Team:BCCS-Bristol/Notebook

From 2009.igem.org

(Difference between revisions)
(10 July 2009)
Line 1: Line 1:
{{:Team:BCCS-Bristol/Header}}
{{:Team:BCCS-Bristol/Header}}
-
==Time Line of Wet-Lab Procedures==
 
-
{| style="color:white; background-color:#0066CC;" cellpadding="20" cellspacing="0" border="2"
+
===Week Zero===
-
!Date
+
-
!Panayiotis
+
-
!Petros
+
-
|-
+
-
|10 July '09
+
-
|Familiarisation with standard lab procedures the past week (bacterial culture growth, Restriction Enzyme Usage, Agarose Gel Electrophoresis)
+
-
|Will start designing some biobricks for the project.
+
-
|}
+
-
===10 July 2009===
+
*Familiarising with standard lab procedures for the past week (bacterial culture growth, restriction enzyme usage, agarose gel electrophoresis).
-
*Panayiotis has been familiarising himself with standard lab procedures for the past week (bacterial culture growth, restriction enzyme usage, agarose gel electrophoresis).
+
*Will start designing some biobricks for the project today.
-
*Petros will start designing some biobricks for the project today.
+
===Week 1===
 +
 
 +
*Isolated 3 canditate proteins to act as carriers for our biobricks. These are FhuA,Fiu & OsmE. Started to design primers to amplify the selected genes via PCR.
 +
 
 +
*Primers designed and ordered. Waiting for their arrival to do PCR! :D
 +
 
 +
*Decided to use 3 reporter genes, 1 RBS, 1 High Copy plasmid backbone for now.
 +
====Reporters====
 +
*RFP(Bba_E1010)
 +
*GFP(Bba_E1040)
 +
*LacZ(Bba_I732005)
 +
====RBS====
 +
*Bba_J61100 - From Anderson Family
 +
====Plasmid Backbone====
 +
*BBa_J04450 ; pSB1A3
 +
 
 +
*Tried to extract DNA from the iGEM biobricks and transfrom into bacteria.
 +
 
 +
*Transformation do not work properly with non-commercial E.coli strain (XL-1).
 +
 
 +
*Transformations worked the 2nd time round with commercial Nova Blue E.coli Strain. DNA samples in toolkit must be of low concentrations!
 +
 
 +
*Regrew bacterial colonies to amplify DNA of reporters,RBS,backbone.
 +
 
 +
*Miniprepped the DNA and made glycerol stocks.
 +
 
 +
*Realised that we are faced with a problem when wanting to assemble biobricks for protein fusions.
 +
 
 +
===Week 2===
 +
 
 +
*Primers finally arrived. Did PCR to amplify carrier genes.
 +
 
 +
*PCR worked. Restricted DNA and inserted into biobrick backbone pSB1A3.
 +
 
 +
*Started working on finding an easy assembly method for in-line protein fusions.
 +
 
 +
*Developed the design for a Bioscaffold-Linker transformer family (inspired by Bioscaffolds). Should allow fusions of proteins and all RFC10 biobricks in-frame after using Bioscaffold specific restriction enzymes.
 +
 
 +
*

Revision as of 09:14, 24 July 2009

BCCS-Bristol
iGEM 2009


Contents

Week Zero

  • Familiarising with standard lab procedures for the past week (bacterial culture growth, restriction enzyme usage, agarose gel electrophoresis).
  • Will start designing some biobricks for the project today.

Week 1

  • Isolated 3 canditate proteins to act as carriers for our biobricks. These are FhuA,Fiu & OsmE. Started to design primers to amplify the selected genes via PCR.
  • Primers designed and ordered. Waiting for their arrival to do PCR! :D
  • Decided to use 3 reporter genes, 1 RBS, 1 High Copy plasmid backbone for now.

Reporters

*RFP(Bba_E1010)
*GFP(Bba_E1040)
*LacZ(Bba_I732005)

RBS

*Bba_J61100 - From Anderson Family

Plasmid Backbone

*BBa_J04450 ; pSB1A3
  • Tried to extract DNA from the iGEM biobricks and transfrom into bacteria.
  • Transformation do not work properly with non-commercial E.coli strain (XL-1).
  • Transformations worked the 2nd time round with commercial Nova Blue E.coli Strain. DNA samples in toolkit must be of low concentrations!
  • Regrew bacterial colonies to amplify DNA of reporters,RBS,backbone.
  • Miniprepped the DNA and made glycerol stocks.
  • Realised that we are faced with a problem when wanting to assemble biobricks for protein fusions.

Week 2

  • Primers finally arrived. Did PCR to amplify carrier genes.
  • PCR worked. Restricted DNA and inserted into biobrick backbone pSB1A3.
  • Started working on finding an easy assembly method for in-line protein fusions.
  • Developed the design for a Bioscaffold-Linker transformer family (inspired by Bioscaffolds). Should allow fusions of proteins and all RFC10 biobricks in-frame after using Bioscaffold specific restriction enzymes.
Retrieved from "http://2009.igem.org/Team:BCCS-Bristol/Notebook"