Team:Exeter/lab book/3gip/wk9

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     <!------------ENTER LAB BOOK HERE: PLEASE INCLUDE DATES WITHIN THE WEEK------------>  
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     <p><b><u>Monday 3rd September</u></b></p>
 +
<p><i><b>Morning</b></i></p>
 +
<p>•<u>3A assembly</u></p> 
 +
<p>BBa_J13002 + Cyc_BBa_B0014 in pSB1K3</p>
 +
<p>BBa_J13002 + has_BBa_B0014 in pSB1K3</p>
 +
<p>ompA + sacB_BBa_B0014 in pSB1K3</p>
 +
<p>Performed with the NEB protocol with some adaptions again. The volume of digestion was changed from 50ul to 20ul by adding less water so as to increase the DNA concentration. The enzymes and buffer concentrations were adapted as below. This was not a Linearized Plasmid Backbone so for the plasmid digestion we used the NEB Biolabs protocol adapted to the amounts shown below. </p>
 +
<p>
 +
</p>
 +
<p><i><b>Afternoon</b></i></p>
 +
<p>•<u>Transformation</u></p>
 +
<p>The ligations were transformed using the Competent Cell protocol and using the Competent Cells made in the lab. </p>
 +
<p>•<u>Adding cultures</u></p> 
 +
<p>Time restraints, weekend and talks had meant there was a backlog of 3A transformations to be miniprepped. All transformations from the 21/08/2012 onwards were added into liquid medium and incubated overnight. Four colonies from each plate. 10μl of broth was used to ensure a good DNA concentration. </p>
 +
<p>Protocol was followed using the relevant antibiotic for the BioBrick part as the selection antibiotic. </p>
 +
 
 +
<p><b><u>Tuesday 4th September</u></b></p>
 +
<p><i><b>Morning</b></i></p>
 +
 
 +
<p>•<u>Mini-Prepping</u></p> 
 +
<p>Following growing up of the cultures the night before, 89 minipreps needed to be performed this morning. Using two teams we took on the task, 24 minipreps at a time. Problems with labelling and timing did occur. </p>
 +
<p>Most of the minipreps were nanodropped with some showing very good concentrations and some not. Some of the tubes were centrifuged by mistake before being lysed and neutralised seriously affecting the final concentration. </p>
 +
 
 +
<p>•<u>Adding cultures</u></p> 
 +
<p>Cells transformed with BBa_J13002 + Cyc_BBa_B0014 in pSB1K3, BBa_J13002 + has_BBa_B0014 in pSB1K3, ompA + sacB_BBa_B0014 in pSB1K3 were all added into liquid medium and incubated overnight. See, Showcasing Polysaccharide Production: 27th - 31st August 2012, Wednesday 05/09/12</p>
 +
<p>Protocol was followed using chloramphenicol for the BioBrick part as the selection antibiotic. </p>
 +
<p><b><u>Wednesday 5th September</u></b></p>
 +
<p>Today was a day for helping out on other projects, tidying up the lab and tying up loos ends. </p>
 +
<p><b><u>Thursday 6th September</u></b></p>
 +
<p><i><b>Morning</b></i></p>
 +
<p>•<u>Gel Digest of DNA from 21/08/2012</u></p>
 +
<p>A digestion using EcoR1 and PstI was run on all of the miniprepped DNA from Tuesday. The tubes were set up and mastermixes made and added. There would not be enough time to set the gel up and run it with the time left available so an the digest was left in the incubator overnight at 37C, the gel was wrapped and stored in the fridge and the prepared DNA was stored at -20C. </p>
 +
<p>For the digestion we had little EcoR1 left so we used Fermantas enzymes instead. The protocol remained the same but we used Ferantas Buffer H instead of the NEB Buffer 2. </p>
 +
<p><i><b>Afternoon</b></i></p>
 +
<p>•<u>Protein Expression</u></p>
 +
<p>The gel showed positive for BBa_J13002 + WbnK_BBa_B0014 and BBa_K764001+ WclY_BBa_B0014. We grew some in 10μl of liquid broth and incubated. When the OC600 reached 0.5A on the spectrometer we induced the cultures with 0.5mM of IPTG with the placI promoter and 50ng/ml, 100ng/ml and 5mg/ml with the Tetr promoter. The samples were placed back in the incubator. 1ml samples were taken at 15.30 and 16.30 and frozen. The remaining samples were placed back in the incubator. </p>
 +
 
