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Gene Knock-in by CRISPR/Cas9 and Cell Sorting in Macrophage and T Cell Lines
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JoVE 杂志 免疫与感染
Gene Knock-in by CRISPR/Cas9 and Cell Sorting in Macrophage and T Cell Lines
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Gene Knock-in by CRISPR/Cas9 and Cell Sorting in Macrophage and T Cell Lines

DOI:
10.3791/62328-v

11:32 min

November 13, 2021

, , , , , , , , ,
1The Laboratory of Genetic Regulators in the Immune System, School of Laboratory Medicine,Xinxiang Medical University, 2Centre d’Immunologie de Marseille-Luminy,Aix Marseille Université

Chapters

  • 00:05Introduction
  • 00:32Design and Plasmid Construction of sgRNAs Targeting Rosa26 Locus
  • 02:28Design and Construction of Targeting Vector as Homologous Recombination Template
  • 03:46Electroporation of Macrophage and T Cell Lines
  • 07:19Cell Sorting to Isolate Putative Knock-in Cells
  • 08:58Screening and Validation of Positive Knock-in Cells
  • 10:16Representative Results
  • 10:52Conclusion

Summary

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This protocol uses fluorescent reporters and cell sorting to simplify knock-in experiments in macrophage and T cell lines. Two plasmids are used for these simplified knock-in experiments, namely a CRISPR/Cas9- and DsRed2-expressing plasmid and a homologous recombination donor plasmid expressing EBFP2, which is permanently integrated at the Rosa26 locus in immune cells.

Tags

CRISPR/Cas9Gene Knock-inMacrophageT Cell LinesROSA26 LocusSgRNA DesignHomologous RecombinationTargeting VectorFluorescent ReporterCell Sorting

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