Template:Kyoto/Notebook/Aug 21

From 2013.igem.org

(Difference between revisions)

Latest revision as of 03:45, 28 September 2013

Aug 21

Plusgrow Medium

Tatsui

material

8/17 Plusgrow medium 50ml
7/22 5000x Ampicillin 10µl

Measuring materials and putting them in a 50ml tube

Liquid culture

Tatsui

Sample	medium
8/20 tRNA-spinach -(1)	8/21 Plusgrow medium(+Amp)
8/20 tRNA-spinach -(2)	8/21 Plusgrow medium(+Amp)
8/20 TetR-aptamer 12_P(1076) -(1)	8/21 Plusgrow medium(+Amp)
8/20 TetR-aptamer 12_P(1076) -(2)	8/21 Plusgrow medium(+Amp)
8/20 TetR-aptamer 12_1R(113) -(1)	8/21 Plusgrow medium(+Amp)
8/20 TetR-aptamer 12_1R(113) -(2)	8/21 Plusgrow medium(+Amp)
8/20 TetR-aptamer 12_1M(105) -(1)	8/21 Plusgrow medium(+Amp)
8/20 TetR-aptamer 12_1M(105) -(2)	8/21 Plusgrow medium(+Amp)
8/20 PT181 attenuator -(1)	8/21 Plusgrow medium(+Amp)
8/20 PT181 attenuator -(2)	8/21 Plusgrow medium(+Amp)
8/20 Fusion1 attenuator -(1)	8/21 Plusgrow medium(+Amp)
8/20 Fusion1 attenuator -(2)	8/21 Plusgrow medium(+Amp)
8/20 Fusion3m2 attenuator -(1)	8/21 Plusgrow medium(+Amp)
8/20 Fusion3m2 attenuator -(2)	8/21 Plusgrow medium(+Amp)
8/20 PT181 antisense -(1)	8/21 Plusgrow medium(+Amp)
8/20 PT181 antisense -(2)	8/21 Plusgrow medium(+Amp)
8/20 Fusion1 antisense -(1)	8/21 Plusgrow medium(+Amp)
8/20 Fusion1 antisense -(2)	8/21 Plusgrow medium(+Amp)
8/20 Fusion6 antisense -(1)	8/21 Plusgrow medium(+Amp)
8/20 Fusion6 antisense -(2)	8/21 Plusgrow medium(+Amp)

incubate 37°C 10hour

Gel Extraction

Nakamoto and Tatsui

Lane	DNA	Enzyme
1	1kbp ladder	--
2	8/20 Ptet -(1)	EcoRI & XbaI
3	8/20 Ptet -(1)	EcoRI & XbaI
5	8/20 RBS-tetR-DT -(2)	EcoRI & SpeI
6	8/20 RBS-tetR-DT -(2)	EcoRI & SpeI
8	8/20 Pconst-RBS-GFP-DT -(1)	EcoRI & SpeI
9	8/20 Pconst-RBS-GFP-DT -(1)	EcoRI & SpeI
11	8/20 RBS-lysis3 -(1)	EcoRI & SpeI
12	8/20 RBS-lysis3 -(1)	EcoRI & SpeI

Name	concentration[µg/mL]	260/280	260/230
Ptet (EcoRI & XbaI)	21	1.55	0.78
RBS-tetR-DT (EcoRI & SpeI)	12	1.45	0.62
Pconst-RBS-GFP-DT (EcoRI & SpeI)	11	1.36	0.60
RBS-lysis3 (EcoRI & SpeI)	10	1.26	0.50

Ristriction Enzyme Digestion

Kojima and Nakamoto

	8/20 Ptet-(1)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
2 cuts	4.5	1	1	3	3	17.5	30
1 cut	0.5	0.2	0	1	1	7.3	10
1 cut	0.5	0	0.2	1	1	7.3	10
NC	0.5	0	0	1	1	7.5	10

	8/20 Pconst-RBS-luxR-DT-(2)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
2 cuts	2.9	1	1	3	3	19.1	30
1 cut	0.3	0.2	0	1	1	7.5	10
1 cut	0.3	0	0.2	1	1	7.5	10
NC	0.3	0	0	1	1	7.7	10

