Revision as of 08:30, 28 August 2015

E. coli

March

2015/03/10

Competent Cells

mami

BL21 (DE3) pLysS

Thawed original competent cells (BL21 (DE3) pLysS) on ice.
Added 5 μL of original competent cells to 2 mL of LB.
Incubated the cells for 16 hrs at 37℃.
Added 5 μL, 50 μL, and 500 μL of original cells to 100 mL of LB.
Incubated the cells at 130 rpm for 14 hrs at 20℃, until OD₆₀₀ reach 0.5.
Took 50 mL of incubated cells to two differnt culture tubes and centrifuged them at 3,000 rpm for 20 min at 4℃.
Removed supernatant and added 75 mL of TB to each tube.
Brought them to a one tube and centrifuged at 3,000 rpm for 20 min at 4℃.
Removed supernatant and added 32 mL of TB.
Added 32 μL of DMSO 10 times.
Took 50 μL and froze with liquid nitrogen.

2015/03/11

PCR

実験者

BBa_R0011

Reagent	Volume
BBa_R0011	1 μL
100bpUP-EX-F 10 μM	1.5 μL
200bpDN-PS-R 10 μM	1.5 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	32 μL
Total	50 μL

BBa_0030 - BBa_E1010

Reagent	Volume
BBa_0030 - BBa_E1010	1 μL
100bpUP-EX-F 10 μM	1.5 μL
200bpDN-PS-R 10 μM	1.5 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	32 μL
Total	50 μL

3 Step Cycle (Tm value ≤ 63℃)

Step	Temp.	Time	Process	Cycle
Start	94℃	120 sec	Initialization
Cycle 1	98℃	10 sec	Denaturation	30 cycle
Cycle 2	62.6℃	30 sec	Annealing	30 cycle
Cycle 3	68℃	1 min	Elongation	30 cycle
Store	4℃	Hold	Store

PCR Purification

実験者

BBa_R0011, BBa_0030 - BBa_E1010
FastGene^TM Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
Purification of PCR products

Digestion

実験者

BBa_R0011

Reagent	Volume
BBa_R0011	44 μL
XbaI	1 μL
Cut Smart	5 μL
Total	50 μL

BBa_0030 - BBa_E1010

Reagent	Volume
BBa_0030 - BBa_E1010	44 μL
XbaI	1 μL
Cut Smart	5 μL
Total	50 μL

Digestion

Step	Temp.	Time	Process
1	37℃	300 min	Digestion
2	60℃	15 min	Inactivation
Store	4℃	Hold	Store

Electrophoresis

実験者

BBa_R0011, BBa_0030 - BBa_E1010

Gel Concentration	Voltage	Time	Buffer
1%	100 V	30 min	2x TBE

Gel Extract

実験者

BBa_R0011, BBa_0030 - BBa_E1010
FastGene^TM Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
DNA extraction from gel

Electrophoresis

実験者

BBa_R0011, BBa_0030 - BBa_E1010

Gel Concentration	Voltage	Time	Buffer
1%	100 V	30 min	2x TBE

May

2015/05/13

Transformation

Onoda

pET15b

Added 1 μL of pET15b to 50 μL of thawed competent cells (DH5alpha) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Spread 50 μL of the culture onto plate with LBA.
Incubated the plate at 37℃ for 16 hours.

Transformation

Onoda

pET16b

Added 1 μL of pET16b to 50 μL of thawed competent cells (DH5alpha) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Spread 50 μL of the culture onto plate with LBA.
Incubated the plate at 37℃ for 16 hours.

