Latest revision as of 00:39, 27 September 2012

GEMOTE Project

Week 11

13th August

Purification by PCR clean-up of BBa_K115017 treated with DPNI. To visualize the fragment, an electrophoresis has been made with a 2% Agarose gel. We are expecting a band at the size of 123 bp.
	New PCR of BBa_K115017 to obtain more quantity of the fragment

PCR program used:

Digestion by DPNI of the BBa_K115017 in order to degrade the matrix plasmid.

Determination of the concentration of plasmid pSB1A2 which has been linearized by HINDIII. We are expecting a band at size (2079+935) ~3kbp
A new PCR of the plasmid pSB1A2 is realized to obtain more quantity of the plasmid. We are expecting a band at size 2079 bp.

PCR program used:

14th August

Determination of the concentration of the BBa_K274100 by electrophoresis on a gel at O.8% Agarose. We are expecting a band at size 2100bp

Digestion of the BBa_K274100 by DPNI to degrade the matrix plasmid.
Stocking up cells with glycerol
- PSB1A3Amil CP + Ampicilline
- PSB1C3 Amil GFP + Chloramphinicol

15th August

French holiday.

16th August

PCR of BBa_K274100 and visualization by 0.8% Agarose gel electrophoresis. We are expecting a band at 3400bp.

PCR program used:

Digestion of the BBa_K274100 by DPNI to degrade the matrix plasmid.

17th august

Visualization of the DPNI’s digestion of the plasmid pSB1A2 by 0.8% Agarose gel electrophoresis. . We are expecting a band at size 2079 bp.

Miniprep of the pSB1A2 plasmid.
Miniprep of BBa_K274100 and BBa_K115017
Gibson assembly of the B construction
Transformation of DH5α competent cells with the Gibson B construction. The Petri dishes are placed at 37°C.

