Week8 8/1/10-8/7/10

From 2010.igem.org

(Difference between revisions)
Line 1: Line 1:
__NOTOC__
__NOTOC__
===Week8 Summary===
===Week8 Summary===
-
We tried our 3A assemblies using circular plasmid backbones extracted from the iGEM kit instead of the PCRed linear backbone plasmid. This solved our 3A assembly problem and all assemblies worked.
+
We tried our 3A assemblies using circular plasmid backbones extracted from the iGEM kit instead of the PCRed linear backbone plasmid. This solved our 3A assembly problem and all assemblies worked. We assembled our CP-LacPi inducible promoter parts. We also made competent ChiA knockout cells. We began assembling our (CP-LacPi)-(GFP) constructs to test/characterize the CP-LacPi parts. We assembled pMAL-CHS3 and tried to stain for chitin using calcofluor white.
 +
 
 +
----
===8/2/10===
===8/2/10===
Line 13: Line 15:
green should be - 3083, 933, 2150
green should be - 3083, 933, 2150
-
 
cP 3A Assembly troubleshooting: How to improve efficiency? Tried Phosphatase in parallel.
cP 3A Assembly troubleshooting: How to improve efficiency? Tried Phosphatase in parallel.
Line 55: Line 56:
Lysed and stained (pMal-CHS3) cells with calcofluor white --> for chitin
Lysed and stained (pMal-CHS3) cells with calcofluor white --> for chitin
-
Transformed ChiA knockout competent cells with _____ --> plan to test competency
+
Transformed ChiA knockout competent cells with pUC19 --> plan to test competency
----
----

Revision as of 21:28, 16 October 2010

Week8 Summary

We tried our 3A assemblies using circular plasmid backbones extracted from the iGEM kit instead of the PCRed linear backbone plasmid. This solved our 3A assembly problem and all assemblies worked. We assembled our CP-LacPi inducible promoter parts. We also made competent ChiA knockout cells. We began assembling our (CP-LacPi)-(GFP) constructs to test/characterize the CP-LacPi parts. We assembled pMAL-CHS3 and tried to stain for chitin using calcofluor white.


8/2/10

cP 3A Assembly troubleshooting: why are there white colonies? --> Ran Gel along with Red and Green (lacp-gfp in cpc)

1050 (rfp default insert), 2150 (bbp), 55+878 (lacp,gfp)

red should be - 3200, 1050, 2150

white should be - 2150

green should be - 3083, 933, 2150

cP 3A Assembly troubleshooting: How to improve efficiency? Tried Phosphatase in parallel.


8/3/10

Gel Results (White, Green, Red Colonies from 3A Assembly)

  • Red colonies look normal
  • Green colonies look normal
  • White colonies --> abnormal bands at 750bp, 1750bp, 2600bp, and 4300bp

The white colonies could be due to aggregation of GFP or RFP protein due to excessive amounts of plasmid.

Inoculated CP1-LacPi1, CP2-LacPi1, CP3-LacPi1, CP1-LacPi2, CP2-LacPi2, CP3-LacPi2, Holin1-XX, Holin2-XX, PMAL, GFP, LacPi1, LacPi2, YdgG Knockout, ChiA Knockout.


8/4/10

Miniprepped CP1-LacPi1, CP2-LacPi1, CP3-LacPi1, CP1-LacPi2, CP2-LacPi2, CP3-LacPi2, Holin1-XX, Holin2-XX, PMAL, GFP, LacPi1, LacPi2.

Miniprepped (CP1-Lacpi1) part --> digested with E/P --> ran a gel

  • Should be 35+1372/1370 = 1405/1407 +20(pre/suffix)

Miniprepped (Holin1-XX) and (Holin2-XX) part --> digested with E/P ran a gel

  • Should be 1257, 317 + 129 = 1386, 446 +20 (prefix/suffix)

Made glycerol stock of ________


8/5/10

Made competent ChiA knockout cells

Made electrocompetent ECNR2 cells

Minipreppred (pMal-CHS3) part

Assembled and transformed (CP1-LacPI1)-(GFP), (CP2-LacPI1)-(GFP),(CP3-LacPI1)-(GFP),(CP1-LacPI2)-(GFP),(CP2-LacPI2)-(GFP), (CP3-LacPI2)-(GFP)


8/6/10

Lysed and stained (pMal-CHS3) cells with calcofluor white --> for chitin

Transformed ChiA knockout competent cells with pUC19 --> plan to test competency