Team:Minnesota/Parts Characterization

From 2009.igem.org

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<h1>Parts Characterization</h1>
<h1>Parts Characterization</h1>
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We chose five promoters that were included in the 2009 iGEM Kit to characterize. Using part [http://partsregistry.org/wiki/index.php/Part:BBa_F2620 BBa_F2620], which was characterized by a group from MIT in 2004, as a template, we characterized the following parts:
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We originally chose five promoters that were included in the 2009 iGEM Kit to characterize. Using part [http://partsregistry.org/wiki/index.php/Part:BBa_F2620 BBa_F2620], which was characterized by a group from MIT in 2004, as a template, we examined the following parts:
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<h2>Challenges</h2>
<h2>Challenges</h2>
A day by day catalog of what we did for parts characterization can be found on our Google calendar on the https://2009.igem.org/Team:Minnesota/Notebook Experiments and Calendar] page. Clearly, despite the summary above, some of these steps we had to redo over and over. Often, our DNA after plasmid preparation and restriction enzyme digest was not very pure and had a low concentration, which necessitated picking colonies, growing more cultures and ]prepping more plasmids. Sequencing, which was performed by the [http://www.agac.umn.edu/ BMGC] on the U of MN campus, provided us with a huge challenge because often, our sequences were not clean so we were not sure that we had the correct parts. Running samples out on a gel and specing samples can be very helpful in double-checking the size and purity of fragments, but sequencing was a very important step that really told us whether our procedure was viable. When we received wonky results-- that is, the signals were mixed and the samples appeared to have multiple products-- we hypothesized that this was due to the primer setting down in the wrong location during the sequence reaction or perhaps a hairpin loop structures getting in the way of the sequencing (we gratefully acknowledge John Barrett for his suggestions).
A day by day catalog of what we did for parts characterization can be found on our Google calendar on the https://2009.igem.org/Team:Minnesota/Notebook Experiments and Calendar] page. Clearly, despite the summary above, some of these steps we had to redo over and over. Often, our DNA after plasmid preparation and restriction enzyme digest was not very pure and had a low concentration, which necessitated picking colonies, growing more cultures and ]prepping more plasmids. Sequencing, which was performed by the [http://www.agac.umn.edu/ BMGC] on the U of MN campus, provided us with a huge challenge because often, our sequences were not clean so we were not sure that we had the correct parts. Running samples out on a gel and specing samples can be very helpful in double-checking the size and purity of fragments, but sequencing was a very important step that really told us whether our procedure was viable. When we received wonky results-- that is, the signals were mixed and the samples appeared to have multiple products-- we hypothesized that this was due to the primer setting down in the wrong location during the sequence reaction or perhaps a hairpin loop structures getting in the way of the sequencing (we gratefully acknowledge John Barrett for his suggestions).
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<br />
 +
<h2>Sequencing</h2>
 +
We utilized the software [http://www.genecodes.com/ Sequencher] through the Minnesota Supercomputing Institute [https://www.msi.umn.edu/ (MSI)] to trim the ends of sequences we received from the BMGC and align them. We wanted to compare both sequencing reactions we had as of 16 July 2009 to each other and to the sequences of the parts that were available on the [http://partsregistry.org/Main_Page Registry]. We obtained successful alignments for parts I14032, J13002 and K091101, which were regulated by IPTG, aTc and both inducers, respectively. It is interesting to note that while our samples appeared to have multiple products, that is, on the chromatogram that accompanied our sequence output, we saw multiple signals for each base pair, the sequence products not only aligned with each other, but with the sequences on the Registry. So we ordered new primers for another sequencing reaction and, based on these alignments as well as the fact that part R0011 had already been characterized and I14013 was regulated by LasR as well as aTc, we reduced our number of parts to characterize to three.
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<h2>References</h2>
<h2>References</h2>
Shetty, R.P.; Endy, D.; Knight, T.F.  2008.  Engineering BioBrick vectors from BioBrick parts.  Journal of Biological Engineering 2.
Shetty, R.P.; Endy, D.; Knight, T.F.  2008.  Engineering BioBrick vectors from BioBrick parts.  Journal of Biological Engineering 2.

