Team:Tokyo Metropolitan/Notebook/Pattern/2010/08/30

From 2010.igem.org

Revision as of 06:21, 28 September 2010 by Mizuki (Talk | contribs)


Contents

2010/08/30

1:PCR

<Member>
Mariko, Hitomi, Taka


<Sample>
・E-coli (having BBa_I13521 plasmid)

・E-coli (having BBa_K208017 plasmid)

・E-coli JM109 (NIPPON GENE)


<Protocol>
See Protocol 2

・Tube (temperature in annealing)
1.Promoter~signal (72.0℃)
3. mRFP~Terminator (69.0)
4. Promoter (70.0)
5. RBS~signal (70.0)
7. Terminator (69.0/67.5/66.0)
8. CRP (72.5)

Total 8 tubes.


2:DNA Digestion

<Member>
nito


<Sample, Materials>
・PCR productions

  • 1L(8/25) 8μl
  • 2L(8/26) 8μl
  • 4H(8/26) 16μl
  • 5H(8/26) 16μl

・Digest enzyme

  • AvrⅡ
  • NheⅠ
  • SpeⅠ


<Protocol>
See Protocol 9


3:Electrophoresis

<Member>
Mariko, Taka


<Sample>
・PCR products


<Protocol>
SeeProtocol 8


<Result>
File:Matsuura 2010-08-30 15hr 17min.tif

4:Electrophoresis

<Member>
nito


<Sample>

  • 1L(8/25)
  • 2L(8/26)
  • 4H(8/26)
  • 5H(8/26)

(after digestion)


<Protocol>
SeeProtocol 8

And cut off gels included DNA.

<Result>
File:Matsuura 2010-08-30 15hr 59min.tif

5:DNA Ligation

<Member>
nito


<Sample>

  • 1L(8/25)
  • 2L(8/26)
  • 4H(8/26)
  • 5H(8/26)

(after digestion)


<Protocol>
See Protocol 3

We ligated 1 and 2, 4 and 5.


6:Electrophoresis

<Member>
nito


<Sample>

  • 1L(8/25)
  • 2L(8/26)
  • 4H(8/26)
  • 5H(8/26)

(after ligation)


<Protocol>
SeeProtocol 8


<Result>
Matsuura 2010-08-06 20hr 02min (8).JPG