"

From 2014.igem.org

Revision as of 13:49, 22 July 2014 (view source) Maschi (Talk | contribs) (→Monday 21st July) ← Older edit		Revision as of 13:01, 23 July 2014 (view source) SC (Talk | contribs) (→2 - Results: Transformation of DY330 via pJBEI6409) Newer edit →
Line 17:		Line 17:
	{| class="wikitable"		{| class="wikitable"
-	|+Number of colonies per dish	+	|+Number of colonies per dish (source of bacteria: electroporation cuvettes prepared on the [https://2014.igem.org/Team:Paris_Saclay/Notebook/July/18 18th July])
	|-		|-
		+	! Volume of plasmid used
	! 50μl from cuvette		! 50μl from cuvette
	! 100μl		! 100μl
-	! remainder	+	! remainder (850µl)
	|-		|-
		+	! 2μl of plasmid
	| 0		| 0
	| 4		| 4
	| 30		| 30
-	! 2μl of plasmid
	|-		|-
		+	! 4μl
	| 3		| 3
	| 6		| 6
	| 45		| 45
-	! 4μl
	|-		|-
		+	! Control
	| 0		| 0
	| 0		| 0
	| 0		| 0
-	!Control
	|}		|}
		+
		+	'''Conclusion: The increase in colony number is proportional to the increase in volume used. The control yielded nothing. The results are coherent.'''
	===3 - Oligo's design===		===3 - Oligo's design===

---

Revision as of 13:01, 23 July 2014

Contents 1 Monday 21st July 1.1 Lab Work 1.1.1 1 - Results: Transformation of supercompetent cells with CaCl2 1.1.2 2 - Results: Transformation of DY330 via pJBEI6409 1.1.3 3 - Oligo's design 1.1.4 4 - Liquid Bacterial Culture 1.1.5 5 - Electrophoresis

Monday 21st July

Lab Work

1 - Results: Transformation of supercompetent cells with CaCl₂

by Romain

Strains transformed: MG1655, MG1655Z1. from Bacterial Cultures transformed the 18th July

Results: Nothing has grown.

2 - Results: Transformation of DY330 via pJBEI6409

by Sean

Transformation performed on the 18th July

Number of colonies per dish (source of bacteria: electroporation cuvettes prepared on the 18th July)

Volume of plasmid used	50μl from cuvette	100μl	remainder (850µl)
2μl of plasmid	0	4	30
4μl	3	6	45
Control	0	0	0

Conclusion: The increase in colony number is proportional to the increase in volume used. The control yielded nothing. The results are coherent.

3 - Oligo's design

by Romain

4 - Liquid Bacterial Culture

by Marie, Romain & Sean

• DY330 pJBEI6409 with 10µl Cm in 10ml LB (x2)
• BT340 Cm and Amp
• The new strains received

5 - Electrophoresis

by Fabio (process A) and Mathieu (process B and C)

We used 2µl of DNA of the following Biobricks in a 1% Agarose Gel. The PCRs came from Mathias' manipulation made the 18th July.

Process A

1. J23119 Cl1
2. J23119 Cl2
3. J23106 Cl1
4. J23100 Cl2
5. PCR 1
6. PCR 2
7. PCR 3
8. PCR 4
9. PCR 5
10. PCR 6
11. PCR 7
12. PCR 8
13. PCR 9
14. PCR 10

Process B

1. J23100 Cl1
2. J23100 Cl2
3. J23106 Cl1
4. J23106 Cl2
5. J23114 Cl1
6. J23114 Cl2

Process C

Pooling and purifying PCR 9 and 10 from process A.

1. PCR purified products. IPS70 / IPS71 of pOsV230 (Apramycin)
2. BT 340 (plasmid's flipase)

Results:

• A: From 1 to 4: Success, DNAs have the expected size.
• A: From 5 to 12: Failure, No PCR products.
• A: Numbers 13 and 14: Success, PCR products have the expected size.
• B: All 6 extractions were successful.
• C: Number 1: successful concentration of pOsV230's PCR product.
• C: Number 2 had no migration.

Protocol

People there:

• Instructors and advisors: Solenne and Sylvie.
• Students: Arnaud, Fabio, Juliette, Mathieu, Marie, Pierre, Romain, Sean and Terry.

Back to the calendar