Competent Cells

Onoda

rosetta

Thawed original competent cells (rosetta) on ice.
Added 5 μL of original competent cells to 2 mL of LB.
Incubated the cells for 16 hrs at 37℃.
Added 5 μL, 50 μL, and 500 μL of original cells to 100 mL of LB.
Incubated the cells at 130 rpm for 培養時間 hrs at 20℃, until OD₆₀₀ reach 0.5.
Took 50 mL of incubated cells to two differnt culture tubes and centrifuged them at 3,000 rpm for 20 min at 4℃.
Removed supernatant and added 75 mL of TB to each tube.
Brought them to a one tube and centrifuged at 3,000 rpm for 20 min at 4℃.
Removed supernatant and added 32 mL of TB.
Added 32 μL of DMSO 10 times.
Took 50 μL and froze with liquid nitrogen.

2015/05/27

Transformation

Mimata, Onoda

GFP

Added 1 μL of GFP to thawed competent cells (Rosetta and DH5α) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Added 200 μL of LB.
Spread 300 μL of the culture onto plate with LBA.
Incubated the plate at 37℃ for 16 hours.

Transformation

Mimata, Onoda, Ono

mRFP

Added 1 μL of mRFP to thawed competent cells (Rosetta and DH5α) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Added 200 μL of LB.
Spread 300 μL of the culture onto plate with LBA.
Incubated the plate at 37℃ for 16 hours.

2015/05/29

Mini-prep

Mimata, Onoda, Ono

GFP, mRFP
FastGene^TM Plasmid mini kit (Nippon Genetics Co.,Ltd)
standard protocol

PCR

Onoda, Ono

GFP

Reagent	Volume
GFP	1 μL
67-F-primer 10 μL	1 μL
14-R-primer 10 μL	1 μL
KOD FX NEO	1 μL
KOD FX NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

mRFP

Reagent	Volume
mRFP	1 μL
67-F-primer 10 μL	1 μL
14-R-primer 10 μL	1 μL
KOD FX NEO	1 μL
KOD FX NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

2 Step Cycle (Tm value ≥ 63℃)

Step	Temp.	Time	Process	Cycle
Start	94℃	120 sec	Initialization
Cycle 1	98℃	10 sec	Denaturation	30 cycles
Cycle 2	68℃	60 sec	Annealing / Elongation	30 cycles
Store	4℃	Hold	Store

2015/05/30

Electrophoresis

Mimata, Onoda, Ono

GFP, mRFP

Gel Concentration	Voltage	Time	Buffer
2%	100 A	30 min	2x TBE

Gel Extract

Onoda, Ono

GFP, mRFP
FastGene^TM Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
DNA extraction from gel

Digestion

Onoda, Ono

GFP

Reagent	Volume
GFP	20 μL
DW	5 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	3 μL
Total	30 μL

mRFP

Reagent	Volume
mRFP	20 μL
DW	5 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	3 μL
Total	30 μL

Digestion

Step	Temp.	Time	Process
1	37℃	120 min	Digestion
2	60℃	15 min	Inactivation
Store	4℃	Hold	Store

Digestion

Onoda, Ono

pET15b

Reagent	Volume
pET15b	10 μL
DW	6 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	2 μL
Total	20 μL

pET16b

Reagent	Volume
pET16b	10 μL
DW	6 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	2 μL
Total	20 μL

pSB1A3

Reagent	Volume
pSB1A3	10 μL
DW	6 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	2 μL
Total	20 μL

pSB4C5

Reagent	Volume
pSB4C5	2 μL
DW	14 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	2 μL
Total	20 μL

Digestion

Step	Temp.	Time	Process
1	37℃	120 min	Digestion
2	60℃	15 min	Inactivation
Store	4℃	Hold	Store

2015/05/31

Electrophoresis

Mimata, Onoda, Ono

GFP, RFP, pET15b, pET16b, pSB1A3, pSB4C5

Gel Concentration	Voltage	Time	Buffer
1%	100 V	30 min	1/2x TBE

Gel Extract

Mimata, Onoda, Ono

GFP, RFP, pET15b, pET16b, pSB1A3
FastGene^TM Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
DNA extraction from gel

