Team:Kyoto/Notebook

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Revision as of 04:28, 4 September 2013

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template

Transformation

じっけんしゃ

Name	Well	Sample	Competent Cells	Total	Plate
いでんし	ぱーつのうぇる	なんちゃらµL	ごにょごにょµL	ほにゃららµL	こーせーぶっしつ
いかどうよう

Restriction Enzyme Digestion

じっけんしゃ

DNA	Buffer	restricion enzymeµL	restriction enzyme µL	MilliQ µL	total
（°°）

Electrophoresis

じっけんしゃ

DNA	Buffer	restricion enzymeµL	restriction enzyme µL	MilliQ µL	total
（°Д°）

Ligation

じっけんしゃ

Vecter(name & concentration)	quantity µL
(＞o＜)

Gel Extraction

じっけんしゃ

Lane	DNA	Enzyme
（＞ω・）b

Name	quantity	concentration	280/260	260/230
（´ω｀）
（ΦωΦ^）

Colony PCR

No name

Sample	base pair
(｀・ω・´)

PreDenature	Denature	Annealing	Extension	cycle
°C	°C	°C	°C	-
（◎Д◎）

Liquid Culture

No name

Sample	medium
(・ω・)
（・Ｘ・）

Miniprep

DNA	concentration	µg/µL	260/280	260/230
(・▽・)

Master Plate

No name

material

Aug 19

Colony PCR

Kojima

numbar	Sample	base pair
1	8/18 J23100 control -(1)	1142
2	8/18 J23100-RBS-GFP-DT -(1)	1156
3	8/18 J23100-RBS-GFP-DT -(2)	1156
4	8/18 J23100-RBS-luxR-DT -(1)	1271
5	8/18 J23100-RBS-luxR-DT -(2)	1271
6	8/18 J23100-RBS-lacZα-DT -(1)	670
7	8/18 J23100-RBS-lacZα-DT -(2)	670
8	8/18 RBS-lysis3 -(1)	997
9	8/18 RBS-lysis3 -(2)	997
10	8/18 P0440(RBS-tetR-DT) -(1)	1154
11	8/18 P0440(RBS-tetR-DT) -(2)	1154
12	negative control	-

PreDenature	Denature	Annealing	Extension	cycle
94°C	94°C	55°C	68°C	-
5min	30s	30s	1min	30cycles

File:Igku Aug19electrophoresis1.png

numbar	Sample	base pair
17	8/18 RBS control -(1)	-
18	8/18 R0040(Ptet) -(1)	686
19	8/18 R0040(Ptet) -(2)	686
20	negative control	-

PreDenature	Denature	Annealing	Extension	cycle
94°C	94°C	55°C	68°C	-
5min	30s	30s	30s	30cycles

File:Igku Aug19electrophoresis2.png

Gel Extraction

Ashida

Lane	DNA	Enzyme
1	100bp ladder	-
3	8/18 K117000(lysis1) -1	XbaI & PstI
5	8/18 K117000(lysis2) -1	XbaI & PstI

File:Igku Aug19electrophoresis3
File:Igku Aug19electrophoresis4

LB Liquid Mideum Culture

Nakamoto

volume	200ml
Bacto T2ypton	2g
Bacto yeast extract	1g
NaCl	1g
Agar Pouder	2g

Restriction Enzyme Digestion

Tatsui

lysis2-1	XbaⅠ	PstⅠ	BSA	10xbuffer	MilliQ	total
10µL	1µL	1µL	3µL	3µL	12µL	30µL
2µL	0.2µL	--	1µL	1µL	5.8µL	10µL
2µL	--	0.2µL	1µL	1µL	5.8µL	10µL
2µLL	--	--	1µL	1µ	6µL	10µL

at 37°C, for 1h

Murata and Okazaki

8/19 lysis1-1	10xbuffer	XbaⅠ	PstⅠ	BSA	MilliQ	total
2µL	2µL	0.5µL	0.8µL	2µL	13µL	20µL
0.5µL	1µL	0.2µL	--	1µL	7.3µL	10µL
0.5µL	1µL	--	0.2µL	1µL	7.3µL	10µL
0.5µL	1µL	--	--	1µL	7.5µL	10µL

at 37℃, for 1h

Transformation

Murata and Kojima

Name	Well	Sample	Competent Cells	Total	Plate
8/18 Plux-RBS-GFP-DT	ぱーつのうぇる	2µL	20µL	ほにゃららµL	CP
8/18 Plux(NC)		2µL	20µL	µL	CP
8/19 RBS+lysis2		2µL	20µL	µL	Amp
8/15 Pbad-araC		2µL	20µL	µL	Kana

