User:Puja Mody/Notebook/Chem 571: Gold Nanoparticles/2012/11/06: Difference between revisions
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==Procedure== | ==Procedure== | ||
* Please refer to the [[User:Puja Mody/Notebook/Chem 571: Gold Nanoparticles/2012/09/26| | * Please refer to the FPLC [[User:Puja Mody/Notebook/Chem 571: Gold Nanoparticles/2012/09/26| instructions]] that was previously employed. No changes were made in this procedure. 3 fracs of ADA were collected. Frac 2 had the most protein present with small amounts present in fracs 1 and 3. The only difference this time was that because there were not two separate samples of protein, everything could be run through the FPLC at once. the flow rate was 5mL/minute | ||
* The transformation and plating of PCR product that was done on [[User:Puja Mody/Notebook/Chem 571: Gold Nanoparticles/2012/10/24| 2012/10/24]] was unsuccessful and had to be repeated. the Original protocol for PCR mutation can be found [[AU Biomaterials Design Lab:Protocols/PCR Mutation Protocol| here]]. The following modifications were made: | * The transformation and plating of PCR product that was done on [[User:Puja Mody/Notebook/Chem 571: Gold Nanoparticles/2012/10/24| 2012/10/24]] was unsuccessful and had to be repeated. the Original protocol for PCR mutation can be found [[AU Biomaterials Design Lab:Protocols/PCR Mutation Protocol| here]]. The following modifications were made: | ||
**20μL DNA solution was added to 30μL solution with E. Coli cells. | **20μL DNA solution was added to 30μL solution with E. Coli cells. |
Revision as of 12:34, 24 November 2012
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FPLC and TransformationGoals
Procedure
Conclusions |