Electrophoresis

Mimata, Onoda, Ono

GFP, mRFP

Gel Concentration	Voltage	Time	Buffer
1%	100 V	30 min	1/2x TBE

PCR

Mimata, Onoda

GFP

Reagent	Volume
GFP	1 μL
67-F-primer 10 μM	1 μL
14-R-primer 10 μM	1 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

mRFP

Reagent	Volume
mRFP	1 μL
67-F-primer 10 μM	1 μL
14-R-primer 10 μM	1 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

2 Step Cycle (Tm value ≥ 63℃)

Step	Temp.	Time	Process	Cycle
Start	94℃	120 sec	Initialization
Cycle 1	98℃	10 sec	Denaturation	30 cycle
Cycle 2	68℃	60 sec	Annealing / Elongation	30 cycle
Store	4℃	Hold	Store

June

2015/06/10

Digestion

Mimata, Onoda

GFP

Reagent	Volume
GFP	16 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	2 μL
Total	20 μL

mRFP

Reagent	Volume
mRFP	16 μL
Spe1	1 μL
EcoR1	1 μL
Cut Smart	2 μL
Total	20 μL

Digestion

Step	Temp.	Time	Process
1	37℃	600 min	Digestion
2	60℃	15 min	Inactivation
Store	4℃	Hold	Store

2015/06/16

PCR

Mimata

thanatin fragment for TA cloning

Reagent	Volume
TA forward primer	1 μL
TA reverse primer	1 μL
Kapa Taq	25 μL
DW	23 μL
Total	50 μL

3 Step Cycle (Tm value ≤ 63℃)

Step	Temp.	Time	Process	Cycle
Start	95℃	180 sec	Initialization
Cycle 1	95℃	30 sec	Denaturation	35 cycle
Cycle 2	63℃	30 sec	Annealing	35 cycle
Cycle 3	72℃	10 sec	Elongation	35 cycle
	72℃	60 sec
Store	4℃	Hold	Store

2015/06/17

Electrophoresis

Mimata

thanatin fragment for TA cloning

Gel Concentration	Voltage	Time	Buffer
2%	100 A	30 min	2x TBE

→failed

Annealing Oligos and Elongation

実験者

thanatin fragment for TA cloning

Reagent	Volume
TA-forward primer 1 μM	1 μL
TA-reverse primer 1 μM	1 μL
Kapa Taq	25 μL
DW	23 μL
Total	50 μL

Annealing Oligos and Elongation

Step	Temp.	Time	Process	Cycle
Start	95℃	1 min	Initialization
Cycle1	95℃ to 23℃	45 min	Annealing	1 cycle
Cycle 2	72℃	1 min	Elongation	1 cycle
Store	4℃	Hold	Store

2015/06/19

Electrophoresis

実験者

thanatin fragment for TA cloning

Gel Concentration	Voltage	Time	Buffer
2%	100V	30min	2x TBE

Gel Extract

実験者

thanatin fragment for TA cloning
FastGene^TM Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
DNA extraction from gel

Ligation

実験者

thanatin fragment for TA cloning / Tvector pGEM

Reagent	Volume
Tvector pGEM	1.7μL
thanatin fragment for TA cloning	0.15μL
Mighty Mix	1.85μL
T4 Ligase	0.18μL
DW	6.12μL
Total	10μL

Ligation

Step	Temp.	Time	Process
1	16℃	30 min	Ligation
2	65℃	10 min	Inactivation
Store	4℃	Hold	Store

2015/06/21

Transformation

実験者

Tvector pGEM

Added 1 μL of thanatin fragment to 50 μL of thawed competent cells (rosseta/DH5α) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Spread 300 μL of the culture onto plate with LBA.
Incubated the plate at 37℃ for 19 hours.

July

2015/07/25

Transformation

Onoda

dT on pSB1C3

Added 1 μL of dT on pSB1C3 to 50 μL of thawed competent cells (DH5α Turbo) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Added 500 μL of LB.
Incubated the cells for 2 hrs at 37℃.
Spread 300 μL of the culture onto plate with LBCp.
Incubated the plate at 37℃ for 16 hours.

