Team:Caltech/Project/Oxidative Burst

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Pathogen Defense by Oxidative Burst


Introduction

In order to help guard against infections of the gut, we wish to engineer a strain of E. coli capable of killing bacterial pathogens. White blood cells called neutrophils are already very efficient at killing bacteria. Neutrophils kill bacteria by bombardment it with a variety of reactive oxygen species including superoxide, hydrogen peroxide and hydrochlorous acid. The reactive oxygen species kill the bacteria by shredding biological molecules by way of their potent oxidizing properties. However neutrophils do not to migrate to the large intestinal lumen where pathogens can reside. Because bacteria are well adapted to live in the gut, this project’s goal is to engineer a strain of E. coli to detect and kill invading bacterial pathogens by means of a sudden burst of hydrogen peroxide.

Detection

Figure 1 - Quorum sensing in gram negative bacteria

Bacteria are able to communicate between individuals of the same species by way of quorum sensing. Small molecules serve as the signal between individual cells. Gram negative bacteria use acylhomoserine lactones (AHL), which can freely diffuse across the cell membrane. The quorum sensing machinery relies in two enzymes, LuxI, an AHL producer, and LuxR, an AHL-dependent transcriptional activator. Figure 1 illustrates how the quorum sensing system works. In isolation, each bacterium constitutively produces a small amount of AHL, which quickly diffuses into the surroundings. If other bacteria of the same species are also nearby, the AHL will diffuse across their membrane where it will bind to LuxR. LuxR activates transcription of several genes, including luxI. A positive feedback loop is created, in which more AHL induces more LuxI, which in turn produces more AHL. Each species of gram negative bacteria produces a unique AHL, requiring unique LuxI and LuxR proteins, and so avoids crosstalk between species. A group of bacteria can thus toggle between an “off” state and an “on” state by using quorum sensing.

Figure 2 - Detection scheme used by our engineered E. coli

Our engineered strain will not participate directly in quorum sensing, but instead will eavesdrop on the conversation. It will be engineered to constitutively express a LuxR able to detect a species AHL. By taking advantage of the specificity of quorum sensing, our engineered strain will be able to be tuned to specifically respond to a variety of bacterial pathogens. Once the AHL is bound, LuxR will activate a set of genes which will lead to the overproduction of hydrogen peroxide, killing the invading cell.

Response

After sensing the presence of an invading pathogen, we want to engineer our E. coli to produce lethal amounts of hydrogen peroxide relatively quickly. We are not concerned with having the engineered E. coli survive either, as it is reasonable to assume that there are “unactivated” cells far away from the pathogen that could sustain the population. Even if all of the oxidative burst cells were wiped out, the population could be regenerated. In combination with the population variation project, the "master cell line" would differentiate into the oxidative burst state, thus reseeding the population. After LuxR binds AHL, it will activate transcription of pyruvate oxidase, which uses pyruvate to produce hydrogen peroxide in the following reaction:

Pyruvate + phosphate + O2 --> H2O2 + CO2 + acetyl phosphate

Streptococcus pneumoniae naturally uses pyruvate oxidase to kill off competing bacteria when infecting the lungs. Having already known its activity and antibacterial properties in vivo, pyruvate oxidase was an attract oxidase with which to work.

Even though our activated engineered cells will eventually die from their oxidative burst, we want them to survive long enough to produce large amounts of the oxidase so they can produce large amounts of hydrogen peroxide. If the cells were left to produce hydrogen peroxide without any protection, they would produce just enough to be cytotoxic and then fissle, killing only themselves and little else. To avoid this problem, an E. coli catalase will be constitutively expressed, and then turned off shortly after pyruvate oxidase expression is triggered. We’re accomplishing this by putting katG (on of two E. coli catalase genes) behind the tetR sensitive promoter (tetR P) and having tetR co-transciptionally expressed with the oxidase. The time it takes for tetR to accumulate in the cell provides the delay in repressing katG expression. To ensure katG is rapidly cleared from the cells, it has a C-terminal ssrA degradation tag, which should reduce the protein’s half life to the order of minutes. In this way, the cell can be temporarily protected from hydrogen peroxide, but large amounts can accumulate before the substrate is exhausted.The final strain will have deletions of both catalases, ensuring no complementation.

System Design

Figure 3 - System design for the oxidative burst.

The entire system will be engineered onto a high copy plasmid in E. coli as seen in Figure 3. Promoters are shown as bent, thin arrows, genes as thick arrows, ribosome binding sites as blue ovals, and a double transcriptional terminator as two red circles. Initially, the system will function independently, with luxR under a constitutive promoter. Later, luxR will be put under the control of a recombinase system that will only turn on the pathway randomly in a subset of cells. This will be one of three fates the master strain will be able to differenciate into. For more information, visit the population variation page.

An ideal system would behave as outlined in Figure 4. It shows the relative abundances of the proteins and molecules used in the system. It is only meant to show if a particular species is relatively high or low, not its absolute concentration.

Figure 4 - Ideal system response for the engineered E. coli after being exposed to AHL.

