5. If H+ leaves HCl it is staying back Cl and it will be export from the transport of chlorine channel.
6. The emitted CO² is taken out by diffusion.
7. Finally, the uncovered GABA is thrown out from the transmembrane protein GadC.

When the given data checked, it is obvious that the produced GadE is functional and makes E. coli survive in the acidic microenvironment in comparison to negative control results. Based on the data given, the E. coli with overexpressed GadE can survive in pH 2 gastric juice for 5-9 hours.

By sequence analysis, H. pylori TlpB is organized like a typical member of the MCP superfamily of transmembrane receptors with two transmembrane helices (tm1, tm2) per subunit bracketing an extracellularsensing domain[2,7]. The extracellular-sensing domain is responsible for detecting ligands directly or indirectly via interactions with periplasmic-binding proteins. Continuing from tm2, the C-terminal portion of the MCP is cytoplasmic and mostly helical. It contains a histidine kinase, adenylyl cyclase, methyl-binding protein, phosphatase (HAMP) domain, followed by a helical domain and a segment that binds to the CheA/CheW histidine autoki-nase complex[2,8]. Phosphorylation of CheA in response to an extracellular signal in turn controls downstream compo-nents that modulate activity of the flagellar motor. MCPs dimerize at the membrane, forming a four helix bundle with ligand-binding domains in the periplasm, whereas trimers of dimers assemble with CheA and CheW to form a high-perfor-mance signaling array located in the cytoplasm[2,9].

In low pH conditions , TlpB’s periplasmic domain is in a ‘‘relaxed’’ or expanded state due to decreased hydrogen bonding to urea and consequent lowered urea-binding affinity. However, in high or more neutral pH conditions, TlpB’s periplasmic domain is in a ‘‘tense’’ or condensed state with increased urea-binding affinity. The state of the periplasmic domain is relayed through the transmembrane region, which affects CheA’s phosphorylation state, ultimately affecting the flagellar motor anddictating stopping behavior

References

SOFT AGAR PLUG ASSAY

HNS/HNST108I

Figure 2: Fluorescence anisotropy of H-NS-FliG interactions. Increasing amounts of FliG were added to fluorescein-labeled H-NS. Ten anisotropy values were measured at each FliG concentration and averaged. Graph is representative of two separate experiments. .

Figure 3: H-NS-FliG cross-linked complexes. Reactions were incubated at room temperature and equal amounts were electrophoresed on denaturing poly acrylamide gels. A, Coomassie-stained 4–20%SDSpolyacrylamidegradient gel; B, 12% SDS-polyacrylamide gel transferred to nitrocellulose, and probed with H-NS antiserum; C, second half of gel in B probed with FliG antiserum. Protein. Standard sizes are indicated by lines; lmw, low molecular weight markers; hmw, high molecular weight markers; protein monomers, dimers, and H-NS-FliG complexes are indicated by arrows. Reactions for all panels: 1, wild-type H-NS only; 2, H-NST108I only; 3, FliG only; 4, wild-type H-NS with cross-linker; 5, H-NST108I with cross-linker; 6, FliG with cross-linker;7, 1:1 molar ratio of wild-type H-NS to FliG with cross-linker; 8, 1:1molar ratio of H-NST108I to FliG with cross-linker.

Figure 2. Schematic diagram of the proton-driven bacterial flagellar motor. The flagellar motor consists of a reversible rotor made of FliF, FliG, FliM and FliN and a dozen stators, each of which consists of MotA and MotB. FliF forms the MS ring within the cytoplasmic membrane. FliG, FliM and FliN form the C ring on the cytoplasmic face of the MS ring. OM, outer membrane; PG, peptidoglycan layer; CM, cytoplasmic membrane.

RESULTS FOR PotB59/PomA

Helicobacter Pylori Sensing:

Helicobacter pylori lives in stomach, by connecting to epithelium cells under the mucus layer.This bacteria releases some molecules around which comes from its metabolic waste. Two of these molecules are Auto-inducer 2 and ammonia.

Ammonia (NH3)

H. pylori synthesizes urease to buffer the pH of its microenvironment within the stomach. H. pylori dedicates several genes to the biosynthesis of its cytosolic urease, a Ni2+-containing enzyme which hydrolyses urea into NH3 and CO2. Bacteria has urea channel which is regulated positively by protons, opening at acidic pH values to allow more urea in to buffer cytosolic and surface pH, and closing at neutral pH to avoid over-alkalinization [1].

Ammonia (NH3) buffers the cytosol and periplasm, and creates a neutral layer around the bacterial surface[1].With this surface created by bacteria, protects itself against low acid coditions of the stomach.

Figure 1: Helicobacter Pylori Environment.

Autoinducer 2 (AI-2)

Such as many gram-negative and gram positive bacteria has the quorum sensing (QS) molecule, H. Pylori has this molecule too. QS molecules are specific, low-molecular-weight signal molecules which used by bacteria to regulate expression of genes in response to changes in population density.[2]

H. pylori has Quorum Sensing molecule “Autoinducer-2 (AI-2)” which is produced depended on the activity of the LuxS enzyme [3].

Based on the information given above, we expect to find ammonia and Auto-inducer 2 molecules in the existence of H. pylori. Thus we aim to sense both of these molecules to find out if H. Pylori’s presence.

