Phase 2: Plasmid Construction and Bacterial Transformations

From 2006.igem.org

(Difference between revisions)
Jump to: navigation, search
m
Line 4: Line 4:
<br>
<br>
'''2.  Ligated ComQX/P/A and Tsr fragments from Phase 1 into pSB1A3 plasmids'''
'''2.  Ligated ComQX/P/A and Tsr fragments from Phase 1 into pSB1A3 plasmids'''
-
::*Used SpeI and XbaI restriction sites
+
::*Cut at EcoRI, XbaI, and PstI restriction sites (cutting at XbaI site reduces background)
 +
::*pSB1A3 contains amp resistance
 +
::*Concentration of digested vector and inserts determined.  Ligations were set up for between 40:150 to 40ng:300ng ratio vector:insert
 +
<br><br>
 +
'''3.  Bacterial transformation'''
 +
::*Used ''E.coli'' strain XL-1 (null for all MCP receptors)
::*Verified transformation for all fragments and sequenced genes (results positive in all cases).
::*Verified transformation for all fragments and sequenced genes (results positive in all cases).
<br>
<br>
<br>
<br>
-
'''3.  Significance:
+
'''4.  Significance:
::*We now have all the fundamental components for the project ahead
::*We now have all the fundamental components for the project ahead
::*Can proceed in constructing the hybrid quorumtaxis receptor using ComP and Tsr genes
::*Can proceed in constructing the hybrid quorumtaxis receptor using ComP and Tsr genes
::*Will need to perform quick-change mutagenesis for ComA to remove internal SpeI site
::*Will need to perform quick-change mutagenesis for ComA to remove internal SpeI site
 +
<br><br>
 +
[[Rice University 2006|Back to Rice iGEM]]

Revision as of 22:28, 30 October 2006

1. Isolated ptetRBS and pSB1A3 plasmids from BioBricks

  • Attached tet promoter with Ribosome Binding Site to GFP gene, transformed XL-1 E. coli and observed positive expression



2. Ligated ComQX/P/A and Tsr fragments from Phase 1 into pSB1A3 plasmids

  • Cut at EcoRI, XbaI, and PstI restriction sites (cutting at XbaI site reduces background)
  • pSB1A3 contains amp resistance
  • Concentration of digested vector and inserts determined. Ligations were set up for between 40:150 to 40ng:300ng ratio vector:insert



3. Bacterial transformation

  • Used E.coli strain XL-1 (null for all MCP receptors)
  • Verified transformation for all fragments and sequenced genes (results positive in all cases).



4. Significance:

  • We now have all the fundamental components for the project ahead
  • Can proceed in constructing the hybrid quorumtaxis receptor using ComP and Tsr genes
  • Will need to perform quick-change mutagenesis for ComA to remove internal SpeI site



Back to Rice iGEM

Personal tools
Past/present/future years