	8/17 DT	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
2 cuts	5.3	1	1	3	3	16.7	30
1 cut	0.5	0.2	0	1	1	7.3	10
1 cut	0.5	0	0.2	1	1	7.3	10
NC	0.5	0	0	1	1	7.5	10

incubate at 37°C for 1h

Electrophoresis

Kojima and Nakamoto

Lane	Sample	Enzyme1	Enzyme2
1	1kbp ladder	--	--
2	8/20 Ptet -(1)	EcoRI	XbaI
3	8/20 Ptet -(1)	EcoRI	--
4	8/20 Ptet -(1)	--	XbaI
5	8/20 Ptet -(1)	--	--
6	8/20 J23100-RBS-luxR-DT -(2)	EcoRI	XbaI
7	8/20 J23100-RBS-luxR-DT -(2)	EcoRI	--
8	8/20 J23100-RBS-luxR-DT -(2)	--	XbaI
9	8/20 J23100-RBS-luxR-DT -(2)	--	--
10	8/20 DT	EcoRI	XbaI
11	8/20 DT	EcoRI	--
12	8/20 DT	--	XbaI
13	8/20 DT	--	--
14	1kbp ladder	--	--
15	8/20 Ptet -(1)	EcoRI	XbaI

The reason why lane 2 and 15 were same is that the well of lane 2 might be broken.

Kojima

Lane	Sample	Enzyme1	Enzyme2
1	1kbp ladder	--	--
2	8/20 J23100-RBS-luxR-DT -(2)	EcoRI	XbaI
3	8/20 DT	EcoRI	XbaI

Gel Extraction

Honda

Lane	DNA	Enzyme
1	1kb ladder	--
2	8/21 J23100-RBS-luxR-DT 25µL	EcoRI+XbaI
3	8/21 J23100-RBS-luxR-DT 25µL	EcoRI+XbaI
4	--	--
5	8/21 Ptet 25µL	EcoRI+XbaI
6	8/21 Ptet 25µL	EcoRI+XbaI

Electrophoresis

Honda

Lane	Sample	EcoRI	XbaI
1	1kb ladder	--	--
2	8/21 DT	+	+
3	8/21 DT	+	--
4	8/21 DT	--	+
5	8/21 DT	--	--

Ligation

No name

state	Vector		Inserter		Ligation High ver.2	total
experiment	8/21 Pcn-RBS-luxR-DT(+Amp)	2.3	8/21 Pcn-RBS-GFP-DT	1.7	2	6
NC	8/21 Pcn-RBS-luxR-DT(+Amp)	2.3	MilliQ	1.7	2	6
experiment	8/18 Plux(+CP)	1.1	8/19 RBS-GFP-DT	5	3.1	9.2
NC	8/18 Plux(+CP)	1.1	MilliQ	5	3.1	9.2
experiment	8/18 RBS(+Amp)	2.2	8/19 lysis1	6.0	4.1	12.3
experiment	8/18 RBS(+Amp)	2.2	8/19 lysis2	3.6	2.9	8.7
NC	8/18 RBS(+Amp)	2.2	MilliQ	3.6	2.9	8.7
experiment	8/21 Ptet	1.5	8/20 RBS-tetR-DT (2)	2.1	1.8	5.4
NC	8/21 Ptet	1.5	MilliQ	2.1	1.8	5.4

Transformation

Okazaki

Name	Sample	Competent Cells	Total	Plate
8/21 Pcon-RBS-GFP-DT+Pcon-RBS-GFP-DT	1µL	10µL	11µL	Amp
8/21 Pcon-RBS-GFP-DT NC	1µL	10µL	11µL	Amp
8/18 RBS+8/19 lysis1	1µL	10µL	11µL	Amp
8/18 RBS+8/19 lysis2	1µL	10µL	11µL	Amp
8/18 RBS NC	1µL	10µL	11µL	Amp
8/18 Plux+8/18 RBS-GFP-DT	1µL	10µL	11µL	CP
8/18 Plux+8/18 RBS-GFP-DT	1µL	10µL	11µL	CP
8/21 Ptet(pm)+8/20 RBS-tetR-DT(2)	1µL	10µL	11µL	CP
8/21 Ptet(pm)+8/20 RBS-tetR-DT(2) NC	1µL	10µL	11µL	CP
8/21 pSB1C3	1µL	10µL	11µL	CP

LB Medium Plate

Gel Extraction

Okazaki

Lane	DNA	Enzyme
1	1kb ladder	--
2	--	--
3	8/21 DT	EcoRI & XbaI
4	8/21 DT	EcoRI & XbaI

