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Generating Neurons by Reprogramming Human Dermal Fibroblast Cells


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Prepare a cellular suspension of 1,320,000 cells in 13.2 milliliters of fibroblast medium in order to achieve 100,000 cells per milliliter of medium. After aspirating the gelatin from the plate, wash the plate with Dulbecco's phosphate-buffered saline twice. Then, add 500 microliters of cell suspension to each of the wells, and incubate at 37 degrees Celsius overnight.

Warm 13.2 milliliters of fibroblast medium to 37 degrees Celsius. Then, thaw the lentiviral vector in the laminar hood at room temperature. Add the required volume of lentivirus necessary to infect the adult human dermal fibroblasts at a multiplicity of infection of 20 to the medium without any transduction enhancers.

Then, replace the medium with 500 microliters of fibroblast medium with the addition of the lentiviral vector. Incubate the plate at 37 degrees Celsius overnight. The following day, replace the medium containing lentivirus with fresh fibroblast medium without the lentiviral vector. On the third day after viral transduction, remove the fibroblast medium and add 500 microliters of early neuronal conversion medium.

Twice or thrice a week, replace 225 microliters of old medium from each well with 250 microliters of fresh, early neuronal conversion medium. On the 18th day after viral transduction, remove the early neuronal conversion medium and replace with 500 microliters of late neuronal conversion medium. Keep changing the medium every two to three days as before until the 25th day or the experimental endpoint.

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