future of High-Throughput RNAi Screening: Will CRISPR Cut Out the Competition or Can RNAi Help Guide the Way?J Biomol Screen. 2015 Sep;20(8):1040-51. doi: 10.1177/1087057115590069. Epub 2015 Jun 5. J Biomol Screen. 2015. PMID: 26048892 Review.
Cited by
-
A multilineage screen identifies actionable synthetic lethal interactions in human cancers.Nat Genet. 2024 Nov 18. doi: 10.1038/s41588-024-01971-9. Online ahead of print. Nat Genet. 2024. PMID: 39558023
-
Streamlined analysis of drug _targets by proteome integral solubility alteration indicates organ-specific engagement.Nat Commun. 2024 Oct 16;15(1):8923. doi: 10.1038/s41467-024-53240-2. Nat Commun. 2024. PMID: 39414818 Free PMC article.
-
Genome-Wide High-Throughput RNAi Screening for Identification of Genes Involved in Protein Production.Methods Mol Biol. 2024;2810:317-327. doi: 10.1007/978-1-0716-3878-1_20. Methods Mol Biol. 2024. PMID: 38926288
-
Identification of Host Factors of Paramyxoviruses by siRNA Genome-Wide Screens.Methods Mol Biol. 2024;2808:105-120. doi: 10.1007/978-1-0716-3870-5_8. Methods Mol Biol. 2024. PMID: 38743365
-
Identifying regulators of aberrant stem cell and differentiation activity in colorectal cancer using a dual endogenous reporter system.Nat Commun. 2024 Mar 12;15(1):2230. doi: 10.1038/s41467-024-46285-w. Nat Commun. 2024. PMID: 38472198 Free PMC article.
References
-
- Rana TM. Illuminating the silence: understanding the structure and function of small RNAs. Nature Rev Mol Cell Biol. 2007;8:23–36. - PubMed
-
- Boutros M, Ahringer J. The art and design of genetic screens: RNA interference. Nature Rev Genetics. 2008;9:554–566. - PubMed
-
- Grimm S. The art and design of genetic screens: mammalian culture cells. Nature reviews Genetics. 2004;5:179–189. - PubMed
-
- Zhuang JJ, Hunter CP. RNA interference in Caenorhabditis elegans: uptake, mechanism, and regulation. Parasitology. 2012;139:560–573. - PubMed
-
- Bernards R, Brummelkamp TR, Beijersbergen RL. shRNA libraries and their use in cancer genetics. Nature Methods. 2006;3:701–706. - PubMed
Publication types
MeSH terms
Substances
Grants and funding
LinkOut - more resources
Full Text Sources
Other Literature Sources
Medical
Molecular Biology Databases
