Team:ESBS-Strasbourg/Project/Strategy

Our device construction is divided into 4 components :

1. Degradation system
2. Light detection system
3. Protein Tagging
4. Light controllable protease

Notebook

The work of the former IGEM Team had a great influence on our choice, particularly those of The ESBS 2008 Team. Their goal was to control cells’ state by linking the natural variability of life to the binary system of computing. In the project of The ESBS 2008 Team, the incrementing from one bit to another required a protease which was expressed during the mitosis in yeast. Renaud Renault of the actual iGEM team had thus the idea of inventing a degradation system which would be not only temporally controllable but also specific.

Based on this idea we chose to create a light-controllable specific protein degradation system. The system contains several parts: degradation system with the bacterial ClpXP protease from Escherichia coli (E.Coli), the light detection system with the photoreceptor protein Phytochrome B and the Phytochrome Interacting Factor (PIF 3 or 6) from Arabidopsis thaliana (A. thaliana) and the protein tagging with the DAS/LAA recognition sequences for ClpX represent the main parts of our system.

The different parts, their basic ideas and their strategic development will be discussed in detail in the following separated parts. The choice of the host organism will also be explained, followed by the final structure of the light controllable protease.

The ClpXP from E.coli protease rapidly established itself as an evident choice. Indeed, this protease has been very well studied, notably by the Tania Baker Team from Berkeley.

Description

Basically, ClpXP is an AAA protease present in bacteria, consisting of two main components, ClpX and ClpP. The ClpX is a hexamer consisting of six identical subunits. It recognizes specific degradation tags of target substrate proteins, unfolds them in an ATP-consuming hydrolysis reaction, and uses additional cycles of ATP hydrolysis to translocate the unfolded polypeptide into an interior chamber of ClpP, where proteolysis takes place. ClpP is a multi-subunit serine peptidase, in which the proteolytic active sites reside within a barrel-shaped structure.

                       The figure on the left shows the two heptamers forming ClpP in our light controllable protease
The figure on the right shows the hexamers of ClpX in our light controllable protease

How using the ClpXP protease ? : The question of the use of an adaptator

This question was really critical. We focused on different strategies before making a definitive choice.
The publication of Tania Baker (Baker and Sauer 2006) based on the ClpXP protease of E. Coli which degrades substrates bearing the specific SsrA recognition sequence, has been the starting point of our reflection. In this work Baker and colleagues designed a series of modified ssrA tags which have weakened interactions with ClpXP to engineer controlled degradation. In E. coli, the adaptor SspB tethers ssrA-tagged substrates to the ClpXP protease, causing a modest increase in their rate of degradation. In the absence of SspB , substrates bearing the artificially altered DAS-tag were stable, in contrast the degradation of substrates bearing these engineered peptide tags was 100-fold more efficiently when SspB was present.

Upon these findings our first idea consisted in using the native ClpX with the mutated tag and a modified SspB whose binding to ClpX should be controlled by light in order to control protein degradation. Forcing cells to produce an inactive form of an adaptator seem to be a good solution to be able to stop the degradation at a certain point. This could be realized by producing two parts of the adaptator which could interconnect them after light-induction by fusing them to proteins which had this capacity, for instance the couple Phytochrome/PIF.

However, the use of the adaptor-based system posed some major problems concerning the complexity. Subsequent to another finding of Baker et. al., we decided to fuse our phytochrome directly to the N-terminal of ClpX, as it is not required for the basic enzymatic functions of ClpX (Baker and Sauer 2006).

Further, we decided to fuse the target protein, additionally to the specific degradation tag, with PIF which will assume the role of the adaptor protein SspB .

 

 

As told before, the Phytochrome/PIF system has been chosen as light detection system. Many reasons have motivated our choice: it is well-characterized, offers a second timescale control which is an order of magnitude faster than previous chemically induced translocation systems and are very near the physical limits for whole-cell diffusion. It has also been proven to be robust being cycled over a hundred times by alternating red and infrared illumination with no measurable decrease in recruitment ratios over time (Lim & Voigt 2009)

 

 

  The figure shows the phytochromes B
        in our light controllable protease

Description

Phytochromes are photoreceptive signaling proteins responsible for mediating many light-sensitive processes in plants, including seed germination, seedling de-etiolation and shade avoidance. They detect red and near-infrared light through the photoisomerization of a covalently bound tetrapyrrole chromophore such as phycocyanobilin (PCB) for plant phytochromes. This photoisomerization event is coupled to an allosteric transition in the phytochrome between two conformational states called Pr (red-absorbing) and Pfr (far-red-absorbing).

Upon stimulation with red light (650 nm), the phytochrome B (PhyB) protein binds directly to a downstream transcription factor, the phytochrome interaction factor (PIF). PIF is a nuclear-localized, basic helix–loop–helix (bHLH) factor initially isolated as interacting with the non-photoactive, C-terminal domain of Arabidopsis PhyB.

