Team:Paris/July 28

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Latest revision as of 16:59, 13 August 2008

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DNA Extraction

Results of the extraction : Electrophoresis

conditions of electrophoresis:

10µl of ladder 1 kb
xµl of extraction added with 2µl of loading Dye 6x
migration ~30min at 100W

Gel 1, 2, 3, 4 = 0,8%
2µl of extraction added with 2µl of loading Dye 6x

Gel 5, 6 = 0,8%
3µl of extraction added with 2µl of loading Dye 6x

Gel 7 = 0,8%
5µl of extraction added with 2µl of loading Dye 6x

Gel 8 = 1,5%
10µl of extraction added with 2µl of loading Dye 6x

Results :

gel1 gel2 gel3 gel4 gel5

gel6 gel7 gel8

Name	BioBrick	Tube N°	Enz 1	Enz 2	Obs	Exp Size	Mea Size	Conc (ng/µl)	Gel	Band
D100	B0034	1	XbaI	PstI	BI	34 pb	-	-	8	5
D100	B0034	2	XbaI	PstI	BI	34 pb	-	-	-
D101	B0034	3	EcoRI	XbaI	FV	2076 pb	- & 2000 pb	- & 7	1 & 7	2 & 2
D102	B0034	4	SpeI	PstI	BV	2077 pb	2000 pb	- & 5	1 & 7	3 & 3
D102	B0034	5	SpeI	PstI	BV	2077 pb	2000 pb	- & 10	1 & 7	4 & 4
D103	J23101	1	SpeI	PstI	BV	2100 pb	2000 pb	-	1	5
D103	J23101	2	SpeI	PstI	BV	2100 pb	2000 pb	10	1	6
D104	J23109	1	SpeI	PstI	BV	2100 pb	2000 pb	20	1	7
D104	J23109	2	SpeI	PstI	BV	2100 pb	2000 pb	20	1	8
D105	R0079	1	SpeI	PstI	BV	2222 pb	2000 pb	5	2	2
D105	R0079	2	SpeI	PstI	BV	2222 pb	2000 pb	5	2	3
D106	R0040	1	SpeI	PstI	BV	2119 pb	- & 2000 pb	- & 5	2 & 7	4 & 5
D106	R0040	2	SpeI	PstI	BV	2119 pb	- & 2000 pb	- & 8	2 & 7	5 & 6
D107	S03154	1	SpeI	PstI	BV	2750 pb	- & 3000 pb	- & 5	2 & 7	6 & 7
D108	S03154	2	XbaI	PstI	BI	707 pb	- & -	- & -	2 & 7	7 & 8
D108	S03154	3	XbaI	PstI	BI	707 pb	- & -	- & -	2 & 7	8 & 9
D109	S03154	4	EcoRI	SpeI	FI	708 pb	- & -	- & -	3 & 7	2 & 10
D110	S03879	1	SpeI	PstI	BV	2768 pb	3000 pb	20	3	3
D111	S03879	2	XbaI	PstI	BI	725 pb	-	-	3	4
D111	S03879	3	XbaI	PstI	BI	725 pb	-	-	3	5
D112	S03879	4	EcoRI	SpeI	FI	726 pb	-	-	3	6
D113	C0079	1	EcoRI	SpeI	FI	779 pb	800 pb	20	3	7
D114	C0079	2	XbaI	PstI	BI	778 pb	800 pb	20	3	8
D115	C0179	1	EcoRI	SpeI	FI	746 pb	- & -	- & -	4 & 7	2 & 11
D116	C0179	2	XbaI	PstI	BI	745 pb	- & -	- & -	4 & 7	3 & 12
D117	E0030	1	EcoRI	SpeI	FI	746 pb	700 pb	5	4	4
D118	E0030	2	XbaI	PstI	BI	745 pb	700 pb	5	4	5
D119	E0040	1	EcoRI	SpeI	FI	743 pb	- & 800 pb	- & 10	4 & 7	6 & 13
D120	E0040	2	XbaI	PstI	BI	742 pb	- & 800 pb	- & 10	4 & 7	7 & 14
D121	E1010	1	EcoRI	SpeI	FI	704 pb	700 pb	5	4	8
D122	E1010	2	XbaI	PstI	BI	703 pb	800 pb	10	5	2
D123	J23100	1	SpeI	PstI	BV	2100 pb	2000 pb	10	5	3
D123	J23100	2	SpeI	PstI	BV	2100 pb	2000 pb	10	5	4
D124	J23107	1	SpeI	PstI	BV	2100 pb	2000 pb	10	5	5
D124	J23107	2	SpeI	PstI	BV	2100 pb	2000 pb	15	5	6
D125	B0015	1	EcoRI	XbaI	FV	3303 pb	3000 pb	15	5	7
D125	B0015	2	EcoRI	XbaI	FV	3303 pb	3000 pb	15	5	8
D126	I0500	1	SpeI	PstI	FV	5621 pb	6000 pb	10	5	9
D126	I0500	2	SpeI	PstI	FV	5621 pb	6000 pb	10	5	10
D127	B0030	1	XbaI	PstI	BI	37 pb	- & -	- & -	8	3
D127	B0030	2	XbaI	PstI	BI	37 pb	- & -	-	-	-
D128	B0030	3	EcoRI	XbaI	FV	2079 pb	2000 pb	10	5	11
D129	B0030	4	SpeI	PstI	BV	2080 pb	2000 pb	10	5	12
D129	B0030	5	SpeI	PstI	BV	2080 pb	2000 pb	10	5	13
D130	E0422	1	XbaI	PstI	BI	939 pb	1100 pb	10	5	14
		2						10	5	15
		3						10	5	16
D131	E0840	1	XbaI	PstI	BI	900 pb	1000 pb	5	6	3
		2						10	6	4
		3						5	6	5

