Team:Paris/August 6

From 2008.igem.org

(Difference between revisions)

Latest revision as of 14:06, 13 August 2008

Cloning of flagella gene promotors into J61002 plasmid

We have to digest (by EcoRI and SpeI) the PCR products of yesterday (amplification of pFlgA (MP124), pFlgB (MP125), pFlhB (MP126) and pFlhDC (MP127) in order to clone them into the J61002 plasmid (that we must extract and then digest by EcoRI and SpeI).

Plasmid extraction

The J61002 plasmid was extracted from overnight bacteria culture using the QIAspin Miniprep Kit (QIAGEN) by QIACube.

Number of this plasmid extraction : MP123
Carried out 3 times (3 tubes)

Quantification of DNA

In order to quantify the DNA contained either in the Miniprep product of MP123 or in the PCR products of MP124, MP125, MP126 and MP127 previously purifed yesterday by the QIAquick Gel Extraction Kit, we carried out :

By electrophoresis

Assay to quantify DNA

10µl of 100pb DNA ladder
5 µL of the sample + 1 µL of 6X blue loading dye
Migration in a 1,5% agarose gel; ~30' at 100W.

Band	2	3	4	5	6
Name	MP123	MP124 PCR product	MP125 PCR product	MP126 PCR product	MP127 PCR product
Promotor	J61002	pFlgA	pFlgB	pFlhB	pFlhDC

==>Results : The MP123 plasmid is clearly visible but the PCR products (purified by QIAquick Gel Extraction) aren't. There might be a problem during the purification step using the QIAquick Gel Extraction. Whatever, we still go on with the digestion.

By Spectrophotometer

Besides the MP123 sample (J61002 plasmid) was quantified using a Bio Photometer (Eppendorf).

Name	concentration	A280/A260
MP123 n°1 (J61002)	102 µg/mL	1,77
MP123 n°2 (J61002)	120 µg/mL	1,69
MP123 n°3 (J61002)	130 µg/mL	1,73

==> Conclusion :we took the MP123 n°2 to do digestions

Digestion

Name	DNA to digest	Enzyme 1	Enzyme 2
D132	pFlgA	EcoRI	SpeI
D133	pFlgB	EcoRI	SpeI
D134	pFlhB	EcoRI	SpeI
D135	pFlhDC	EcoRI	SpeI
D136	J61002	EcoRI	SpeI

For each sample (MP123 and PCR products of MP124, MP125, MP126 and MP127):

10 µL of DNA (Miniprep eluate or PCR products)
12,5 µL water
2,5 µL buffer 2
0,25 µL BSA
1 µL EcoRI

Incubation 1h30 at 37°C
Incubation 1h30 more after adding 1 µL of SpeI

Electrophoresis of the digested J61002 plasmid

Electrophoresis of digested J61002 (D136)

10µl of 1 kb DNA ladder
30µL of the digestion + 5 µL of 6X blue loading dye
3µl of not digested plasmid + 1µl of 6X blue loading dye
Migration in a 0,5% agarose gel; ~30' at 100W.

Band	2	3	4	5	6
Name	D136	D136	-	MP123
Description	digested J61002	digested J61002	-	control with undigested J61002

==>Conclusion :' we observe a band near 3000 pb, and we excpeted a size of 3002 pb. So we observe the linearise plamsid (only one band at the good size).

Analysis of the purified digested DNA:

gel 2 : D136

Excision, dissolution and purification of the band of interest using the Wizard SV Gel and PCR Clean-Up System (Promega).

Purification of the digested PCR products using the same kit.

band 1 : ladder 1kb 10µL
band 2 : D136 4µL + 1µL Loading dye

=> Concentration : +/- 12ng/4µL -> 3ng/µL

Ligation

Protocol

For each sample,

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

Incubated O/N at 4°C (in the fridge)

List of ligations

Name	Vector	Insert	Antibio	Vol. vector (µl)	Vol. insert (µl)	Vol. H20 (µl)
L128	D136	D132	A	5	5	7
L129	D136	D133	A	5	5	7
L130	D136	D134	A	5	5	7
L131	D136	D135	A	5	5	7
Control	D136	-	A	5	-	6

Cloning of pflhDC

Yesterday the isolation of pflhDC did not work : the PCR product measured more than 1.5 kb. We checked the primers, they are well designed but they contain a sequence similarity with other sequences in E.coli K12. To amplify more precisely the promoter, we decided to do a PCR with gradient.

