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| {{:Team:Tuebingen/Template/Tuebingen}} | | {{:Team:Tuebingen/Template/Tuebingen}} |
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- | __TOC__
| + | * [[Team:Tuebingen/ProjectOverview|Overview]] <br /> A short introduction including an animation film. |
- | | + | * [[Team:Tuebingen/ProjectQuestions|Questions]] <br /> Every project should start with important questions, here are ours. |
- | == Overview ==
| + | * [[Team:Tuebingen/ProjectMechanism|Mechanism]] <br /> An in-depth explanation of our genetically engineered system. |
- | | + | * [[Team:Tuebingen/ProjectImplementation|Implementation]] <br /> Assembly and plasmid construction to implement the system. |
- | Our general aim is to establish a simple synthetic organisim which will
| + | * [[Team:Tuebingen/Parts|Submitted Parts]] <br /> All of our submitted Parts. |
- | be capable to measure the influence of endocrine disruptors on the
| + | * [[Team:Tuebingen/References|References]] <br /> Scientific literature used to design our project. |
- | natural balance of sexual determination in all kind of vertebrates. The
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- | measurement itself will be cost-efficient, environment-friendly and
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- | sensitive.
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- | | + | |
- | Naturally occuring iron receptors of the PAQR family are found to
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- | repress the fet3 promotor on high level of extra-cellular iron.
| + | |
- | According to Smith et al. human mPR expressed in yeast induced the same
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- | signal when binding to progesterone. Relying on this results we will
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- | express various mPRs of Danio rerio and Xenopus laevis in yeast to
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- | measure endocrine substances that influence fish and amphibians.
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- | | + | |
- | We will transform the negative signal (fet3 repression) into a positive
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- | signal by regulating a repressor (rox1 or mig1) with Pfet3. This
| + | |
- | repressor will in turn regulate the expression of the reporter gene
| + | |
- | (firefly luciferase or beta-galactosidase) and allow quantitative
| + | |
- | measurement.
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- | | + | |
- | == Motivation ==
| + | |
- | | + | |
- | ''Why do we want to establish a mechanism for steroid measurement?''
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- | | + | |
- | Steroid hormones, especially estrogens, occur in all vertebrates and
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- | play a crucial role in sexual differentiation. In recent times the
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- | pollution of waters with these hormones has become an increasing problem
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- | for the aquatic fauna.
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- | | + | |
- | Particularly waters functionalized by humans or adjacent to human
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- | settlements, e.g. in areas with agricultural use, show increased
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- | concentrations of estrogen.
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- | | + | |
- | Scientific studies based on ''Danio rerio'' showed that the consequences
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- | are devastating.
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- | | + | |
- | High concentrations of 17α-ethinylestradiol, a hormone in most
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- | birth-control pills, affected the sex differentiation of ''Danio rerio''
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- | leading to development of ovotestis or complete feminization (Andersenc,
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- | 2002).
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- | | + | |
- | Intersex-fish have been reported in UK rivers since 1978 downstream of
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- | an sewage treatment plant.
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- | | + | |
- | We believe that a first step in finding a solution to this environmental
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- | problem is an accurate and reliable method to quantify steroid
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- | concentrations.
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- | | + | |
- | == Occurring Questions ==
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- | | + | |
- | On our way designing the major pathway to express a specific reporter
| + | |
- | gene to demonstrate the presence of steroid hormones, we had and still
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- | have to deal with several questions concering the choice of BioBricks,
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- | genes and vectors to construct a firm method to determine "pollution" by
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- | steroids. As a conclusion, we have to meet two major requirements for
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- | our system:
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- | | + | |
- | * It should be as cost-efficient as possible for easy and regular application | + | |
- | * It should be resistant to yeast's own metabolism (no disturbance by unexpected expression).
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- | | + | |
- | At first we had to find an appropriate receptor to bind steroid
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- | hormones in efluents. It should fulfill the following requirements:
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- | | + | |
- | * It should only be responsible to substrates we wish to detect, so the results of the test will not be falsified.
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- | * It has to be easiliy integrated into yeast's cell membrane.
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- | * Its nucleic acid sequence should not be too long so we can put it onto a plasmid vector.
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- | | + | |
- | We chose the membrane progesterone receptor of the zebra fish (''Danio rerio'') and the African clawed frog (''Xenopus laevis''). We focused on
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- | these receptors, since they are easy to duplicate and interact with a
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- | broad bandwith of sex-determining hormones.