==> Conclusion : for most of the samples we have enough signal to determine the concentration of the digestion to do the ligation.

For the samples we don't succeed to obtain signals, we have migrated a second gel ( gel n°7).

==> Conclusion : The gel n°7 allowed us to know the concentration of other digestion undetermined.

Ligation

Protocol

For each samples,

1 µl Ligase
X µl Vector
Y µl Insert (3x more than vector)
2 µl Ligase Buffer 10x
20 µl qsp H2O

Incubates O/N at 4°C (in the fridge)

List of ligations

Name	Vector	Insert	Antibio	Vol. vector (µl)	Vol. insert (µl)	Vol. H20 (µl)
L100	D110	D130	A	3	6	8
L101	D110	D131	A	3	6	8
L102	D129	D118	A	5	10	2
L103	D129	D122	A	5	5	7
L104	D129	D114	A	5	4	8
L105	D123	D130	A	5	4	8
L106	D123	D131	A	5	8	4
L107	D103	D130	A	5	8	4
L108	D103	D131	A	5	8	4
L109	D124	D130	A	4	7	6
L110	D124	D131	A	4	7	6
L111	D104	D130	A	3	5	9
L112	D104	D131	A	3	5	9
L113	D126	D130	K	5	2.5	9.5
L114	D126	D131	K	5	2.5	9.5
L115	D105	D130	A	7	11	-
L116	D105	D131	A	7	11	-
L117	D125	D117	A	4	3	10
L118	D125	D121	A	4	2	11
L119	D125	D113	A	4	2	11
L120	D106	D130	A	6	7.5	3.5
L121	D106	D131	A	6	7.5	3.5
L122	D107	D130	A	7	3.5	6.5
L123	D107	D131	A	7	3.5	6.5
L124	D102	D122	A	6	5	4
L125	D102	D1118	A	6	10	1
L126	D102	D114	A	6	4	7
L127	D125	D119	A	6	3	8
C1	D110	-	A	3	-	14
C2	D129	-	A	5	-	12
C3	D123	-	A	5	-	12
C4	D103	-	A	8	-	9
C5	D124	-	A	7	-	10
C6	D104	-	A	3	-	14
C7	D126	-	A	2.5	-	14.5
C8	D105	-	A	11	-	6
C9	D125	-	A	2	-	15
C10	D106	-	A	7.5	-	9.5
C11	D107	-	A	3.5	-	13.5
C12	D102	-	A	10	-	7

Purification of the B0034 and B0030 BioBricks

We performed PCR on the B0034 BioBrick (MP 100) and the B0030 BioBrick (MP 120) to amplify the sequence in order to have enough amount of DNA to carry out the following of our experiments.

PCR Protocol

For each samples,

1 µl dNTP
10 µl Buffer Phusion 5x
2,5 µl VR2 (O18)
2,5 µl VF (O19)
1 µl Phusion
50 µl qsp H2O (33µl)

Electrophoresis - Purification

When the PCR cycles were finished,

Add 10 µL of 6X loading dye.
Load the samples (2 x 30 µL per sample) on a 1,5% agarose gel.
Migration 30' at 100W.

After electrophoresis,

Excision and purification of the bands corresponding to MP 100 and MP 120, using the QIAquick DNA Gel Extraction Kit (QIAGEN).
Elution in 50 µL of water.

Because the intensity of the band corresponding to MP 120 was very low, we only continued with MP 100.

DNA Digestion

MP 100 was digested by EcoRI & SpeI (Forward Insert) or by XbaI & PstI (D100 : Backward Insert)

Digestion reaction (total volume : 50 µL)

25 µL DNA
5 µL buffer 2 (10X)
2 µL enzyme 1
2 µL enzyme 2
0.5 µL BSA (100X)
15,5 µL water

The reaction was incubated 2 hours at 37°C.
The samples (2 x 30 µL per sample) were then analysed by electrophoresis.