Protocol

10µL Phusion buffer 5X
1µL dNTP
2.5 µL Oligo F (O111) 10mM
2.5 µL Oligo R (O113) 10mM
1µL template DNA
0.5µL Phusion polymerase

PCR Program

   PROMOTE2
   * LID : 105 °C
   *1. T: 95°C     5min
   *2. T: 95°C     1min
   *3. T: 55°C     30s  ~>G: 5°C
   *4. T: 72°C     1min30
   *5. GO TO: 2 REP: 29
   *6. T: 72°C     5min    
   *7. HOLD: 10°C

Results

PCR with gradient : amplification of pflhDC

On the left side, the temperature was 50°C, in the center 55°C and on the right 60°C.

We can't see anything on this electrophoresis (except the ladder) !

Remarks :

We forgot the negative control
The temperature should be 60°C +- 5°C
For a promoter, 45s of elongation is enough (~1min per kb)
We could have used a taq polymerase instead of the phusion one
We will do it again

The return of PCRs for amplification of promoters

As our results were not very encouraging, we started again a PCR to amplify:

pflhDC ( 12 times with 12 different temperatures between 55°C and 65°C)
pflgA (60°C)
pflgB (60°C)
pflhB (60°C)
Negative control

Protocol

We used the taq polymerase, following a typical protocol.

Program

The PCR Program was a new version of PROMOTE2 :

   PROMOTE2
   * LID : 105 °C
   *1. T: 95°C     5min
   *2. T: 95°C     1min
   *3. T: 60°C     30s  ~>G: 5°C
   *4. T: 72°C     45 sec
   *5. GO TO: 2 REP: 29
   *6. T: 72°C     5min    
   *7. HOLD: 10°C

Results

We will have the results tomorrow

Culture for glycerol stocks and MiniPreps

E.coli K12 strain MG1655, to create a glycerol stock of this wonderful bacteria
pJ61002

Protocol :

5 mL LB with the appropriate antibiotic (here 5µL Amp 1000X)
With a toothpick, we select a single colony
37°C 225 rpm, overnight

Isolation of colonies

We isolated colonies of several strains on a petri dish (streaked):

