Team:TMU-Tokyo/Notebook/Experiment/1st week (8.13 - 8.19)

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(Difference between revisions)

Latest revision as of 15:06, 26 September 2012

■Experiment
1st week (8.13 - 8.19)
2nd week (8.20 - 8.26)
3rd week (8.27 - 9. 2)
4th week (9. 3 - 9. 9)
5th week (9.10 - 9.16)
6th week (9.17 - 9.23)
7th week (9.24 - 9.30)

Experiment

■1st week (8.13 - 8.19)

■ 14th Aug
(Construction of Device3) ・PCR of vector (BBa_K299009) and insert (fdh4AB) ・Preparation of 1.5 % Agarose Gel Electrophoresis
→Failure: because of Preparation of Gel protocol miss

・Preparation of 1.5 % Agarose Gel Electrophoresis (again)
→Failure: because of Preparation of Gel protocol miss

・Preparation of 1.5 % Agarose Gel
→Failure: because of PCR protocol miss

・PCR of vector (BBa_K299009) and insert (fdh4AB) ・Preparation of 0.8 % Agarose Gel ・Correction of the PCR protocol and Preparation of Gel protocol

■15th Aug

(Construction of Device3)
・Electrophoresis of previous sample
→Failure: because of PCR protocol miss
・PCR of vector (BBa_K299009) and insert (fdh4AB)
・Preparation of 0.8 % Agarose Gel Electrophoresis
→Failure: because of smear
・PCR of vector (BBa_K299009)

・Digestion
1. Mixed following: total 20µL
(DW 15µL / DNA solution 2µL / 10x L buffer 2µL / SacI 1µL;)
2. Incubated at 37 °C for 1 hour.
3. Heat inactivated at 65 °C for 10 minutes.
4. Mixed: Total 50µL
(DW 24µL / Reaction solution 20µL / 10x K buffer 5µL / BamHI 1µL;)
5. Incubated at 37 °C for 1 hour 40 minutes.

・Electrophoresis
Put an agalose gel into the tank, and poured TBE buffer.
Mixed DNA samples: loading buffer = 9: 1. Loaded samples into wells.
Electrophoresed, stopped when samples move to 2/3.

・Gel extraction
Excised the DNA fragment from an agarose gel. For each 100 mg of agarose gel added 200µL Buffer NT.
Incubated sample for 5 – 10 minutes at 50 C. Vortexed the sample briefly every 2 – 3 minuets until the gel slice was completely dissolved.
Placed a NucleoSpin Extract II Columu into a Collection Tube and loaded the sample. Centrifuged for 30 seconds at 11,000x g. Discarded flow-through and placed the column backed into the collection tube.
Added 700µL Buffer NT3 to the NucleoSpin Extact II Column. Centrifuged for 30 s at 11,000x g. Discarded flow-through and placed the column backed into the collection tube.
Centrifuged for 1 min at 11,000x g to remove Buffer NT3 completely.
Placed the NucleoSpin Extract II Column into a new 1.5 ml microcetrifuge tube. Added 30µL Buffer NE and incubated at room temperature for 1 min. Centrifuged for 1 min at 11,000x g.

・Densitometry
Diluted DNA samples 50 times with a solvent.
Turned on the machine; GeneQuant 100.
Poured the solvent 100µL into a cuvette and adjusted 0.
Threw the solvent, poured the DNA sample.
Measured the concentration.

・Results
Concentration of a back bone plasmid was 53 ng /μl.
We could not obtain the target fragments of fdh4AB.

■16th Aug

(Construction of Device3)
・Preparation of 0.8 % Agarose Gel Electrophoresis
→Success: We observed appropriate bands!
・PCR of insert (fdh4AB) ・Check the fdh4AB primer’s sequence

・Refine of PCR products: fdh4AB and Backbone plasmid
Mixed 1 volume of sample with 2 volumes of Buffer NT.
Placed a NucleoSpin Extract II Column into a Collection Tube and loaded the sample. Centrifuged for 30 s at 11,000x g. Discarded flow-through and placed the column back into the collection tube.
Added 700µL Buffer NT3 to the NucleoSpin Extract II Column. Centrifuged for 30 s at 11,000x g. Discarded flow-though and placed the column back into the collection tube.
Centrifuged for 1 minute at 11,000x g to remove Buffer NT3 completely.
Placed the NucleoSpin Extract II Column into a new 1.5 ml microcentrifuge tube. Added 30µL Buffer NE and incubated at room temperature for 1 min. Centrifuged for 1 minute at 11,000x g.