Results

Constructs

Figure X - Constructs made to characterize the performance of SpxB and KatG, as well as their genetic control elements.

The constructs shown in figure X were made using the standard assembly method. They were made to test the various regulatory elements and the functionality of the oxidase and catalase.

Characterization of LuxR Inducer

Figure X - Characterization of LuxR inducer and TetR inverter by flow cytometry. The figure shows the fluorescence of GFP in the constructs luxR-GFP and luxR-tetR-GFP. The left axis corresponds to the LuxR data and the right axis corresponds to the TetR data. At 100 nM AHL, cells with the luxR-GFP construct grew very poorly.

The TetR inverter was characterized by using a luxR-tetR-GFP construct. In this context, GFP provides a relative gauge of expression levels of KatG in the final construct. Figure 4 shows the tetracycline inverter behaved as expected. At high concentrations of AHL, the TetR inverter shows near full repression, as compared to the lower concentrations of AHL. Similar to the LuxR inducer, the TetR inverter showed a 50 fold difference in expression between the uninduced (low AHL) and induced (high AHL) states. However the absolute maximum level of expression from the TetR inverter was much lower than that from the LuxR inducer (compare the scale of the left TetR axis to the scale of the left LuxR axis). The low expression levels can be explained by the leakiness of the LuxR promoter, resulting in a basal level of repression from the TetR inverter. The low expression level is advantageous for the engineered E. coli because catalase is a very efficient scavenger of hydrogen peroxide. The low expression level ensures there is enough KatG to buffer any leaky pyruvate oxidase expression, yet still clear quickly from the cytoplasm. Additionally, in the uninduced state there should be extremely low levels of KatG. The LAA degradation tag should reduce KatG levels even further.

Characterization of TetR Inverter

Production of Hydrogen Peroxide

Functionality of KatG

Coculture Assay

Current Progress

  • Characterization of LuxR receiver: The luxR receiver (F2622)is able to turn on transcription of GFP reporter in the presense of acyl-homoserine lactone (AHL). The part begins to switch on around 100pM AHL and has a 43x fold increase in GFP flourescence between the induced (10nM AHL) and uninduced states. Although saturation of the luxR switch was not observed at 10nM AHL, it is difficult to characterize behavior at 100 nM or 1000 nM AHL because the cells grow very poorly. Presumably, this is due to a high protein load. Therefore, saturation of the luxR reciever likely occurs between 100 and 1000 nM AHL. Flow cytometry data did show the receiver to be leaky, as compared to a control without a GFP reporter, even in the uninduced state. In the final construct, the GFP reporter will be replaced by the oxidase. Thus this data shows our engineered cells will be able to activate the appropriate gene in response to detecting an invading pathogen, although there will likely be a basal level of oxidase expression. All cells (DH10B) were grown in M9 + 2% glucose prior to flow cytometry.
  • Characterization of TetR inverter: Besides turning on an oxidase, the engineered E. coli need to turn off transcription of their protective catalase. In the uninduced state, the catalase serves as a buffer against leaky oxidase expression. Flow cytometry data shows that when the tetR inverter (Q04400) is cloned downstream of the luxR receiver, it is able to repress GFP expression to that of the negative control (no GFP reporter). This bods very well as catalase will need to be tightly repressed in order to allow H2O2 to accumulate to bactericidal concentrations. The addition of an LAA tag to the catalase should not only ensure fast clearance of the catalase one the cell is induced, but also further reduced any possible leaky expression.
  • Galactose oxidase characterization: Galactose oxidase has proven to be a difficult enzyme to get to function in vivo. Every in vitro test (essentially just lysing the cells in a sodium phosphate buffer containing CuSO4 and testing the soluble fraction) has shown galactose oxidase to be consistently very active. However cells expressing galactose oxidase fail to produce detectable amounts of H2O2 in the supernatant. This is true even of JI377 cells (DE katE, katG, ahp) which cannot scavenge hydrogen peroxide. The leading hypothesis for this inactivity is that galactose oxidase doesn't have sufficient access to its cofactor, Cu2+. Cells grown with copper, thoroughly washed, and then lysed show a great reduction in the activity of galactose oxidase. For this reason, we are looking into the alternative oxidase, pyruvate oxidase.
  • Pyruvate oxidase: Pyruvate oxidase (spxB) from Streptococcus pnumoniea (R6) is being explored for its ability to produce H2O2 in vivo. This enzyme is responsible for the hydrogen peroxide that this pathogen naturally produces when it infects the lungs of humans. The most attractive part of this enzyme it that there should be no transport issues for its substrait (pyruvate) into the cell. Pyruvate oxidase is currently being tested in E. coli in a catalase proficient strain (DH10B) and a catalase deficient strain (JI377), either under the control of a strong constitutive promoter (J23100.B0034) or an AHL inducible promoter (F2622.B0034). The first bit of good news is that catalase deficient cells cannot grow when constitutively expressing pyruvate oxidase, while catalse proficient cells can. This suggests the toxicity is mediated by H2O2 rather than high protein loads or the toxicity of pyruvate oxidase.

References

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