Team:Peking/Project/BioSensors/HcaR

From 2013.igem.org

(Difference between revisions)
Line 207: Line 207:
#FigurePic1{position:absolute; top:650px; width:600px; left:200px; }
#FigurePic1{position:absolute; top:650px; width:600px; left:200px; }
-
#FigurePic2{position:absolute; top:1800px; width:600px; left:200px; }
+
#FigurePic2{position:absolute; top:1750px; width:600px; left:200px; }
#FigureData1{position:absolute; top:2220px; width:700px; left:150px; }
#FigureData1{position:absolute; top:2220px; width:700px; left:150px; }

Revision as of 07:01, 27 September 2013

Biosensors

A FAST, EASY AND ACCURATE METHOD TO DETECT TOXIC AROMATIC COMPOUNDS

HcaR Mechanism Build Our Own Sensor!

Escherichia coli play an essential role in the circulation of materials in the nature, especially for aromatic compounds. The gene clusters related to the aromatic compounds mainly include hca (for 3-phenylpropionic acid and cinnamic acid), mhp (for 3-hydroxyphenylpropionate and phenylpropionate), paa (for phenylacetic acid) and hpa (for 4-hydroxyphenylacetic acid). All of them have the regulators to control the expression of corresponding genes, according to which we could design biosensors detecting aromatic compounds.

HcaR is a 32,838 Da (296 amino acids) protein, which belongs to LysR family. Its’ N-terminal domain functions in DNA binding via a helix-turn-helix motif, while C-terminal domain functions in multimerization. As an activator, HcaR activates the expression of hca cluster at the presence of ligands. It detects limited range of ligands, including 3-phenylpropionic acid (PPA) and cinnamic acid (CnA) [1]

MhpR is a 31,767 Da (281 amino acids) protein. It belongs to IclR family, which forms helix-turn-helix motif at N-terminal. MhpR behaves as an activator to initiate the expression of mhp cluster when contacts with its ligands, 3-hydroxyphenylpropionate (3-HPPA), 3-hydoxycinnamate (3-HCnA) and 3-(2, 3-dihydroxyphenyl) propionic acid (2,3-DHPPA). [2]

hca and mhp clusters are involved in the catabolism of PPA and CnA in E. coli (Fig.1). The enzymes encoded by hca cluster degrade PPA and CnA to 2,3-DHPPA and 2,3-DHCnA respectively, which serve as the substrates of the mhp cluster. The enzymes in mhp cluster function in the cleavage of aromatic ring.

Compared with the sole 2,3-DHPPA, the special induction effect of PPA and 2,3-DHPPA is obtained, although PPA don’t behave as ligand alone. Based on the result and the observation of different binding site of PPA with MhpR, it is deduced that PPA and 2,3-DHPPA have synergistic effect to the activation of MhpR expression [3]. (That is to say, PPA enhances the activation effect as a cooperator of 2,3-DHPPA instead of a ligand.) The same effect is observed in 3-HPPA along with PPA.

The synergistic effect seems to be explained by pre-activation mechanism. It is that 2,3-DHPPA is a product of PPA degradation by hca cluster, and it will accumulate before activating the expression of the downstream mhp cluster. 2,3-DHPPA has cytotoxicity to the bacteria. The pre-activation mechanism activates the downstream cluster at low ligand concentration so that bacteria consume it to prevent accumulation of toxicity. The mechanism reflects the precise control across several pathways in bacteria, and also contributes to the sensor application [3].

Based on the information, our team constructed the Ph/HcaR expression system. The coding sequence of HcaR was obtained from the genome of E. coli K12 via PCR. Constitutive Pc promoters are used to initiate the expression of hcaR on pSB4K5, and sfGFP, as a reporter gene, is under the control of Ph, the cognate promoter of HcaR.

We also created a Pc library to obtain the optical performance of this expression system which gets the best induction ratio. The library consists of a series of Pc promoters with different expression intensity, including BBa_J23113, J23109, J23114 and J23106. Primary test following protocol 1 showed that HcaR performed best under the control of BBa_J23106. Then the best performed expression system is subjected to the On-Off test about 78 aromatics according to protocol 1. Results showed that HcaR worked as a specific sensor to PPA (Fig.2).

Figure 1.The degradation pathway of PPA and CnA

Figure 2. Results of On-Off test about biosensor HcaR. HcaR specifically responds to PPA (1000 μM) with the induction ration over 2.

Reference:
[1] Díaz, E., Ferrández, A., & García, J. L. (1998). Characterization of the hca Cluster Encoding the Dioxygenolytic Pathway for Initial Catabolism of 3-Phenylpropionic Acid in Escherichia coliK-12. Journal of bacteriology, 180(11), 2915-2923.
[2] Ferrández, A., García, J. L., & Díaz, E. (1997). Genetic characterization and expression in heterologous hosts of the 3-(3-hydroxyphenyl) propionate catabolic pathway of Escherichia coli K-12. Journal of bacteriology, 179(8), 2573-2581.
[3] Manso, I., Torres, B., Andreu, J. M., Menéndez, M., Rivas, G., Alfonso, C., ... & Galán, B. (2009). 3-Hydroxyphenylpropionate and phenylpropionate are synergistic activators of the MhpR transcriptional regulator from Escherichia coli. Journal of Biological Chemistry, 284(32), 21218-21228.