・Densitometry
Diluted DNA samples 50 times with a solvent.
Turned on the machine; GeneQuant 100.
Poured the solvent 100 μl into a cuvette and adjusted 0.
Threw the solvent, poured the DNA sample.
Measured the concentration.

・Results
Concentration of fdh4AB was 210 ng/ μl.
Backbone plasmid No. 01 was 110 ng/ μl
No. 02 was 60 ng/ μl

・Digestion
1. Mixed following
Fdh4AB: total 25µL (milliQ 6.5µL / DNA solution 15µL / 10x L buffer 2.5µL / SacI 1µL)
Backbone plasmid: total 25µL (milliQ 1.5µL / DNA solution 20µL / 10x L buffer 2.5µL / SacI 1µL)
2. Incubated for 1 hour at 37 °C.
3. Heat inactivated at 65 °C for 10 minutes.
4. Mixed following; total 50µL (milliQ 19µL / Reaction solution 25 µL / 10x K buffer 5µL / BamHI 1µL)
5. Incubated at 37 °C for 1 hour.

・Gel extraction
Excised the DNA fragment from an agarose gel. For each 100 mg of agarose gel added 200 μl Buffer NT.
Incubated sample for 5 – 10 minutes at 50 °C. Vortexed the sample briefly every 2 – 3 minuets until the gel slice was completely dissolved.
Placed a NucleoSpin Extract II Columu into a Collection Tube and loaded the sample. Centrifuged for 30 seconds at 11,000 x g. Discarded flow-through and placed the column back into the collection tube.
Added 700 μl Buffer NT3 to the NucleoSpin Extact II Column. Centrifuged for 30 seconds at 11,000 x g. Discarded flow-through and placed the column back into the collection tube.
Centrifuged for 1 minute at 11,000 x g to remove Buffer NT3 completely.
Placed the NucleoSpin Extract II Column into a new 1.5 ml microcentrifuge tube. Added 50 μl Buffer NE and incubated at room temperature for 1 minute. Centrifuged for 1 minute at 11,000 x g.

・Results
We could not obtain the target band of fdh4AB.

・Densitometry
Diluted DNA samples 50 times with a solvent.
Turned on the machine; GeneQuant 100.
Poured the solvent 100 μl into a cuvette and adjusted 0.
Threw the solvent, poured the DNA sample.
Measured the concentration.

・Results
Concentration of backbone plasmid was 48 ng/ μl.

■17th Aug

(Construction of Device3)
・Preparation of 0.8 % Agarose Gel ・Electrophoresis →Failure: because of different bands ・PCR of insert (fdh4AB) ・Preparation of 0.8 % Agarose Ge

Electrophoresis of PCR products: before digestion of fdh4AB, after PCR products clean-up of fdh4AB, before PCR products clean-up of fdh4AB and diluted 100 times of PCR products of fdh4AB.
Put an agalose gel into the tank, and poured TBE buffer.
Mixed DNA samples: loading buffer = 9: 1. Loaded samples into wells.
Electrophoresed, stopped when samples move to 2/3.

・Results
Every sample was smeared. It seemed that PCR didn’t run well.

■18th Aug

(Construction of Device3)
・Electrophoresis
→Failure: because of deterioration of Loading buffer
・Preparation of 0.8 % Agarose Gel
・Electrophoresis
→Failure: because of miss of fdh4AB primer’s sequence
・Redesign and Order new fdh4AB primer

