Cardiomyocyte Preparation: Difference between revisions

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# Wash ventricles in 70% Leibovitz-15 (L15) medium (AL15) w/ pen-strep
# Wash ventricles in 70% Leibovitz-15 (L15) medium (AL15) w/ pen-strep
# Store ventricles O.N. at 25C in AL15 w/ pen-strep
# Store ventricles O.N. at 25C in AL15 w/ pen-strep
# Digest ventricles 2ml d.sol for 8h in a shaking water bath at 27C. Change the enzyme solution every 1-2h.
# Digest ventricles 2ml d.sol
''Note: D.sol''
* aPBS w/
* aPBS w/
* 0.5% Bactotrypsin (Difco)
* 0.5% Bactotrypsin (Difco)
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* 0.3% glucose  
* 0.3% glucose  
* gentamycin (50ug/ml)
* gentamycin (50ug/ml)
for 8h in a shaking water bath at 27C. Change the enzyme solution every 1-2h.
# Neutralize cell suspensions w/ complete  4ml AL-15 medium (AL-15 w/ 10% FBS and pen-strep)
# Neutralize cell suspensions w/ complete  4ml AL-15 medium (AL-15 w/ 10% FBS and pen-strep)
# Pass through a 100um microsieve (reason for this???? And what to collect – flowthrough or the retenate… cardiomyocytes are min 150um in length…)
# Pass through a 100um microsieve (reason for this???? And what to collect – flowthrough or the retenate… cardiomyocytes are min 150um in length…)

Revision as of 08:44, 11 March 2015

(Bettencourt-Dias & Laube F combined)

Procedure:

  1. Collect hearts in 70% Leibovitz-15 (L15) medium (AL15) w/ pen-strep
  2. Wash them once in 70% Leibovitz-15 (L15) medium (AL15) w/ pen-strep
  3. Remove the newt ventricles
  4. Wash ventricles in 70% Leibovitz-15 (L15) medium (AL15) w/ pen-strep
  5. Store ventricles O.N. at 25C in AL15 w/ pen-strep
  6. Digest ventricles 2ml d.sol
  • aPBS w/
  • 0.5% Bactotrypsin (Difco)
  • 380U/ml collagenase (Sigma)
  • 0.15% BSA
  • 0.3% glucose
  • gentamycin (50ug/ml)

for 8h in a shaking water bath at 27C. Change the enzyme solution every 1-2h.

  1. Neutralize cell suspensions w/ complete 4ml AL-15 medium (AL-15 w/ 10% FBS and pen-strep)
  2. Pass through a 100um microsieve (reason for this???? And what to collect – flowthrough or the retenate… cardiomyocytes are min 150um in length…)
  3. Centrifuge the neutralized suspensions for 10min at 500 rpm .
  4. Resuspend in complete AL15 (volume???)
  5. preplate in uncoated 6cm culture dishes for 3 days at 25C in a humidified CO2 incubator. Note: Blood cells, connective tissue and some pigmented cells attach to the culture dish during this step, while the cardiomyocytes remain in suspension (non-adhere)
  6. Transfer the supernatant onto laminin coated dishes (15ug/ml in serum-free medium, coating for 60 min) *at a density of 4000 cells/cm2* (is it necessary at such density?)
  7. Change the medium only when 3 days have passed since plating.