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| <p>Cyanobacteria are prokaryotic photoautotrophs and they are believed to be the only group of organisms to | | <p>Cyanobacteria are prokaryotic photoautotrophs and they are believed to be the only group of organisms to |
- | evolve oxygenic photosynthesis about 2.4 billion years ago (1). Although this biochemical breakthrough can’t | + | evolve oxygenic photosynthesis about 2.4 billion years ago [[#1|1]]. Although this biochemical breakthrough can’t |
| be understated, several cyanobacteria species also play a crucial role in the planet nitrogen cycle as marine | | be understated, several cyanobacteria species also play a crucial role in the planet nitrogen cycle as marine |
- | diazotrophs (2). They are found almost in every environment in earth´s surface and interestingly, they | + | diazotrophs [[#2|2]]. They are found almost in every environment in earth´s surface and interestingly, they |
| are the only prokaryote known to have circadian rhythms, probably accounting for their photosyntethic | | are the only prokaryote known to have circadian rhythms, probably accounting for their photosyntethic |
- | lifestyle (3).</p> | + | lifestyle [[#3|3]].</p> |
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| <p><i>Synechocystis PCC6803</i> is a gram negative non-filamentous cyanobacteria and it was the third | | <p><i>Synechocystis PCC6803</i> is a gram negative non-filamentous cyanobacteria and it was the third |
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| <p>Given the reasons mentioned above, it is of no surprise that <i>Synechocystis PCC6803</i> (among other | | <p>Given the reasons mentioned above, it is of no surprise that <i>Synechocystis PCC6803</i> (among other |
- | cyanobacteria) has been extensively used for biotechnological applications and proposed as the “green <i>E.coli</i>”(4).</p> | + | cyanobacteria) has been extensively used for biotechnological applications and proposed as the “green <i>E.coli</i>”[[#4|4]].</p> |
| <p>With the dawn of Synthetic Biology, research has made use of <i>Synechocystis</i> for | | <p>With the dawn of Synthetic Biology, research has made use of <i>Synechocystis</i> for |
- | commodity chemicals production and detection of water soluble pollutants among other applications(5, 6).</p> | + | commodity chemicals production and detection of water soluble pollutants among other applications[[#5|5]],[[#6|6]].</p> |
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| | | |
| <p>While aware of these practical applications, we (UC_Chile) are particulary interested in the well | | <p>While aware of these practical applications, we (UC_Chile) are particulary interested in the well |
- | characterized circadian behavior of this chassis (7) and its implications. There are several | + | characterized circadian behavior of this chassis [[#7|7]] and its implications. There are several |
| genes known to oscillate in a daily basis, most of them related to respiration, photosynthesis and energy | | genes known to oscillate in a daily basis, most of them related to respiration, photosynthesis and energy |
- | metabolism (8), and it has been shown that reporter systems using these promoters show a | + | metabolism [[#8|8]], and it has been shown that reporter systems using these promoters show a |
- | similar expression pattern (9).</p> | + | similar expression pattern [[#9|9]].</p> |
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Motivational drive
Natural cycles have always fascinated mankind, probably due to the mysterious mechanisms involved in them and the power they exert in our everyday life. Since the dawn of synthetic biology, engineering oscillatory systems has been a recurrent topic, being Ellowitz's represillator a classical example. Nevertheless, to date no iGEM team has accomplished the implementation of a robust oscillatory system. That will be our challenge for this year's iGEM project.
To reach our goal we designed a synthethic circuit that links to the endogenous circadian rhythm of Synechocystis PCC6803. As a proof of concept we are going to engineer the first light-rechargeable biological lamp: Synechocystis PCC 6803 cells that emit light only by night while recovering and producing the substrates in the day. We strongly believe this will serve as an enabling tool to any project requiring time control over a biological behaviour independently of the user's input.
Furthermore, the characterization of this chassis is a fundamental step to explore new systems with minimal inputs to replace E. coli, for example, in the biotechnological industry in order to achieve greener processes.
