Team:Pasteur Paris/Composite Part

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FIGHT INFECTIONS

RIP secretion : BBa_K2616001

To easily measure the effect of RIP on Staphylococcus aureus, we designed an initial construct allowing us to simply produce RIP after IPTG induction. Thus, we designed a part containing a T7 promotor, a ribosome binding site (RBS) upstream, followed by a signal sequence for secretion fused to the RIP sequence downstream of the coding sequence.

Eight different secretion systems have currently been identified in Escherichia coli, and more generally in Gram-negative bacteria [1]. Type I and type II secretion systems are the most commonly used for secretion of recombinant proteins. We chose to use Type II to secrete RIP [2].
Type II secretion system is a two-steps system: proteins are first exported to the periplasmic space, between E. coli’s two membranes, and then secreted to the medium [2].
We target RIP to the periplasm using the Sec-dependent secretion system [1], [3]. Our peptide is fused to an amino-terminal signal sequence that gets recognized by the chaperone SecB, then addressed to SecA and then translocated across the inner membrane through the SecYEG complex. One advantage of this system is that the signal sequence gets cleaved during translocation through SecYEG [1]. Several different signal sequences have been characterized (all formed of 18 to 30 amino acids) [3].
Following the advice of Dr. Jean-Michel Betton, Research Director in the Structural Biology Department at the Institut Pasteur, we chose to try two different signal sequences to export our peptides, which he knew about and which are known to be efficient: MalE and DsbA [2], [4], [5]. A secretion machinery called “secreton” then enables the release of proteins extracellularly. However, this system is not very well characterized yet, and it is a complex machinery composed of more than 10 proteins, so we did not plan to use it. However, since RIP is only a 7 amino acid protein, leaky release from the periplasm to the medium should be enough to obtain RIP in the medium [6].

RIP secretion following S. aureus detection: BBa_K2616003

In order not to produce RIP continuously but only in presence of S. aureus, we engineered a sensor device in our modified E. coli capable of detecting S. aureus and producing RIP after detection.

Our modified E. coli expresses under a constitutive promoter BBa_J23107the sensor device of S. aureus agr operon. It is composed of agrA and agrC, and we took it from BBa_I746100 from iGEM Cambridge 2007 team. Staphylococcus communicate through a quorum sensing mechanism, which consists in producing and detecting signaling peptides called AIP (Auto-Inducing Peptide). If S. aureus approaches our system, AIP will be detected by the transmembrane protein agrC, launching the phosphorylation of agrA which then activates promotor P2 ( Bba_K1351037 , characterized by LMU-Munich 2014 team). Our RIP sequence fused to a signal sequence for periplasmic export is placed after promotor P2 and will consequently be expressed only if S. aureus approaches our biofilm.

NERVE GROWTH FACTOR (NGF) SECRETION: BBa_K2616000

Part description

We built a part which should permit to secrete proNGF directly in the extracellular medium using E. coli type I secretion system. We used an inducible promoter T7 in order to control proNGF production thanks to IPTG induction. We added an His-tag in order to purify it.

Secretion

Type I secretion system transports proteins in one step across the two cellular membranes [2]. It is composed of an inner membrane protein HlyB, a periplasmic channel protein HlyD and an outer membrane protein TolC. As every secretion system, secretion through this one too is mediated by the specific recognition of a signal sequence, which in this case are the sixty C-terminal amino acids of alpha-haemolysin HlyA. This sequence binds with the HlyB-HlyD complex and is then translocated into the channel [7].


There are several problems to address when secreting recombinant proteins through the Type I secretion system:

  • First, the signal sequence HlyA is not cleaved when crossing the channel, but it needs to be cleaved to obtain a functional protein in the medium. That is why we fused the proNGF sequence with this sixty-amino acid long sequence, separated by the cleavage site for Tobacco Etch Virus protease (TEV). As we co-express TEV protease, the signal sequence will be eliminated once it is out the cell, and our proNGF can be active.
  • Secondly, if TolC endogenously exists within E. coli, this is not the case of the transporter complex HlyB-HlyD. Thus, we co-transformed our bacteria with another plasmid pVDL 9.3, generously provided by Dr. Victor de Lorenzo, from Centro Nacional de Biotecnologia of Madrid, bearing HlyB and HlyD sequences, in order to get a chance to secrete NGF out of the cell. [8]

KILL SWITCH : BBa_K2616002

Since we imagined a technology which requires to integrate engineered bacteria in humans, we need to ensure that the engineered bacteria are contained in the specific environment they are designed for. That is why we thought of using a “kill switch” that cause them to die if they are released in the environment. Our kill switch is based on temperature: it enables bacteria to survive at human body temperature (37°C) but die at lower temperatures.

The kill-switch we use is based on a toxin/antitoxin combination, CcdB/CcdA [9]. CcdB is a lethal toxin for E. coli and its production is placed under the regulation of a temperature-sensitive promoter [9]. In permissive conditions, i.e. in human body, the expression of the toxin is repressed and the antitoxin is expressed at a constitutive low level in order to counteract any leaky expression of the toxin. This is done thanks to the modification of the Plac promoter, which is explained precisely in the KILL-SWITCH part of this wiki. When the temperature goes lower, the repression is lifted and toxin expression increases. The constitutive low level of antitoxin is no longer sufficient to counter the effects of the toxin, and the bacteria die.

REFERENCES

  • E. R. Green and J. Mecsas, "Bacterial Secretion Systems - An overview," Am. Soc. Microbiol., vol. 4, no. 1, pp. 1-32, 2015.

  • S. H. Yoon, S. K. Kim, and J. F. Kim, "Secretory production of recombinant proteins in Escherichia coli.," Recent Pat. Biotechnol., vol. 4, no. March, pp. 23-9, 2010.

  • J. H. Choi and S. Y. Lee, "Secretory and extracellular production of recombinant proteins using Escherichia coli," Appl. Microbiol. Biotechnol., vol. 64, no. 5, pp. 625-635, 2004.

  • G. L. Rosano and E. A. Ceccarelli, "Recombinant protein expression in Escherichia coli: Advances and challenges," Front. Microbiol., vol. 5, no. APR, pp. 1-17, 2014.

  • N. Ke and M. Berkmen, "Production of Disulfide-Bonded Proteins in Escherichia coli," Curr. Protoc. Mol. Biol., vol. 108, no. 1, p. 16.1B.1-16.1B.21, 2014.

  • A. Giacometti et al., "RNA III Inhibiting peptide inhibits in vivo biofilm formation by drug-resistant Staphylococcus aureus," Antimicrob. Agents Chemother., vol. 47, no. 6, pp. 1979-1983, 2003.

  • S. Thomas, I. B. Holland, and L. Schmitt, "The Type 1 secretion pathway - The hemolysin system and beyond," Biochim. Biophys. Acta - Mol. Cell Res., vol. 1843, no. 8, pp. 1629-1641, 2014.

  • B. D. Tzschaschel, C. A. Guzmán, K. N. Timmis, and V. De Lorenzo, "An Escherichia coli hemolysin transport system-based vector for the export of polypeptides: Export of Shiga-like toxin IIeB subunit by Salmonella typhimurium aroA," Nat. Biotechnol., vol. 14, no. 3, pp. 303-308, 1996.

  • F. Stirling et al., "Rational Design of Evolutionarily Stable Microbial Kill Switches," Mol. Cell, vol. 68, no. 4, p. 686-697.e3, Nov. 2017.