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- | | + | |
- | The next step was to select an appropriate organism to express these
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- | receptors. After some research, we could narrow our options down to two
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- | organisms:
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- | | + | |
- | * ''Escherichia coli''
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- | * ''Saccharomyces cerevisiae''
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- | | + | |
- | Finally we decided for yeast, since it has been done more research with
| + | |
- | it according to our prefered receptors. In addition yeast is an
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- | eukaryote making it more easier to integrate mPRs into their cell
| + | |
- | membrane.
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- | | + | |
- | == '''Mechanism''' ==
| + | |
- | | + | |
- | [[File:MechanismScheme.png|right|400px|Mechanism]] | + | |
- | [[File:Igem_2.3.jpg|thumb|right|Planned mechanism]] | + | |
- | | + | |
- | | + | |
- | Naturally occuring iron receptors of the PAQR family are found to repress
| + | |
- | fet3 promotor on high levesl of extra-cellular iron. According to
| + | |
- | [http://www.ncbi.nlm.nih.gov/pubmed/18603275 J Smith et al.]
| + | |
- | human mPR expressed in yeast induced the same signal binding to estrogen. Relying
| + | |
- | on this results we will try to express various mPRs of ''Danio rerio'',
| + | |
- | ''Xanophus laevis'' in yeast which we find fitting to measure
| + | |
- | endocrine substances that influence fish.
| + | |
- | | + | |
- | We will transform the negative signal (fet3 repression) into a positive signal by regulating a repressor (rox1 or mig1) with Pfet3. This repressor will in turn regulate the expression of the reporter gene (firefly luciferase or beta-galactosidase) and allow quantitative measurement.
| + | |
- | | + | |
- | === Receptors ===
| + | |
- | | + | |
- | Membrane progesterone receptors are membrane bound, seven-transmembrane receptors and belong to the PAQR family (progesterone adiponectin Q receptor). These G-protein coupled receptors activate inhibitory Gi units.
| + | |
- | | + | |
- | === Inhibitors and their targets ===
| + | |
- | | + | |
- | An appropriate inhibitor/promotor combination is a crucial step in our
| + | |
- | pathway and should be selected wisely.
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- | | + | |
- | Finally we chose FET3 as our promoter and both ROX1 and MIG1 as
| + | |
- | inhibitors. It is very likely, that they don't seem to repress any gene
| + | |
- | expression that are crucial for yeast.
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- | | + | |
- | === Reporter genes ===
| + | |
- | | + | |
- | The last station of our signaling pathway should be a reporter gene
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- | which amplifies our initial signal to allow a quantitative measurement.
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- | | + | |
- | The enzyme '''luciferase''' fulfills these conditions and is our
| + | |
- | candidate of choice.
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- | | + | |
- | == Implementation ==
| + | |
- | | + | |
- | | + | |
- | === Promoter ===
| + | |
- | [[File:PRS313_Padh1_Danio_Tadh1.png|promoter1]] | + | |
- | [[File:PRS313_Padh1_Xenopus_Tadh1.png|promoter2]]
| + | |
- | === Inhibitor ===
| + | |
- | [[File:PRS315_Pfet3_rox1_Tadh1_V3.png|inhibitor1]] | + | |
- | [[File:pRS315_Pfet3_mig1_Tadh1.png|inhibitor2]]
| + | |
- | === Reporter ===
| + | |
- | [[File:PRS316_Panb1_lacZ_Tadh1.png|reporter1]] | + | |
- | [[File:pRS316_Psuc2_lacZ_Tadh1.png|reporter2]]
| + | |
- | [[File:PRS316_Psuc2_Luciferase_Tadh1.png|reporter3]] | + | |
- | | + | |
- | == Measurement ==
| + | |
- | | + | |
- | The measurement itself should be limited to an optical one. With this
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- | idea in mind, we decided for reporter genes like lacZ and luciferase,
| + | |
- | because these produce signals which can simply be quantified by optical
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- | measurement methods.