Transformation

Onoda

pLac - B0034 on pSB1C3

Added 1 μL of pLac - B0034 on pSB1C3 to 50 μL of thawed competent cells (DH5α Turbo) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Added 500 μL of LB.
Incubated the cells for 2 hrs at 37℃.
Spread 300 μL of the culture onto plate with LBCp.
Incubated the plate at 37℃ for 16 hours.

Transformation

Onoda

pTet - B0034 on pSB1C3

Added 1 μL of pTet - B0034 on pSB1C3 to 50 μL of thawed competent cells (DH5α Turbo) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Added 500 μL of LB.
Incubated the cells for 2 hrs at 37℃.
Spread 300 μL of the culture onto plate with LBCp.
Incubated the plate at 37℃ for 16 hours.

Transformation

Onoda

B0034 on pSB1A2

Added 1 μL of B0034 on pSB1A2 to 50 μL of thawed competent cells (DH5α Turbo) on ice.
Incubated on ice for 30 min.
Heat-shocked for 30 sec at 42℃.
Added 500 μL of LB.
Spread 300 μL of the culture onto plate with LBA.
Incubated the plate at 37℃ for 16 hours.

PCR

Onoda

dT on pSB1C3

Reagent	Volume
10% dT on pSB1C3	1 μL
100bpUP-EX-F 10 μM	1 μL
200bpDN-PS-R 10 μM	1 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

pLac - B0034 on pSB1C3

Reagent	Volume
10% pLac - B0034 on pSB1C3	1 μL
100bpUP-EX-F 10 μM	1 μL
200bpDN-PS-R 10 μM	1 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

pTet - B0034 on pSB1C3

Reagent	Volume
10% pTet - B0034 on pSB1C3	1 μL
100bpUP-EX-F 10 μM	1 μL
200bpDN-PS-R 10 μM	1 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

B0034 on pSB1A2

Reagent	Volume
10% B0034 on pSB1A2	1 μL
100bpUP-EX-F 10 μM	1 μL
200bpDN-PS-R 10 μM	1 μL
KOD Plus NEO	1 μL
KOD Plus NEO 10x Buffer	5 μL
2 mM dNTPS	5 μL
25 mM MgSO₄	3 μL
DW	33 μL
Total	50 μL

3 Step Cycle (Tm value ≤ 63℃)

Step	Temp.	Time	Process	Cycle
Start	94℃	120 sec	Initialization
Cycle 1	98℃	10 sec	Denaturation	30 cycle
Cycle 2	62.6℃	30 sec	Annealing	30 cycle
Cycle 3	68℃	60 sec	Elongation	30 cycle
Store	4℃	Hold	Store

Electrophoresis

Onoda

dT on pSB1C3, pLac - B0034 on pSB1C3, pTet - B0034 on pSB1C3, B0034 on pSB1A2

Gel Concentration	Voltage	Time	Buffer
2%	100 A	30 min	2x TBE

2015/07/26

Liquid Culture

Ono

pTet - B0034 on pSB1A2

Reagent	Volume
Single Colony	-
LB	2000 μL
Ampicillin	2 μL

Cultured for 15 hours.

Mini-prep

実験者

pLac - B0034 on pSB1C3, dT on pSB1C3, B0034 on pSB1A2
FastGene^TM Plasmid mini kit (Nippon Genetics Co.,Ltd)
standard protocol

Electrophoresis

実験者

pTet - B0034 on pSB1C3, pLac - B0034 on pSB1C3, B0034 on pSB1A3, dT on pSB1C3

Gel Concentration	Voltage	Time	Buffer
2%	100 A	30 min	2x TBE

Gel Extract

Ono

pLac - B0034 on pSB1C3, pTet - B0034 on pSB1C3, B0034 on pSB1A2, dT on pSB1C3
FastGene^TM Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
DNA extraction from gel

2015/07/27

Mini-prep

Ono

pTet - B0034 on pSB1A2
FastGene^TM Plasmid mini kit (Nippon Genetics Co.,Ltd)
standard protocol

