Team:Brown/Notebook/Timeline

From 2008.igem.org

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*Team Toxipop created a timeline back in May to follow throughout the summer.   
*Team Toxipop created a timeline back in May to follow throughout the summer.   
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====Timeline as presented to Faculty Mentors and Graduate Advisors in May:====  
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===Timeline as presented to Faculty Mentors and Graduate Advisors in May:===  
* Week 1: Obtaining DNA from Texas lab or outsourcing production. Run experiments testing known methods of lysis & resistance measurements—change procedure and apparatus as necessary.
* Week 1: Obtaining DNA from Texas lab or outsourcing production. Run experiments testing known methods of lysis & resistance measurements—change procedure and apparatus as necessary.
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* Weeks 9 - 10: Allowance for any delays, further experimentation, begin second project.
* Weeks 9 - 10: Allowance for any delays, further experimentation, begin second project.
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====Actual Timeline====
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===Actual Timeline===
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====Week One====
*We were able to get the multiple strains from Vivek Jain and John Mekalanos at the Harvard Medical School.   
*We were able to get the multiple strains from Vivek Jain and John Mekalanos at the Harvard Medical School.   
*1 pRG1 DH5alpha cells containing the S,R,Rz lysis cassette under a Plac promoter. Ampicillin Resistance.  
*1 pRG1 DH5alpha cells containing the S,R,Rz lysis cassette under a Plac promoter. Ampicillin Resistance.  
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*3 '''pVJ4 SM10 cells.  Lysis cassette from RY100 cloned into pBAD18.mob 1.''' Amp Resistant.
*3 '''pVJ4 SM10 cells.  Lysis cassette from RY100 cloned into pBAD18.mob 1.''' Amp Resistant.
*4 pVJ13 DH5alpha cells clonded into pBAD33. Chloramphenicol Resistant.
*4 pVJ13 DH5alpha cells clonded into pBAD33. Chloramphenicol Resistant.
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*We worked with the Freeze-Thaw Method of Lysis in the few first days of summer.  In addition, the FastLyse reagent was ordered but could not be used due to the significant changes in resistance caused due to the FastLyse alone.  A change in resistance due to the intracellular ionic content of the E. coli bacteria could not be detected with the addition of FastLyse.
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 +
====Week Two====
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*The S,R,Rz genes were provided already transformed.  We spent most of week two working on two separate projects: 1. Testing lysis with Optical Density measurements and 2. Construction of a precise and accurate measurement apparatus. 
 +
*Multiple versions of the testing apparatus were made throughout the summer.  Initial designs included legos, skewers, pipette tips, and copper electrodes.  As the summer progressed, our apparatus became more complex.  We quickly made the transition from standard voltmeter to a Data Acquisition Card coupled with LabView Computer Software.  We quickly ditched the multi-stranded copper wires for Gold plated and Gold electrodes.  In addition, we moved to an alternating current to prevent the ions from settling on the electrodes and affecting current. 
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===Week Three===
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*Continued apparatus work in cooperation with Professor Jerry Daniels in Engineering and Daniel Ludwig, Biomedical Engineering '09.

Revision as of 12:34, 27 October 2008



  • Team Toxipop created a timeline back in May to follow throughout the summer.

Contents

Timeline as presented to Faculty Mentors and Graduate Advisors in May:

  • Week 1: Obtaining DNA from Texas lab or outsourcing production. Run experiments testing known methods of lysis & resistance measurements—change procedure and apparatus as necessary.
  • Week 2: Insert S-R-Rz cassette into plasmid and transform into bacteria. Screen bacteria to verify transformation success.
  • Week 3: Create testing apparatus for resistance measurement. Begin modeling.
  • Weeks 4-7: Experimentation
  • Week 8: Analysis of Data, Graphing, Presentation
  • Weeks 9 - 10: Allowance for any delays, further experimentation, begin second project.

Actual Timeline

Week One

  • We were able to get the multiple strains from Vivek Jain and John Mekalanos at the Harvard Medical School.
  • 1 pRG1 DH5alpha cells containing the S,R,Rz lysis cassette under a Plac promoter. Ampicillin Resistance.
  • 2 pDKL02 S17-1 cells with the lysis cassette under an IPTG promoter (also containing the mob element). Kanamycin Resistant.
  • 3 pVJ4 SM10 cells. Lysis cassette from RY100 cloned into pBAD18.mob 1. Amp Resistant.
  • 4 pVJ13 DH5alpha cells clonded into pBAD33. Chloramphenicol Resistant.
  • We worked with the Freeze-Thaw Method of Lysis in the few first days of summer. In addition, the FastLyse reagent was ordered but could not be used due to the significant changes in resistance caused due to the FastLyse alone. A change in resistance due to the intracellular ionic content of the E. coli bacteria could not be detected with the addition of FastLyse.

Week Two

  • The S,R,Rz genes were provided already transformed. We spent most of week two working on two separate projects: 1. Testing lysis with Optical Density measurements and 2. Construction of a precise and accurate measurement apparatus.
  • Multiple versions of the testing apparatus were made throughout the summer. Initial designs included legos, skewers, pipette tips, and copper electrodes. As the summer progressed, our apparatus became more complex. We quickly made the transition from standard voltmeter to a Data Acquisition Card coupled with LabView Computer Software. We quickly ditched the multi-stranded copper wires for Gold plated and Gold electrodes. In addition, we moved to an alternating current to prevent the ions from settling on the electrodes and affecting current.

Week Three

  • Continued apparatus work in cooperation with Professor Jerry Daniels in Engineering and Daniel Ludwig, Biomedical Engineering '09.
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