Incubate at 17°C

Gel Extraction

Master Plate

Ashida

Use LB plate(+Amp)
8/18 J23100-6pp(Amp)
8/18 J23100-luxR(Amp)
8/18 J23100-luxR(Amp)
8/18 J23100+LacZα(Amp)
8/18 RBS-lysis3(Amp)
8/18 RBS-lysis3(Amp)

Use LB plate(+CP)
8/18 Ptet
8/18 RBS-tetR-DT
8/18 RBS-tetR-DT

Miniprep

Aug 20

Miniprep

Kojima

DNA	concentration[µg/µL]	260/280	260/230
8/18 Ptet -1	220	1.69	1.87
8/18 Ptet -2	210	1.69	1.71
8/18 RBS-tetR-DT -1	236	1.63	1.69
8/18 RBS-tetR-DT -2	182	1.65	1.98
8/18 J23100-RBS-GFP-DT -1	334	1.71	2.12
8/18 J23100-RBS-luxR-DT -1	440	1.67	1.60
8/18 J23100-RBS-luxR-DT -2	344	1.68	1.83
8/18 J23100-RBS-lacZα-DT -1	280	1.70	1.81
8/18 RBS-lysis3 -1	282	1.67	1.76
8/18 RBS-lysis3 -2	212	1.30	1.35

LB Culture Medium

Okazaki

volume	200mL
Bacto Trypton	2g
Bacto yeast extract	1g
Nacl	1g
Agar Powder	2g
Amp	40µl

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 Digestion

Kojima and Ashida

8/20 Ptet -1(220µg/mL)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
4.5	1	1	3	3	17.5	30
0.5	0.2	0	1	1	7.3	10
0.5	0	0.2	1	1	7.3	10
0.5	0	0	1	1	7.5	10

8/20 RBS-tetR-DT -2(182µg/mL)	EcoRI	SpeI	10x buffer H	MilliQ	total
5.5	1	1	3	19.5	30
0.6	0.2	0	1	8.2	10
0.6	0	0.2	1	8.2	10
0.6	0	0	1	8.4	10

8/20 J23100-RBS-GFP-DT(334µg/ml)	EcoRI	SpeI	10x buffer H	MilliQ	total
3.0	1	1	3	22	30
0.3	0.2	0	1	8.5	10
0.3	0	0.2	1	8.5	10
0.3	0	0	1	8.7	10

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
0.3	0.2	0	1	1	7.5	10
0.3	0	0.2	1	1	7.5	10
0.3	0	0	1	1	7.7	10

8/20 RBS-lysis3 -1(282µg/mL)	EcoRI	SpeI	10x buffer H	MilliQ	total
3.5	1	1	3	21.5	30
0.4	0.2	0	1	8.4	10
0.4	0	0.2	1	8.4	10
0.4	0	0	1	8.6	10

8/17 DT -1(188µg/mL)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
5.3	1	1	3	3	16.7	30
0.3	0.2	0	1	1	7.5	10
0.3	0	0.2	1	1	7.5	10
0.3	0	0	1	1	7.7	10

incubate XX°C for Xh

Transformation

Nakamoto

Name	Sample	Competent Cells(XL10-gold)	Total	Plate
tRNA-Spinach-tRNA	1µL	10µL	11µL	8/19 LB+Amp
tetR-aptamer 12_PC(076)	1µL	10µL	11µL	8/19 LB+Amp
tetR-aptamer 12_1R(113)	1µL	10µL	11µL	8/19 LB+Amp
tetR-aptamer 12_1M(105)	1µL	10µL	11µL	8/19 LB+Amp
pT181 attenuator	1µL	10µL	11µL	8/19 LB+Amp
Fusin1 attenuator	1µL	10µL	11µL	8/19 LB+Amp
Fusion3m2 attenuator	1µL	10µL	11µL	8/19 LB+Amp
pT181 antisense	1µL	10µL	11µL	8/19 LB+Amp
Fusion1 antisense	1µL	10µL	11µL	8/19 LB+Amp
Fusion6 antisense	1µL	10µL	11µL	8/19 LB+Amp

