Pooled protein tagging, cellular imaging, and in situ sequencing for monitoring drug action in real time

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Figure 1.
Figure 1.

Pooled GFP intron-tagging of metabolic enzymes. (A) Schematic outline of the approach. (B) Identification of targetable introns within metabolic genes. (C) FACS sorting of clones with successful GFP-tagging by signal enrichment over background mCherry intensity used as control for autofluorescence. (D) Representative image of sorted GFP-tagged cell pool. Scale bar, 25 µm. (E) Comparison of RNA-seq expression in HAP1 cells between genes for which GFP-tagged cells could be isolated and genes that were targeted in the sgRNA library but did not result in successful clone isolation.

This Article

  1. Published in Advance November 17, 2020, doi: 10.1101/gr.261503.120 Genome Res. 30: 1846-1855

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