21/08/13

From 2013.igem.org

(Difference between revisions)
(hydrodynamic shearing of Herring Sperm DNA)
 
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*20ul of lysozyme was added to each of these 8 samples.
*20ul of lysozyme was added to each of these 8 samples.
* A maxwell robot was then used to complete the DNA extraction process.
* A maxwell robot was then used to complete the DNA extraction process.
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==hydrodynamic shearing of Herring Sperm DNA==
+
==Hydrodynamic shearing of Herring Sperm DNA==
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*a 20G syringe was used ~24 times squirt the herring sperm DNA in order to make it less viscous.
+
*A 20G syringe was used ~24 times to squirt the herring sperm DNA in order to make it less viscous.
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*30G syringe was also used .
+
*30G syringe was also used  
*This method seems to work better than the sonification.
*This method seems to work better than the sonification.

Latest revision as of 13:55, 22 August 2013

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Reculturing Bacteria

  • The P. putida grew overnight, which proved that we had viable cells.
  • The bacteria was then re-streaked to single colonies and left to grow overnight in a 37C incubator.

Isolation of P. putida DNA

  • 8 1.5ml samples were isolated from each of the 2 broths that were prepared yesterday.
  • The first few steps of CTAB protocol was used to prep cells for DNA isolation;
  • The 8 samples were spun down at 10000 rpm for 5 mins.
  • The supernatant was discarded.
  • cells were then resuspended in 1ml of TE.
  • 740ul of this new mixture was transferred to 8 new eppendorf tubes.
  • 20ul of lysozyme was added to each of these 8 samples.
  • A maxwell robot was then used to complete the DNA extraction process.

Hydrodynamic shearing of Herring Sperm DNA

  • A 20G syringe was used ~24 times to squirt the herring sperm DNA in order to make it less viscous.
  • 30G syringe was also used
  • This method seems to work better than the sonification.