Team:Heidelberg/Templates/DelH week13

From 2013.igem.org

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* Of each miniprep, 3 µl were loaded  
* Of each miniprep, 3 µl were loaded  
[[File:Heidelberg_20130724 miniprepBB.png|200px|thumb|right|'''Fig.13.1''' Analytical gel for checking concentration of purified BB (PSB6A1-lacI-mRFP) (loaded 3 µL of PCR) <br>''l1'' 2log ladder ''l2:'' pSB6A1-lacI-mRFP  <br>  bands at 5 Kb = is ok, because BB is not linear]]
[[File:Heidelberg_20130724 miniprepBB.png|200px|thumb|right|'''Fig.13.1''' Analytical gel for checking concentration of purified BB (PSB6A1-lacI-mRFP) (loaded 3 µL of PCR) <br>''l1'' 2log ladder ''l2:'' pSB6A1-lacI-mRFP  <br>  bands at 5 Kb = is ok, because BB is not linear]]
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At 3Kb and at 8 Kb, there are bands visible.  
At 3Kb and at 8 Kb, there are bands visible.  
:=> Minipreps are fine.
:=> Minipreps are fine.
<br/>
<br/>
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====PCR Conditions BB.W13.A====
====PCR Conditions BB.W13.A====
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Expected band: 5 Kb
Expected band: 5 Kb
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<br/>
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[[File:Heidelberg_20130725 PCRofBB.png|200px|thumb|right|'''Fig.13.2''' gel of BB(PSB6A1-lacI-mRFP) (loaded 3 µL of PCR) <br>''l1:'' BB amplified with HM11 & HM12,  ''l2:'' BB amplified with HM11 & HM12,''l3:''  2log ladder <br>  specific bands at 5 Kb on both lanes = BB is ok]]
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[[File:Heidelberg_20130725 PCRofBB cut.png|200px|thumb|right|'''Fig.13.3''' gel of BB(PSB6A1-lacI-mRFP) (loaded 3 µL of PCR) <br>''l1:'' BB amplified with HM11 & HM12,  ''l2:'' BB amplified with HM11 & HM12,''l3:''  2log ladder <br>  specific bands at 5 Kb on both lanes = was cut out]]
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[[File:Heidelberg_20130725 PCRofBB cut.png|200px|thumb|right|'''Fig.13.3''' gel of BB(PSB6A1-lacI-mRFP) (loaded 3 µL of PCR) <br>''l1:'' BB amplified with HM11 & HM12,  ''l2:'' BB amplified with HM11 & HM12,''l3:''  2log ladder <br>  specific bands at 5 Kb on both lanes = was cut out]]
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<div class="tright" style="clear:none">[[File:Heidelberg_20130725 PCRofBB.png|200px|thumb|right|'''Fig.13.2''' gel of BB(PSB6A1-lacI-mRFP) (loaded 3 µL of PCR) <br>''l1:'' BB amplified with HM11 & HM12,  ''l2:'' BB amplified with HM11 & HM12,''l3:''  2log ladder <br>  specific bands at 5 Kb on both lanes = BB is ok]]</div>
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====Analysis of G0, G1 & G2b on Gel====
====Analysis of G0, G1 & G2b on Gel====
[[File:Heidelberg_20130725 G0 G1 G2b 2log.png|200px|thumb|right|'''Fig.13.4''' analyse-gel for checking concentration of DelH fragments (loaded 3 µL of PCR) <br>''l1'' 1Kb+ ladder ''l2:'' G0 complete DelH-fragment (DN11 & HM08), ''l3'' G1/2a DelH-fragment (DN11 & HM06), ''l4:'' G2b DelH-fragment (DHM07 & HM08)  <br> all bands are as expected = result shown in table below]]
[[File:Heidelberg_20130725 G0 G1 G2b 2log.png|200px|thumb|right|'''Fig.13.4''' analyse-gel for checking concentration of DelH fragments (loaded 3 µL of PCR) <br>''l1'' 1Kb+ ladder ''l2:'' G0 complete DelH-fragment (DN11 & HM08), ''l3'' G1/2a DelH-fragment (DN11 & HM06), ''l4:'' G2b DelH-fragment (DHM07 & HM08)  <br> all bands are as expected = result shown in table below]]
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====Overview on Fragments====
====Overview on Fragments====
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* Washing step with QX1 was not performed, because it is only to remove the residual agarose and we don't want to loose any DNA.
* Washing step with QX1 was not performed, because it is only to remove the residual agarose and we don't want to loose any DNA.
====Electroporation====
====Electroporation====
