Modified myotube prep: Difference between revisions

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If desired, myotubes can be purified away from contaminating mononucleate cells and replated using the following procedure.  The yield from 2 x 10 cm plates of myotubes should be about 5,000-10,000 myotubes. Myotubes should be plated onto a fibronectin coated substratum.
If desired, myotubes can be purified away from contaminating mononucleate cells and replated using the following procedure.  The yield from 2 x 10 cm plates of myotubes should be about 5,000-10,000 myotubes. Myotubes should be plated onto a fibronectin coated substratum.


== Materials ==
== Material ==
* 1 x 0,5%  serum AEMEM (low serum media)
* 1 x 0,5 %  serum AEMEM (low serum media)
* 2 x 100 um filters cut into 2 cm  x 2 cm squares
* 2 x 100 um filters cut into 2 cm  x 2 cm squares
* 2 x 35 um filters
* 2 x 35 um filters
* 1 x 6cm plate containing 2mls of low serum media (0,5% serum AEMEM)
* 1 x 6 cm plate containing 2mls of low serum media (0,5% serum AEMEM)
* 1 x 96 well plate coated  with 20 µg/ml fibronectin in SF media
* 1 x 96 well plate coated  with 20 µg/ml fibronectin in SF media
* 1 x scalpel number 22
* 1 x scalpel number 22
* 1 x tweezers
* 1 x tweezers
* 5 x universal (25 ml) tubes,  
* 5 x universal (25 ml) tubes,  
* 1 x TE (trypsin –edta )
* 1 x TE (trypsin – edta )
* 1 x APBS (100 ml PBS + 25 ml ddH2O
* 1 x APBS (100 ml PBS + 25 ml ddH2O
*    sterile pipettes(2* 5mls, 2*10mls, 1*20mls)
*    sterile pipettes(2 * 5mls, 2 * 10mls, 1 * 20mls)
*    sterile pasteur pipettes unplugged
*    sterile pasteur pipettes unplugged
* 2 x 60 ul of fibronectin at 1mg/ml (in –20 degrees C freezer, drawer number 3 )
* 2 x 60 ul of fibronectin at 1mg/ml (in –20 degrees C freezer, drawer number 3 )
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== Execution ==
== Procedure ==
1 Put 3.3mls SF MEM  into the 5ml tube add 1 tube of fibronectin , mix (thaw fibronectin on ice)
# Put 3.3mls SF MEM  into the 5ml tube add 1 tube of fibronectin , mix (thaw fibronectin on ice)
2
# (Using multipipette 500ul) put 30ul of fibronectin mix in each well of the 96 well plate, distribute the liquid so that it wets the bottom evenly
(Using multipipette 500ul) put 30ul of fibronectin mix in each  
# Incubate at RT for at least 2 hours ( or overnight at 4 degrees C )
well of the 96 well plate, distribute the liquid so that it  
# Label the universal tubes:2 with “100um”, 2 with “35 um” and 1 with” myotubes”
wets the bottom evenly
# Put filters on the tubes and fix  at 3 points  with a hot scalpel ( leave the scalpel for 20 seconds in the flame, wait 8 sec., then use hot blade to melt filter onto the top of the tube )
# Put 9 mls low serum media in universal tube “ myotube” and 2 mls low serum media in the 6 cm plate
3
# Check myotubes on microscope
Incubate at RT for at least 2 hours ( or overnight at 4 degrees C )
# Take 2 X10 cm plate of myotubes and aspirate off the media
4 Label the universal tubes:2 with “100um”, 2 with “35 um”
# Rinse the myotubes with 5mls APBS (aspirate)
and 1 with” myotubes”
# Add 2mlTE to each plate-trypsinize very briefly until chunks of cells start coming off
5 Put filters on the tubes and fix  at 3 points  with a hot
# Quickly stop TE with 6mls low serum  media
scalpel ( leave the scalpel for 20 seconds in the flame, wait 8 sec., then use hot blade to melt filter onto the top of the tube )
# Detach cells from plate, using pipette
6 Put 9 mls low serum media in universal tube “ myotube”
# Slowly pipette the liquid through the 100 um filter, rinse with 2 mls low serum media (do it with both tube)
and 2 mls low serum media in the 6 cm plate
# Remove 100 um filters from the tubes
7 Check myotubes on microscope
# Drip a small volume of L. S. media through the 35 um filter
8 Take 2 X10 cm plate of myotubes and aspirate off the media
# Pipette the filtrate through the 35um filter and wash with 2 mls of low serum media
9 Rinse the myotubes with 5mls APBS (aspirate)
# Place filter face down in a 6cm dish
10 Add 2mlTE to each plate-trypsinize very briefly until chunks of cells start coming off
# Wash the filter with 2mls low serum (and then discard the filter)  
11 Quickly stop TE with 6mls low serum  media
# Repeat steps 14-16 with the other tube
12 Detach cells from plate, using pipette
# Then pipette the liquid  from the 6cm plate and put it into the myotube tube , wash  the plate with some low serum media from the “ myotube”
13 Slowly pipette the liquid through the 100 um filter, rinse  
# Aspirate off the fibronectin  from the 96 well-plate
with 2 mls low serum media ( do it with both tubes )
# Cut off tip of 5 ml pipette
14 Remove 100 um filters from the tubes
# (Using multipipette) put 150 ul per well from “ myotube” into each well of the 96 well plate
15 Drip a small volume of L. S. media through the 35 um filter
# Look in the microscope for myotubes
16 Pipette the filtrate through the 35um filter and wash with 2 mls of low serum media
# Label the 96 well-plate with name, date and myotube in low serum ( L. S. )
17 Place filter face down in a 6cm dish
# Put cells in incubator
18 Wash the filter with 2mls low serum( and then discard
the filter),
19 Repeat steps 14-16 with the other tube
20
Then pipette the liquid  from the 6cm plate and put it into  
the myotube tube , wash  the plate with some low serum
media from the “ myotube”
21 Aspirate off the fibronectin  from the 96 well-plate
22 Cut off tip of 5 ml pipette
23 ( Using multipipette) put 150 ul per well from “ myotube” into each well of the 96 well plate
24 Look in the microscope for myotubes
25 Label the 96 well-plate with name,date and
                          myotube in low serum ( L. S. )
26 Put cells in incubator