Figure 2:Our “AND GATE” system diagram: According to our system, TnrA transcription factor represses TnrA promoter which produce Toehold. In the presence of NH3 this press will be eliminated and Toehold will be produced. Lsr transcription factor represses pLsr promoter which produce Trigger mRNA. In the presence of AI-2 (Autoinducer-2) this press will be eliminated and Trigger mRNA will be produced. In conclusion Trigger mRNA opens the toehold system and TEV-Protease will be formed.

As a result, our “SENSING” system composed of three parties:

1.NH3 sensitive TnrA promoter

2. AI-2 sensitive Lsr promoter

3. Toehold system

1. NH3 Sensitive TnrA Promoter

Bacteria use nitrogen which is present in nearly all macromolecules such as proteins, carbonhydrates and peptidoglycan. Prokaryotes have developed transport and assimilation systems for a variety of nitrogen sources for living under optimal conditions and regulate their own systems. This regulatory network allows an adequate response to situations of nitrogen limitation.

In the Bacillus subtilis, ammonium assimilation occurs via the glutamine synthetase - glutamate synthase pathway. Bacillus subtilis faces nitrogen- limiting conditions when it consumes glutamate as a prior nitrogen source, while glutamine is the secondly preferred nitrogen source [3].

Two transcription factors, TnrA and GlnR, and one enzyme, the Glutamine Synthase, are the major players in the B. Subtilis nitrogen regulatory network [3]. We use TnrA transcription factor in our system.

Under nitrogen-limited conditions, TnrA works as an activator and a repressor both. TnrA represses expression of glnRA (Glutamine Synthase) [4], gltAB (Glutamate Synthase) [5] and other genes. Also the form of Glutamine Synthase which is feedback inhibited by excess glutamine, directly interacts with and unbinds from TnrA, thus blocks its DNA-binding activity [6]. Based on all this information, if the amount of NH3 is not sufficient, glutamine synthase will not work properly, glutamine will be produced in a low amount, TnrA will bind to promoter and Toehold production will be repressed. But if there is a sufficient amount of NH3, glutamine will be produced in a high level, TnrA will not repress the promoter as previous and Toehold – Tev Protease will be produced in a high amount.

Figure 3: If there is a sufficient amount of NH3, Toehold and TEV protease will be produced. If there isn’t a sufficient amount of NH3, Toehold and TEV Protease will not be produced.

Seventeen TnrA targets were detected by a combination of DNA microarray hybridization, a genome-wide search for TnrA boxes, and gel retardation assays [7]. The TnrA box consensus delimited in this study to a 17- bp interrupted, inverted repeat sequence, TGTNANAWWWTNTNACA.

2. AI-2 Sensitive Lsr Promoter

Figure 4:LsrR-binding site recognition and regulatory characteristics in Escherichia Coli AI-2 quorum sensing (Ting Xue, Liping Zhao, Haipeng Sun, Xianxuan Zhou and Baolin Sun).

In quorum sensing (QS) process, bacteria regulate gene expression by utilizing small signaling molecules called autoinducers in response to a variety of environmental cues. QS molecules secreted by bacteria are small, diffusible signaling molecules called autoinducers that accumulate in the external environment. When the concentration of the autoinducers reaches a threshold, an alteration of gene expression is induced, allowing the bacteria to adopt behaviors that are only productive when the bacteria are working together as a group [8].

Many quorum sensing molecules have been identified until now. In contrast to other autoinducers that are specific for a narrow range of organisms, the widely conserved AI-2 has been hypothesized to be a universal language for interspecies communication [9]. In every case, AI-2 is synthesized by LuxS, which functions in the pathway for metabolism of S-adenosylmethionine (SAM), a major cellular methyl donor. In a metabolic pathway known as the activated methyl cycle, SAM is metabolized to S-adenosylhomocysteine, which is subsequently converted to adenine, homocysteine, and 4,5-dihydroxy-2,3-pentanedione (DPD, the precursor of AI-2) by the sequential action of the enzymes Pfs and LuxS [10].

The regulatory network for AI-2 uptake is comprised of two other important components, lsrR and lsrK, which are located adjacent, but divergently transcribed from the lsr operon (Figure 1). LsrR is the repressor of the lsr operon and itself. LsrK is a kinase responsible for converting AI-2 to phospho-AI-2, which is required for relieving LsrR repression. It has also been postulated that phospho- AI-2 binds to LsrR and inactivates it to derepress the transcription of lsr [11].Since LsrR contains a helix-turn-helix (HTH) DNA-binding domain, it was hypothesized that LsrR represses the expression of lsr operon and itself by binding to their promoter regions [12].

Two independent groups demonstrated that H. pylori secretes AI-2 into its extracellular environment by a luxS-dependent mechanism.[13,14] Therefore we planned to use LsrR system to sense AI-2 molecules synthesized by H. Pylori.

In the absence of Autoinducer-2, LsrR repress the LsrR promoter to bind LsrR-Binding Site. In the presence of AI-2 extracellular AI-2 is imported into the cell (cytoplasmic AI-2) via LsrACDB transporter, where it is phosphorylated by LsrK. LsrK is a kinase responsible for converting AI-2 to phospho-AI-2, which is required for relieving LsrR repression. Phospho-AI-2 has been reported to bind to LsrR and relieve its repression effect on the lsrR promoter.