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* Electroporation into freshly prepared electrocompetent cell following [[Electroporation of E. coli DH10β|Protocol]]
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* Electroporation into freshly prepared electrocompetent cell following [https://2013.igem.org/Team:Heidelberg/Project/Methods the protocol]
* Streaked on LB Amp plates and incubated ON at 37°C
* Streaked on LB Amp plates and incubated ON at 37°C
 +
====Result====
====Result====
There were no colonies on any of the plates. Ginson assembly and electroporation have to be repeated.
There were no colonies on any of the plates. Ginson assembly and electroporation have to be repeated.
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<br/>
[[File:Heidelberg_20130728 2log BB G0.png|200px|thumb|right|'''Fig.13.5''' Analytical gel of backbone (pSB6A1-lacI-mRFP) and complete DelH fragment = G0 (loaded 5 µL of PCR) <br> ''l1:''2log ladder, ''l2:''BB,''l3:'' G0 <br> BB and DelH show the expected band at 18 Kb and 4.4 Kb]]
[[File:Heidelberg_20130728 2log BB G0.png|200px|thumb|right|'''Fig.13.5''' Analytical gel of backbone (pSB6A1-lacI-mRFP) and complete DelH fragment = G0 (loaded 5 µL of PCR) <br> ''l1:''2log ladder, ''l2:''BB,''l3:'' G0 <br> BB and DelH show the expected band at 18 Kb and 4.4 Kb]]
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No product visible of correct size. There is a light band at ~1.5 Kb.
No product visible of correct size. There is a light band at ~1.5 Kb.
:=> Most probably too little DNA loaded.
:=> Most probably too little DNA loaded.
<br/>
<br/>
 +
<div style="clear:both"></div>
====Electroporation====
====Electroporation====
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* Electroporation into freshly prepared electrocompetent cell following [[Electroporation of E. coli DH10β|Protocol]]
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* Electroporation into freshly prepared electrocompetent cell following [https://2013.igem.org/Team:Heidelberg/Project/Methods the protocol]
* Streaked on LB Amp plates and incubated ON at 37°C
* Streaked on LB Amp plates and incubated ON at 37°C
<br/>
<br/>
 +
====Result====
====Result====
There were few colonies on the plates. Red colonies were picked and screenied by colony-PCR, but none of them was positive. The Gibson assembly has to be repeated.
There were few colonies on the plates. Red colonies were picked and screenied by colony-PCR, but none of them was positive. The Gibson assembly has to be repeated.
<br/>
<br/>
====Preparation of Electrocompetent ''E.coli'' DH10ß====
====Preparation of Electrocompetent ''E.coli'' DH10ß====
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According to [[Electrocompetent bacteria|Protocol]]
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According to [https://2013.igem.org/Team:Heidelberg/Project/Methods the protocol]
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<br/>
<br/>
<br/>
 +
===Amplification of Backbone pSB6A1-lacZ-mRFP===
===Amplification of Backbone pSB6A1-lacZ-mRFP===
====Test Restriction Digest====
====Test Restriction Digest====
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<br/>
<br/>
[[File:Heidelberg_20130728 M testdigestofBB.png|200px|thumb|right|'''Fig.13.6'''test digest of Backbone (pSB6A1-lacZ-mRFP) (loaded 20 µL of PCR) <br> ''l1:''2log ladder, ''l2:''BB digested with NotI <br> digested BB show expected band at 4 Kb and 1 Kb => The backbone is ok.]]
[[File:Heidelberg_20130728 M testdigestofBB.png|200px|thumb|right|'''Fig.13.6'''test digest of Backbone (pSB6A1-lacZ-mRFP) (loaded 20 µL of PCR) <br> ''l1:''2log ladder, ''l2:''BB digested with NotI <br> digested BB show expected band at 4 Kb and 1 Kb => The backbone is ok.]]
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Gel shows shows expeted bands at 4 Kb and 1 Kb.
Gel shows shows expeted bands at 4 Kb and 1 Kb.
:=> Backbone is fine.
:=> Backbone is fine.
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<br/>
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<div style="clear:both"></div>

