Human primary fibroblast culture

Ching-Chieh Chou, Judith Frydman

Published: 2023-11-09 DOI: 10.17504/protocols.io.36wgq3edklk5/v1

ASAPCRN

Fibroblast

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Abstract

This is a protocol for human primary fibroblast culture.

Steps

Preparing culture medium

1.

Fibroblast medium @4°C lasts for 1 month. A total of 500 mL:

  • 435 ml DMEM (High glucose, GlutaMAX) (Thermo Fisher Scientific)
  • 50 ml Fetal bovine serum (FBS) (Thermo Fisher Scientific)
  • 5 ml Penicillin-Streptomycin (Thermo Fisher Scientific)
  • 5 ml MEM NEAA (100X; Thermo Fisher Scientific)
  • 5 ml Sodium pyruvate (Thermo Fisher Scientific)
  • 0.5 ml beta-mercaptoethanol (Thermo Fisher Scientific)
  • Sterilized by filtration through a 0.22 µm filter

Thawing, subculturing and freezing fibroblasts

2.

Remove a cryogenic vial containing the frozen human primary fibroblasts from liquid nitrogen storage and thaw in a 37°C bead bath for a few min. Constantly check the content.

3.

After the content is thawed, immediately transfer and slowly add to a 15 mL conical tube containing 5 mL of cell culture medium.

4.

Centrifuge at 200xG for 5 min to pellet the cells.

5.

Remove the supernatant, add 10 mL of fresh culture medium for culturing cells in a 10-cm dish.

Note
If the cell numbers are low, recommend to first culture the cells in a well of a 6-well plate filled with 2 mL of fresh culture medium to improve cell survival and growth.

6.

Replace medium every 3-4 days. Fibroblasts should be confluent after one week.

7.

For subculturing, rinse the dish with sterile 1x PBS to remove all complete medium before splitting.

8.

Add 0.05% Trypsin-EDTA to cover the bottom of the dish. Incubate at 37°C with 5% CO2 for ~5 minutes. Cells should round up and become dislodged.

9.

Neutralize trypsin-EDTA activity by adding the complete media.

10.

Gently pipette to resuspend the cells and transfer the cell-containing medium to a 15 mL conical tube.

11.

Centrifuge at 200xG for 5 min to pellet the cells.

12.

Remove the supernatant, add fresh culture medium and split the cells at 1:3 ratio.

13.

Replace medium every 3 to 4 days. Fibroblasts should be 80 to 90% confluent after one week and ready for experiments.

Note
Avoid subculture at low-density as it will age the cells.

14.

If want to freeze the cells, after centrifugation (Step 11), remove the supernatant, and add 1 to 2 mL of Recovery Cell Culture Freezing Medium (Thermo Fisher Scientific).

Note
Recommend freezing cells at a high concentration.

15.

Gently pipette to resuspend the cells and transfer the cell-containing medium to a cryogenic vial. Then store the cryogenic vial in a cryo-freezing container that limits the decrease in temperature at ~1°C per min at -80°C.

16.

For long-term preservation, transfer the cryogenic vial from a -80°C freezer to a liquid nitrogen tank.

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