3. Toehold System

Toehold switches provide a high level of orthogonality and can be forward engineered to provide average dynamic range above 400. Toehold switches, with their wide dynamic range, orthogonality, and programmability, represent a versatile and powerful platform for regulation of translation, offering diverse applications in molecular biology, synthetic biology, and biotechnology.New classes of regulatory components that offer wide dynamic range, low system crosstalk, and design flexibility represent a much-needed, enabling step toward fully realizing the potential of synthetic biology in areas such as biotechnology and medicine. (Khalil and Collins, 2010).

Engineered riboregulators consist of cognate pairs of RNAs: a transducer strand that regulates translation or transcription and a trans-acting RNA that binds to the transducer to modulate its biological activity. Riboregulator designs can be classified according to the initial RNA-RNA interaction that drives hybridization between the transducer and trans-acting RNAs. Reactions initiated between loop sequences in both RNAs are termed loop-loop interactions, whereas those that occur between a loop sequence and an unstructured RNA are termed loop-linear(Takahashi and Lucks, 2013).

A common limitation for riboregulators has been their dynamic range (Liu et al., 2012). Previous prokaryotic translational riboregulators have typically modulated biological signals by up to a maximum of 55-fold for activators (Callura et al., 2012) and up to 10-fold for repressors (Mutalik et al., 2012). In contrast, protein-based transcriptional regulators have demonstrated dynamic ranges over an order of magnitude higher, with widely-used inducible promoters regulating protein expression over 350-fold (Lutz and Bujard, 1997) and sigma factor-promoter pairs providing up to 480-fold modulation (Rhodius et al., 2013).Despite the inherent programmability of RNA-based systems, efforts at constructing large sets of orthogonal riboregulators have been limited to libraries of at most seven parts with crosstalk levels of 20% (Takahashi and Lucks, 2013). Typical RNA-based regulators employ interaction domains consisting of30 nts, which corresponds to a sequence space of over 1018 potential regulatory elements. Thus, the sheer diversity of possible RNA-based parts suggests that previous devices have not come close to realizing the potential of highly orthogonal regulation.

Figure 5: (A and B) Design schematics of conventional riboregulators (A) and toehold switches (B). Variable sequences are shown in gray, whereas conserved or constrained sequences are represented by different colors.

Much of this discrepancy arises from the significant sequence constraints imposed on riboregulators engineered thus far (Figure1A). Like natural riboregulators, engineered riboregulators of translation have invariably used base pairing to the ribosome binding site (RBS) to prevent ribosome binding, thereby preventing translation (Callura et al., 2012; Isaacs et al., 2004; Mutaliket al., 2012; Rodrigo et al., 2012). Because repression is caused by RBS binding, trigger RNAs that activate translation are engineered to contain an RBS sequence to displace the repressing sequence, which in turn reduces the potential sequence space for the riboregulator.

Previous riboregulators have also relied on U-turn loop structures to drive loop-loop and loop-linear interactions between RNAs (Figure 1A) (Callura et al., 2012; Isaacs et al., 2004; Luckset al., 2011; Takahashi and Lucks, 2013). U-turn loops are common RNA structural motifs formed by tertiary interactions that have been identified in ribozymes, ribosomal RNAs, and transfer RNA anticodon loops (Gutell et al., 2000). Although recent work has begun to show that loops with canonical U-turn sequences are not essential for riboregulators (Mutalik et al., 2012; Rodrigoet al., 2012), the engineered systems reported to date have continued their reliance on the loop-mediated RNA interactions from natural systems. Although these loop interactions have been selected by evolution in nature, alternative approaches employing linear-linear RNA interactions are amenable to rational engineering and exhibit more favorable reaction kinetics and thermodynamics, factors that could be exploited to increase riboregulator dynamic range.

A riboregulator that activates gene expression must switch from a secondary structure that prevents translation to a configuration that promotes translation upon binding of a cognate trans-acting RNA. Although the Shine-Dalgarno sequence is an important factor in determining the efficiency of translation from a given mRNA, studies have found that secondary structure in regions near by the start codon also plays a critical role (Kudla et al., 2009).Furthermore, genome-wide analyses have revealed strong biases toward low secondary structures around the start codon of mRNAs from a panel of hundreds of bacterial genomes.

Toehold switch systems are composed of two RNA strands referred to as the switch and trigger (Figure 1B). The switch RNA contains the coding sequence of the gene being regulated. Upstream of this coding sequence is a hairpin-based processing module containing both a strong RBS and a start codon that is followed by a common 21 nt linker sequence coding for low-molecular-weight amino acids added to the N terminus of the gene of interest. A single-stranded toehold sequence at the 50 end of the hairpin module provides the initial binding site for the trigger RNA strand. This trigger molecule contains an extended single stranded region that completes a branch migration process with the hairpin to expose the RBS and start codon, thereby initiating translation of the gene of interest. The hairpin processing unit functions as a repressor of translation in the absence of the trigger strand. Unlike previous riboregulators, the RBS sequence is left completely unpaired within the 11 nt loop of the hairpin. Instead, the bases immediately before and after the start codon are sequestered within RNA duplexes that are 6 bp and 9 bp long, respectively. The start codon itself is left unpaired in the switches we tested, leaving a 3 nt bulge near the midpoint of the 18 nt hairpin stem. Because the repressing domain b (Figure 1B) does not possess complementary bases to the start codon, the cognate trigger strand in turn does not need to contain corresponding start codon bases, thereby increasing the number of potential trigger sequences. The sequence in the hairpin added after the start codon was also screened for the presence of stop codons, as they would prematurely terminate translation of the gene of interest when the riboregulator was activated. We employed a 12 nt Toehold domain at the 50 end of the hairpin to initiate its interaction with the cognate trigger strand. The trigger RNA contains a 30 nt single-stranded RNA sequence that is complementary to the toehold and stem of the switch RNA.

