Difference between revisions of "Transfecting Cells"

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* Work deep inside the hood
 
* Work deep inside the hood
  
===Steps===
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===Transfection mix (for this example)===
Transfection mix (for this example)
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#Take sterile tubes for as many transfections you have, label (in this example we needed six tubes)
Take sterile tubes for as many transfections you have, label
+
#Put 150 ul of media into tubes  
In this example we needed six tubes
+
(You can reuse the tip if you don’t touch anything)
Put 150 ul of media into tubes  
+
# Make sure you don’t go over any open tubes or bottles, close tubes and bottles right away
You can reuse the tip if you don’t touch anything
+
# Into the 150 ul of media add about 1-2 ug of DNA (optimize DNA concentration first)
Make sure you don’t go over any open tubes or bottles, close tubes and bottles right away
+
# Tap gently to mix
Into the 150 ul of media add about 1-2 ug of DNA (optimize DNA concentration first)
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# Add 6.5 ul of lipofectamine (transfection media)  
Tap gently to mix
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# Pipette directly in the tube, flush, and tap
Add 6.5 ul of lipofectamine (transfection media)  
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# re-cap / close
Pipette directly in the tube, flush, and tap
+
# Let it sit for 5-10 minutes (helps enhance transfection efficiency)  
re-cap / close
+
# After optional 5-10 minutes, grab cell plates from incubator (careful not to open lid yet)
Let it sit for 5-10 minutes (helps enhance transfection efficiency)  
+
# Make sure tubes and plates are in order (1-6), set pipette to 170 (ish) ul, take up media from tube and add to plate (pipette at an angle so nothing falls in) spread media in drops in a circle  
After optional 5-10 minutes, grab cell plates from incubator (careful not to open lid yet)
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# Give the dishes a gentle swirl, and place in incubator for a minimum of 24 hours and a maximum of three days. After 24 hours the DNa will be taken up, but after three days they will over grow and die
Make sure tubes and plates are in order (1-6), set pipette to 170 (ish) ul, take up media from tube and add to plate (pipette at an angle so nothing falls in) spread media in drops in a circle  
+
Give the dishes a gentle swirl, and place in incubator for a minimum of 24 hours and a maximum of three days. After 24 hours the DNa will be taken up, but after three days they will over grow and die
+

Latest revision as of 21:30, 20 July 2018

Summary

Cos 1 (African green monkey, from kidney cells). Cells are heterozygous, they all look different. We are transfecting Cos 1, 6 cm plates

  • Make sure everything is clean and sterile

Materials

  • DNA, transfection lipofectamine 2000
  • Antibiotic free DMEM (no serum), kept in the fridge
  • Sterile tips, tubes, pipettes (sprayed)
  • Make sure cells are 50-70% confluent
  • Work deep inside the hood

Transfection mix (for this example)

  1. Take sterile tubes for as many transfections you have, label (in this example we needed six tubes)
  2. Put 150 ul of media into tubes

(You can reuse the tip if you don’t touch anything)

  1. Make sure you don’t go over any open tubes or bottles, close tubes and bottles right away
  2. Into the 150 ul of media add about 1-2 ug of DNA (optimize DNA concentration first)
  3. Tap gently to mix
  4. Add 6.5 ul of lipofectamine (transfection media)
  5. Pipette directly in the tube, flush, and tap
  6. re-cap / close
  7. Let it sit for 5-10 minutes (helps enhance transfection efficiency)
  8. After optional 5-10 minutes, grab cell plates from incubator (careful not to open lid yet)
  9. Make sure tubes and plates are in order (1-6), set pipette to 170 (ish) ul, take up media from tube and add to plate (pipette at an angle so nothing falls in) spread media in drops in a circle
  10. Give the dishes a gentle swirl, and place in incubator for a minimum of 24 hours and a maximum of three days. After 24 hours the DNa will be taken up, but after three days they will over grow and die