Insulin Preparation

From Tanaka Wiki
Revision as of 12:09, 19 July 2018 by Benjamin.wachtel (talk | contribs)
(diff) ← Older revision | Latest revision (diff) | Newer revision → (diff)
Jump to navigation Jump to search
The printable version is no longer supported and may have rendering errors. Please update your browser bookmarks and please use the default browser print function instead.

Media for passaging A1 cells.

  • For 400 mls
  • FCS 40 ml
  • Eagle's MEM 252 ml
  • DdH2O 100 ml
  • 100xPen/Strep 2 ml
  • 100x Glutamine 2 ml
  • Insulin (stock 1 mg/ml) 2 ml

Insulin Materials:

  • 250 mg insulin (sigma I 5500)
  • 0.1 M HCL
  • 2x 400 ml tissue culture bottles
  • 225 ml APBS (4 parts PBS, 1 part ddH2O)
  • steri top 200ml
  • 6-7 50 ml conical tubes

Execution

  1. put the insulin powder into the 400 ml tissue culture bottle
  2. add 25 mls of 0.1 M HCL and swirl until dissolved
  3. while swirling slowly add 225 mls APBS ( final solution should be clear )
  4. filter sterilize the solution ( use the steri top )
  5. aliquot 4 ml per tube and store in freezer
  6. label the tubes with insulin (red)


Gelatin Materials:

  • Gelatin (Sigma, Porcine skin, 300 bloom)—in chemical room
  • 500 ml ddH2O
  • 2X500 ml Cell culture bottles
  • Water bath
  • Steritop
  • 12-13 50 ml conicals

Execution:

  1. Weigh 3.75 g gelatin and put into the bottle
  2. Add 500 ml ddH2O
  3. Mix and heat to 65 C for about 15 minutes
  4. Check that is all dissolved
  5. Under the tissue culture hood, while the gelatin is still hot, vacuum filter the gelatin into a new 500 ml bottle
  6. Aliquot the gelatin, 40 ml/conical tube
  7. Store at 4 C.
Retrieved from "https://wiki.tanakalab.org/index.php?title=Insulin_Preparation&oldid=880"