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-{{Team:Paris-Saclay/Follow}}
+='''Week 11'''=
-[[Category:Team:Paris-Saclay/Project Gemote/Notebook|5]]
-__NOTOC__
-====6th August====
-*Sending of the B1 sample to sequencing with two pairs of primers
-**K-274100 Forward and Reverse
-**Plasmid pSB1A2 Forward and Reverse
+[[Category:Team:Paris-Saclay/Project Gemote/Notebook|k]]
+__NOTOC__
+====13th August====
-====7th August====
+{| width="85%"
+|-
+| style="width: 50%;"|Purification by PCR clean-up of BBa_K115017 treated with DPNI. To visualize the fragment, an electrophoresis has been made with a 2% Agarose gel. We are expecting a band at the size of 123 bp.
+| style="width: 35%;"| [[File:Week11-1.jpg|right|280px]]
+|-
+| style="width: 50%;"|[[File:Week11-2.jpg|left|280px]]
+| style="width: 35%;"| New PCR of BBa_K115017 to obtain more quantity of the fragment
+|}
-*Liquid culture of B1 in order to prepare a glycerol stock
-**Receipt of new primers
-**2 Forward
-**3 Reverse
-**Plasmid Reverse
+PCR program used:
+[[File:Week11-3.jpg|500px]]
-====8th August====
+*Digestion by DPNI of the BBa_K115017 in order to degrade the matrix plasmid.
 {| width="85%"
 |-
-| style="width: 50%;"| Amplification of the plasmid pSB1A2, BBa_K274100 and BBa_K115017 by PCR with the new primers. Visualization by electrophoresis on a 2% Agarose gel for BBa_K115017 and a 0.8% Agarose gel for BBa_K274100 and the plasmid pSB1A2. We are expecting a band at 147 bp for BBa_K115017, 3408 bp for BBa_K274100 and 2079 for the plasmid.
+| style="width: 50%;"|Determination of the concentration of plasmid pSB1A2 which has been linearized by HINDIII. We are expecting a band at size (2079+935) ~3kbp
-| style="width: 35%;"| [[File:Week10-2.jpg|right|330px]]
+| style="width: 35%;"| [[File:Week11-4.jpg|right|280px]]
+|-
+| style="width: 50%;"|A new PCR of the plasmid pSB1A2 is realized to obtain more quantity of the plasmid. We are expecting a band at size 2079 bp.
+| style="width: 35%;"| [[File:Week11-5.jpg|right|280px]]
 |}
 PCR program used:
-[[File:Week10-3.jpg|600px]]
+[[File:Week11-6.jpg|500px]]
-====9th August====
+====14th August====
 {| width="85%"
 |-
-| style="width: 50%;"|New amplification by PCR of the plasmid pSB1A2, BBa_K274100 and BBa_K115017 as it has been done the day before.
+| style="width: 50%;"|Determination of the concentration of the BBa_K274100 by electrophoresis on a gel at O.8% Agarose. We are expecting a band at size 2100bp
-| style="width: 35%;"| [[File:Week10-4.jpg|right|330px]]
+| style="width: 35%;"| [[File:Week11-7.jpg|right|280px]]
 |}
-*Digestion by EcoRI of the plasmid that contains BBa_K274100.
+*Digestion of the BBa_K274100 by DPNI to degrade the matrix plasmid.
+*Stocking up cells with glycerol
+**PSB1A3Amil CP + Ampicilline
+**PSB1C3 Amil GFP + Chloramphinicol
+====15th August====
-====10th August====
+French holiday.
+====16th August====
 {| width="85%"
 |-
-| style="width: 50%;"|Amplification by PCR of BBa_K274100 already digested by EcoRI. Visualization by electrophoresis on a 0.8% Agarose gel.
+| style="width: 50%;"|PCR of BBa_K274100 and visualization by 0.8% Agarose gel electrophoresis. We are expecting a band at 3400bp.
-| style="width: 35%;"| [[File:Week10-5.jpg|right|300px]]
+| style="width: 35%;"| [[File:Week11-8.jpg|right|280px]]
 |}
 PCR program used:
-[[File:Week10-8.jpg|400px]]
+[[File:Week11-9.jpg|500px]]
-{| width="85%"
+*Digestion of the BBa_K274100 by DPNI to degrade the matrix plasmid.
-|-
-| style="width: 50%;"|Miniprep of BBa_K274100 followed by Nanovue to determine the concentration of the sample
-| style="width: 35%;"| [[File:Week10-6.jpg|right|330px]]
-|-
-| style="width: 50%;"|Miniprep of the Plasmid pSB1A2 followed by Nanovue to determine the concentration of the sample
-| style="width: 35%;"| [[File:Week10-7.jpg|right|330px]]
-|}
-*Digestion by HindIII of the plasmid pSB1A2 in order to linearize it.
+====17th august====
 {| width="85%"
 |-
-| style="width: 50%;"|Digestion of BBa_K115017 by DPNI to eliminate the plasmid matrix. Visualization by electrophoresis on a 2% Agarose gel. We are expecting a band at 123 bp.
+| style="width: 50%;"|Visualization of the DPNI’s digestion of the plasmid pSB1A2 by 0.8% Agarose gel electrophoresis. . We are expecting a band at size 2079 bp.
-| style="width: 35%;"| [[File:Week10-1.jpg|right|280px]]
+| style="width: 35%;"| [[File:Week11-10.jpg|right|220px]]
 |}
+*Miniprep of the pSB1A2 plasmid.
+*Miniprep of BBa_K274100 and BBa_K115017
+*Gibson assembly of the B construction
+*Transformation of DH5α competent cells with the Gibson B construction. The Petri dishes are placed at 37°C.
 {{Team:Paris-Saclay/Follow}}
+</div>
 </div>
 </div>
 {{Team:Paris-Saclay/Footer}}

Team:Paris-Saclay/Project/Notebook/Week 11

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Latest revision as of 00:39, 27 September 2012

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Week 11

13th August

14th August

15th August

16th August

17th august