Latest revision as of 13:28, 27 October 2010

RBS digestion: Revenge

Reagent	Amount
1-2M	10 uL
DW	4 uL
10x M Buffer	2 uL
BSA	2 uL
Xba I	1 uL
Pst I	1 uL
Total	20 uL

->Incubated at 37C for 60 min

Added 4 uL of 6x Sample Buffer making it total of 12 uL per lane and electrophoresed

->Extracted for gel
->Electrophoresed 10 uL of Extracted DNA

Used TSUDA Marker 1

Failure

After better inspection of Kit specs it came to lite that retreavel rate for 50 bp and less is 26%
- RBS is just quite small when cut

Ligation

Preparation of DNA Solution for Ligation

Part	By comparison toλ/Hind III (ng/10 uL)	ng/uL	ratio	size(bp)	required(ng)	used(uL)
Vector	50 ng/10 uL	5 ng/uL	1	2996 bp	10 ng	2 uL
RFP	250 ng/10 uL	25 ng/uL	2	700 bp	7 ng	0.3 uL
terminator	5 ng/10 uL	0.5 ng/uL	2	200 bp	2 ng	4 uL
Total						6.3 uL

Ligation and Transformation

Reagent	Amount
DNA solution	6.3 uL
Ligation solution	6.3 uL
T4 ligase	1 uL
Total	13.6 uL

Incubated at 16C for 30 min
Transformation: Added all to 50 uL of competent cell
Incubated at 0C for 30 min
Heat shocked at 42C for 60 sec
5 min on ice
Added 100 uL of LB
Incubated at 37C for 120 min
Spread onto the LBC plate
Incubated at 37C for 20 hrs

RBS Retry

Digestion

Reagent	Amount
（RBS）1-2M	10 uL
DW	4 uL
10x M Buffer	2 uL
BSA	2 uL
Xba I	1 uL
Pst I	1 uL
Total	20 uL

->Incubated at 37C for 60 min

Ethanol Precipication

Added 2 uL of sodium acetate(3 M)
Added 44 uL of Ethanol
Transfered to 1.5 mL tube and frozen with liquid nitrogen
Melted and centrifuged at 15000 rpm, 4C for 5 min
Transfered supernatant to another tube
- Driven by precaution centrifuged the supernatant and discarded it's supernatant
Rinsed the tube walls with 100 uL of 70% Ethanol and centrifuged at 15000 rpm, 4C for 5 min
Discarded the supertenant and dried via vacuum desiccator
Melted in 5 uL of TE

Electrophoresis

Electrophoresis after Ethanol presipication

Added 1 uL of 6x SB to DNA Solution of 1 uL
Did the same to supernatant　retreaved for precaution