incubate 37°C overnight 20:34~

Electrophoresis

Kojima

Lane	Sample	Enzyme1	Enzyme2
1	8/20 Ptet -1	EcoRI	XbaI
2	8/20 Ptet -1	EcoRI	-
3	8/20 Ptet -1	-	XbaI
4	8/20 Ptet -1	-	-
5	8/20 RBS-tetR-DT -2	EcoRI	SpeI
6	8/20 RBS-tetR-DT -2	EcoRI	-
7	8/20 RBS-tetR-DT -2	-	SpeI
8	8/20 RBS-tetR-DT -2	-	-
9	1kbp ladder	-	-
10	8/20 J23100-RBS-GFP-DT -1	EcoRI	SpeI
11	8/20 J23100-RBS-GFP-DT -1	EcoRI	-
12	8/20 J23100-RBS-GFP-DT -1	-	SpeI
13	8/20 J23100-RBS-GFP-DT -1	-	-
14	8/20 J23100-RBS-luxR-DT -1	EcoRI	XbaI
15	8/20 J23100-RBS-luxR-DT -1	EcoRI	-
16	8/20 J23100-RBS-luxR-DT -1	-	XbaI
17	8/20 J23100-RBS-luxR-DT -1	-	-
18	1kbp ladder	-	-
19	8/20 RBS-lysis3 -1	EcoRI	SpeI
20	8/20 RBS-lysis3 -1	EcoRI	-
21	8/20 RBS-lysis3 -1	-	SpeI
22	8/20 RBS-lysis3 -1	-	-
23	1kbp ladder	-	-
24	8/17 DT	EcoRI	XbaI
25	8/17 DT	EcoRI	-
26	8/17 DT	-	XbaI
27	8/17 DT	-	-

Aug 21(changing)

Miniprep

Kojima

DNA	concentration[µg/µL]	260/280	260/230
8/18 Ptet -1	220	1.69	1.87
8/18 Ptet -2	210	1.69	1.71
8/18 RBS-tetR-DT -1	236	1.63	1.69
8/18 RBS-tetR-DT -2	182	1.65	1.98
8/18 J23100-RBS-GFP-DT -1	334	1.71	2.12
8/18 J23100-RBS-luxR-DT -1	440	1.67	1.60
8/18 J23100-RBS-luxR-DT -2	344	1.68	1.83
8/18 J23100-RBS-lacZα-DT -1	280	1.70	1.81
8/18 RBS-lysis3 -1	282	1.67	1.76
8/18 RBS-lysis3 -2	212	1.30	1.35

LB Culture Medium

Okazaki

volume	200mL
Bacto Trypton	2g
Bacto yeast extract	1g
Nacl	1g
Agar Powder	2g
Amp	40µl

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 Digestion

Kojima and Ashida

8/20 Ptet -1(220µg/mL)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
4.5	1	1	3	3	17.5	30
0.5	0.2	0	1	1	7.3	10
0.5	0	0.2	1	1	7.3	10
0.5	0	0	1	1	7.5	10

8/20 RBS-tetR-DT -2(182µg/mL)	EcoRI	SpeI	10x buffer H	MilliQ	total
5.5	1	1	3	19.5	30
0.6	0.2	0	1	8.2	10
0.6	0	0.2	1	8.2	10
0.6	0	0	1	8.4	10

8/20 J23100-RBS-GFP-DT(334µg/ml)	EcoRI	SpeI	10x buffer H	MilliQ	total
3.0	1	1	3	22	30
0.3	0.2	0	1	8.5	10
0.3	0	0.2	1	8.5	10
0.3	0	0	1	8.7	10

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
0.3	0.2	0	1	1	7.5	10
0.3	0	0.2	1	1	7.5	10
0.3	0	0	1	1	7.7	10

8/20 RBS-lysis3 -1(282µg/mL)	EcoRI	SpeI	10x buffer H	MilliQ	total
3.5	1	1	3	21.5	30
0.4	0.2	0	1	8.4	10
0.4	0	0.2	1	8.4	10
0.4	0	0	1	8.6	10