Revision as of 19:51, 21 July 2009

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Contents

Parts Characterization

We originally chose five promoters that were included in the 2009 iGEM Kit to characterize. Using part [http://partsregistry.org/wiki/index.php/Part:BBa_F2620 BBa_F2620], which was characterized by a group from MIT in 2004, as a template, we examined the following parts:

PartDescriptionRegulatorsPeople
[http://partsregistry.org/Part:BBa_I14032 I14032]Constitutive promoter classified as repressibleIPTGPrinceton 2004
[http://partsregistry.org/Part:BBa_J13002 J13002]Two TetR binding sites and RBSaTcUT Austin 2005
[http://partsregistry.org/Part:BBa_I14015 I14015]LasR, 3OC12HSL aTc regulated promoterLasR, 3C12HSL, aTcPrinceton 2004
[http://partsregistry.org/Part:BBa_K091101 K091101]TTL AND gateIPTG, aTcDavidson Missouri-Western 2008
[http://partsregistry.org/Part:BBa_R0011 R0011]Inverting regulatory region controlled by LacI; for comparison since already characterizedIPTGRegistry

We chose these parts because they had the same regulators as the promoters we examined in our project. Part [http://partsregistry.org/Part:BBa_K091101 K091101] was particularly interesting because it was one of the constructs of the Tet and Lac operators that we examined for our research. Since Tet and Lac are commonly studied operators in synthetic biology, we wanted parts that involved them to be well-characterized to ensure the viability of future research.

We decided to characterize these promoters by attaching them to part [http://partsregistry.org/Part:Bba_K081012 K081012], which consists of a strong RBS and GFP. This 'PoPS generator' takes [http://parts2.mit.edu/wiki/index.php/Abstraction_hierarchy_and_PoPS PoPS] (Polymerase Per Second) as an input and gives GFP as an output, allowing us to indirectly measure PoPS and characterize our parts.

BiobrickVector.jpg

The picture at the right, from [http://www.jbioleng.org/content/2/1/5 Shetty et al. Journal of Biological Engineering 2008] demonstrates how to combine standard biological parts to form a new composite part. In our case, the prefix part was each of our 5 promoters and these were digested with restriction enzymes EcoRI and SpeI. The suffix part was the PoPS generator in every case except part [http://partsregistry.org/Part:BBa_J13002 J13002], which already contained an RBS. This [http://partsregistry.org/wiki/index.php?title=Part:BBa_B0034 RBS] is defined as efficiency 1.0 while the RBS contained on our PoPS generator, which has an efficiency of 0.6. We decided to characterize the entire part that [http://parts2.mit.edu/wiki/index.php/UT_Austin_2005 UT Austin 2005] submitted, which included their RBS. These suffix parts were cut using restriction enzymes XbaI and PstI.

We ligated these parts to make a composite BioBrick part in [http://partsregistry.org/Part:pSB3K3 pSB3K3], a low-medium copy plasmid with kanamycin resistance.

The 2009 iGEM Judging Criteria gives MIT's characterization of part [http://partsregistry.org/wiki/index.php/Part:BBa_F2620 BBa_F2620] as an exemplar of parts characterization. We gratefully acknowledge their pioneering work with parts characterization and hope that our work continues to maintain the high standard for characterization of parts.

Like MIT in 2004, we characterized our 5 promoters included with the 2009 iGEM kit in terms of:

  1. Transfer Function: the equilibrium relationship between the input and output
  2. Specificity: the ability of the devide to distinguish between its true input and similar inputs
  3. Response time: the time taken for the output to respond to a change in input
  4. Stability: how transfer function changes across multiple rounds of cell division and culture

In the Lab

Initially, we resuspended the DNA for the promoters, PoPS generator and GFP in water and transformed them into [http://openwetware.org/wiki/TOP10_chemically_competent_cells Top10 chemically competent cells]. The plasmid backbone we transformed into CCDB-resistant cells. Then, we allowed the cells to grow overnight on the appropriate antibiotic plate based on the plasmid that the part was on. We picked colonies and inoculated liquid media. Once these cultures entered [http://en.wikipedia.org/wiki/Stationary_phase_(biology) stationary phase], we prepped the plasmids using the [http://www1.qiagen.com/products/plasmid/qiaprepminiprepsystem/qiaprepspinminiprepkit.aspx QIAprep Spin Miniprep Kit] for each promoter, the PoPS generator, GFP and the plasmid backbone (psB3K3) into which everything would be ligated. We quantified the purity of our DNA before performing polymerase chain reaction [http://en.wikipedia.org/wiki/Polymerase_chain_reaction (PCR)] to amplify the DNA we had from the plasmid prep.