←Notebook Top

@@ Line 603: / Line 603: @@
 </ol>
 <!-- Transformaion（プレ培養なし） END -->
+<h2 id="july">July</h2>
+<h3>2015/07/25</h3>
+<!-- Transformaion（プレ培養あり） -->
+<h4>Transformation</h4>
+<p>Onoda</p>
+<p>dT on pSB1C3</p>
+<ol>
+	<li>Added 1 μL of dT on pSB1C3 to 50 μL of thawed competent cells (DH5α Turbo) on ice.</li>
+	<li>Incubated on ice for 30 min.</li>
+	<li>Heat-shocked for 30 sec at 42℃.</li>
+	<li>Added 500 μL of LB.</li>
+	<li>Incubated the cells for 2 hrs at 37℃.</li>
+	<li>Spread 300 μL of the culture onto plate with LBCp.</li>
+	<li>Incubated the plate at 37℃ for 16 hours.</li>
+</ol>
+<!-- Transformaion（プレ培養あり） END -->
+<!-- Transformaion（プレ培養あり） -->
+<h4>Transformation</h4>
+<p>Onoda</p>
+<p>pLac - B0034 on pSB1C3</p>
+<ol>
+	<li>Added 1 μL of pLac - B0034 on pSB1C3 to 50 μL of thawed competent cells (DH5α Turbo) on ice.</li>
+	<li>Incubated on ice for 30 min.</li>
+	<li>Heat-shocked for 30 sec at 42℃.</li>
+	<li>Added 500 μL of LB.</li>
+	<li>Incubated the cells for 2 hrs at 37℃.</li>
+	<li>Spread 300 μL of the culture onto plate with LBCp.</li>
+	<li>Incubated the plate at 37℃ for 16 hours.</li>
+</ol>
+<!-- Transformaion（プレ培養あり） END -->
+<!-- Transformaion（プレ培養あり） -->
+<h4>Transformation</h4>
+<p>Onoda</p>
+<p>pTet - B0034 on pSB1C3</p>
+<ol>
+	<li>Added 1 μL of pTet - B0034 on pSB1C3 to 50 μL of thawed competent cells (DH5α Turbo) on ice.</li>
+	<li>Incubated on ice for 30 min.</li>
+	<li>Heat-shocked for 30 sec at 42℃.</li>
+	<li>Added 500 μL of LB.</li>
+	<li>Incubated the cells for 2 hrs at 37℃.</li>
+	<li>Spread 300 μL of the culture onto plate with LBCp.</li>
+	<li>Incubated the plate at 37℃ for 16 hours.</li>
+</ol>
+<!-- Transformaion（プレ培養あり） END -->
+<!-- Transformaion（プレ培養なし） -->
+<h4>Transformation</h4>
+<p>Onoda</p>
+<p>B0034 on pSB1A2</p>
+<ol>
+	<li>Added 1 μL of B0034 on pSB1A2 to 50 μL of thawed competent cells (DH5α Turbo) on ice.</li>
+	<li>Incubated on ice for 30 min.</li>
+	<li>Heat-shocked for 30 sec at 42℃.</li>
+	<li>Added 500 μL of LB.</li>
+	<li>Spread 300 μL of the culture onto plate with LBA.</li>
+	<li>Incubated the plate at 37℃ for 16 hours.</li>
+</ol>
+<!-- Transformaion（プレ培養なし） END -->
+<!-- PCR 3STEP-->
+<h4>PCR</h4>
+<p>Onoda</p>
+<p>dT on pSB1C3</p>
+<table>
+	<tr><th>Reagent</th><th>Volume</th></tr>
+	<tr><td>10% dT on pSB1C3</td><td>1 μL</td></tr>
+	<tr><td>100bpUP-EX-F 10 μM</td><td>1 μL</td></tr>
+	<tr><td>200bpDN-PS-R 10 μM</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO 10x Buffer</td><td>5 μL</td></tr>