8/17 DT -1(188µg/mL)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
5.3	1	1	3	3	16.7	30
0.3	0.2	0	1	1	7.5	10
0.3	0	0.2	1	1	7.5	10
0.3	0	0	1	1	7.7	10

incubate XX°C for Xh

Transformation

Nakamoto

Name	Sample	Competent Cells(XL10-gold)	Total	Plate
tRNA-Spinach-tRNA	1µL	10µL	11µL	8/19 LB+Amp
tetR-aptamer 12_PC(076)	1µL	10µL	11µL	8/19 LB+Amp
tetR-aptamer 12_1R(113)	1µL	10µL	11µL	8/19 LB+Amp
tetR-aptamer 12_1M(105)	1µL	10µL	11µL	8/19 LB+Amp
pT181 attenuator	1µL	10µL	11µL	8/19 LB+Amp
Fusin1 attenuator	1µL	10µL	11µL	8/19 LB+Amp
Fusion3m2 attenuator	1µL	10µL	11µL	8/19 LB+Amp
pT181 antisense	1µL	10µL	11µL	8/19 LB+Amp
Fusion1 antisense	1µL	10µL	11µL	8/19 LB+Amp
Fusion6 antisense	1µL	10µL	11µL	8/19 LB+Amp

incubate 37°C overnight 20:34~

Electrophoresis

Kojima

Lane	Sample	Enzyme1	Enzyme2
1	8/20 Ptet -1	EcoRI	XbaI
2	8/20 Ptet -1	EcoRI	-
3	8/20 Ptet -1	-	XbaI
4	8/20 Ptet -1	-	-
5	8/20 RBS-tetR-DT -2	EcoRI	SpeI
6	8/20 RBS-tetR-DT -2	EcoRI	-
7	8/20 RBS-tetR-DT -2	-	SpeI
8	8/20 RBS-tetR-DT -2	-	-
9	1kbp ladder	-	-
10	8/20 J23100-RBS-GFP-DT -1	EcoRI	SpeI
11	8/20 J23100-RBS-GFP-DT -1	EcoRI	-
12	8/20 J23100-RBS-GFP-DT -1	-	SpeI
13	8/20 J23100-RBS-GFP-DT -1	-	-
14	8/20 J23100-RBS-luxR-DT -1	EcoRI	XbaI
15	8/20 J23100-RBS-luxR-DT -1	EcoRI	-
16	8/20 J23100-RBS-luxR-DT -1	-	XbaI
17	8/20 J23100-RBS-luxR-DT -1	-	-
18	1kbp ladder	-	-
19	8/20 RBS-lysis3 -1	EcoRI	SpeI
20	8/20 RBS-lysis3 -1	EcoRI	-
21	8/20 RBS-lysis3 -1	-	SpeI
22	8/20 RBS-lysis3 -1	-	-
23	1kbp ladder	-	-
24	8/17 DT	EcoRI	XbaI
25	8/17 DT	EcoRI	-
26	8/17 DT	-	XbaI
27	8/17 DT	-	-

Aug 21

Plusgrow medium(+Amp)

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

incubate 37°C 10hour

Ristriction Enzyme Digestion

Kojima and Nakamoto

8/20 Ptet-(1)	EcoRI	XbaI	10x BSA	10x buffer M	MilliQ	total
4.5	1	1	3	3	17.5	30
0.5	0.2	0	1	1	7.3	10
0.5	0	0.2	1	1	7.3	10
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
2.9	1	1	3	3	19.1	30
0.3	0.2	0	1	1	7.5	10
0.3	0	0.2	1	1	7.5	10
0.3	0	0	1	1	7.7	10