Miniprep

Tatsui, Kojima, and Nakamoto

DNA	concentration [µg/mL]	260/280	260/230
tRNA-spinach-(1)	234	1.64	2.14
tRNA-spinach-(2)	440	1.60	1.91
tetR-aptamer 12-p(1076)-(1)	150	1.61	2.03
tetR-aptamer 12-p(1076)-(2)	374	1.45	1.66
tetR-aptamer 12-1R(113)-(1)	304	1.68	2.21
tetR-aptamer 12-1R(113)-(2)	382	1.47	1.66
tetR-aptamer 12-1M(105)-(1)	374	1.68	2.20
tetR-aptamer 12-1M(105)-(2)	286	1.31	1.43
PT181 attenuator-(1)	330	1.66	2.11
PT181 attenuator-(2)	270	1.68	2.18
Fusion1 attenuator-(1)	306	1.67	2.20
Fusion1 attenuator-(2)	282	1.60	1.94
Fusion3m2 attenuator-(1)	332	1.68	2.25
Fusion3m2 attenuator-(2)	326	1.67	2.10
PT181 antisense-(1)	178	1.64	1.68
PT181 antisense-(2)	116	1.63	1.95
Fusion1 antisense-(1)	300	1.67	2.21
Fusion1 antisense-(2)	164	1.42	1.46
Fusion6 antisense-(1)	336	1.65	2.18
Fusion6 antisense-(2)	192	1.65	2.01

@@ Line 5: / Line 5: @@
 *material
 :*8/17 Plusgrow medium 50ml
-:*7/22 5000x　Ampicillin 10&micro;l
+:*7/22 5000x Ampicillin 10&micro;l
 # Measuring materials and putting them in a 50ml tube
 </div>
@@ Line 61: / Line 61: @@
 ===Gel Extraction===
 <div class="experiment">
-<span class="author">Nakamoto and TaTsui</span>
+<span class="author">Nakamoto and Tatsui</span>
 {| class="wikitable"
 !Lane||DNA||Enzyme
@@ Line 84: / Line 84: @@
 |}
 [[File:Igku Aug21 Gel Extraction(Ptet‐(1))before.jpg]]
-[[File:xxxx.jpg]]
+[[File:Igku Aug21 Gel Extraction 2-2.jpg]]
-[[fig after]]
 {| class="wikitable"
 !Name||concentration[&micro;g/mL]||260/280||260/230
@@ Line 178: / Line 177: @@
 |}
 * The reason why lane 2 and 15 were same is that the well of lane 2 might be broken.
-[[fig]]<br>
+[[File:Igku Aug21 Electorophoresis Rtet E+X.jpg]]<br>
 <span class="author">Kojima</span>
 {| class="wikitable"
@@ Line 189: / Line 188: @@
 |3||8/20 DT||EcoRI||XbaI
 |}
-[[File:Igku Aug21 Electrophoresis(J23100‐RBS,DT-E+X)bykojima.jpg]]<br>
+[[File:Igku Aug21 Electrophoresis(J23100‐RBS,DT-E+X)bykojima.jpg ]]<br>
 </div>
@@ Line 201: / Line 200: @@
 |1||1kb ladder||--
 |-
-|2||8/21 J23100-RBS-luxR-DT 25&micro;L||E+X
+|2||8/21 J23100-RBS-luxR-DT 25&micro;L||EcoRI+XbaI
 |-
-|3||8/21 J23100-RBS-luxR-DT 25&micro;L||E+X
+|3||8/21 J23100-RBS-luxR-DT 25&micro;L||EcoRI+XbaI
 |-
 |4||--||--
 |-
-|5||8/21 Ptet 25&micro;L||E+X
+|5||8/21 Ptet 25&micro;L||EcoRI+XbaI
 |-
-|6||8/21 Ptet 25&micro;L||E+X
+|6||8/21 Ptet 25&micro;L||EcoRI+XbaI
 |}
 [[File:Igku Aug21 Gel Extraction(J23100,Ptet①)before.jpg]]<br>
@@ Line 217: / Line 216: @@
 ===Electrophoresis===
-<!-- こっから -->
 <div class="experiment">
 <span class="author">Honda</span>
@@ Line 235: / Line 233: @@
 [[File:Igku_Aug21electrophoresis.jpg]]<br>
 </div>
-<!-- ここまでをコピーしてね -->
 ===Ligation===
@@ Line 312: / Line 309: @@
 |4
 |}
-[[File:Igku Aug21 Gel Extraction(DT E+X 12,5μL①)before.jpg]]<br>
-[[File:Igku Aug21 Gel Extraction(DT E+X 12,5μL②)after.jpg]]<br>
 </div>

Template:Kyoto/Notebook/Aug 21

From 2013.igem.org

Latest revision as of 03:45, 28 September 2013

Contents

Aug 21

Plusgrow Medium

Liquid culture

Gel Extraction

Ristriction Enzyme Digestion

Electrophoresis

Gel Extraction

Electrophoresis

Ligation

Transformation

LB Medium Plate

Gel Extraction

Miniprep