Background
Synechocystis PCC 6803
Cyanobacteria are prokaryotic photoautotrophs and they are believed to be the only group of organisms to
evolve oxygenic photosynthesis about 2.4 billion years ago 1. Although this biochemical breakthrough can’t
be understated, several cyanobacteria species also play a crucial role in the planet nitrogen cycle as marine
diazotrophs 2. They are found almost in every environment in earth´s surface and interestingly, they
are the only prokaryote known to have circadian rhythms, probably accounting for their photosyntethic
lifestyle 3.
Synechocystis PCC6803 is a gram negative non-filamentous cyanobacteria and it was the third
prokaryote and the first photoautotroph whose genome was sequenced. Consequently, is has become a model organism as its genetic background has been widely studied.
Given the reasons mentioned above, it is of no surprise that Synechocystis PCC6803 (among other
cyanobacteria) has been extensively used for biotechnological applications and proposed as the “green E.coli”4.
With the dawn of Synthetic Biology, research has made use of Synechocystis for
commodity chemicals production and detection of water soluble pollutants among other applications5,6.
While aware of these practical applications, we (UC_Chile) are particulary interested in the well
characterized circadian behavior of this chassis 7 and its implications. There are several
genes known to oscillate in a daily basis, most of them related to respiration, photosynthesis and energy
metabolism 8, and it has been shown that reporter systems using these promoters show a
similar expression pattern 9.
Lastly, there are a lot of biobricks designed especially for Synechocystis or from its genome´s
sequence by previous iGEM teams (references) but sadly no one has ever characterized them in this chassis
and the registry lacks a set of tools for its transformation with standard biological parts. Moreover, to our
knowledge, no iGEM team has ever accomplished a successful direct Synechocystis transformation with naked DNA.
Lux Operon (faltan referencias!!)
The lux operon is a group of genes that are responsible for density-dependent bioluminescent behavior
in various prokariotic organisms such as Vibrio fischeri and Photorabdus luminescens. In V. fischeri, the operon is composed of 8 genes: LuxA and LuxB encode for the monomers of a heterodimeric luciferase; LuxC, LuxD and LuxE code for fatty acid reductases enzymes and LuxR and LuxI are responsible for the regulation of the whole operon.
Lastly LuxG is believed to act as a FMNH2 dependent FADH reductase, although luminescence is barely affected
in its absence. The n-decanal ( n= 9 to 14) substrate oxidization to n-decanoic acid by the LuxAB heterodimer is coupled with the reduction of FMNH to FMNH2 and the releasing of oxygen and x photons of light at x wavelength.
The carboxylic group of the product is then reduced to aldehyde by CDE proteins allowing the reaction to
start over.
LuxAB genes have been widely used as reporters dependent on the addition of n-decanal to the culture
media and in 2010, the Cambridge iGEM team engineered LuxABCDEG to an E. coli-optimized biobrick
format, uncoupling it from the LuxR and LuxI regulation.
As a team we decided to work with this operon for a number of reasons, first of all, the luminescence
produced by this pathway is much more visually appealing than other systems from the registry (i.e XFPs),
moreover, the light production doesn´t depend on a single peptide but on a whole pathway involving several genes, which makes it much more tunable, for instance, decoupling in time the substrate recovery from the luciferase reaction itself.
Experimental Strategy
We have devised different strategies to achieve bioluminescence controlled under circadian rhythms. Here we describe the strategies used for building the constructs to reach our goals.
Splitting the Lux operon and choosing promoters
We decided that we would separate LuxAB (the luciferase part of the operon) and LuxCDEG (the substrate producing enzymes LuxCDE with LuxG the FMNH2/FMN reducing enzyme) to allow phase-dependent expression of the parts. Using specific promoters of Synechocystis PCC. 6803 we can have fine-tunning of the production of bioluminescence. Recent work on global gene expression in Synechocystis aided on finding adecuate promoters 7, 8 . (Images at right from cited papers.)
