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Creating parts of Tar methylation region

Date:8/9

Colony PCR

Reagent

TaKaRa Ex Taq(5units/μL) 0.5μL
10×Ex Taq buffer 10μL
dNTP Mixture(2.5Meach) 8μL
Primer F(10μM) 4μL
Primer R(10μM) 4μL
Template(E.coli DH5α)

→Reflection:We Took E.coli too many.You should take less E.coli.

Conditions of the thermal cycler

95°C(5min)
94°C(30sec)
61°C(30sec)
71°C(40sec)
72°C(1min)
4°C(Save)
- 2-4:35cycle→Reflection:The number of cycles was less.So,We increased The number of cycles in 8/11.(50 cycles)
- gradient:60-61°C(+0.1°C)

Date:8/11

The purified DNA

Electrophoresis
- Marker:dye 1μL,DNA molecule 2μL,TE buffer 3μL
- Sample:dye 1μL,sample 5μL
- Gel concentration:1.2%,Migration time:30min

→Reflection:Band was less.

Storage

PCR Product

Electrophoresis
- The gel check and cut
DNA purification
Confirmation of electrophoresis
PCR
- 50cycle
Storage

Date:8/13

Confirmed of electrophoresis by PCR product and Ligation of the TA vector

Electrophoresis
- Gel concentration:1.2%,Migration time:30min
- Marker:Flash Gel 5μL
- Sample:dye 1μL,sample 5μL
Check and Colony PCR
Add to TA vector
- PCR product 2μL
- pMD20-Tvector 1μL
- D₂W 2μL
- Ligation Mighty Mix 5μL
Heat insulation(16°C,30min)
Storage(-20°C)

Date:8/14

Transformation

Put competent cells on ice(10-15min)
Add Ligation reaction solution(10μL) and tapping
On the ice(30min)[Transformation]
Add LB medium(0.7mL)
Incubate(60min,37°C)
Add X-gal(40μL) and ampicillin(10μL)[200μg/mL] on LB agar medium(IPTG)
Add one incubated(100μL)
Cultivation(overnight)

Creating parts of azurin

Date:8/16

Colony PCR

Reagent

TaKaRa Ex Taq(5units/μL) 0.5μL
10×Ex Taq buffer 10μL
dNTP Mixture(2.5Meach) 8μL
Primer F(10μM) 4μL
Primer R(10μM) 4μL
Template(E.coli DH5α)
sterilized water(73.5μL)

Conditions of the thermal cycler

95°C(5min)
94°C(30sec)
61°C(30sec)
71°C(40sec)
72°C(1min)
4°C(Save)
- 2-4:30cycle
- gradient:57-62°C(+0.1c)

Ligation

Reagent

sterilize water 2μL
PCR product 2μL
vector DNA 1μL
Ligation Mighty Mix 5μL

Method

Incubation(1h,16°C)
Storage Overnight(-4°C)

Date:8/18

Colony PCR

Reagent

TaKaRa Ex Taq(5units/μL) 0.5μL
10×Ex Taq buffer 10μL
dNTP Mixture(2.5Meach) 8μL
Primer F(10μM) 4μL
Primer R(10μM) 4μL
Template(E.coli DH5α)
sterilized water(73.5μL)

Conditions of the thermal cycler

95°C(5min)
94°C(30sec)
61°C(30sec)
71°C(40sec)
72°C(1min)
4°C(Save)
- 2-4:30cycle
- gradient:57-62°C(+0.1c)