Figure 6: (C) Flow cytometry GFP fluorescence histograms for toehold switch number 2 compared to E. coli autofluorescence and a positive control. Autofluorescence level measured from induced cells not bearing a GFP-expressing plasmid.(D) GFP mode fluorescence levels measured for switches in their ON and OFF states in comparison to positive control constructs and autofluorescence. Error bars are the SD from at least three biological replicates.
Based on all information given above, we decided to use Toehold-Trigger RNA system fort he AND Gate part of our project.

At last, here is the place of toehold-trigger RNA system in our project as a diagram:

Sources:

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[8]: Ahmer BM. Cell-to-cell signalling in Escherichia coli and Salmonella enterica. Mol Microbiol 2004; 52:933-945
[9]: Federle MJ, Bassler BL. Interspecies communication in bacteria. J Clin Invest 2003; 112:1291-1299.
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[11]: Taga ME, Miller ST, Bassler BL. Lsr-mediated transport and processing of AI-2 in Salmonella typhimurium. Mol Microbiol 2003; 50:1411-1427.
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[15]:Green, A., Silver, P., Collins, J., & Yin, P. (n.d.). Toehold Switches: De-Novo-Designed Regulators of Gene Expression. Cell, 925-939.

TnrA-pAlsT -RFP

Main goal of this part is to show TnrA protein’s repressor activity on pAlst promoter and derepression of this promoter in the presence of NH3. Thereby we combined TnrA protein’s and pAlst’s gene sequences on the same biobrick. As a reporter, we put RFP gene sequence in front of the pAlst sequence. To make sure the repressive protein TnrA is produced in a high amount, we combined TnrA-pAlst-RFP gene sequence with T7 promoter which has a high transcription rate. Also, we put a Lac operator which LacI protein can bind, between this sequence and T7 promoter, in order to create a controllable system. We searched to find an expression vector working in harmony with this system, peT45-b expression vector was serving this purpose. . When we ordered our genes, we put RFC10 prefix site on 3’ end of TnrA-pAlst-RFP gene sequence and also BamHI restriction enzyme recognition site for cloning to peT45-b. We added RFC10 suffix site on 5’ end of the same gene sequence and also XhoI restriction enzyme recognition site for cloning to peT-45 vector, again.

As shown above,we planned to clone the ordered TnrA-pAlst-RFP gene into peT45-b vector by using BamHI and XhoI enzymes. Final construct after this cloning is, T7 promoter-Lac operator(LacO)-HisTag-TnrA-pAlst-RFP, respectively. Besides, a constitutive promoter called LacI promoter and LacI protein sequence in front of that, found on peT45-b vector’s another part. It is obvious that this part is IPTG-dependent, so Western Blot can be performed easily with the help of His Tag.

According to this system, under the absence of IPTG; TnrA production will be repressed, pAlsT promoter will be derepressed and RFP won’t be produced. If IPTG is present, TnrA will be produced , pAlsT promoter becomes derepressed and red colored bacteria will be observed with production of RFP. After showing stability of TnrA-pAlst sytem by using the RFP fluorescence protein, Toehold-TEV protease will be replaced with RFP for binding to AND gate system.

QS dependent promoter pLsr

There are two promoters on LsrR’s operon Lsr . these promoters are called LsrA and LsrR, and they are repressed in the absence of AI-2. The location LsrR binds on these promoters(p-lsr-Box) are shown below. Dark ones indicate the common sequences in both promoters. We preferred to use lsR promoter as it is one of ATOMS Team’s parts in 2013.

FIGURE 5:LsrR-binding site recognition and regulatory characteristics in Escherichia Coli AI-2 quorum sensing (Ting Xue, Liping Zhao, Haipeng Sun, Xianxuan Zhou and Baolin Sun).

We aimed to show repression of LsrR protein on pLsr promoter and dereppession of it in the presence of AI-2. For this purpose, we gathered LsrR protein gene sequence and pLsr sequence on the same biobrick. We put RFP as a reporter in front of pLsr promoter. To produce th repressor protein Lsr in a high amount, we put LsrR-pLsr-RFP gene sequence in front of J23100 constutive promoter . We added RFC prefix on 3’end , RFC suffix on 5’ end of LsrR-pLsr-RFP gene sequence.

LsrABCD operon, which makes AI-2 getting into the cell, already present in E.coli; so it is expected to be enough when an AI-2 sensing promoter system placed into E. coli. Thereby under the absence of AI-2, Lsr promoter will be heavily repressed by LsrR protein. If Quorum Sensing molecule sensed successfully AI-2 will be phosphorylated and LsrR’s suppression on pLsr will disappear. Thus RFP expression will occur.

We chose to use the part J23100-LsrR-pLsR-RFP(BBa_K1202108) as 2013 ATOMS IGEM TEAM designed. After showing LsrR-pLsrR system’s stability by using RFP, Trigger RNA will be replaced with RFP to connect the inputs to the And gate system.