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

incubate 37°C 1h

Electrophoresis

Aug 22

Liquid culture

Nakamoto

Sample	Medium
8/21 Pcon-RBS-GFP-DT-Pcon-RBS-luxR-DT (1)	8/21 Plusgrow medium(+Amp)
8/21 Pcon-RBS-GFP-DT-Pcon-RBS-luxR-DT (2)	8/21 Plusgrow medium(+Amp)
8/21 Pcon-RBS-GFP-DT control (1)	8/21 Plusgrow medium(+Amp)
8/21 Pcon-RBS-GFP-DT control (2)	8/21 Plusgrow medium(+Amp)
8/21 RBS-lysis1 (1)	8/21 Plusgrow medium(+Amp)
8/21 RBS-lysis1 (2)	8/21 Plusgrow medium(+Amp)
8/21 RBS control (1)	8/21 Plusgrow medium(+Amp)
8/21 RBS control (2)	8/21 Plusgrow medium(+Amp)
8/21 Ptet(pm)-RBS-tetR-DT (1)	8/21 Plusgrow medium(+Amp)
8/21 Ptet(pm)-RBS-tetR-DT (2)	8/21 Plusgrow medium(+Amp)
8/21 Ptet(pm) control (1)	8/21 Plusgrow medium(+Amp)
8/21 Ptet(pm) control (2)	8/21 Plusgrow medium(+Amp)
8/21 Plux-RBS-GFP-DT (1)	8/21 Plusgrow medium(+Amp)
8/21 pSB1C3(BBa_J04450) (1)	8/21 Plusgrow medium(+Amp)
8/21 pSB1C3(BBa_J04450) (2)	8/21 Plusgrow medium(+Amp)

incubate 37°C 10hour

Colony PCR

Kojima

Sample	base pair
8/21 RBS-lysis1(1)	400
8/21 RBS-lysis1(2)	400
8/21 RBS control(1)
8/21 RBS control(2)
negative control

PreDenature	Denature	Annealing	Extension	cycle
94°C	94°C	55°C	68°C	-
5min	30s	30s	30s	30cycles

Sample	base pair
8/21 Pcon-GFP-DT-Pcon-RBS-luxR-DT (1)	2143
8/21 Pcon-GFP-DT-Pcon-RBS-luxR-DT (2)	2143
8/21 Pcon-RBS-luxR control(1)
8/21 Pcon-RBS-luxR control(2)
negative control

PreDenature	Denature	Annealing	Extension	cycle
94°C	94°C	55°C	68°C	-
5min	30s	30s	30s	30cycles

Sample	base pair
8/21 Ptet(pm)-RBS-tetR-DT (1)
8/21 Ptet(pm)-RBS-tetR-DT (2)
8/21 Ptet(pm) control (1)
8/21 Ptet(pm) control (2)
8/21 Plux-RBS-GFP-DT (1)
8/21 pSB1C3(BBa_J04450) (1)
8/21 pSB1C3(BBa_J04450) (2)
negative control

PreDenature	Denature	Annealing	Extension	cycle
94°C	94°C	55°C	68°C	-
5min	30s	30s	30s	30cycles