S119
S120
E0240
pSB3K3

Culture : 37°C overnight

@@ Line 1: / Line 1: @@
 {{Paris/Calendar_Links|August 5|August 7}}
-[[Image:KR000109.jpg‎ ]]
-==Assay to clone different flagella gene promotors into the J61002 plasmid==
-We have to digest (by EcoRI and SpeI) the PCR products of yesterday (amplification of '''pFlgA''' (MP124), '''pFlgB''' (MP125), '''pFlhB''' (MP126) and '''pFlhDC''' (MP127) in order to '''clone''' them into the '''J61002 plasmid''' (that we must extract and then digest by EcoRI and SpeI).
+=='''Cloning of flagella gene promotors into J61002 plasmid'''==
+''We have to digest (by EcoRI and SpeI) the PCR products of yesterday (amplification of '''pFlgA''' (MP124), '''pFlgB''' (MP125), '''pFlhB''' (MP126) and '''pFlhDC''' (MP127) in order to '''clone''' them into the '''J61002 plasmid''' (that we must extract and then digest by EcoRI and SpeI).''
 <br>
 ===Plasmid extraction===
-The J61002 plasmid was extracted from overnight bacteria culture using the QIAspin Miniprep Kit (QIAGEN).
+The '''J61002 plasmid''' was extracted from overnight bacteria culture using the QIAspin Miniprep Kit (QIAGEN) by QIACube.
-* Number of this plasmid extraction : MP123
+* Number of this plasmid extraction : '''MP123'''
 * Carried out 3 times (3 tubes)
 <br>
-===Assay to quantify DNA===
-In order to quantify the DNA contained either in the Miniprep product of MP123 or in the PCR products of MP124, MP125, MP126 and MP127 previously purifed yesterday by the QIAquick Gel Extraction Kit, we carried out an '''electrophoresis''' assay in a '''1,5% agarose gel'''.
-* 5 µL of the sample
+===Quantification of DNA===
-* 1 µL of 6X blue loading dye
+In order to quantify the DNA contained either in the Miniprep product of MP123 or in the PCR products of MP124, MP125, MP126 and MP127 previously purifed yesterday by the QIAquick Gel Extraction Kit, we carried out :
+====By electrophoresis====
+[[Image:Gel 080806.JPG|thumb|Assay to quantify DNA]]
+* 10µl of 100pb DNA ladder
+* 5 µL of the sample + 1 µL of 6X blue loading dye
+* Migration in a '''1,5% agarose gel'''; ~30' at 100W.
 {| Border="1"
-|align="center"|'''1'''
+|align="center"|'''Band'''
-|align="center"|'''2'''
+|align="center"|2
-|align="center"|'''3'''
+|align="center"|3
-|align="center"|'''4'''
+|align="center"|4
-|align="center"|'''5'''
+|align="center"|5
-|align="center"|'''6'''
+|align="center"|6
 |-
-|align="center"|100 bp DNA ladder
+|align="center"|'''Name'''
-|align="center"|MP123 ('''J61002''')
+|align="center"|MP123
-|align="center"|MP124 PCR product ('''pFlgA''')
+|align="center"|MP124 PCR product
-|align="center"|MP125 PCR product ('''pFlgB''')
+|align="center"|MP125 PCR product
-|align="center"|MP126 PCR product ('''pFlhB''')
+|align="center"|MP126 PCR product
-|align="center"|MP127 PCR product ('''pFlhDC''')
+|align="center"|MP127 PCR product
 |-
+|align="center"|'''Promotor'''
+|align="center"|J61002
+|align="center"|pFlgA
+|align="center"|pFlgB
+|align="center"|pFlhB
+|align="center"|pFlhDC
 |}
-[[Image:Gel 080806.JPG|thumb|Assay to quantify DNA]]
-'''Results''' : The MP123 plasmid is clearly visible but the PCR products (purified by QIAquick Gel Extraction) aren't. There might be a problem during the purification step using the QIAquick Gel Extraction. Whatever, we still go on with the digestion.
-<br>Besides the MP123 sample (J61002 plasmid) was quantified using a '''Bio Photometer (Eppendorf)'''.
+==>'''Results''' : The MP123 plasmid is clearly visible but the PCR products (purified by QIAquick Gel Extraction) aren't. There might be a problem during the purification step using the QIAquick Gel Extraction. Whatever, we still go on with the digestion.
+====By Spectrophotometer====
+<br>''Besides the MP123 sample (J61002 plasmid) was quantified using a '''Bio Photometer (Eppendorf)'''.''
 {| Border="1"
@@ Line 47: / Line 62: @@
 |align="center"|'''A280/A260'''
 |-
-|align="center"|MP123 ('''J61002''')
+|align="center"|MP123 n°1 ('''J61002''')
+|align="center"|'''102 µg/mL'''
+|align="center"|'''1,77'''
+|-
+|align="center"|MP123 n°2 ('''J61002''')