Trigger RNA-Toehold-GFP System

We aimed to show Toehold switch system’s incapability of protein expression when it is alone, which means the Trigger RNA and Toehold Switch must coexist for protein expression. To observe Toehold swtich’s and and Toehold Swtich-Trigger RNA’s coexisting results both, we designed Toehold switch and trigger RNA in different biobricks. Because of origin incompatibility process, we had to clone these two different gene sequences into different plasmids. Thus we cloned Toehold-GFP into ColA originated PColA plasmid, and Trigger RNA into ColE originated PSB1C3 plasmid.

The ordered form of Toehold G-blocks is shown above. We preferred to use T7 promoter, which is a very strong promoter in this gene’s design. Thus there won’t be any difficulty in Toehold-GFP RNA’s production. The RBS of GFP presented in Toehold structure. To clone Toehold-GFP sequence into PSB2C3 and pColA plasmids both, we added RFC 10 suffix region on 3’ end and RFC 10 prefix region on 5’ end of Toehold-GFP. We also put BamHI restriction sitebetween Toehold and GFP. After GFP expression, which shows that Toehold-trigger system works, any protein could be replaced with GFP. In our project, GFP will be replaced with TEV protease.

Trigger RNA, which turns on Toehold switch system, is shown above in its ordered form as G-Blocks. In the design of this biobrick, we used T7 promoter, which has a strong mRNA production rate. By doing these, an enough amount of Trigger RNA will be produced to open Toeholds. There is no RBS in this product, because Trigger RNA doesn’t codes a protein. Its only task is opening Toehold switch in order to produce protein. To clone Trigger RNA sequence into PSB1C3 plasmid, we added RFC10 prefix on 3’ end and RFC10 suffix on 5’ end.

Figure: Toehold switch and Trigger RNA deatiled design

NH3 Sensitive Promoter and TnrA

PSB1C3-TnrA-pAlst-RFP CLONING

We cloned IDT G-Blocks GadE gene into PSB1C3 vector in order to make it ready to be submitted and have many copies of it. For this purpose we digested PSB1C3 vector and TnrA-pAlst-RFP G-Blocks with ECoRI and PstI restriction enzymes. Then we ligated these cut genes into the plasmid by using T4 DNA Ligase . Ocurring products were transformed into BL21 competent cell strain.

To check if the cloning is correct, a colony PCR was perfomed with Verify Forward and Verify Reverse primers. If the cloning isn’t made properly t the band should be 314 bp long, but if colony PCR worked, then bands should be 1800 bp long.

As the result of Colony PCR experiments, we observed bands are either negative or less molecule-weighted than we expected. We made liquid cultures of the not negative colonies, and isolated DNA from these colonies after incubating for 16 hours. we did cut-check with EcoRI and PstI enzymes in order to control occurring DNA’s.

After cut-check, we observed less molecule-weighted bands again. Therefore we decided to control our ordered G-Blocks and did a PCR experiment with CMV forward and SV40 reverse primers. The gel image of this PCR is shown below.

TnrA-pTnrA-RFP PCR

After that PCR, we observed less molecule-weighted bands than normal.

pET45 -TnrA-pTnrA-RFP CLONNING

We questioned if the plasmid is incorrect because the results of PSB1C3 cloning weren’t matching with our expected results. We cut the G-Block with BamHI and XhoI and ligated it with pET45-b which was cut with same enzymes. We transformed this ligated product into BL21 bacteria strain, which has T7 RNA polymerase.

In order to control if the cloning is made correctly, we did a colony PCR with T7 Promoter reverse and T7 promoter forward. If cloning isn’t made properly, the band should be at 360 bp line and if is made properly the band should be at 1779 bp line.

In colony PCR results, we observed lower molecule-weighted bands than expected, again. In this case we realized that this gene sequence was wrong.

We didn’t have enough time to order and clone this gene so we didn’t continue to do this part’s experiments.

AI-2Sensitive Promoter and LsrR

We got the results of Lsr promoter part from 2013 ATOMS iGEM team. Their results are shown below.

Inducible promoter experiment

To observe inducible promoters response, we co incubated two different bacteria. The first bacteria culture is expressing enzyme system and the second culture is including inducible promoter. At the experiment, we incubated them seperately for 16 hours and mixed them into one flask and 4 hour later, we add 0,1 mM SAH (with 10x PBS containing %1 BSA). Incubate with SAH for one day and, took 2 ml of liquid culture to santrifuge tube.Centrifuged it. We saw the red color at the pellet as you see below.

So, it means the enzyme system is working and inducible promoter is succesfully induced from AI-2.

Toehold-Trigger RNA-GFP

PSB1C3-Toehold-GFP/Trigger RNA CLONING

We cloned these two IDT G-Block genes into PSB1C3 vector in order to make it ready to be submitted and have many copies of it. For this purpose we digested PSB1C3 vector and TnrA-pAlst-RFP G-Blocks with ECoRI and PstI restriction enzymes. Then we ligated these cut genes into the plasmid by using T4 DNA Ligase . Ocurring products were transformed into BL21 competent cell strain.

To check if the cloning is correct, a colony PCR was perfomed with Verify Forward and Verify Reverse primers. If the cloning isn’t made properly t the band should be 314 bp long, but if colony PCR worked, Toehold-GFP’s band should be at 1294 bp line and Trigger RNA’s should be at 443.