@@ Line 18: / Line 18: @@
 <Br>
 <B>■Experiment</B><Br>
-st week (8.13 - 8.19)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/1st_week_(8.13_-_8.19)">1st week (8.13 - 8.19)</A></B><Br>
-nd week (8.20 - 8.26)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/2nd_week_(8.20_-_8.26)">2nd week (8.20 - 8.26)</A></B><Br>
-rd week (8.27 - 9. 2)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/3rd_week_(8.27_-_9._2)">3rd week (8.27 - 9. 2)</A></B><Br>
-th week (9. 3 - 9. 9)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/4th_week_(9._3_-_9._9)">4th week (9. 3 - 9. 9)</A></B><Br>
-th week (9.10 - 9.16)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/5th_week_(9.10_-_9.16)">5th week (9.10 - 9.16)</A></B><Br>
-th week (9.17 - 9.23)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/6th_week_(9.17_-_9.23)">6th week (9.17 - 9.23)</A></B><Br>
-th week (9.24 - 9.30)<Br>
+<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Experiment/7th_week_(9.24_-_9.30)">7th week (9.24 - 9.30)</A></B><Br>
 <Br>
 <Br>
-<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Protocol/">■Protocols</A></B><Br>
-Plasmid DNA Purification<Br>
-Genome DNA Purification<Br>
-Restruction Enzyme Degestion<Br>
-DNA Fragment Ligation<Br>
-Transformation<Br>
-Electrophoresis<Br>
-LB Medium<Br>
-<Br>
-<Br>
-<B><A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Assay">■Assay</A></B><Br>
-Device1 Assay<Br>
-Device2 Assay<Br>
-Device3 Assay<Br>
@@ Line 61: / Line 48: @@
 <b>■1st week (8.13 - 8.19)</b><Br></p>
 <Br>
-th Aug<br />
+<p class="description3">
-Digestion<br />
+<b>■ 14th Aug</b><br />
-. Mixed following<br />
+(Construction of Device3)
-DW			15 μl<br />
+ <b>・PCR of vector (BBa_K299009) and insert (fdh4AB)</b>
-DNA solution		 2 μl<br />
+ ・Preparation of 1.5 % Agarose Gel Electrophoresis<Br>
-x L buffer		 2 μl<br />
+ →Failure: because of Preparation of Gel protocol miss<Br>
-SacI			 1 μl
+<Br>
-Total		20 μl
+ ・Preparation of 1.5 % Agarose Gel Electrophoresis (again)<Br>
-	<br />
+ →Failure: because of Preparation of Gel protocol miss<Br>
+<Br>
+ ・Preparation of 1.5 % Agarose Gel<Br>
+ →Failure: because of PCR protocol miss<Br>
+<Br>
+ <b>・PCR of vector (BBa_K299009) and insert (fdh4AB)</b>
+ ・Preparation of 0.8 % Agarose Gel
+・Correction of the PCR protocol and Preparation of Gel protocol<Br>
+<Br>
+<Br>
+<b>■15th Aug</b><br />
+<Br>
+(Construction of Device3)<Br>
+・Electrophoresis of previous sample<Br>
+→Failure: because of PCR protocol miss<Br>
+  <b>・PCR of vector (BBa_K299009) and insert (fdh4AB)</b><Br>
+  ・Preparation of 0.8 % Agarose Gel Electrophoresis<Br>
+→Failure: because of smear<Br>
+  <b>・PCR of vector (BBa_K299009)</b><Br>
+<Br>
+<b>・Digestion</b><br />
+. Mixed following: total 20µL<br />
+(DW 15µL / DNA solution 2µL / 10x L buffer 2µL / SacI 1µL;)<Br>
 . Incubated at 37 °C for 1 hour.<br />
 . Heat inactivated at 65 °C for 10 minutes.<br />
-. Mixed<br />
+. Mixed: Total 50µL<br />
-DW			24 μl<br />
+(DW 24µL / Reaction solution 20µL / 10x K buffer 5µL / BamHI 1µL;)<Br>
-Reaction solution	20 μl<br />
-x K buffer		 5 μl<br />
-BamHI			 1 μl
-Total		50 μl
-<br />
 . Incubated at 37 °C for 1 hour 40 minutes.<br />
 <br />
-Electrophoresis<br />
+<b>・Electrophoresis</b><br />
 Put an agalose gel into the tank, and poured TBE buffer.<br />
 Mixed DNA samples: loading buffer = 9: 1. Loaded samples into wells.<br />
 Electrophoresed, stopped when samples move to 2/3.<br />
 <br />
-Gel extraction<br />
+<b>・Gel extraction</b><br />
-Excised the DNA fragment from an agarose gel. For each 100 mg of agarose gel added 200 μl Buffer NT.<br />
+Excised the DNA fragment from an agarose gel. For each 100 mg of agarose gel added 200µL Buffer NT.<br />