+	<tr><td>2 mM dNTPS</td><td>5 μL</td></tr>
+	<tr><td>25 mM MgSO<sub>4</sub></td><td>3 μL</td></tr>
+	<tr><td>DW</td><td>33 μL</td></tr>
+	<tr><td><b>Total</b></td><td><b>50 μL</b></td></tr>
+</table>
+<p>pLac - B0034 on pSB1C3</p>
+<table>
+	<tr><th>Reagent</th><th>Volume</th></tr>
+	<tr><td>10% pLac - B0034 on pSB1C3</td><td>1 μL</td></tr>
+	<tr><td>100bpUP-EX-F 10 μM</td><td>1 μL</td></tr>
+	<tr><td>200bpDN-PS-R 10 μM</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO 10x Buffer</td><td>5 μL</td></tr>
+	<tr><td>2 mM dNTPS</td><td>5 μL</td></tr>
+	<tr><td>25 mM MgSO<sub>4</sub></td><td>3 μL</td></tr>
+	<tr><td>DW</td><td>33 μL</td></tr>
+	<tr><td><b>Total</b></td><td><b>50 μL</b></td></tr>
+</table>
+<p>pTet - B0034 on pSB1C3</p>
+<table>
+	<tr><th>Reagent</th><th>Volume</th></tr>
+	<tr><td>10% pTet - B0034 on pSB1C3</td><td>1 μL</td></tr>
+	<tr><td>100bpUP-EX-F 10 μM</td><td>1 μL</td></tr>
+	<tr><td>200bpDN-PS-R 10 μM</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO 10x Buffer</td><td>5 μL</td></tr>
+	<tr><td>2 mM dNTPS</td><td>5 μL</td></tr>
+	<tr><td>25 mM MgSO<sub>4</sub></td><td>3 μL</td></tr>
+	<tr><td>DW</td><td>33 μL</td></tr>
+	<tr><td><b>Total</b></td><td><b>50 μL</b></td></tr>
+</table>
+<p>B0034 on pSB1A2</p>
+<table>
+	<tr><th>Reagent</th><th>Volume</th></tr>
+	<tr><td>10% B0034 on pSB1A2</td><td>1 μL</td></tr>
+	<tr><td>100bpUP-EX-F 10 μM</td><td>1 μL</td></tr>
+	<tr><td>200bpDN-PS-R 10 μM</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO</td><td>1 μL</td></tr>
+	<tr><td>KOD Plus NEO 10x Buffer</td><td>5 μL</td></tr>
+	<tr><td>2 mM dNTPS</td><td>5 μL</td></tr>
+	<tr><td>25 mM MgSO<sub>4</sub></td><td>3 μL</td></tr>
+	<tr><td>DW</td><td>33 μL</td></tr>
+	<tr><td><b>Total</b></td><td><b>50 μL</b></td></tr>
+</table>
+<p>3 Step Cycle (Tm value &le; 63℃)</p>
+<table>
+	<tr><th>Step</th><th>Temp.</th><th>Time</th><th>Process</th><th>Cycle</th></tr>
+	<tr><td>Start</td><td>94℃</td><td>120 sec</td><td>Initialization</td><td></td></tr>
+	<tr><td>Cycle 1</td><td>98℃</td><td>10 sec</td><td>Denaturation</td><td>30 cycle</td></tr>
+	<tr><td>Cycle 2</td><td>62.6℃</td><td>30 sec</td><td>Annealing</td><td>30 cycle</td></tr>
+	<tr><td>Cycle 3</td><td>68℃</td><td>60 sec</td><td>Elongation</td><td>30 cycle</td></tr>
+	<tr><td>Store</td><td>4℃</td><td>Hold</td><td>Store</td><td></td></tr>
+</table>
+<!-- PCR 3STEP END -->
+<!-- Electrophoresis -->
+<h4>Electrophoresis</h4>
+<p>Onoda</p>
+<p>dT on pSB1C3, pLac - B0034 on pSB1C3, pTet - B0034 on pSB1C3, B0034 on pSB1A2</p>
+<table>