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- | | + | |
- | == References ==
| + | |
- | | + | |
- | * [1] Jessica L. Smith, Brian R. Kupchak, Ibon Garitaonandia, L. Kim Hoang, Andrew S. Maina, Lisa M. Regalla, and Thomas J. Lyons - 2008 - Heterologous expression of human mPRα, mPRβ and mPRγ in yeast confirms their ability to function as membrane progesterone receptors
| + | |
- | * [2] Sumpter, Johnson (2008) Reflections on endocrine disruption in the aquatic environment
| + | |
- | <!-- | + | |
- | * Liew et. al. - 2012 Polygenic Sex Determination System in Zebrafish
| + | |
- | * Hanna et al. - 2006 - Cell-surface expression, progestin binding, and
| + | |
- | rapid nongenomic signaling of zebrafish membrane progestin receptors
| + | |
- | alpha and beta in transfected cells
| + | |
- | * Reupke - 2011 - Detektion dopingrelevanter anaboler Steroide in
| + | |
- | Pferdeurin und Pferdeplasma mithilfe eines Reportergen-Assays in
| + | |
- | Hefezellen. (Detection of doping relevant anabolic steroids in horse
| + | |
- | urin and blood plasma using yeast reporter gene assays)
| + | |
- | * “Assault on the male”, BBC 1996. Video report
| + | |
- | http://www.youtube.com/watch?v=LkxIJJI37bQ
| + | |
- | * Dr. Volker Scheil, The impact of potential environmental stressors on
| + | |
- | early development and cellular and biochemical biomarkers in fish,
| + | |
- | Main research: Fish embryotoxicity, histopathology and stress protein
| + | |
- | (hsp 70) responses.
| + | |
- | * Harris et al. - 2011 - The consequences of feminization in breeding
| + | |
- | groups of wild fish
| + | |
- | * Liew et al. - 2012 - Polygenic Sex Determination System in Zebrafish
| + | |
- | * Sumpter, Johnson - 2008 - 10th Anniversary Perspective Reflections on
| + | |
- | endocrine disruption in the aquatic environment from known knowns to
| + | |
- | unknown unknowns (and many things in between)
| + | |
- | * Werner, Palace, Wautier - 2006 - Reproductive fitness of lake trout
| + | |
- | (Salvelinus namaycush) exposed to environmentally relevant
| + | |
- | concentrations of the potent estrogen ethynylestradiol (EE2) in a
| + | |
- | whole lake exposure experiment
| + | |
- | * Fenske, M., Maack, G., Schäfers, C., & Segner, H. (2005). An
| + | |
- | environmentally relevant concentration of estrogen induces arrest of
| + | |
- | male gonad development in zebrafish, Danio rerio. Environmental
| + | |
- | toxicology and chemistry / SETAC, 24(5), 1088-98. Retrieved from
| + | |
- | http://www.ncbi.nlm.nih.gov/pubmed/16110986 (kein PDF)
| + | |
- | * Schäfers, C., Teigeler, M., Wenzel, A., Maack, G., Fenske, M., &
| + | |
- | Segner, H. (2007). Concentration- and time-dependent effects of the
| + | |
- | synthetic estrogen, 17alpha-ethinylestradiol, on reproductive
| + | |
- | capabilities of the zebrafish, Danio rerio. Journal of toxicology and
| + | |
- | environmental health. Part A, 70(9), 768-79.
| + | |
- | doi:10.1080/15287390701236470
| + | |
- | * Segner, H., Caroll, K., Fenske, M., Janssen, C. R., Maack, G., Pascoe,
| + | |
- | D., Schäfers, C., et al. (2003). Identification of
| + | |
- | endocrine-disrupting effects in aquatic vertebrates and invertebrates:
| + | |
- | report from the European IDEA project. Ecotoxicology and environmental
| + | |
- | safety, 54(3), 302-14. Retrieved from
| + | |
- | http://www.ncbi.nlm.nih.gov/pubmed/12651186 (kein PDF)
| + | |
- | * Hanna et al. - 2006 - Cell-surface expression, progestin binding, and
| + | |
- | rapid nongenomic signaling of zebrafish membrane progestin receptors
| + | |
- | alpha and beta in transfected cells
| + | |
- | * Thomas et al. - 2007 - Steroid and G protein binding characteristics
| + | |
- | of the seatrout and human progestin membrane receptor alpha subtypes
| + | |
- | and their evolutionary origins
| + | |
- | * Thomas - 2008 - Characteristics of membrane progestin receptor alpha
| + | |
- | (mPR ) and progesterone membrane receptor component 1 (PGMRC1) and
| + | |
- | their roles in mediating rapid progestin actions
| + | |
- | * Jessica L. Smith, Brian R. Kupchak, Ibon Garitaonandia, L. Kim Hoang,
| + | |
- | Andrew S. Maina, Lisa M. Regalla, and Thomas J. *Lyons - 2008 -
| + | |
- | Heterologous expression of human mPRα, mPRβ and mPRγ in yeast confirms
| + | |
- | their ability to function as membrane progesterone receptors
| + | |
- |
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- | -->
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