Difference between revisions of "Team:HZAU-China/Design"

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                 <div class="h2">Surface Display</div>
 
                 <div class="h2">Surface Display</div>
 
                 <p>In order to enable bacteria to have the greater targeting ability towards tumor, we improved part <a href="http://parts.igem.org/Part:BBa_J36850">OmpA</a> to  
 
                 <p>In order to enable bacteria to have the greater targeting ability towards tumor, we improved part <a href="http://parts.igem.org/Part:BBa_J36850">OmpA</a> to  
                     OmpA-RGD protein to achieve this goal.
+
                     <a class="noul_link part_link" href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K2632008">OmpA-RGD</a> protein to achieve this goal.
 
                     RGD is a well-studied tumor homing tripeptide that specifically binds to alpha v beta 3 (αvβ3)
 
                     RGD is a well-studied tumor homing tripeptide that specifically binds to alpha v beta 3 (αvβ3)
 
                     integrin, which is widely overexpressed on cancer cells and blood vessels during cancer
 
                     integrin, which is widely overexpressed on cancer cells and blood vessels during cancer

Revision as of 13:22, 15 October 2018

Modification of Bacteria

Gene sifA is a vital gene located in Salmonella pathogenicity island, taking the role of maintaining the stability of Salmonella-Containing Vacuole (SCV) only after Salmonella infection.1,2,3,4. We also knocked out the sifA gene from Salmonella Typhimurium str. SL1344 genome by conjugational transfer. The aim is to reduce the toxicity of Salmonella and allow the protein, which is able to rupture the phospholipid bilayer of the cell membrane from the inner side purely, to release into the cytoplasma of the tumor cell.

Targeting
Surface Display

In order to enable bacteria to have the greater targeting ability towards tumor, we improved part OmpA to OmpA-RGD protein to achieve this goal. RGD is a well-studied tumor homing tripeptide that specifically binds to alpha v beta 3 (αvβ3) integrin, which is widely overexpressed on cancer cells and blood vessels during cancer angiogenesis. We intended to display RGD on the surface of bacteria, so as to target the αvβ3 on the surface of tumor cells.

Figure 1.

Thus we needed a method to display RGD in the outer membrane. We chose Lpp signal peptide and outer membrane protein A (OmpA) system, which has been extensively used todisplay a diverse group of proteins, including Green Fluorescent Protein(GFP)5, Organophosphorus Hydrolase (OPH),single chain Fv fragments (scFv), Cellulomonas fimi exoglucanase Cexand its cellulose-binding domain(CBScex)6. Therefore, we expressed Lpp-OmpA-RGD fusion protein under the control of Ara promoter in our system. The fusion protein would be anchored in the outer membrane of bacteria and display RGD on the surface. Then RGD would lead the Salmonella to bind with tumor cells which have αvβ3 integrin on their surface7.

Figure 2.
Regulation of Pyroptosis
Chemical Induction

We decided to use anhydrotetracycline transcriptional regulation system to express GSDMD-N275 protein. It is one of the commonest methods to express toxin protein because of its low expression noise, high response speed and the good linear relation between the inducer and the expression of product. Anhydrotetracycline transcriptional regulation system is a one-component signal transduction system that regulates the expression of the tetracycline resistance determinant encoded by tetA, the anhydrotetracycline efflux pumping in Escherichia coli8. In this system, promoter Ptet expresses the repression protein TetR. With the presence of ATc (anhydrotetracycline), TetR will integrate ATc and. This induces a conformational change in TetR and its dissociation from the operon of Ptet and abolishes the repression9.

Figure 3.

We decided to use this system to regulate the expression ofour GSDMD-N275 protein, which controlled by Ptet promoter.

Figure 4.

However, we worried that the leakage of GSDMD-N275 will induce cytotoxicity. So we replaced different strength of RBS to choose the suitable RBS to control the leakage of GSDMD-N275. Owing to testing the linear stability of ATc induction and to transfer the expression of GSDMD-N275 to the concentration of ATc, we also constructed the TetR::EGFP (enhanced green fluorescent) fusion protein in E.coli (Fig.5) as an essay suggested10. And we induced Salmonella with gradients of ATc and measured the fluorescence accordingly. More details to our experimental method has been listed in our notebook and the ATc induction model. Finally, we constructed the EGFP::GSDMD-N275 expressed by the anhydrotetracycline transcriptional regulation system to proof our final circuit.

Figure 5.
The Intracellular Specific Induction

Once delivered into the host cell, Gram-negative bacteria Salmonella always express its virulence genes to alter host cell functions with the advantage of the pathogen. These genes are in Salmonella Pathogenicity Island and enterobactin gene cluster1,11. Owing to the feature of expressing intracellularly, we used promoters of these genes to express GSDMD-N275 after its entrance to tumor cells. To achieve this goal, we constructed PsifA::GSDMD-N275 and transferred it via electroporation (see details in our Methods). The figure below shows their functions (Fig 6.). Promoters in the circuits won't work outside cells but only express GSDMD-N275 after the entry to tumor cells.

Reference

1. Garmendia, J., Beuzón, C. R., Ruiz-Albert, J. & Holden, D. W. The roles of SsrA-SsrB and OmpR-EnvZ in the regulation of genes encoding the Salmonella typhimurium SPI-2 type III secretion system. Microbiology 149, 2385–2396 (2003).

2. Beuzon, C. R. Salmonella maintains the integrity of its intracellular vacuole through the action of SifA. EMBO J. 19, 3235–3249 (2000).

3. Steele-Mortimer, O. The Salmonella-containing vacuole-Moving with the times. Curr. Opin. Microbiol. 11, 38–45 (2008).

4. Nevozhay, D., Adams, R. M., Murphy, K. F., Josic, K. & Balazsi, G. Negative autoregulation linearizes the dose-response and suppresses the heterogeneity of gene expression. Proc. Natl. Acad. Sci. 106, 5123–5128 (2009).

5. Shi, H. & Wen Su, W. Display of green fluorescent protein on Escherichia coli cell surface. Enzyme Microb. Technol. 28, 25–34 (2001).

6. Earhart, C. F. Use of a n Lpp-OmpA Fusion Vehicle for Bacterial Surface Display. Methods Enzymol. 326, 506–516 (2000).

7. Desgrosellier, J. S. & Cheresh, D. A. Integrins in cancer: Biological implications and therapeutic opportunities. Nat. Rev. Cancer 10, 9–22 (2010).

8. Cuthbertson, L. & Nodwell, J. R. The TetR Family of Regulators. Microbiol. Mol. Biol. Rev. 77, 440–475 (2013).

9. Kisker, C., Hinrichs, W., Tovar, K., Hillen, W. & Saenger, W. The complex formed between Tet repressor and tetracycline-Mg2+ reveals mechanism of antibiotic resistance. J. Mol. Biol. 247,260–280 (1995).

10. Nevozhay, D., Adams, R. M., Murphy, K. F., Josic, K. & Balazsi, G. Negative autoregulation linearizes the dose-response and suppresses the heterogeneity of gene expression. Proc. Natl. Acad. Sci. 106, 5123–5128 (2009).

11. Crouch, M. L. V, Castor, M., Karlinsey, J. E., Kalhorn, T. & Fang, F. C. Biosynthesis and IroC-dependent export of the siderophore salmochelin are essential for virulence of Salmonella enterica serovar Typhimurium. Mol. Microbiol. 67, 971–983 (2008).

Description
Design

Modification of Bacteria

Targeting

Regulation of pyroptosis

Reference

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