+	<tr><th>Gel Concentration</th><th>Voltage</th><th>Time</th><th>Buffer</th></tr>
+	<tr><td>2%</td><td>100 A</td><td>30 min</td><td>2x TBE</td></tr>
+</table>
+<!-- Electrophoresis END -->
+<h3>2015/07/26</h3>
+<!-- Liquid Culture -->
+<h4>Liquid Culture</h4>
+<p>Ono</p>
+<p>pTet - B0034 on pSB1A2</p>
+<table>
+	<tr><th>Reagent</th><th>Volume</th></tr>
+	<tr><td>Single Colony</td><td>-</td></tr>
+	<tr><td>LB</td><td>2000 μL</td></tr>
+	<tr><td>Ampicillin</td><td>2 μL</td></tr>
+</table>
+<p>Cultured for 15 hours.</p>
+<!-- Liquid Culture END -->
+<!-- Mini-prep -->
+<h4>Mini-prep</h4>
+<p>実験者</p>
+<p>pLac - B0034 on pSB1C3, dT on pSB1C3, B0034 on pSB1A2
+	<br>FastGene<sup>TM</sup> Plasmid mini kit (Nippon Genetics Co.,Ltd)
+	<br>standard protocol</p>
+<!-- Mini-prep END -->
+<!-- Electrophoresis -->
+<h4>Electrophoresis</h4>
+<p>実験者</p>
+<p>pTet - B0034 on pSB1C3, pLac - B0034 on pSB1C3, B0034 on pSB1A3, dT on pSB1C3</p>
+<table>
+	<tr><th>Gel Concentration</th><th>Voltage</th><th>Time</th><th>Buffer</th></tr>
+	<tr><td>2%</td><td>100 A</td><td>30 min</td><td>2x TBE</td></tr>
+</table>
+<!-- Electrophoresis END -->
+<!-- Gel Extract -->
+<h4>Gel Extract</h4>
+<p>Ono</p>
+<p>pLac - B0034 on pSB1C3, pTet - B0034 on pSB1C3, B0034 on pSB1A2, dT on pSB1C3
+	<br>FastGene<sup>TM</sup> Gel/PCR Extraction kit (Nippon Genetics Co.,Ltd)
+	<br>DNA extraction from gel</p>
+<!-- Gel Extract END -->
+<h3>2015/07/27</h3>
+<!-- Mini-prep -->
+<h4>Mini-prep</h4>
+<p>Ono</p>
+<p>pTet - B0034 on pSB1A2
+	<br>FastGene<sup>TM</sup> Plasmid mini kit (Nippon Genetics Co.,Ltd)
+	<br>standard protocol</p>
+<!-- Mini-prep END -->

Difference between revisions of "Team:HokkaidoU Japan/Notebook/ecoli"

Revision as of 08:30, 28 August 2015

E. coli

March

2015/03/10

Competent Cells

2015/03/11

PCR

PCR Purification

Digestion

Electrophoresis

Gel Extract

Electrophoresis

May

2015/05/13

Transformation

Transformation

Competent Cells

2015/05/27

Transformation

Transformation

2015/05/29

Mini-prep

PCR

2015/05/30

Electrophoresis

Gel Extract

Digestion

Digestion

2015/05/31

Electrophoresis

Gel Extract

Electrophoresis

PCR

June

2015/06/10

Digestion

2015/06/16

PCR

2015/06/17

Electrophoresis

Annealing Oligos and Elongation

2015/06/19

Electrophoresis

Gel Extract

Ligation

2015/06/21

Transformation

July

2015/07/25

Transformation

Transformation

Transformation

Transformation

PCR

Electrophoresis

2015/07/26

Liquid Culture

Mini-prep

Electrophoresis

Gel Extract

2015/07/27

Mini-prep