Date:8/20

DNA extraction and purification of P.aeruginosa

Centrifuge culture medium(6,000rpm,5min,4°C)
Remove supernatant,Add saline[0.85%](1.5mL)
Centrifuge(6,000rpm,5min,4°C)
Add 5mMEDTA 1mL
Add 10%SDS 100μL
Add proteinase K 50methodL
Vortex
Incubation(30min,55°C)
Add phenol mixture(TE saturated phenol:chloroform:isoamyl alcohol=25:24:1)
Shake vigorously(1min)
- At this time,It became muddy white in color.
Centrifuge(16,000rpm,10min,4°C)
Pick up supernatant,remove new microtube
Repeat step 7-11
Add 3M-sodium acetate 40μL,chilled isopropanol 400μL
Vortex
Wind the DNA by a thin glass rod.
Rinse chilled 70%-ethanol(500μL)
Pick up DNA,air dry
Add TE buffer 500μL
Add RNase A 50μL
Incubation(20min,37°C)
Add proteinase K 50μL
Incubation(1h,37°C)
Add phenol mixture
Vortex(1min)
Centrifuge(16,000rpm,10min,4°C)
Pick up supernatant,remove new microtube
Add 3M-sodium acetate 40μL,chilled isopropanol 400μL
Wind the DNA by a thin glass rod.
Rinse chilled 70%-ethanol(500μL,about 30s)
Pick up DNA,air dry
Add TE buffer 200μL
- Melt DNA in buffer