Once the PCR completed, we usually ran some of the products out on an agarose gel to ensure that our DNA was the right size. We also sent some of our DNA to be sequenced and gratefully acknowledge the [http://www.bmgc.umn.edu/facilities/home.html BioMedical Genomics Center (BMGC)] at the University of Minnesota for their resources and expertise. The gel and sequencing helped us ensure that we had the correct plasmids.

We performed the restriction enzyme digest on PCR products and adjusted the reaction conditions based on the concentration of the DNA from the plasmid prep. This reaction ran for between 2 and 3 hours. We ran these products out on an agarose gel and excised the DNA with razor blades. Then, we purified the DNA using a QIAquick Gel Extraction Kit.

The purified DNA we ligated overnight at 16C. One of the challenges of this step was determining the appropriate ratio of insert to backbone because we were performing double insert rather than a single insert. The ratio for a single insert is 3:1 of insert to backbone. We still wanted to maximize insertion efficiency but minimize cancatamerization of inserts, so we ligated at a 6:1 ratio of inserts to backbone.

We transformed the ligation products into Top10 cells after their overnight ligation and plated them on LB + kanamycin plates since our plasmid backbone contained kanamycin resistance. This selected for non-transformants. The CCDB toxin built into the plasmid backbone also selected against uncut plasmid backbone and the gel purification step also allowed us to select the correct DNA. We grew these plates overnight and grew cultures from colonies that grew. Then, we were able to characterize the parts in terms of the four areas above: transfer function, specificity, response time, and stability.

Challenges

A day by day catalog of what we did for parts characterization can be found on our Google calendar on the https://2009.igem.org/Team:Minnesota/Notebook Experiments and Calendar] page. Clearly, despite the summary above, some of these steps we had to redo over and over. Often, our DNA after plasmid preparation and restriction enzyme digest was not very pure and had a low concentration, which necessitated picking colonies, growing more cultures and ]prepping more plasmids. Sequencing, which was performed by the [http://www.agac.umn.edu/ BMGC] on the U of MN campus, provided us with a huge challenge because often, our sequences were not clean so we were not sure that we had the correct parts. Running samples out on a gel and specing samples can be very helpful in double-checking the size and purity of fragments, but sequencing was a very important step that really told us whether our procedure was viable. When we received wonky results-- that is, the signals were mixed and the samples appeared to have multiple products-- we hypothesized that this was due to the primer setting down in the wrong location during the sequence reaction or perhaps a hairpin loop structures getting in the way of the sequencing (we gratefully acknowledge John Barrett for his suggestions).

Sequencing

We utilized the software [http://www.genecodes.com/ Sequencher] through the Minnesota Supercomputing Institute (MSI) to trim the ends of sequences we received from the BMGC and align them. We wanted to compare both sequencing reactions we had as of 16 July 2009 to each other and to the sequences of the parts that were available on the [http://partsregistry.org/Main_Page Registry]. We obtained successful alignments for parts I14032, J13002 and K091101, which were regulated by IPTG, aTc and both inducers, respectively. It is interesting to note that while our samples appeared to have multiple products, that is, on the chromatogram that accompanied our sequence output, we saw multiple signals for each base pair, the sequence products not only aligned with each other, but with the sequences on the Registry. So we ordered new primers for another sequencing reaction and, based on these alignments as well as the fact that part R0011 had already been characterized and I14013 was regulated by LasR as well as aTc, we reduced our number of parts to characterize to three.


References

Shetty, R.P.; Endy, D.; Knight, T.F. 2008. Engineering BioBrick vectors from BioBrick parts. Journal of Biological Engineering 2.