Team:Evry/Project FUR

From 2013.igem.org

Revision as of 00:03, 5 October 2013 by Batou (Talk | contribs)

Iron coli project

FUR system

Iron is an essential element in the development of E. coli, but it can also be toxic and E. coli can be killed, if iron is absorbed in high quantity. Using the ferric-uptake regulator protein (Fur), bacteria developed an advanced system to regulate their iron homeostasis.

FUR protein (Ferric Uptake Regulator)

The Fur protein is a transcriptional repressor for more than 90 genes involved, in majority, in iron homeostasis1,2. It plays an important role in the control of the intracellular concentration of iron in E. coli.

Fur acts as a positive repressor in presence of ferrous ion (Fe2+), its co-repressor. Then, Fe2+ binds to the Fur protein (one ferrous ion per subunit of Fur). This interaction leads to a structural modification and induces the dimerization of Fur and Fe2+. Then the homodimeric Fur-Fe2+ complex will bind to the DNA on a Fur binding site and inhibit the mRNA transcription. In absence of Fe2+, a disinhibiting effect occurs and mRNA can be transcribed.

Meca_FurBS
Figure 1: Regulation by the Fur transcriptional factor. In absence of iron mRNA can be transcribed. In presence of iron, Fur binds the DNA, on the Fur binding site and mRNA expression is inhibited.

Fur is found at a level of 5000 copies in E. coli during exponential growth and it can be up to 10’000 copies in stationary phase. Note that this high number of Fur protein is essential to E. coli during its development. As explain previously, Fur regulates the expression of gene involved in the iron absorption, so it avoids an over absorption of iron which could be really toxic and kill E. coli.

FUR binding site architecture

Meca_RyhB
Figure 2: Consensus palindromic sequence of Fur binding site.

The Fur Binding site also named “Fur box” or “iron box” is localized between -35 and -10 site at the promoters of Fur-repressed genes. As shown in the Figure 2, the Fur binding site is composed of 19-base pair that are organized as a palindromic consensus sequence. It must be noted that this consensus sequence is not an exact sequence. Others sequences of Fur binding sites can be found into E. coli’s genome.

Often, Fur binding site is repeated (as shown in the Figures 3 and 4). It means that several homodimer of Fur-Fe2+ can bind among the DNA. Then Fur binding sites can be localized in a larger region than between -35 and -10 of the promoter region (defined previously). The affinity of these Fur binding site to Fur-Fe2+ is different. In a first time the complex Fur-Fe2+ binds to the 1st Fur binding site, which presents a higher affinity for its complex. Then, others Fur-Fe2+ bind to the following Fur binding sites which present a weaker affinity. A polymer of Fur protein is formed among the DNA which allows a stronger inhibition of the expression of the gene downstream these Fur binding sites.

Meca_RyhB
Figure 3: Repeated Fur binding site sequences.
Meca_RyhB
Figure 4: Repeated Fur binding site sequences on a double strand DNA.

Natural inverter system

It had been shown that Fur could be involved in a positive regulation of several genes of E. coli (fntA, bfr, acnA, fumA, sdh operon, sodB). In fact E. coli uses an inverter system mediated by a small RNA named RhyB.
RhyB is a 90 nucleotids long sRNA which is regulated by the Fur transcriptional factor, then it is expressed at low concentration of iron3.

Meca_RyhB
Figure 5: Regulation by the Fur transcriptional and the RhyB sRNA, acting as an inverter. In absence of iron mRNA is binded by the RhyB and then it is degradated. In presence of iron, Fur binds the DNA, the RhyB expression is inhibited and the mRNA can be transcribed.

As shown in Figure 5, and if we apply it to the sodB gene expression system. In iron starvation, Fur-Fe2+ cannot be formed and RyhB transcription is disinhibited. RyhB is expressed in the intracellular environment and it can binds to sodB mRNA which contains RyhB’s target sequence. Once RyhB binds to SodB mRNA, RNA degrading enzymes, such as RNaseE and RNase III, are recruited and the new formed complex is digested.
However, if the iron concentration is high enough, Fur-Fe2+ complex is formed and it can inhibit the RyhB transcription. SodB is not repressed and can be synthesized3. That is why Fur is described as an activator transcriptional factor in such a case.

Siderophores

In lack of iron, bacteria produced siderophores, small molecules, that can catch any atom of iron in the environment to feed the bacteria. There is different types of siderophores, depending on their structure and their interaction with iron:

  • Catecholate,
  • phenolate,
  • hydroxymate,
  • carboxylate types.

We focus more specifically on enterobactins which are catecholate siderophore (composed with catechol = bi-phenol) produced by E. coli. Enterobactins present a very high affinity for ferric iron K = 1052 M-14. This number is greater than the affinity of heme B and EDTA metal chelator for iron, respectively K = 1039 M−1 and 1025 M−1. De facto, enterobactins are one of the most powerfull siderophore known: it can extract iron from hemic source and even from air!

Enterobactines Structure
Figure 7: Structure of Enterobactin molecule.

Ferric iron Fe3+ established hydrogen bound with the alcohol groupment of enterobactins.

Enterobactines
Figure 8: 3D structure of enterobaction without (A) or with (B) Ferric Iron5.

Genes of enterobactin pathway are under the regulation of the Fur protein in E.coli. It means that genes of enterobactin pathway are expressed only in lack of iron.

Enterobactine Synths
Figure 9: Pathway of the synthese of the enterobactin.

In our project, we want to produce enterobactin. Then we focus on the 6 enzymes (EntA, EntB, EntC, EntD, EntE and EntF) of it biosynthesis started from chorismic acid. However, we want to produce enterobactin in presence of iron, in order to reduce an excess of iron.

Constructions

Meca_RyhB
Figure 10: Enterobactine production using the Fur-inverter system.

Our goal is to decrease the iron absorption from the intestines to the blood by using an iron chelating bacteria, Iron Coli.
We have design a system that could produce enterobactins from chorimsic acid, under the regulation of an iron sensor with an inverter. When the iron is present in the environment (ie intestine) in high concentration, our Iron Coli will produce siderophores to chelate the iron and hence reduce the amount of iron that could be absorbed by the patient.
We also model enterobactin production of our Iron Coli and the potential efficiency of our treatment to cure iron overload.

References:

  1. Revue
  2. “Iron and metal regulation in bacteria”, Klaus Hantke)
  3. (ref: Amanda G., “Iron responsive Bacterial small RNAs: variation on a theme”)
  4. Zheng, T. 2012, "Siderophore-Mediated Cargo Delivery to the Cytoplasm of Escherichia coli and Pseudomonas aeruginosa : Syntheses of Monofunctionalized Enterobactin Scaffolds and Evaluation of Enterobactin–Cargo Conjugate Uptake".
  • Raymond, K. N. 2003; link to the pdf