To try our approach, we selected various promoter which could serve the purpose. Our rational for selecting candidate promoters involved amplitude of oscillation, peak activity, hour, absence of restriction sites, predicted strength of promoter according to the role of the gene and reproducibility between experiments (based on the literature available). We looked for promoters which would have peak expression nearby dusk hours and that were slightly out of phase to optimize production of bioluminescence according to our mathematical models (LINK OVER HERE!). We prioritized promoters from genes that would be involved in central energetic metabolism as we thought that their expression would be most robust and reliable. We choose the transaldolase promoter (specific name here and code in Synechocystis Genome) to direct the expression of the LuxAB genes and we found a couple of other promoters which filled the other requirements from above. Pcaa3 (NAME HERE AND DESCRIPTION OF ENDOGENOUS ACTIVITY) and PsigE (NAME HERE AND DESCRIPTION OF ENDOGENOUS ACTIVITY), the former being already in Biobrick format (courtesy from the Utah team iGEM 2010).
Building constructs
As transformation in Synechocystis is undergone through double recombination of DNA strands, we designed two constructs that have different recombination locations in the Synechocystis chromosome.
pSB1C3_IntK
The first of our constructs is an integrative plasmid which targets neutral recombination sites (slr0370 and slr03770 DOUBLECHECK this). We selected this locus because it has been extensively used in the literature (CAPAZ EXAGERE?) and it shown to have no deleterious effects on Synechocystis viability. We selected Kanamycin resistance as our transformation marker. [PUT LINK TO CONSTRUCT HERE].
pSB1C3_IntS
We designed another construct that besides serving as a double recombination plasmid it makes Synechocystis susceptible to copper concentrations higher than X uM (Giner-Lamia, J., Lopez-Maury, L., Reyes, J. C., & Florencio, F. J. (2012). The CopRS two-component system is responsible for resistance to copper in the cyanobacterium Synechocystis sp. PCC 6803. Plant physiology, 159(August), 1806-1818.). We have designed this construct to interrupt the CopS gene as a biosafety measure to avoid the possibility of having a leakage of recombinant DNA to the environment. This plasmid has Spectynomycin resistance as the transformation marker. [PUT LINK TO CONSTRUCT HERE]
pSB1A2_IntC (Utah 2010 iGEM Team integration plasmid)
Alternatively, we designed our LuxCDEG contructs for the Utah 2010 iGEM Team plasmid backbone pSB1A2_IntC. [PUT LINK TO CONSTRUCT HERE].
(1) Evolution of photosynthesis. Hohmann-Marriott MF, Blankenship. Annual Review of Plant Biology Vol. 62: 515-548
</div>
(2) Nitrogen fixation by marine cyanobacteria. Jonathan P. Zehr. Trends in microbiology, Volume 19, Issue 4,
April 2011, Pages 162–17
(3) Carl Hirschie Johnson and Susan S. Golden. CIRCADIAN PROGRAMS IN CYANOBACTERIA: Adaptiveness
and Mechanism. Annual Review of Microbiology, Vol. 53: 389-409
(4) Ducat, D. C., Way, J. C., & Silver, P. a. (2011). Engineering cyanobacteria to generate high-value products.
Trends in biotechnology, 29(2), 95-103.
(5) Huang, H.-H., Camsund, D., Lindblad, P., & Heidorn, T. (2010). Design and characterization of molecular
tools for a Synthetic Biology approach towards developing cyanobacterial biotechnology. Nucleic acids
research, 38(8), 2577-93
(6) Peca, L., Kós, P. B., Máté, Z., Farsang, A., & Vass, I. (2008). Construction of bioluminescent cyanobacterial
reporter strains for detection of nickel, cobalt and zinc. FEMS microbiology letters, 289(2), 258-64.
(7) Kucho, K.-ichi, Okamoto, K., Tsuchiya, Y., Nomura, S., Nango, M., Kanehisa, M., Ishiura, M., et al. (2005).
Global Analysis of Circadian Expression in the Cyanobacterium Synechocystis sp . Global Analysis of Circadian
Expression in the Cyanobacterium. Society.
(8) Layana, C., & Diambra, L. (2011). Time-course analysis of cyanobacterium transcriptome: detecting
oscillatory genes. PloS one, 6(10), e26291.
(9) Kunert, a, Hagemann, M., & Erdmann, N. (2000). Construction of promoter probe vectors for
Synechocystis sp. PCC 6803 using the light-emitting reporter systems Gfp and LuxAB. Journal of
microbiological methods, 41(3), 185-94.