Electrophoresis

ladder	EcoRI & SpeI	EcoRI & SpeI	-	XbaI & PstI	XbaI & PstI
1	2	3	4	5	6

The sequence of MP 100 (B0034) digested by EcoRI & SpeI (35 bp) or XbaI & PstI (34 bp) was too short and we didn't manage to visualise it on the gel.

==> Conclusion : small parts like B0034 can't be cloned as an insert.

@@ Line 406: / Line 406: @@
 ! rowspan="1"| 6
 |-
-! rowspan="2" style="background: #ccccff;"|D124
+! rowspan="2" style="background: #ccccff;"|D125
-! rowspan="2" style="background: #ccccff;"|J23107
+! rowspan="2" style="background: #ccccff;"|B0015
 |align=center|1
 ! rowspan="2"|EcoRI
@@ Line 532: / Line 532: @@
-==> Conclusion : for most of the samples we have enough signal to determine the concentration of the digestion to do the ligation.
+==> ''Conclusion :'' for most of the samples we have enough signal to determine the concentration of the digestion to do the ligation.
@@ Line 538: / Line 538: @@
-==> Conclusion : The gel n°7 allowed us to know the concentration of other digestion undetermined.
+==> ''Conclusion :'' The gel n°7 allowed us to know the concentration of other digestion undetermined.
 == Ligation ==
@@ Line 555: / Line 552: @@
 * 2 µl Ligase Buffer 10x
 * 20 µl qsp H2O
 * Incubates O/N at 4°C (in the fridge)
+=== List of ligations ===
 {| border="1"
@@ Line 891: / Line 888: @@
 |}
-== Attempt to excise and purify the B0034 and B0030 BioBricks ==
+== Purification of the B0034 and B0030 BioBricks ==
-We performed PCR on the B0034 BioBrick (MP 100) and the B0030 BioBrick (MP 120) to amplify the sequence in order to have enough amount of DNA to carry out the following of our experiments.
+''We performed PCR on the B0034 BioBrick (MP 100) and the B0030 BioBrick (MP 120) to amplify the sequence in order to have enough amount of DNA to carry out the following of our experiments.''
 === PCR Protocol ===
-For each samples,
+''For each samples,''
 * 1 µl dNTP
@@ Line 906: / Line 903: @@
 * 50 µl qsp H2O (33µl)
-When the PCR cycles were finished, 10 µL of 6X loading dye were added. The samples were then loaded (2 x 30 µL per sample) on a 1,5% agarose gel. After electrophoresis, the bands corresponding to MP 100 and MP 120 were excised and purified using the QIAquick DNA Gel Extraction Kit (QIAGEN). The elution was made in 50 µL of water. Because the intensity of the band corresponding to MP 120 was very low, we only continued with MP 100. MP 100 was digested by EcoRI & SpeI (Forward Insert) or by XbaI & PstI (D100 : Backward Insert).
+=== Electrophoresis - Purification ===
+''When the PCR cycles were finished,''
+* Add 10 µL of 6X loading dye.
+* Load the samples (2 x 30 µL per sample) on a 1,5% agarose gel.
+* Migration 30' at 100W.
+''After electrophoresis,''
+* Excision and purification of the bands corresponding to MP 100 and MP 120, using the QIAquick DNA Gel Extraction Kit (QIAGEN).
+* Elution in 50 µL of water.
+''Because the intensity of the band corresponding to MP 120 was very low, we only continued with MP 100.''
 === DNA Digestion ===
-Digestion reaction (total volume : 50 µL)
+''MP 100 was digested by EcoRI & SpeI (Forward Insert) or by XbaI & PstI (D100 : Backward Insert)
+Digestion reaction (total volume : 50 µL)''
 * 25 µL DNA
 * 5 µL buffer 2 (10X)
@@ Line 918: / Line 934: @@
 * 15,5 µL water
-The reaction was incubated 2 hours at 37°C. The samples (2 x 30 µL per sample) were then analysed by electrophoresis.
+* The reaction was incubated 2 hours at 37°C.
+* The samples (2 x 30 µL per sample) were then analysed by electrophoresis.
 ===Electrophoresis===
-{|1|2|3|4|5|6
 {| border="1"
@@ Line 940: / Line 958: @@
 |}
-[[Image:Image gel.jpg]]
+[[Image:Image_gel.jpg|thumb|]]
 The sequence of MP 100 (B0034) digested by EcoRI & SpeI (35 bp) or XbaI & PstI (34 bp) was too short and we didn't manage to visualise it on the gel.
-Conclusion : small parts like B0034 can't be cloned as an insert.
+==> ''Conclusion'' : small parts like B0034 can't be cloned as an insert.