2020
DOI: 10.1016/j.chembiol.2020.02.004
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Targeted In Situ Protein Diversification and Intra-organelle Validation in Mammalian Cells

Abstract: Engineered proteins must be phenotypically selected for function in the appropriate physiological context. Here, we present a versatile approach that allows generating panels of mammalian cells that express diversified heterologous protein libraries in the cytosol or subcellular compartments under stable conditions and in a single-variant-per-cell manner. To this end we adapt CRISPR/Cas9 editing technology to diversify targeted stretches of a protein of interest in situ. We demonstrate the utility of the appro… Show more

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Cited by 31 publications
(57 citation statements)
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“…The G-quartets stabilize rigid chromophore conformations by stacking interactions that largely govern the photophysical properties 34 36 . Unlike the near-planar fluorinated ligands DFHBI and DFHO in Spinach and Corn 7 , 20 , 21 , the fluorophores DMHBO + and DMHBI + in Chili adopt moderately twisted conformations, resembling those found in some LSS fluorescent proteins such as LSSmKate1 19 and mCRISPred 37 (Supplementary Fig. 20 and Supplementary Table 3 ).…”
Section: Discussionmentioning
confidence: 94%
“…The G-quartets stabilize rigid chromophore conformations by stacking interactions that largely govern the photophysical properties 34 36 . Unlike the near-planar fluorinated ligands DFHBI and DFHO in Spinach and Corn 7 , 20 , 21 , the fluorophores DMHBO + and DMHBI + in Chili adopt moderately twisted conformations, resembling those found in some LSS fluorescent proteins such as LSSmKate1 19 and mCRISPred 37 (Supplementary Fig. 20 and Supplementary Table 3 ).…”
Section: Discussionmentioning
confidence: 94%
“…[65][66][67][68] These approaches, however, require up-front development of a template sequence carrying the desired mutation of interest. Although useful for validation studies, targeted mutations, and singlesite saturation, 69 it remains difficult to envision the successful use of Figure 6. Overview of Currently Available Approaches for CRISPR-Directed Evolution Five classes of CRISPR-based genome editing systems are highlighted.…”
Section: Discussionmentioning
confidence: 99%
“…This makes it difficult to compare and quantify brightness across mutants without re-cloning them behind the original RBS. Emerging strategies for directed evolution in mammalian cells are potential solutions to this limitation [15,16]. Spontaneous mutagenesis in continuous style may further boost its screening efficiency with high throughput and minimal human intervention [17].…”
Section: Discussionmentioning
confidence: 99%