==Aug 23==

@@ Line 346: / Line 346: @@
 ===Miniprep===
-==Aug 19==
+==Aug 20==
-===Colony PCR===
+===Miniprep===
 <div class="experiment">
-<span class="author">Kojima</span>
+<span class="author">Kojima </span>
-{| class="wikitable"
+{|class="wikitable"
-!numbar||Sample||base pair
+!DNA!!concentration[&micro;g/&micro;L]!!260/280!!260/230
 |-
-|1||8/18 J23100 control -(1)||1142
+|8/18 Ptet -1||220||1.69||1.87
 |-
-|2||8/18 J23100-RBS-GFP-DT -(1)||1156
+|8/18 Ptet -2||210||1.69||1.71
 |-
-|3||8/18 J23100-RBS-GFP-DT -(2)||1156
+|8/18 RBS-tetR-DT -1||236||1.63||1.69
 |-
-|4||8/18 J23100-RBS-luxR-DT -(1)||1271
+|8/18 RBS-tetR-DT -2||182||1.65||1.98
 |-
-|5||8/18 J23100-RBS-luxR-DT -(2)||1271
+|8/18 J23100-RBS-GFP-DT -1||334||1.71||2.12
 |-
-|6||8/18 J23100-RBS-lacZ&alpha;-DT -(1)||670
+|8/18 J23100-RBS-luxR-DT -1||440||1.67||1.60
 |-
-|7||8/18 J23100-RBS-lacZ&alpha;-DT -(2)||670
+|8/18 J23100-RBS-luxR-DT -2||344||1.68||1.83
 |-
-|8||8/18 RBS-lysis3 -(1)||997
+|8/18 J23100-RBS-lacZα-DT -1||280||1.70||1.81
 |-
-|9||8/18 RBS-lysis3 -(2)||997
+|8/18 RBS-lysis3 -1||282||1.67||1.76
 |-
-|10||8/18 P0440(RBS-tetR-DT) -(1)||1154
+|8/18 RBS-lysis3 -2||212||1.30||1.35
+|}
+</div>
+===LB Culture Medium===
+<div class="experiment">
+<span class="author">Okazaki</span>
+{|class="wikitable"
+!volume||200mL
 |-
-|11||8/18 P0440(RBS-tetR-DT) -(2)||1154
+|Bacto Trypton||2g
 |-
-|12||negative control||-
+|Bacto yeast extract||1g
-|}
-{| class="wikitable"
-!PreDenature||Denature||Annealing||Extension||cycle
 |-
-|94&deg;C||94&deg;C||55&deg;C||68&deg;C||-
+|Nacl||1g
 |-
-|5min||30s||30s||1min||30cycles
+|Agar Powder||2g
+|-
+|Amp||40&micro;l
 |}
-[[File:igku_Aug19electrophoresis1.png]]
-<br>
+.Measuring  reagents and put they in the Erlenmeyer flask<br>
-{| class="wikitable"
+.diluting in measuring cylinder to 200ml total <br>
-!numbar||Sample||base pair
+.autoclaving<br>
+.adding ampicirine 40ml
+not written yet
+</div>
+===Ristriction Enzyme Digestion===
+<div class="experiment">
+<span class="author">Kojima and Ashida</span>
+{|class="wikitable"
+!8/20 Ptet -1(220&micro;g/mL)!!EcoRI!!XbaI!!10x BSA!!10x buffer M!!MilliQ!!total
 |-
-|17||8/18 RBS control -(1)||-
+|4.5||1||1||3||3||17.5||30
 |-
-|18||8/18 R0040(Ptet) -(1)||686
+|0.5||0.2||0||1||1||7.3||10
 |-
-|19||8/18 R0040(Ptet) -(2)||686
+|0.5||0||0.2||1||1||7.3||10
 |-
-|20||negative control||-
+|0.5||0||0||1||1||7.5||10
 |}
-{| class="wikitable"
+{|class="wikitable"
-!PreDenature||Denature||Annealing||Extension||cycle
+!8/20 RBS-tetR-DT -2(182&micro;g/mL)!!EcoRI!!SpeI!!10x buffer H!!MilliQ!!total
 |-
-|94&deg;C||94&deg;C||55&deg;C||68&deg;C||-
+|5.5||1||1||3||19.5||30
 |-
-|5min||30s||30s||30s||30cycles
+|0.6||0.2||0||1||8.2||10
+|-
+|0.6||0||0.2||1||8.2||10
+|-
+|0.6||0||0||1||8.4||10
 |}
-[[File:igku_Aug19electrophoresis2.png]]
+{|class="wikitable"
-</div>
+!8/20 J23100-RBS-GFP-DT(334&micro;g/ml)!!EcoRI!!SpeI!!10x buffer H!!MilliQ!!total
-===Gel Extraction===
-<div class="experiment">
-<span class="author">Ashida</span>
-{| class="wikitable"
