Team:Heidelberg/Project

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Project Idea

Ecolicence to kill: Engineering E.coli for targeting pathogenic microorganisms

Pathogenic microorganisms represent a major challenge to both medicine and industry. Microbial communities known as biofilms prove to be particularly resistant to conventional therapies [1] and demonstrate the need for alternative methods to fight bacterial growth. The formation of biofilms, as well as other processes such as virulence, antibiotic production, and sporulation, are regulated by communication circuits that depend on small signalling molecules called autoinducers. Our aim is to exploit this communication mechanism by engineering synthetic bacteria that are able to target potentially harmful autoinducer-secreting species and kill them. Working with E. coli as a model system, we plan to engineer separate “killer” and “prey” cells, and divide our project into two complementary modules. The “sensing module” comprises the modification of E. coli’s chemotaxis [2] system to make killer cells move towards prey cells. This requires the engineering of a “sensing module” which propagates a prey-specific stimulus to the downstream signalling cascades, prompting the cells to swim towards the gradient of such a stimulus. The directed swimming stops only in the region where the stimulus is maximal, i.e. in the vicinity of the prey. The “killing module” ensures that once in the vicinity of the prey, a bacteriocidal mechanism is activated. Computer models will show how both modules behave in concert and probe the efficiency of the system in defined spatial environments. Future directions, which are beyond the scope of this project, include the modification of the sensory and killing modules, adjusting the range of targets to real pathogens, but also other organisms, specific cell types or even cancer cells.

Fig. 1: A killer cell senses the specific signal of autoinducer-2 secreted by prey cells and chases them with chemotaxis
Fig. 2: Once the preys are caught the killer cells are induced by a second specific signal, autoinducer-1, to activate a killer mechanism.

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Deutsche Übersetzung:

Ecolizenz zum Töten: Eine E. coli-Konstruktion zum gezielten Angriff auf pathogene Mikroorganismen

Pathogene Mikroorganismen stellen eine große Herausforderung sowohl für die Medizin als auch für die Industrie dar. Gemeinschaften aus Mikroorganismen, die in der Fachsprache als Biofilme bezeichnet werden, haben sich als äußerst resistent gegenüber konventionellen Therapien erwiesen [1]. Um deren Wachstum zu bekämpfen bedarf es daher alternativen Ansätzen. Die Entstehung von Biofilmen, genauso wie die der Virulenz, der Produktion von Antibiotika oder der Bildung von Sporen werden durch Kommunikations-Schaltkreise reguliert, die auf kleinen Signalmolekülen - den sogennanten Autoinduzierern (AI) - basieren. Unser Ziel ist es, diese Kommunikationsmechanismen in der Weise zu integrieren, dass synthetische Bakterien potenziell gefährliche, AI-ausschüttende Spezies aufspüren und töten können. Mit E. coli als Modellorganismus beabsichtigen wir zwei separate Stämme - einen Killer- und einen Beutestamm - zu entwerfen. Das Projekt gliedert sich in zwei ergänzende Module: Die Signalerkennung umfasst die Modifizierung des Chemotaxis-Systems von E. coli [2], um Killer-Zellen zu den Beute-Zellen schwimmen zu lassen. Dafür ist es notwendig, dass ein Erkennungsmodul einen Beute-spezifischen Stimulus an die Signalkaskade für Chemotaxis weiterleitet, so dass die Killer-Zellen entgegen des Gradienten des Stimulus schwimmen. Das gerichtete Schwimmen kommt nur zum Erliegen, wenn sich die Killer-Zellen in der unmittelbaren Umgebung der Beute-Zellen befinden - dort, wo die Stimuluskonzentration maximal ist. Das Killer-Modul gewährt, dass - einmal in der Nähe der Beute angekommen - ein bakterizider Mechanismus aktiviert wird. Computermodelle werden ergänzend zeigen, wie sich die beiden Modelle im Zusammenspiel verhalten, und wie die Effizienz des Gesamtsystems in seiner räumlichen Umgebung einzuschätzen ist. In Zukunft - sicherlich außerhalb der Reichweite unseres Projekts - könnte die Spezifität auf relevante Pathogene, genauso wie auf andere Organismen, Gewebe oder sogar Krebszellen erweitert werden.

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Project Realization

Have you ever wondered, why numbers of iGEM team members are limited to a maximum of twelve students? Apart from financial resources, this limit is only natural: efficient work with larger team sizes requires a subtle organization and project management, in particular when the team is still green! On top, team formation and project work have to be conducted within a short time interval and under liabilities to the academic curriculum - both on the student and the advisor sides. The social abilities for reliable team formation, in particular communication, team integration, and consequence to work towards common team goals, must therefore be substantial and dedicated to compensate these circumstances. When you visit our portraits, however, you will realize that we are not so green and that each of us has an active past often intricately connected with scientific work. In our project description we provide a sincere answer to the apparent question, if 16 "greenhorns" can push forward in only four months to contribute research on an international level!

In order to streamline our horse-power, we divide the project into four columns, which are simultaneously developed by us and can merge in the end with a synergistic effect to a complex population system (modeling inclusive). At the same time the global progress is robust towards each column, consequently a delay or failure in one column will not lead to a breakdown of the overall project. In accordance with current scientific standards demanded in systems and synthetic biology, we pursue an interdisciplinary approach combining mathematics, experimental, and quantitative biology [3].

The first column (Project - Sensing) comprises the design and development of a sensing module. Chemotaxis is a very effective mechanism of bacteria to move towards nutrients. Using the natural signals for bacterial quorum communication, we re-design a chemotactic receptor for detection of a quorum signal and its transmission to the chemotaxis signaling network. A prey strain, which is to be found via the sensing mechanism, will be engineered to secrete the specific quorum signal. We dedicate two columns to the development of a killing mechanism to secure a higher implementation confidence: One column, the second (Project - Killing I/Phages), is based on bacteriophages, which are conjugated once the killers are in the vicinity of the preys. Induction of conjugation is dependent on a second signal molecule - also from the family of quorum molecules. The mechanism can be considered as a pattern recognition of molecular exudation. In the third column (Project - Killing II/Colicins) the killing mechanism - which is activated by the same pattern - is based on colicin production. Colicins are bactericide substances, for which the producing host possesses resistance. In a fourth column (Modeling) we model the system behavior of these two bacterial strains - the killer and the prey - in a 2D landscape. One approach is based on partial differential equations and simulates chemotaxis and the colicin killing mechanism; the second approach based on delay differential equations analyzes the killing dynamics with bacteriophages. Visualization - the architrave - with microscopy is finally employed to quantify bacterial density landscapes in space and time - allowing a phenotypic connection and comparison with our modeling work.


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Literature

[1] K. Brenner et al., Engineered bidirectional communication mediates a consensus in a microbial biofilm consortium, PNAS, Vol. 104 (44), pp. 17300-17304 (2007)
[2] G. H. Wadhams and J. P. Armitage, Making sense of it all: bacterial chemotaxis, Nat. Rev. Mol. Cel. Bio., Vol. 5, pp. 1024-1037 (2004)
[3] N. Wingreen and D. Botstein, Back to future: education for systems-level biologists, Nat. Rev. Mol. Cel. Bio., Vol. 7(11), pp. 829-832

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Phips the Phage

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