Lane	DNA
2	TSUDA Marker 1
3	supernatant
4	DNA solution

DNA solution band is visible
- Looks OK

@@ Line 27: / Line 27: @@
 |style="border-top:1px solid #996"|'''20 uL'''
 |}
-→Incubated at 37C for 60 min
+->Incubated at 37C for 60 min
 * Added 4 uL of 6x Sample Buffer making it total of 12 uL per lane and electrophoresed
-→Extracted for gel <br>
+->Extracted for gel <br>
-→Electrophoresed 10 uL of Extracted DNA
+->Electrophoresed 10 uL of Extracted DNA
 * Used [https://2010.igem.org/Image:HokkaidoU_Pictures_DNA_Marker.png TSUDA Marker 1]
@@ Line 39: / Line 39: @@
 =Ligation=
 ===Preparation of DNA Solution for Ligation===
-{|style="text-align:center;" class="protocol"
+{|border="1px" style="text-align:center;" class="protocol"
 |-
 !Part
-![https://2010.igem.org/Image:HokkaidoU_Pictures_DNA_Marker.png Lambda/''Hin''d III] と比べて (ng/10 uL)
+!By comparison to[https://2010.igem.org/Image:HokkaidoU_Pictures_DNA_Marker.png λ/''Hin''d III]<br>(ng/10 uL)
 !ng/uL
-!割合
+!ratio
-!size (bp)
+!size(bp)
-!必要 (ng)
+!required(ng)
-!使用 (uL)
+!used(uL)
 |-
 |Vector
@@ Line 65: / Line 65: @@
 |0.3 uL
 |-
-|double terminator
+|terminator
 |5 ng/10 uL
 |0.5 ng/uL
@@ Line 77: / Line 77: @@
 |}
-===Ligation & Transformation===
+===Ligation and [[Team:HokkaidoU_Japan/Protocols|Transformation]]===
 {|style="text-align:center;" class="protocol"
 !Reagent
@@ Line 95: / Line 95: @@
 |}
-* 16℃，30 min
+* Incubated at 16C for 30 min
-* competent cell 50 uLに全量加えた（Transformation）
+* Transformation: Added all to 50 uL of competent cell
-* 0℃，30 min
+* Incubated at 0C for 30 min
-* 42℃，60 sec
+* Heat shocked at 42C for 60 sec
 * 5 min on ice
-* add LB 100 uL
+* Added 100 uL of LB
-* 37℃，120 min
+* Incubated at 37C for 120 min
-* spread onto the LBC
+* Spread onto the LBC plate
-* 37℃，15~20 hrs
+* Incubated at 37C for 20 hrs
-=RBS 再リベンジ=
+=RBS Retry=
 ==Digestion==
 {|style="text-align: center" class="protocol"
@@ Line 132: / Line 132: @@
 |style="border-top:1px solid #996"|'''20 uL'''
 |}
-→37℃，60 min
+->Incubated at 37C for 60 min
-==エタ沈==
+==[[Team:HokkaidoU_Japan/Protocols|Ethanol Precipication]]==
-* 2 uLの3 M 酢酸ナトリウムを加えた
+* Added 2 uL of sodium acetate(3 M)
-* 44 uLのエタノールを加えた
+* Added 44 uL of Ethanol
-* 液体窒素の中で凍らせた（'''1.5 mLのチューブに移す'''）
+* Transfered to 1.5 mL tube and frozen with liquid nitrogen
-* 溶かしてから15,996 rpm @4℃で５分間遠心した
+* Melted and centrifuged at 15000 rpm, 4C for 5 min
-* 上清をほかのチューブに移した（一応これも遠心し，上清を捨て，同じ操作をした）
+* Transfered supernatant to another tube
-* 100 uLの70%エタノールで壁をリンスし，15,996 rpm @4℃で５分間遠心した
+** Driven by precaution centrifuged the supernatant and discarded it's supernatant
-* 上清を捨て，真空デシケータで乾燥させた
+* Rinsed the tube walls with 100 uL of 70% Ethanol and centrifuged at 15000 rpm, 4C for 5 min
-* TE 5 uLで溶かした
+* Discarded the supertenant and dried via vacuum desiccator
+* Melted in 5 uL of TE
-==電気泳動==
+==Electrophoresis==
-[[Image:HokkaidoU Japan 20100818b.JPG‎|200px|right|thumb|]]
+[[Image:HokkaidoU Japan 20100818b.JPG‎|200px|right|thumb| Electrophoresis after Ethanol presipication]]
-* TEで溶かしたDNA Solution 1 uLに6x SB 1 uLを加えた
+* Added 1 uL of 6x SB to DNA Solution of 1 uL
-* 最初にとった上清も同じ操作をした
+* Did the same to supernatant　retreaved for precaution
 {| class="protocol"
@@ Line 155: / Line 156: @@
 |-
 |2
-|TSUDA Marker 1
+|[https://2010.igem.org/Image:HokkaidoU_Pictures_DNA_Marker.png TSUDA Marker 1]
 |-
 |3
-|上清
+|supernatant
 |-
 |4
 |DNA solution
 |}
-* DNA solutionにしっかり回収されていた
+* DNA solution band is visible
+** Looks OK

Team:HokkaidoU Japan/Notebook/August18

From 2010.igem.org

Latest revision as of 13:28, 27 October 2010

RBS digestion: Revenge

Failure

Ligation

Preparation of DNA Solution for Ligation

Ligation and Transformation

RBS Retry

Digestion

Ethanol Precipication

Electrophoresis