 Incubated sample for 5 – 10 minutes at 50 C. Vortexed the sample briefly every 2 – 3 minuets until the gel slice was completely dissolved.<br />
-Placed a NucleoSpin Extract II Columu into a Collection Tube and loaded the sample. Centrifuged for 30 seconds at 11,000 x g. Discarded flow-through and placed the column backed into the collection tube.<br />
+Placed a NucleoSpin Extract II Columu into a Collection Tube and loaded the sample. Centrifuged for 30 seconds at 11,000x g. Discarded flow-through and placed the column backed into the collection tube.<br />
-Added 700 μl Buffer NT3 to the NucleoSpin Extact II Column. Centrifuged for 30 seconds at 11,000 x g. Discarded flow-through and placed the column backed into the collection tube.<br />
+Added 700µL Buffer NT3 to the NucleoSpin Extact II Column. Centrifuged for 30 s at 11,000x g. Discarded flow-through and placed the column backed into the collection tube.<br />
-Centrifuged for 1 minute at 11,000 x g to remove Buffer NT3 completely.<br />
+Centrifuged for 1 min at 11,000x g to remove Buffer NT3 completely.<br />
-Placed the NucleoSpin Extract II Column into a new 1.5 ml microcetrifuge tube. Added 30 μl Buffer NE and incubated at room temperature for 1 minute. Centrifuged for 1 minute at 11,000 x g.<br />
+Placed the NucleoSpin Extract II Column into a new 1.5 ml microcetrifuge tube. Added 30µL Buffer NE and incubated at room temperature for 1 min. Centrifuged for 1 min at 11,000x g.<br />
 <br />
-Densitometry<br />
+<b>・Densitometry</b><br />
 Diluted DNA samples 50 times with a solvent.<br />
 Turned on the machine; GeneQuant 100.<br />
-Poured the solvent 100 μl into a cuvette and adjusted 0.<br />
+Poured the solvent 100µL into a cuvette and adjusted 0.<br />
 Threw the solvent, poured the DNA sample.<br />
 Measured the concentration. <br />
 <br />
-Results<br />
+<b>・Results</b><br />
 Concentration of a back bone plasmid was 53 ng /μl.<br />
 We could not obtain the target fragments of fdh4AB.<br />
 <br />
-th Aug<br />
+<Br>
-Refine of PCR products: fdh4AB and Backbone plasmid<br />
+<b>■16th Aug</b><br />
+<Br>
+(Construction of Device3)<Br>
+・Preparation of 0.8 % Agarose Gel Electrophoresis<Br>
+→Success: We observed appropriate bands!<Br>
+  ・PCR of insert (fdh4AB)
+・Check the fdh4AB primer’s sequence
+<Br>
+<Br>
+<Br>
+<b>・Refine of PCR products</b>: fdh4AB and Backbone plasmid<br />
 Mixed 1 volume of sample with 2 volumes of Buffer NT.<br />
-Placed a NucleoSpin Extract II Column into a Collection Tube and loaded the sample. Centrifuged for 30 seconds at 11,000 x g. Discarded flow-through and placed the column back into the collection tube.<br />
+Placed a NucleoSpin Extract II Column into a Collection Tube and loaded the sample. Centrifuged for 30 s at 11,000x g. Discarded flow-through and placed the column back into the collection tube.<br />
-Added 700 μl Buffer NT3 to the NucleoSpin Extract II Column. Centrifuged for 30 seconds at 11,000 x g. Discarded flow-though and placed the column back into the collection tube.<br />
+Added 700µL Buffer NT3 to the NucleoSpin Extract II Column. Centrifuged for 30 s at 11,000x g. Discarded flow-though and placed the column back into the collection tube.<br />
-Centrifuged for 1 minute at 11,000 x g to remove Buffer NT3 completely.<br />
+Centrifuged for 1 minute at 11,000x g to remove Buffer NT3 completely.<br />
-Placed the NucleoSpin Extract II Column into a new 1.5 ml microcentrifuge tube. Added 30 μl Buffer NE and incubated at room temperature for 1 minute. Centrifuged for 1 minute at 11,000 x g.<br />