As the result of colony PCR, the possible right cloned colonies were incubated in liquid culture for 16 hours. After this incubation, we isolated plasmid DNA from this bacteria culture by miniprep plasmid isolation method. We controlled obtained colonies with cut-check as a second control of cloning. We used EcorI and PstI restriction enzymes for cut-check.

RESULT FOR TOEHOLD-GFP

RESULT FOR TRIGGER RNA

In order to make And gate work, Toehold-GFP and Trigger RNA must be transformed into the same bacteria. Origin incompatibility prevents us to transform two different originated plasmids in the same bacteria. Therefore we decided to clone Toehold-GFP into a ColA originated plasmid and clone Trigger RNA into a ColE originated plasmid. PSB1C3 plasmid has a ColE origin so we cloned Trigger RNA into it. We designed this ColA originated plasmid for cloning Toehold-GFP sequence and named it ‘pColA’.

pColA-Toehold GFP CLONING

After cloning Toehold-GFP into PSB1C3 vector successfully, as we are planning to transform this gene into the same bacteria with Trigger RNA, we cloned it into pColA plasmid. In order to do cloning into this vector, we removed the gene from PSB1C3-Toehold GFP plasmid by cutting it with NotI enzyme. Then we ligated these cut genes into the plasmid by using T4 DNA Ligase . Ocurring products were transformed into BL21 competent cell strain.

To check if the cloning is correct, a colony PCR was perfomed with ColA Forward and ColA Reverse primers. If the cloning isn’t made properly t the band should be 192 bp long, but if colony PCR worked, Toehold-GFP’s band should be at 1196 bp line.

As the result of colony PCR, the possible right cloned colonies were incubated in liquid culture for 16 hours. After this incubation, we isolated plasmid DNA from this bacteria culture by miniprep plasmid isolation method. We controlled obtained colonies with cut-check as a second control of cloning. We used NotI restriction enzyme for cut-check.

PSB1C3-Trigger RNA/pColA-Toehold-GFP Cotransformation:

To show And Gate system works properly, these two plasmids with different origins should be transformed into the same bacteria. T7 is the promoter which produces Trigger RNA and Toehold-GFP mRNA’s , so we assured that they were cotransformed into a bacteria strain including T7 RNA polymerase. BL21 served this purpose, and after cotransformation, we observed grown colonies.

Functional Assay:

We designed a functional assay setup in order to figure out if Toehold-Trigger RNA system is functional. The main goal of this setup is to show that; Toehold-GFP doesn’t give fluorecence alone but if it comes together with Trigger RNA, GFP fluorescences. GFP production is also IPTG-dependent.

For the purposes given above, we made liquid culture of two different bacteria together; bacteria including only pColA-Toehold-GFP plasmid and bacteria including pCola-Toehold-GFP and PSB1C3-Trigger RNA. We incubated these bacteria in liquid culture for 13 hours at 37C and added IPTG into their mediums at 13. hour. After adding IPTG, we incubated them for more 3 hours at 37C. At the end of three hours, we firstly measured GFP fluorescence of the grown cultures by using VarioScan device. The results of measurements are given above. They were made twice.

When the results are analyzed, it is obvious that Toehold-Trigger RNA parts gave very high amounts of flourescence together while Toehold-GFP part gave flourescence in a very low amount. There is almost 15 times difference between these two fluoroscence amounts. This proves that Toehold-Trigger system works successfully. Also it is shown that systems work IPTG-dependently.

The graphs of measurement results are given below. The difference between two systems can be observed clearly.

Figure : GFP flourescent measurrement in LB mediums.

We also observed the liquid cultures under the fluorescence microscope.

Figure 2: Flourescence microscope image of GFP producing E. coli.

For better results, we isolated protein and we fluorimetrically measured them. Firstly we centrifuged the liquid cultures which were incubated for 16 hours. We took pictures of tubes after centrifugation, they are shown belown.

Figure : Pellets can be seen after 16 hours of liquid culter precipitated.

We applied Standard protein isolation protocol after this centrifuge and managed to isolate protein from the occured pellets. We made GFP fluorescence measurement with VarioScan from those isolated proteins. The results of measurements are shown below.

The measurement results of isolated proteins indicate that Toehold-Trigger system works very efficiently. GFP fluorescence amount of Toehold-trigger RNA including bacteria is about 175 times more than only Toehold including bacteria’s. also the leak of this system is almost negligible. In the absence of Trigger RNA, Toehold’s GFP fluorescence is almost zero. This indicates that our system works very efficient and in a very specific way.

Figure : Protein extract GFP florasans measurement

Pexiganan

According to our researches, a very efficient protein called pexiganan, a molecule showing a broad spectrum of potent antimicrobial activities against both gram negative and positive bacteria, seemed beneficial for killing H. Pylori.(Figure 1) Antimicrobial peptides (AMP) are very popular because of their bactericidal activity and they seem potential alternatives to current antibiotics. Also, antimicrobial peptides are not affected by classical antibiotic mechanisms of antibiotic resistance, so this class of peptide have advantages to eradicate H.pylori instead of using current antibiotics. The other advantage of AMPs is that there aren’t any resistance to them-yet. This was shown in a study too. (Figure 2)

