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Viral-Mediated Labeling and Transplantation of Medial Ganglionic Eminence Cells for In Vivo Studies

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Harvest the medial ganglionic eminence tissue, containing cortical interneuron progenitors, from genetically modified mouse embryos. 

Add a cationic polymer and dissociate the tissue into a single-cell suspension.

Add lentiviral vectors carrying a Cre recombinase-dependent GFP reporter flanked by lox sites. Incubate.

The polymer neutralizes the viral- and host-cell-membrane charges, enabling viral fusion and RNA release.

The viral RNA is reverse-transcribed and integrated into the host genome.

Centrifuge and discard the supernatant. Absorb excess media.

Transfer the cells to a hydrophobic surface and load them into an injection device.

Inject the cells into an anesthetized mouse pup's cortex.

Allow the pup to recover and grow.

The transplanted progenitors differentiate into mature interneurons in the cortex.

A subgroup of these interneurons co-expresses Cre recombinase and RFP.

In these interneurons, Cre excises the lox sites, flipping the GFP gene and enabling its expression.

Visualize the RFP and GFP co-expression to identify Cre-expressing interneurons.

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Viral-Mediated Labeling and Transplantation of Medial Ganglionic Eminence Cells for In Vivo Studies

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