+Placed the NucleoSpin Extract II Column into a new 1.5 ml microcentrifuge tube. Added 30µL Buffer NE and incubated at room temperature for 1 min. Centrifuged for 1 minute at 11,000x g.<br />
 <br />
-Densitometry<br />
+<b>・Densitometry</b><br />
 Diluted DNA samples 50 times with a solvent.<br />
 Turned on the machine; GeneQuant 100.<br />
@@ Line 120: / Line 139: @@
 Measured the concentration. <br />
 <br />
-Results<br />
+<b>・Results</b><br />
 Concentration of 	fdh4AB			was 210 ng/ μl.<br />
 			Backbone plasmid No. 01	was 110 ng/ μl<br />
 			                  No. 02 was 60 ng/ μl<br />
-Digestion<br />
+<Br>
-Mixed following<br />
+<b>・Digestion</b><br />
-Fdh4AB<br />
+. Mixed following<br />
-milliQ			6.5 μl<br />
+Fdh4AB: total 25µL (milliQ 6.5µL / DNA solution 15µL / 10x L buffer 2.5µL / SacI 1µL)<br />
-DNA solution		15 μl<br />
+Backbone plasmid: total 25µL (milliQ 1.5µL / DNA solution 20µL / 10x L buffer 2.5µL / SacI 1µL)<br />
-x L buffer		2.5 μl<br />
-SacI			 1 μl
-Total		25 μl
-<br />
-Backbone plasmid<br />
-milliQ			1.5 μl<br />
-DNA solution		20 μl<br />
-x L buffer		2.5 μl<br />
-SacI			 1 μl
-Total		25 μl
-<br />
 . Incubated for 1 hour at 37 °C.<br />
 . Heat inactivated at 65 °C for 10 minutes.<br />
-. Mixed following<br />
+. Mixed following; total 50µL (milliQ 19µL / Reaction solution	25 µL / 10x K buffer 5µL / BamHI 1µL)<br />
-milliQ			19 μl<br />
-Reaction solution	25 μl<br />
-x K buffer		 5 μl<br />
-BamHI			 1 μl
-Total		50 μl
-<br />
 . Incubated at 37 °C for 1 hour.<br />
 <br />
-Gel extraction<br />
+<b>・Gel extraction</b><br />
 Excised the DNA fragment from an agarose gel. For each 100 mg of agarose gel added 200 μl Buffer NT.<br />
 Incubated sample for 5 – 10 minutes at 50 °C. Vortexed the sample briefly every 2 – 3 minuets until the gel slice was completely dissolved.<br />
@@ Line 159: / Line 161: @@
 Placed the NucleoSpin Extract II Column into a new 1.5 ml microcentrifuge tube. Added 50 μl Buffer NE and incubated at room temperature for 1 minute. Centrifuged for 1 minute at 11,000 x g.<br />
 <br />
-Results<br />
+<b>・Results</b><br />
 We could not obtain the target band of fdh4AB.<br />
 <br />
-Densitometry<br />
+<b>・Densitometry</b><br />
 Diluted DNA samples 50 times with a solvent.<br />
 Turned on the machine; GeneQuant 100.<br />
@@ Line 169: / Line 171: @@
 Measured the concentration. <br />
 <br />
-Results<br />
+<b>・Results</b><br />
 Concentration of backbone plasmid was 48 ng/ μl.<br />
 <br />
-th Aug<br />
+<Br>
-Electrophoresis of PCR products: before digestion of fdh4AB, after PCR products clean-up of fdh4AB, before PCR products clean-up of fdh4AB and diluted 100 times of PCR products of fdh4AB.<br />
+<b>■17th Aug</b><br />
-<br />
+<Br>
+(Construction of Device3)<Br>
+・Preparation of 0.8 % Agarose Gel
+・Electrophoresis
+→Failure: because of different bands
+・<b>PCR of insert (fdh4AB)</b>
+・Preparation of 0.8 % Agarose Ge<Br>
+<Br>
+<b>Electrophoresis of PCR products</b>: before digestion of fdh4AB, after PCR products clean-up of fdh4AB, before PCR products clean-up of fdh4AB and diluted 100 times of PCR products of fdh4AB.<br />
 Put an agalose gel into the tank, and poured TBE buffer.<br />
 Mixed DNA samples: loading buffer = 9: 1. Loaded samples into wells.<br />
 Electrophoresed, stopped when samples move to 2/3.<br />
 <br />
-Results<br />
+<b>・Results</b><br />
 Every sample was smeared. It seemed that PCR didn’t run well.<br />
+<Br>
+<b>■18th Aug</b><br />
+<Br>
+(Construction of Device3)<Br>
+・Electrophoresis<Br>
+→Failure: because of deterioration of Loading buffer<Br>
+・Preparation of 0.8 % Agarose Gel<Br>
+・Electrophoresis<Br>
+→Failure: because of miss of fdh4AB primer’s sequence<Br>
+<b>・Redesign and Order new fdh4AB primer</b>
+<Br>
 <Br>