In a paper, pexiganan’s killer activity is proved under both in vitro and in vivo conditions. (Xiao-Lin Zhang et al. 2015) It has exhibited a broad-spectrum antibacterial activity in vitro, and it has been tested against 3109 clinical isolate strains of Gram-negative and Gram-positive, aerobic and anaerobic bacteria. (Ge, Y; MacDonald, D,L et al. 1999). By using normal H.Pylori treatment way, complete eradication is not possible because of the low antibiotic concentration in gastric mucosa. In addition, in the low pH of the gastric fluid, antibiotics are unstable. As a result of gastric emptying, the residence time is short for antibiotics in the stomach. Therefore, our strategy depends on providing production of pexiganan enter the mucosa according to presence of H.pylori or not. This system is based on the penetration of our engineered E.coli under the mucosa, and production of pexiganan under the control of the AND GATE system. After the production of pexiganan under the mucose, if this peptide is toxic for mammalian cells, this cannot be used for H.pylori eradication in the gastric mucosa. Therefore, toxicity level of pexiganan for mammalian cells must be higher than the requirement of H.pylori eradication. The potential toxicity of pexiganan has been investigated systematically by measuring the peptide’s hemolytic activity in human red blood cells in other studies. The reports suggested that at least 250 μg/mL is necessary to induce 100% hemolysis. (Navon, V; Feder, R et al. 2002 and Eren,T; Som, A et al. 2008) Two phase III clinical trials have reported that no adverse side effects have been found for pexiganan.
(The Synthetic Antimicrobial Peptide Pexiganan and ItsNanoparticles (PNPs) Exhibit the Anti-Helicobacter pylori Activity in Vitro and in Vivo)

DAMP

(A Simple and Low-Cost Platform Technology forProducing Pexiganan Antimicrobial Peptide in E. Coli,Chun-Xia Zhao, Mirjana Dimitrijev Dwyer, Alice Lei Yu, Yang Wu, Sheng Fang, Anton P.J. Middelberg)

DAMP, a four-helix bundle protein connected to Pexiganan, used to ensure pexiganan’s intracellular antimicrobial activity was prevented successfully. A design, as showed above, was used to attach DAMP to Pexiganan with a cleavage site. That cleavage site makes it possible to release Pexiganan in an exact concentration. In addition, DAMP provides high levels of solubles in recombinant bacteria. It also forms a four helix bundle structure that has thermo stability and remains soluble at high salt levels. Finally, pexiganan embeds into DAMP and this provides limitted electrostatic of pex. It prevents damage to the cell membrane in the E. coli.

TEV Protease

As a protease needed to cut the cleavage site between DAMP and Pexiganan, TEV protease is chosen to serve this purpose. TEV protease is the common name for the 27 kDa catalytic domain of the Nuclear Inclusion a (NIa) protein encoded by the tobacco etch virus (TEV). Because its sequence specificity, TEV protease is a very useful reagent for cleaving fusion proteins. It is also relatively easy to overproduce and purify large quantities of the enzyme. (Macromollecular Crystallography Laboratory, Protein Engineering Section, David Waugh)

The project's main goal on this part is producing the inactive form of the pexiganan which have antimicrobial effects; DAMP-Pexiganan and producing TEV Protease which will activate DAMP-Pexiganan. For producing this proteins abundantly we use T7 promoter ,which has extremely strong transcription rate, while we designing our parts. We also decided to have Lac Operator site (that LacI protein can bind) between our gene sequences and T7 promoters to make protein expressions controllable. We researched for the expression vector that satisfy these requirements, and we found we could use the pet45-b expression vector provides the conditions we want. While we genes to order we added RFC10 prefix domain to the 3 'end of DAMP-Pexiganan and TEV Protease and we also added BamHI restriction enzyme recognition sequence for clonning inside to Pet45-b vector. We added RFC10 Suffix domain to the 5’ end of the same gene sequences, same way we added XhoI restriction enzyme recognition sequence for cloning inside to Pet45-b plasmid. In line with our ultimate goal we aim producing of these two proteins in the same bacteria. To make this happen we need to ligate these two gene sequences with two plasmids these have different types of origin(Origin incompatibility). Therefore, we have designed Damp PEX gene sequence in this manner so that at the same time we can ligate it with pColA vector. pColA plasmit do not include promoter in itself beceuse of that we added T7 promoter to 5' end of DAMP-Pexiganan gene sequence.

As stated above, we planned clonning ordered DAMP-Pexiganan and TEV Protease genes in Pet45-b vector with BamHI and XhoI restriction enzymes. When this clonning performed; T7 promoter-Lac operator (LacO)- HisTag- DAMP-pexiganan/TEV protease construction will ocur in order. In addition LacI promoter ,which is a constutive promoter in an other region, and also LacI protein sequence in front of this. In view of the above information DAMP-pexigan and TEV protease protein's production dependent IPTG and with help of His-tag it easily executed via Western blotting.

In addition to this if DAMP-Pexiganan gene sequence insert into pColA vector with NotI enzyme succesfully below stated construction will occur.

PSB1C3-DAMP-PEXIGANAN/TEV PROTEASE CLONNING

We thought to ,ligate our gene sequence whichs ordered from IDT with the g-BLOCKS form, PSB1C3 firstly to clonning and submittions. Therefore we digested both PSB1C3 vector and Damp-Pexigan and TEV protease-G-blocks with EcoRI and PstI restriction enzymes. Then we aimed to insert these cuted g-BLOCKS into plasmid with using T4 DNA Ligase. Following ligation, the resulting plasmids were transformed into BL21 competent bacteria.