Construction choice

We needed to study the different domains of the phytochrome B in order to try to reduce its size which can be a potential sterical hindrance for ClpX activity.
All plant phytochromes can be divided into an N-terminal photo sensory domain and a C-terminal dimerization domain. The Nterminal photo sensory domain comprises four consecutive subdomains called P1, P2/PAS, P3/GAF, and P4/PHY (named sequentially from the N terminus), the C-terminal domain consists of two subdomains, the PAS-A and PAS-B domains and the histidine kinase–related domain (HKRD) (Wu and Lagarias). The PAS domain is named after three proteins in which it occurs: Per (period circadian protein), Arn (Ah receptor nucleartranslocator protein), and Sim (single-minded protein) (Bae and Choi, 2008).
The P1 domain is not essential for the function of PHYB. Deletion of amino acids 1–57 of Arabidopsis PHYB yields a protein with full activity (Quail and Koloszvari). In contrast, the P2/PAS and P3/GAF domains form the essential photo sensory core domain. These domains contain a bilin lyase activity, which is responsible for the binding of the chromophore to a cysteine residue in the P3/GAF domain. The P2/PAS and P3/GAF domains play critical roles in photo sensing, whereas the P4/PHY domain is necessary for fine tuning phytochrome activity. Deletion of the P4/PHY domain increases the dark reversion rate (i.e., the instability of the Pfr conformation) and causes a blue shift in absorption by both Pr and Pfr. A serine/threonine kinase domain that governs phytochrome autophosphorylation and phytochrome-directed phosphorylation of other proteins, such as the phytochrome interacting factor (PIF3) has also been located in the N-terminal domain (Bae and Choi, 2008). The PAS-A and PAS-B domains of PHYB are necessary for dimerization and nuclear localization, whereas PAS-A, PAS-B, and the HKRD domains are necessary for nuclear speckle formation (Bae and Choi, 2008).Dimerization is required for PhyB full activity.

The light-sensitive interaction between PHYB and PIF3 has been mapped to the 650-residue amino-terminal photosensory core of PHYB (Khanna et al., 2004).
The improved understanding of these mechanisms has been helpful for the design of the first engineered photoreceptors. By now there have been three illuminating studies that utilized the interaction between PhyB and PIF3 to achieve light regulation of target proteins.
Leung et al. put the association of the GTPase Cdc42 with its effector protein WASP under red-light control. When in complex with PhyB-Cdc42, PIF3-WASP promoted actin polymerization in vitro; use in vivo was not demonstrated. Based on the interaction between PhyB and PIF3, Muir and coworkers established a protein-splicing system that was moderately regulated by red light in vitro65. Lastly, Lim & Voigt employed the light-dependent interaction between PhyB and PIF6 to activate target proteins in vivo. The nucleotide exchange factors Tiam and intersectin were recruited to the plasma membrane in a red-light-controlled manner where they activated their GTPase effectors Rac1 and Cdc42, respectively. In their activated form, the GTPases promoted formation of cell protrusions, and thus the motility of fibroblasts could be controlled by red light.
With this first successful in-vivo application Lim & Voigt have shown that the PIF-interaction with the PhyB photo sensory core (residues 1–642) is irreversible in infrared light. By assaying PIF6, which has the strongest interactions of all previously reported PIF domains, against different variants of PhyB they demonstrated that the tandem C-terminal PAS domains (residues 1-908) of PHYB are necessary to confer rapid photo reversibility under infrared light. The interaction with PIF3 has been too weak to cause significant translocation.

 

Upon these findings, we decided to tests different variants for the implementation of our system: for the phytochrome constructs we choose PhyB residues 1-908 (PhyB900) and the photo sensory core domain residues 1-642 (PhyB650) in combination with PIF3 (residues 1-100) and PIF6 (residues 1-100).
The choice to include the shorter PhyB650 variant in our tests is reasoned by the risk of a potential sterical hindrance of ClpX due to the fusioned PhyB. Due to its reduced size, the PhyB650 construct provides an additional control for the case that the system implementation using PhyB950 does not produce results. Further, binding strength and kinetic parameters depend on the composition and nature of the individual system, so we thought it a good idea to test the findings of Lim & Voigt in a novel background.

     The figure shows the
  phytochrome B domains
  used in our construction

The question of the chromophore

Since the plant phytochromes PhyA and PhyB employ the modified tetrapyrroles PCB or PΦB which are not available in most tissues and cell types, these chromophores must be supplied either exogenously or endogenously. The PCB chromophore, stemming from heme can be produced by ??? cells by inserting three additional genes into the ??? pathway [3]. Nevertheless, we decided to use the exogenous way by adding exogenous PCB as it has been shown that the endogenous modification of the bacterial metabolism leads to the production of toxic side-products.

Tagging

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Light Inducible Degradation

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