@@ Line 56: / Line 56: @@
 ===Colony PCR===
 Reagent
-:*TaKaRa Ex Taq(5units/μL) 0.5μL
+:*TaKaRa Ex Taq(5units/&mu;L) 0.5&mu;L
-:*10×Ex Taq buffer 10μL
+:*10×Ex Taq buffer 10&mu;L
-:*dNTP Mixture(2.5Meach) 8μL
+:*dNTP Mixture(2.5Meach) 8&mu;L
-:*Primer F(10μM) 4μL
+:*Primer F(10&mu;M) 4&mu;L
-:*Primer R(10μM) 4μL
+:*Primer R(10&mu;M) 4&mu;L
 :*Template(E.coli DH5α)
 ::'''→Reflection:We Took E.coli too many.You should take less E.coli.'''<br>
@@ Line 78: / Line 78: @@
 ===The purified DNA===
 #Electrophoresis
-#*Marker:dye 1μL,DNA molecule 2μL,TE buffer 3μL
+#*Marker:dye 1&mu;L,DNA molecule 2&mu;L,TE buffer 3&mu;L
-#*Sample:dye 1μL,sample 5μL
+#*Sample:dye 1&mu;L,sample 5&mu;L
 #*Gel concentration:1.2%,Migration time:30min
 :::'''→Reflection:Band was less.'''
@@ Line 99: / Line 99: @@
 #Electrophoresis
 #*Gel concentration:1.2%,Migration time:30min
-#*Marker:Flash Gel 5μL
+#*Marker:Flash Gel 5&mu;L
-#*Sample:dye 1μL,sample 5μL
+#*Sample:dye 1&mu;L,sample 5&mu;L
 #Check and Colony PCR
 #Add to TA vector
-#*PCR product 2μL
+#*PCR product 2&mu;L
-#*pMD20-Tvector 1μL
+#*pMD20-Tvector 1&mu;L
-#*D<sub>2</sub>W 2μL
+#*D<sub>2</sub>W 2&mu;L
-#*Ligation Mighty Mix 5μL
+#*Ligation Mighty Mix 5&mu;L
 #Heat insulation(16°C,30min)
 #Storage(-20°C)
@@ Line 115: / Line 115: @@
 ===Transformation===
 #Put competent cells on ice(10-15min)
-#Add Ligation reaction solution(10μL) and tapping
+#Add Ligation reaction solution(10&mu;L) and tapping
 #On the ice(30min)[Transformation]
 #Add LB medium(0.7mL)
 #Incubate(60min,37°C)
-#Add X-gal(40μL) and ampicillin(10μL)[200μg/mL] on LB agar medium(IPTG)
+#Add X-gal(40&mu;L) and ampicillin(10&mu;L)[200&mu;g/mL] on LB agar medium(IPTG)
-#Add one incubated(100μL)
+#Add one incubated(100&mu;L)
 #Cultivation(overnight)
@@ Line 129: / Line 129: @@
 ===Colony PCR===
 Reagent
-:*TaKaRa Ex Taq(5units/μL) 0.5μL
+:*TaKaRa Ex Taq(5units/&mu;L) 0.5&mu;L
-:*10×Ex Taq buffer 10μL
+:*10×Ex Taq buffer 10&mu;L
-:*dNTP Mixture(2.5Meach) 8μL
+:*dNTP Mixture(2.5Meach) 8&mu;L
-:*Primer F(10μM) 4μL
+:*Primer F(10&mu;M) 4&mu;L
-:*Primer R(10μM) 4μL
+:*Primer R(10&mu;M) 4&mu;L
 :*Template(E.coli DH5α)
-:*sterilized water(73.5μL)
+:*sterilized water(73.5&mu;L)
 Conditions of the thermal cycler
 #95°C(5min)
@@ Line 159: / Line 159: @@
 ===Colony PCR===
 Reagent
-:*TaKaRa Ex Taq(5units/μL) 0.5μL
+:*TaKaRa Ex Taq(5units/&mu;L) 0.5&mu;L
-:*10×Ex Taq buffer 10μL
+:*10×Ex Taq buffer 10&mu;L
-:*dNTP Mixture(2.5Meach) 8μL
+:*dNTP Mixture(2.5Meach) 8&mu;L
-:*Primer F(10μM) 4μL
+:*Primer F(10&mu;M) 4&mu;L
-:*Primer R(10μM) 4μL
+:*Primer R(10&mu;M) 4&mu;L
 :*Template(E.coli DH5α)
-:*sterilized water(73.5μL)
+:*sterilized water(73.5&mu;L)
 Conditions of the thermal cycler
 #95°C(5min)
@@ Line 184: / Line 184: @@
 #Centrifuge(6,000rpm,5min,4°C)
 #Add 5mMEDTA 1mL
-#Add 10%SDS 100μL
+#Add 10%SDS 100&mu;L
-#Add proteinase K 50μL
+#Add proteinase K 50methodL
 #Vortex
 #Incubation(30min,55°C)
@@ Line 194: / Line 194: @@
 #Pick up supernatant,remove new microtube
 #Repeat step 7-11
-#Add 3M-sodium acetate 40μL,chilled isopropanol 400μL
+#Add 3M-sodium acetate 40&mu;L,chilled isopropanol 400&mu;L
 #Vortex
 #Wind the DNA by a thin glass rod.
-#Rinse chilled 70%-ethanol(500μL)
+#Rinse chilled 70%-ethanol(500&mu;L)
 #Pick up DNA,air dry
-#Add TE buffer 500μL
+#Add TE buffer 500&mu;L
-#Add RNase A 50μL
+#Add RNase A 50&mu;L
 #Incubation(20min,37°C)
-#Add proteinase K 50μL
+#Add proteinase K 50&mu;L
 #Incubation(1h,37°C)
 #Add phenol mixture
@@ Line 208: / Line 208: @@
 #Centrifuge(16,000rpm,10min,4°C)
 #Pick up supernatant,remove new microtube
-#Add 3M-sodium acetate 40μL,chilled isopropanol 400μL
+#Add 3M-sodium acetate 40&mu;L,chilled isopropanol 400&mu;L
 #Wind the DNA by a thin glass rod.
-#Rinse chilled 70%-ethanol(500μL,about 30s)
+#Rinse chilled 70%-ethanol(500&mu;L,about 30s)
 #Pick up DNA,air dry
-#Add TE buffer 200μL
+#Add TE buffer 200&mu;L
 #*Melt DNA in buffer
 |}

Team:KAIT Japan/Notebook

From 2012.igem.org

Revision as of 03:40, 22 August 2012

Contents

Creating parts of Tar methylation region

Date:8/9

Colony PCR

Date:8/11

The purified DNA

PCR Product

Date:8/13

Confirmed of electrophoresis by PCR product and Ligation of the TA vector

Date:8/14

Transformation

Creating parts of azurin

Date:8/16

Colony PCR

Ligation

Date:8/18

Colony PCR

Date:8/20

DNA extraction and purification of P.aeruginosa