We did colony PCR in order to check the accuracy of cloning with Veritification Forward and Veritification Reverse Primers. If the clonning resulted negative expecting band would be 314 bp. On the other hand if we succesfully clonned these parts, for DAMP-Pex. Expected band would be 1006 bp, for TEV Protease it would be 1062 bp.

After colony PCR consequences we have put the positive resulted clonnings 16 hours liquid culture after that we isolated plasmid DNA with miniprep plasmid izolation method. We make cutcheck to our attained plasmid DNAs for put a second control step. Our restriction enzymes those we used are EcoRI and PstI.

pET45- DAMP-PEXIGANAN/TEV PROTEASE CLONNING

We planned; clonning our genes ,whichs clonned succesfully to PSB1C3 vector, into pET45-b expression vector. For producing abundantly protein. To allow for cloning this vector we withdraw our genes from PSB1C3- DAMP-Pexigan and PSB1C3-TEV protease gene plasmids with using BamHI and XhoI digestion enzymes. We did ligation within using pET45-b vector that digested with the same enzymes. Following ligation, the resulting plasmids were transformed into BL21 competent bacteria which have T7 RNA Polymerase that we know.

We did colony PCR in order to check the accuracy of cloning with using T7 promoter forward and T7 terminator reverse primers. If the clonning resulted negative expecting band would be 360 bp. On the other hand if we succesfully clonned these parts, for DAMP-Pex. Expected band would be 699 bp, for TEV Protease it would be 1041 bp.

After colony PCR consequences we have put the positive resulted clonnings 16 hours liquid culture after that we isolated plasmid DNA with miniprep plasmid izolation method. We make cutcheck to our attained plasmid DNAs for put a second control step. Our restriction enzymes those we used are BamHI and XhoI.

WESTERN BLOTTING

After we clonned to pET45-b succesfully we showed our aim proteins production via western blotting with using His-tag which lacate in N-terminal of these proteins.

RESULT FOR DAMP-Pexiganan

RESULT FOR TEV Protease

PColA- DAMP-PEXIGANAN CLONNIG:

We demonstrated that DAMP-Pexiganan and TEV Protease proteins synthesing succesfully within clonning to pET45-b plasmid. We thought that we should insert both two genes(DAMP-Pexiganan and TEV Protease) at the same time to same bacteria to show TEV Protease breaking linker chain (to releasing active free pexiganan) that is between DAMP and Pexiganan. We have seen with the same origin in two plasmids can not be found in a bacterium simultaneously due to origin incompatibility process. For this reason, we decided to clonning one of these two gene sequences into pet45-b plasmid which have ColE origin and one of the gene sequence clonning into pColA plasmid which have ColA origin which also we designed it.

Before that we achieved to clonning both of two gene sequences into pET45-b vector. Therefore, clonning only one of these genes would be enough for us. We decided to locate TEV Protease gene sequence into pET45-b because our essential want to control protein is TEV Protease. And we decided clonning DAMP-Pexiganan gene sequence into pColA vector. For clonning DAMP-Pexiganan protein sequence into pColA vector we toke out our gene with NotI enzyme from PSB1C3-DAMP-Pexiganan plasmid. We did ligation with pET45-b vector which digested the same enzyme. Following ligation, the resulting plasmids were transformed into BL21 competent bacteria.

We did colony PCR in order to check the accuracy of cloning with using pColA forward and pColA reverse primers. If the clonning resulted negative expecting band would be 192 bp. On the other hand if we succesfully clonned these part, expected band would be 908 bp.

After colony PCR consequences we have put the positive resulted clonnings 16 hours liquid culture after that we isolated plasmid DNA with miniprep plasmid izolation method. We make cutcheck to our attained plasmid DNAs for put a second control step. Our restriction enzymes those we used are XbaI and SpeI.

pColA- DAMP-PEXIGANAN/pET45-TEV PROTEASE COTRANSFORMATION

After we clonning DAMP-Pexiganan gene sequence into pColA plasmid and TEV Protease gene sequence into pET45-b for transformate these both two plasmids into same BL21 bacteria we did cotransformation. After cotransformation process we put bacterias at 37C for 16 hours incubation. End of 16 hours as a result we did not see any bacteria colony over agar plate.

We retried several times this cotransformation process but with these tryings we havent seen any bacteria colony on our agar plates.

TEV protease Activity Control:

After the negative results obtained from cotransformation experiements we designed a new experimental apparatus to demonstrate TEV Protease's breaking or separator effect to DAMP-Pexiganan molecules linker site. We firstly make broth culture secondly put incubation at 37C for 13 hours bacterias which contain pET45-DAMP-Pexiganan and pET45-TEV Protease plasmids. For inducing protein production we added 1mM IPTG into medium at 13rd hour. Next we left these incubation for 3 hours at 37C. We isolated protein from totally 16 hours incubated broth culture. We prepared a suitable buffer to create the conditions necessary to show the TEV Protease’s enzymatic activity.(Conditions are given below). Then we prepare our DAMP-Pex, and TEV protease isolated proteins by mixing in the buffer, we put the resulting mixture overnight incubation at 20° C. After incubation, to observe the fate of DAMP-pexigan proteins we did Western Blot. But in western blotting, we could not get any significant rational result.