 +
<p><b><u>Friday 7th September</u></b></p>
 +
<p><i><b>Morning</b></i></p>
 +
<p>A final sample for the protein expression was taken at 9.00 this morning and frozen. </p>
 +
<p>The biggest Gel I have ever run. </p>
 +
<p><b>Undergraduate iGEM Lesson for the week – don’t take on too much! </b></p>
 +
<p>The frozen samples for protein expression were unfrozen and the 9.00 samples were run on an SDS-page gel. It showed no unique proteins. In future we would always tag proteins to eliminate many of the identification problems. </p>
      
      
     </font>
     </font>

Revision as of 16:05, 25 September 2012

ExiGEM2012 Lab Book 3GP wk6

The 3-Gene Inducible Plasmid: 3rd - 7th September 2012

Monday 3rd September

Morning

3A assembly

BBa_J13002 + Cyc_BBa_B0014 in pSB1K3

BBa_J13002 + has_BBa_B0014 in pSB1K3

ompA + sacB_BBa_B0014 in pSB1K3

Performed with the NEB protocol with some adaptions again. The volume of digestion was changed from 50ul to 20ul by adding less water so as to increase the DNA concentration. The enzymes and buffer concentrations were adapted as below. This was not a Linearized Plasmid Backbone so for the plasmid digestion we used the NEB Biolabs protocol adapted to the amounts shown below.

Afternoon

Transformation

The ligations were transformed using the Competent Cell protocol and using the Competent Cells made in the lab.

Adding cultures

Time restraints, weekend and talks had meant there was a backlog of 3A transformations to be miniprepped. All transformations from the 21/08/2012 onwards were added into liquid medium and incubated overnight. Four colonies from each plate. 10μl of broth was used to ensure a good DNA concentration.

Protocol was followed using the relevant antibiotic for the BioBrick part as the selection antibiotic.

Tuesday 4th September

Morning

Mini-Prepping

Following growing up of the cultures the night before, 89 minipreps needed to be performed this morning. Using two teams we took on the task, 24 minipreps at a time. Problems with labelling and timing did occur.

Most of the minipreps were nanodropped with some showing very good concentrations and some not. Some of the tubes were centrifuged by mistake before being lysed and neutralised seriously affecting the final concentration.

Adding cultures

Cells transformed with BBa_J13002 + Cyc_BBa_B0014 in pSB1K3, BBa_J13002 + has_BBa_B0014 in pSB1K3, ompA + sacB_BBa_B0014 in pSB1K3 were all added into liquid medium and incubated overnight. See, Showcasing Polysaccharide Production: 27th - 31st August 2012, Wednesday 05/09/12

Protocol was followed using chloramphenicol for the BioBrick part as the selection antibiotic.

Wednesday 5th September

Today was a day for helping out on other projects, tidying up the lab and tying up loos ends.

Thursday 6th September

Morning

Gel Digest of DNA from 21/08/2012

A digestion using EcoR1 and PstI was run on all of the miniprepped DNA from Tuesday. The tubes were set up and mastermixes made and added. There would not be enough time to set the gel up and run it with the time left available so an the digest was left in the incubator overnight at 37C, the gel was wrapped and stored in the fridge and the prepared DNA was stored at -20C.

For the digestion we had little EcoR1 left so we used Fermantas enzymes instead. The protocol remained the same but we used Ferantas Buffer H instead of the NEB Buffer 2.

Afternoon

Protein Expression

The gel showed positive for BBa_J13002 + WbnK_BBa_B0014 and BBa_K764001+ WclY_BBa_B0014. We grew some in 10μl of liquid broth and incubated. When the OC600 reached 0.5A on the spectrometer we induced the cultures with 0.5mM of IPTG with the placI promoter and 50ng/ml, 100ng/ml and 5mg/ml with the Tetr promoter. The samples were placed back in the incubator. 1ml samples were taken at 15.30 and 16.30 and frozen. The remaining samples were placed back in the incubator.

Friday 7th September

Morning

A final sample for the protein expression was taken at 9.00 this morning and frozen.

The biggest Gel I have ever run.

Undergraduate iGEM Lesson for the week – don’t take on too much!

The frozen samples for protein expression were unfrozen and the 9.00 samples were run on an SDS-page gel. It showed no unique proteins. In future we would always tag proteins to eliminate many of the identification problems.