Latest revision as of 11:00, 25 October 2013

Contents

22-07 - 28-07-13

Amplification of Backbone pSB6A1-lacZ-mRFP

Miniprep

  • 4 colonies were picked and inoculated in 4x 3 ml LB Amp
  • Incubated ON at 37°C
  • 4x 3 ml were distibuted in 5x 2 ml eppis and centrifuged
  • Supernatant was discarded, cell pellet was used for miniprep
  • Two minipreps were pooled into 1 column and 180ipreps on another one (every eluation was performed with 50 µl)

Result

  • 5 µl were loaded on a gel
=> Gel was not succesful
=> Miniprep didn't work and has to be repeated

Glycerol Stock

Glycerol stocks were prepared from liquid culture not used for miniprep.

Repetiotion of Miniprep

4x 2 ml of Top10 pSB6A1-lacZ-mRFP were minipreped with the Qiagen kit.

Result

Sample Performed Concentration (Nanovue) P2 Buffer
pSB6A1-lacI-mRFP (1) upstairs 88 ng/µl from upstairs
pSB6A1-lacI-mRFP (2) iGEM lab 62 ng/µl new
pSB6A1-lacI-mRFP (3) iGEM lab 104 ng/µl new
pSB6A1-lacI-mRFP (4) iGEM lab 60 ng/µl old
  • Of each miniprep, 3 µl were loaded
Fig.13.1 Analytical gel for checking concentration of purified BB (PSB6A1-lacI-mRFP) (loaded 3 µL of PCR)
l1 2log ladder l2: pSB6A1-lacI-mRFP
bands at 5 Kb = is ok, because BB is not linear

At 3Kb and at 8 Kb, there are bands visible.

=> Minipreps are fine.


PCR Conditions BB.W13.A

Reagent Backbone Backbone
Template Miniprep A Miniprep A
Primer fw 10 µM HM11 HM11
Primer rev 10 µM HM12 HM12
Phusion Flash Ready Mix 10 µl 10 µl
ddH2O 7 µl 7 µl
DMSO - -
Cycles Temperature [°C] Time [s]
1 98 10
12 98 1
68 (touchdown - 0,5) 5
72 1:15 min
18 98 1
67 5
72 1:15 min
1 72 5 min
1 4 inf

Result

Expected band: 5 Kb

Fig.13.3 gel of BB(PSB6A1-lacI-mRFP) (loaded 3 µL of PCR)
l1: BB amplified with HM11 & HM12, l2: BB amplified with HM11 & HM12,l3: 2log ladder
specific bands at 5 Kb on both lanes = was cut out
Fig.13.2 gel of BB(PSB6A1-lacI-mRFP) (loaded 3 µL of PCR)
l1: BB amplified with HM11 & HM12, l2: BB amplified with HM11 & HM12,l3: 2log ladder
specific bands at 5 Kb on both lanes = BB is ok


Specific expected band at 5 Kb

=> Fragment was cut and gel isolated. A: 22 ng/µl, B: 25 ng/µl


Generation of DelH Plasmid 26-07

Analysis of G0, G1 & G2b on Gel

Fig.13.4 analyse-gel for checking concentration of DelH fragments (loaded 3 µL of PCR)
l1 1Kb+ ladder l2: G0 complete DelH-fragment (DN11 & HM08), l3 G1/2a DelH-fragment (DN11 & HM06), l4: G2b DelH-fragment (DHM07 & HM08)
all bands are as expected = result shown in table below
Fragment Size Amount used [µl] Amount used [ng] (by view) Left for Gibson [µl] = [ng] Concentration [ng/µl]
G0 18 Kb 8 5 52 = 35.5 0.68
G1 14 Kb 8 10 12 = 15 1.25
G2b 5 Kb 8 10 12 = 15 1.25


Overview on Fragments

Fragment Concentration [ng/µl]
G0 0.68
G1 1.25
G2b 1.25
BB A 22
BB B 25


Gibson Assembly

Assembly # Fragments Amount used [µl]
1
  • G0
  • BB A
  • 9.5
  • 0.5
2
  • G0
  • BB A
  • 8
  • 2
3
  • 1
  • G2b
  • BB A
  • 7
  • 2.5
  • 0.5
  • Incubated 1 hour at 50°C
  • Stored ON at -20°C

Purification of Gibson Mix

  • Purification performed with the long range gel extraction kit (because of 23 Kb size) of the entire sample (20 µl).
  • Performed the purification by calculating with 100 mg DNA (gel- step1)
  • Washing step with QX1 was not performed, because it is only to remove the residual agarose and we don't want to loose any DNA.