-!Lane||DNA||Enzyme
 |-
-|1||100bp ladder||-
+|3.0||1||1||3||22||30
 |-
-|3||8/18 K117000(lysis1) -1||XbaI & PstI
+|0.3||0.2||0||1||8.5||10
 |-
-|5||8/18 K117000(lysis2) -1||XbaI & PstI
+|0.3||0||0.2||1||8.5||10
+|-
+|0.3||0||0||1||8.7||10
 |}
-[[File:igku_Aug19electrophoresis3]]<br>
+{|class="wikitable"
-[[File:igku_Aug19electrophoresis4]]
+!8/20 J23100-RBS-luxR-DT -2(344&micro;g/mL)!!EcoRI!!XbaI!!BSA!!10x buffer M!!MilliQ!!total
-</div>
-===LB Liquid Mideum Culture===
-<!-- ここから -->
-<div class="experiment">
-<span class="author">Nakamoto</span>
-{| class="wikitable"
-!volume||200ml
 |-
-|Bacto T2ypton || 2g
+|2.9||1||1||3||3||19.1||30
 |-
-|Bacto yeast extract ||1g
+|0.3||0.2||0||1||1||7.5||10
 |-
-|NaCl||1g
+|0.3||0||0.2||1||1||7.5||10
 |-
-|Agar Pouder||2g
+|0.3||0||0||1||1||7.7||10
 |}
-</div>
+{|class="wikitable"
-<!-- ここまでをコピーしてね -->
+!8/20 RBS-lysis3 -1(282&micro;g/mL)!!EcoRI!!SpeI!!10x buffer H!!MilliQ!!total
-===Restriction Enzyme Digestion===
-<!-- こっから -->
-<div class="experiment">
-<span class="author">Tatsui</span>
-{| class="wikitable"
-!lysis2-1||XbaⅠ||PstⅠ||BSA||10xbuffer||MilliQ||total
 |-
-|10&micro;L||1&micro;L||1&micro;L||3&micro;L||3&micro;L||12&micro;L||30&micro;L
+|3.5||1||1||3||21.5||30
 |-
-|2&micro;L||0.2&micro;L||--||1&micro;L||1&micro;L||5.8&micro;L||10&micro;L
+|0.4||0.2||0||1||8.4||10
 |-
-|2&micro;L||--||0.2&micro;L||1&micro;L||1&micro;L||5.8&micro;L||10&micro;L
+|0.4||0||0.2||1||8.4||10
 |-
-|2&micro;LL||--||--||1&micro;L||1&micro;||6&micro;L||10&micro;L
+|0.4||0||0||1||8.6||10
 |}
-</div>
+{|class="wikitable"
-*at 37&deg;C, for 1h
+!8/17 DT -1(188&micro;g/mL)!!EcoRI!!XbaI!!10x BSA!!10x buffer M!!MilliQ!!total
-<div class="experiment">
-<span class="author">Murata and Okazaki</span>
-{| class="wikitable"
-!8/19 lysis1-1||10xbuffer||XbaⅠ||PstⅠ||BSA||MilliQ||total
 |-
-|2&micro;L||2&micro;L||0.5&micro;L||0.8&micro;L||2&micro;L||13&micro;L||20&micro;L
+|5.3||1||1||3||3||16.7||30
 |-
-|0.5&micro;L||1&micro;L||0.2&micro;L||--||1&micro;L||7.3&micro;L||10&micro;L
+|0.3||0.2||0||1||1||7.5||10
 |-
-|0.5&micro;L||1&micro;L||--||0.2&micro;L||1&micro;L||7.3&micro;L||10&micro;L
+|0.3||0||0.2||1||1||7.5||10
 |-
-|0.5&micro;L||1&micro;L||--||--||1&micro;L||7.5&micro;L||10&micro;L
+|0.3||0||0||1||1||7.7||10
 |}
-*at 37℃, for 1h
+incubate  XX&deg;C  for Xh
 </div>
-<!-- ここまでをコピーしてね -->
 ===Transformation===
-<!-- こっから -->
 <div class="experiment">
-<span class="author">Murata and Kojima</span>
+<span class="author">Nakamoto</span>
 {| class="wikitable"
-!Name||Well||Sample||Competent Cells||Total||Plate
+!Name||Sample||Competent Cells(XL10-gold)||Total||Plate
 |-
-|8/18 Plux-RBS-GFP-DT||ぱーつのうぇる||2&micro;L||20&micro;L||ほにゃらら&micro;L||CP
+|tRNA-Spinach-tRNA||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
 |-
-|8/18 Plux(NC)||   ||2&micro;L||20&micro;L|| &micro;L ||CP
+|tetR-aptamer 12_PC(076)||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
 |-
-|8/19 RBS+lysis2 || || 2&micro;L||20&micro;L|| &micro;L||Amp