Notes:
''Notes:''
(Date and passage number on the 10 cm dish)
(Date and passage number on the 10 cm dish)

Latest revision as of 14:24, 8 June 2015

Induce A1 cells on 10 cm plates to form myotubes by

  • wash 1x with 5 mls APBS
  • changing the media to 0.5% serum-AMEM
  • wait 4 days

If desired, myotubes can be purified away from contaminating mononucleate cells and replated using the following procedure. The yield from 2 x 10 cm plates of myotubes should be about 5,000-10,000 myotubes. Myotubes should be plated onto a fibronectin coated substratum.

Material

  • 1 x 0,5 % serum AEMEM (low serum media)
  • 2 x 100 um filters cut into 2 cm x 2 cm squares
  • 2 x 35 um filters
  • 1 x 6 cm plate containing 2mls of low serum media (0,5% serum AEMEM)
  • 1 x 96 well plate coated with 20 µg/ml fibronectin in SF media
  • 1 x scalpel number 22
  • 1 x tweezers
  • 5 x universal (25 ml) tubes,
  • 1 x TE (trypsin – edta )
  • 1 x APBS (100 ml PBS + 25 ml ddH2O
  • sterile pipettes(2 * 5mls, 2 * 10mls, 1 * 20mls)
  • sterile pasteur pipettes unplugged
  • 2 x 60 ul of fibronectin at 1mg/ml (in –20 degrees C freezer, drawer number 3 )
  • 1 x 4 ml tube
  • 500ul multipipette tip
  • 5ul multipipette tip
  • multipipette plus
  • microscope


Procedure

  1. Put 3.3mls SF MEM into the 5ml tube add 1 tube of fibronectin , mix (thaw fibronectin on ice)
  2. (Using multipipette 500ul) put 30ul of fibronectin mix in each well of the 96 well plate, distribute the liquid so that it wets the bottom evenly
  3. Incubate at RT for at least 2 hours ( or overnight at 4 degrees C )
  4. Label the universal tubes:2 with “100um”, 2 with “35 um” and 1 with” myotubes”
  5. Put filters on the tubes and fix at 3 points with a hot scalpel ( leave the scalpel for 20 seconds in the flame, wait 8 sec., then use hot blade to melt filter onto the top of the tube )
  6. Put 9 mls low serum media in universal tube “ myotube” and 2 mls low serum media in the 6 cm plate
  7. Check myotubes on microscope
  8. Take 2 X10 cm plate of myotubes and aspirate off the media
  9. Rinse the myotubes with 5mls APBS (aspirate)
  10. Add 2mlTE to each plate-trypsinize very briefly until chunks of cells start coming off
  11. Quickly stop TE with 6mls low serum media
  12. Detach cells from plate, using pipette
  13. Slowly pipette the liquid through the 100 um filter, rinse with 2 mls low serum media (do it with both tube)
  14. Remove 100 um filters from the tubes
  15. Drip a small volume of L. S. media through the 35 um filter
  16. Pipette the filtrate through the 35um filter and wash with 2 mls of low serum media
  17. Place filter face down in a 6cm dish
  18. Wash the filter with 2mls low serum (and then discard the filter)
  19. Repeat steps 14-16 with the other tube
  20. Then pipette the liquid from the 6cm plate and put it into the myotube tube , wash the plate with some low serum media from the “ myotube”
  21. Aspirate off the fibronectin from the 96 well-plate
  22. Cut off tip of 5 ml pipette
  23. (Using multipipette) put 150 ul per well from “ myotube” into each well of the 96 well plate
  24. Look in the microscope for myotubes
  25. Label the 96 well-plate with name, date and myotube in low serum ( L. S. )
  26. Put cells in incubator

Notes: (Date and passage number on the 10 cm dish)