Team:Kyoto/Notebook

From 2013.igem.org

(Difference between revisions)
(LB Culture Medium)
(Ristriction Enzyme Proccessing)
Line 77: Line 77:
<small>by Kojima and Ashida</small><br>
<small>by Kojima and Ashida</small><br>
{|class="wikitable"  
{|class="wikitable"  
-
|8/20 Ptet -1(220μg/mL)||EcoRI||XbaI||10x BSA||10x buffer M||MilliQ||total
+
!8/20 Ptet -1(220μg/mL)!!EcoRI!!XbaI!!10x BSA!!10x buffer M!!MilliQ!!total
|-
|-
|4.5||1||1||3||3||17.5||30
|4.5||1||1||3||3||17.5||30
Line 88: Line 88:
|}
|}
{|class="wikitable"  
{|class="wikitable"  
-
|8/20 RBS-tetR-DT -2(182μg/mL)||EcoRI||SpeI||10x buffer H||MilliQ||total
+
!8/20 RBS-tetR-DT -2(182μg/mL)!!EcoRI!!SpeI!!10x buffer H!!MilliQ!!total
|-
|-
|5.5||1||1||3||19.5||30
|5.5||1||1||3||19.5||30
Line 99: Line 99:
|}
|}
{|class="wikitable"  
{|class="wikitable"  
-
|8/20 J23100-RBS-GFP-DT(334μg/ml)||EcoRI||SpeI||10x buffer H||MilliQ||total
+
!8/20 J23100-RBS-GFP-DT(334μg/ml)!!EcoRI!!SpeI!!10x buffer H!!MilliQ!!total
|-
|-
|3.0||1||1||3||22||30
|3.0||1||1||3||22||30
Line 110: Line 110:
|}
|}
{|class="wikitable"  
{|class="wikitable"  
-
|8/20 J23100-RBS-luxR-DT -2(344μg/mL)||EcoRI||XbaI||BSA||10x buffer M||MilliQ||total
+
!8/20 J23100-RBS-luxR-DT -2(344μg/mL)!!EcoRI!!XbaI!!BSA!!10x buffer M!!MilliQ!!total
|-
|-
|2.9||1||1||3||3||19.1||30
|2.9||1||1||3||3||19.1||30
Line 121: Line 121:
|}
|}
{|class="wikitable"  
{|class="wikitable"  
-
|8/20 RBS-lysis3 -1(282μg/mL)||EcoRI||SpeI||10x buffer H||MilliQ||total
+
!8/20 RBS-lysis3 -1(282μg/mL)!!EcoRI!!SpeI!!10x buffer H!!MilliQ!!total
|-
|-
|3.5||1||1||3||21.5||30
|3.5||1||1||3||21.5||30
Line 132: Line 132:
|}
|}
{|class="wikitable"  
{|class="wikitable"  
-
|8/17 DT -1(188μg/mL)||EcoRI||XbaI||10x BSA||10x buffer M||MilliQ||total
+
!8/17 DT -1(188μg/mL)!!EcoRI!!XbaI!!10x BSA!!10x buffer M!!MilliQ!!total
|-
|-
|5.3||1||1||3||3||16.7||30
|5.3||1||1||3||3||16.7||30

Revision as of 05:48, 21 August 2013

Home Team Official Team Profile Project Parts Submitted to the Registry Modeling Notebook Material and method Safety Attributions

""m&m""

Contents

RNA Oscillator

Turing Pattern

Aug 20

Miniprep

DNAconcentration[μg/μL]260/280260/230
8/18 Ptet -12201.691.87
8/18 Ptet -22101.691.71
8/18 RBS-tetR-DT -12361.631.69
8/18 RBS-tetR-DT -21821.651.98
8/18 J23100-RBS-GFP-DT -13341.712.12
8/18 J23100-RBS-luxR-DT -14401.671.60
8/18 J23100-RBS-luxR-DT -23441.681.83
8/18 J23100-RBS-lacZα-DT -12801.701.81
8/18 RBS-lysis3 -12821.671.76
8/18 RBS-lysis3 -22121.301.35

LB Culture Medium

by Okazaki
volume - 200mL

Bacto Trypton2g
Bacto yeast extract1g
Nacl1g
Agar Powder2g
Amp40μl

1.Measuring reagents and put they in the Erlenmeyer flask
2.diluting in measuring cylinder to 200ml total
3.autoclaving
4.adding ampicirine 40ml


not written yet

Ristriction Enzyme Proccessing

by Kojima and Ashida

8/20 Ptet -1(220μg/mL)EcoRIXbaI10x BSA10x buffer MMilliQtotal
4.5113317.530
0.50.20117.310
0.500.2117.310
0.500117.510
8/20 RBS-tetR-DT -2(182μg/mL)EcoRISpeI10x buffer HMilliQtotal
5.511319.530
0.60.2018.210
0.600.218.210
0.60018.410
8/20 J23100-RBS-GFP-DT(334μg/ml)EcoRISpeI10x buffer HMilliQtotal
3.01132230
0.30.2018.510
0.300.218.510
0.30018.710
8/20 J23100-RBS-luxR-DT -2(344μg/mL)EcoRIXbaIBSA10x buffer MMilliQtotal
2.9113319.130
0.30.20117.510
0.300.2117.510
0.300117.710
8/20 RBS-lysis3 -1(282μg/mL)EcoRISpeI10x buffer HMilliQtotal
3.511321.530
0.40.2018.410
0.400.218.410
0.40018.610
8/17 DT -1(188μg/mL)EcoRIXbaI10x BSA10x buffer MMilliQtotal
5.3113316.730
0.30.20117.510
0.300.2117.510
0.300117.710

incubate ~20:00

Transformation

Electrophoresis

Retrieved from "http://2013.igem.org/Team:Kyoto/Notebook"