+|tetR-aptamer 12_1R(113)||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
 |-
-|8/15 Pbad-araC|| || 2&micro;L||20&micro;L|| &micro;L||Kana
+|tetR-aptamer 12_1M(105)||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
+|-
+|pT181 attenuator||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
+|-
+|Fusin1 attenuator||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
+|-
+|Fusion3m2 attenuator||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
+|-
+|pT181 antisense||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
+|-
+|Fusion1 antisense||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
+|-
+|Fusion6 antisense||1&micro;L||10&micro;L||11&micro;L||8/19 LB+Amp
 |}
+incubate 37&deg;C overnight 20:34~
 </div>
-*Incubate at 17&deg;C
+===Electrophoresis===
-<!-- ここまでをコピーしてね -->
-===Gel Extraction===
-===Master Plate===
 <div class="experiment">
-<span class="author">Ashida</span>
+<span class="author">Kojima</span>
 {| class="wikitable"
-!Use LB plate(+Amp)
+!Lane||Sample||Enzyme1||Enzyme2
 |-
-|8/18 J23100-6pp(Amp)
+|1||8/20 Ptet -1||EcoRI||XbaI
 |-
-|8/18 J23100-luxR(Amp)
+|2||8/20 Ptet -1||EcoRI||-
 |-
-|8/18 J23100-luxR(Amp)
+|3||8/20 Ptet -1||-||XbaI
 |-
-|8/18 J23100+LacZα(Amp)
+|4||8/20 Ptet -1||-||-
 |-
-|8/18 RBS-lysis3(Amp)
+|5||8/20 RBS-tetR-DT -2||EcoRI||SpeI
 |-
-|8/18 RBS-lysis3(Amp)
+|6||8/20 RBS-tetR-DT -2||EcoRI||-
-|}
-{| class="wikitable"
-!Use LB plate(+CP)
 |-
-|8/18 Ptet
+|7||8/20 RBS-tetR-DT -2||-||SpeI
 |-
-|8/18 RBS-tetR-DT
+|8||8/20 RBS-tetR-DT -2||-||-
 |-
-|8/18 RBS-tetR-DT
+|9||1kbp ladder||-||-
-|}
+|-
+|10||8/20 J23100-RBS-GFP-DT -1||EcoRI||SpeI
+|-
+|11||8/20 J23100-RBS-GFP-DT -1||EcoRI||-
+|-
+|12||8/20 J23100-RBS-GFP-DT -1||-||SpeI
+|-
+|13||8/20 J23100-RBS-GFP-DT -1||-||-
+|-
+|14||8/20 J23100-RBS-luxR-DT -1||EcoRI||XbaI
+|-
+|15||8/20 J23100-RBS-luxR-DT -1||EcoRI||-
+|-
+|16||8/20 J23100-RBS-luxR-DT -1||-||XbaI
+|-
+|17||8/20 J23100-RBS-luxR-DT -1||-||-
+|-
+|18||1kbp ladder||-||-
+|-
+|19||8/20 RBS-lysis3 -1||EcoRI||SpeI
+|-
+|20||8/20 RBS-lysis3 -1||EcoRI||-
+|-
+|21||8/20 RBS-lysis3 -1||-||SpeI
+|-
+|22||8/20 RBS-lysis3 -1||-||-
+|-
+|23||1kbp ladder||-||-
+|-
+|24||8/17 DT||EcoRI||XbaI
+|-
+|25||8/17 DT||EcoRI||-
+|-
+|26||8/17 DT||-||XbaI
+|-
+|27||8/17 DT||-||-
+|}
 </div>
-<!-- ここまでをコピーしてね -->
-===Miniprep===
 ==Aug 21(changing)==

Team:Kyoto/Notebook

From 2013.igem.org

Revision as of 04:28, 4 September 2013

Contents

template

Transformation

Restriction Enzyme Digestion

Electrophoresis

Ligation

Gel Extraction

Colony PCR

Liquid Culture

Miniprep

Master Plate

Aug 19

Colony PCR

Gel Extraction

LB Liquid Mideum Culture

Restriction Enzyme Digestion

Transformation

Gel Extraction

Master Plate

Miniprep

Aug 20

Miniprep

LB Culture Medium

Ristriction Enzyme Digestion

Transformation

Electrophoresis

Aug 21(changing)

Miniprep

LB Culture Medium

Ristriction Enzyme Digestion

Transformation

Electrophoresis

Aug 21

Plusgrow medium(+Amp)

Liquid culture

Ristriction Enzyme Digestion

Electrophoresis

Aug 22

Liquid culture

Colony PCR