 |align="center"|'''120 µg/mL'''
 |align="center"|'''1,69'''
 |-
+|align="center"|MP123 n°3 ('''J61002''')
+|align="center"|'''130 µg/mL'''
+|align="center"|'''1,73'''
 |}
+==> '''Conclusion :'''we took the MP123 n°2 to do digestions
 <br>
 ===Digestion===
@@ Line 97: / Line 123: @@
 <br> Incubation 1h30 at 37°C
 <br> Incubation 1h30 more after adding 1 µL of '''SpeI'''
-<br> '''Electrophoresis''' of the digested '''J61002 plasmid'''
-*1: 1 kb DNA ladder
-*2: digested J61002 (D136)
-*3: digested J61002 (D136)
+====='''Electrophoresis''' of the digested '''J61002 plasmid'''=====
-*4: -
+[[Image:KR000110.jpg|thumb|Electrophoresis of digested J61002 (D136)]]
-*5: control with undigested J61002
+* 10µl of 1 kb DNA ladder
-*6: -
+* 30µL of the digestion + 5 µL of 6X blue loading dye
-[[Image:KR000110.jpg]]
+* 3µl of not digested plasmid + 1µl of 6X blue loading dye
-<br> Excision, dissolution and '''purification''' of the band of interest using the '''Wizard SV Gel and PCR Clean-Up System (Promega)'''.
+* Migration in a '''0,5% agarose gel'''; ~30' at 100W.
-<br> '''Purification''' of the '''digested PCR products''' using the same kit.
+{| Border="1"
+|align="center"|'''Band'''
+|align="center"|2
+|align="center"|3
+|align="center"|4
+|align="center"|5
+|align="center"|6
+|-
+|align="center"|'''Name'''
+|align="center"|D136
+|align="center"|D136
+|align="center"|-
+|align="center"|MP123
+|-
+|align="center"|'''Description'''
+|align="center"|digested J61002
+|align="center"|digested J61002
+|align="center"|-
+|align="center"|control with undigested J61002
+|}
+==>'''Conclusion :'''' we observe a band near 3000 pb, and we excpeted a size of 3002 pb. So we observe the linearise plamsid (only one band at the good size).
+===='''Analysis of the purified digested DNA:'''====
+[[Image:D123.JPG|thumb|gel 2 : D136]]<br> ''Excision, dissolution and '''purification''' of the band of interest using the '''Wizard SV Gel and PCR Clean-Up System (Promega)'''.
+<br> '''Purification''' of the '''digested PCR products''' using the same kit.''
 <br>
-<br> '''Analysis of the purified digested DNA:'''
+<br>
+<br>
 * band 1 : ladder 1kb 10µL
 * band 2 : D136 4µL + 1µL Loading dye
-[[Image:D123_vérif.JPG| gel 2 : D136]]
   '''=> Concentration :''' +/- 12ng/4µL -> 3ng/µL
@@ Line 119: / Line 177: @@
 ==== Protocol ====
-For each sample,
+''For each sample,''
 * 1 µl Ligase
@@ Line 200: / Line 258: @@
      * LID : 105 °C
      *1. T: 95°C     5min
-     *2. T: 95°C     5min
+     *2. T: 95°C     1min
      *3. T: 55°C     30s  ~>G: 5°C
      *4. T: 72°C     1min30
-     *6. GO TO: 2 REP: 29
+     *5. GO TO: 2 REP: 29
+    *6. T: 72°C     5min
      *7. HOLD: 10°C
@@ Line 220: / Line 279: @@
 *We will do it again
 <br>
 ===The return of PCRs for amplification of promoters===
@@ Line 228: / Line 289: @@
 *pflhB (60°C)
 *Negative control
 ====Protocol====
 We used the taq polymerase, following a typical protocol.
@@ Line 236: / Line 298: @@
      * LID : 105 °C
      *1. T: 95°C     5min
-     *2. T: 95°C     5min
+     *2. T: 95°C     1min
      ''*3. T: 60°C     30s  ~>G: 5°C''
      ''*4. T: 72°C     45 sec''
-     *6. GO TO: 2 REP: 29
+     *5. GO TO: 2 REP: 29
+    *6. T: 72°C     5min
      *7. HOLD: 10°C
 ====Results====
 We will have the results [[Team:Paris/August_7|tomorrow]]
 ==Culture for glycerol stocks and MiniPreps==
@@ Line 252: / Line 318: @@
 *With a toothpick, we select a single colony
 *37°C 225 rpm, overnight
 ==Isolation of colonies==

Team:Paris/August 6

From 2008.igem.org

Latest revision as of 14:06, 13 August 2008

Contents

Cloning of flagella gene promotors into J61002 plasmid

Plasmid extraction

Quantification of DNA

By electrophoresis

By Spectrophotometer

Digestion

Electrophoresis of the digested J61002 plasmid

Analysis of the purified digested DNA:

Ligation

Protocol

List of ligations

Cloning of pflhDC

Protocol

PCR Program

Results

The return of PCRs for amplification of promoters

Protocol

Program

Results

Culture for glycerol stocks and MiniPreps

Isolation of colonies