Electroporation

  • Electroporation into freshly prepared electrocompetent cell following the protocol
  • Streaked on LB Amp plates and incubated ON at 37°C

Result

There were no colonies on any of the plates. Ginson assembly and electroporation have to be repeated.

Generation of DelH Plasmid 28-07

NEB Protocol for Gibson Assembly

  • Optimized cloning efficiency is 50–100 ng of vectors with 2–3 fold of excess inserts. Use 5 times more of inserts if size is less than 200 bps. Optimized cloning efficiency is 50-100 ng of vectors with 2-3 fold of excess inserts. Use 5 times more of inserts if size is less than 200 bps.
  • Electrocompetent Cells Transformation Protocol:
  • Thaw electrocompetent cells on ice.
  • Transfer 50 μl of electrocompetent cells to a pre-chilled electroporation cuvette with 1 mM gap.
  • Dilute assembled products 3-fold with H2O prior electroporation. This can be achieved by mixing 5 μl of assembled products with 10 μl of H2O. Add 1 μ l of the diluted assembly product to electrocompetent cells.Mix gently by pipetting up and down or flicking the tube 4–5 times. Do not vortex. Place the mixture on ice for 30 minutes. Do not mix.
  • Mix gently by pipetting up.
  • Once DNA is added to the cells, electroporation can be carried out immediately. It is not necessary to incubate DNA with cells.Add 950 μl of room temperature SOC media* to tubes.
  • Add 950 μl of room temperature SOC media to the cuvette immediately after electroporation.
  • Place the tube at 37°C for 60 minutes. Shake vigorously (250 rpm) or rotate.
  • Warm selection plates to 37°C.
  • Spread 100 μl of the cells onto the plates.
  • Incubate overnight at 37°C.

Gibson Assembly

Fragments Concentraion [ng/µl] Amount [µl]
G0 0.68 9
BB (8.8) 22 1
Gibson Master Mix 2x 10
  • Incubated 1 h at 37 °C in thermocycler
  • 5 µl of mix added to 10 µl ddH2O and stored at -20°C
  • 10 µl stored for isoprop purification

Result

Remaining 5 µl were checked on a gel:
Expected band: 23 Kb

Fig.13.5 Analytical gel of backbone (pSB6A1-lacI-mRFP) and complete DelH fragment = G0 (loaded 5 µL of PCR)
l1:2log ladder, l2:BB,l3: G0
BB and DelH show the expected band at 18 Kb and 4.4 Kb

No product visible of correct size. There is a light band at ~1.5 Kb.

=> Most probably too little DNA loaded.


Electroporation

  • Electroporation into freshly prepared electrocompetent cell following the protocol
  • Streaked on LB Amp plates and incubated ON at 37°C


Result

There were few colonies on the plates. Red colonies were picked and screenied by colony-PCR, but none of them was positive. The Gibson assembly has to be repeated.

Preparation of Electrocompetent E.coli DH10ß

According to the protocol

Amplification of Backbone pSB6A1-lacZ-mRFP

Test Restriction Digest

Fragment DNA [µl] H2O [µl] Enzymes [µl] Buffer 3.1 [µl]
BB A (22 ng/µl) 8 = 200 ng 9 NotI: 1 2
  • Incubated 1.5 h at 37 °C

Result

Expected bands: 4 Kb & 1 Kb

Fig.13.6test digest of Backbone (pSB6A1-lacZ-mRFP) (loaded 20 µL of PCR)
l1:2log ladder, l2:BB digested with NotI
digested BB show expected band at 4 Kb and 1 Kb => The backbone is ok.

Gel shows shows expeted bands at 4 Kb and 1 Kb.

=> Backbone is fine.


Retrieved from "http://2013.igem.org/Team:Heidelberg/Templates/DelH_week13"