Team:SDU-Denmark/Project

From 2009.igem.org

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(Methods)
(Results)
 
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'''Forslag til opbygning:'''
+
=Concept=
-
1. Concept
+
===Bacto-Bandage===
-
2. Metode and results
+
[[Image:SDU-Denmark-real-bandage.jpg|300px|thumb|right|Different kinds of plastic adhesive drapes are already in use today.]]
 +
The main goal of our project was to assemble biobricks in to a plasmid and in this way make ''E. coli'' produce and excrete the quorum-quenching protein ''RIP''.
-
3. Summary of results
+
We propose making a bandage that contains our engineered bacteria behind a semipermeable membrane, allowing only small peptides such as ''RIP'' to pass through, into the wound.
-
4. Implications and development
+
We have [https://2009.igem.org/Team:SDU-Denmark/Background#Quorum-quenching_using_RIP reason to hope] that this will weaken the biofilm formation, thereby making multiresistant bacteria easier to treat with conventional antibiotics. This should also increase the effectiveness of the antibiotics and thereby decrease the amount and range of antibiotics that are needed today, to fight the infections.
 +
Since our system doesn't kill ''S. aureus'' but only prevents it from becoming pathogenic, it is less likely to promote the development of resistant strains.
 +
===Parts===
 +
[[Image:SDU-Denmark-RIP4PART.jpg|300px|thumb|right|Our biological machine, composed of a [http://partsregistry.org/wiki/index.php?title=Part:BBa_J13002 promoter and RBS], our novel ''[http://partsregistry.org/Part:BBa_K237002 RIP]'' part and a [http://partsregistry.org/wiki/index.php?title=Part:BBa_B0015 double terminator].]]
-
=Concept=
+
Our idea is to compose a plasmid containing a promoter, which should either be constitutive or inducible. After the promoter sequence we have a RBS, and then our ''RIP'' sequence, which we based on the amino acid sequence of the protein and made in PCR via two flanking primers. We are working with a clean ''RIP'' sequence and a ''RIP'' sequence with an export sequence on it, called ''sRIP''. Following the ''RIP'' sequence we have a terminator.
-
The concept of our project is to assemble biobricks in to a plasmid and in this way get ''E. Coli'' to produce and excrete the quorum quenching protein RIP.
+
All the four parts were incorporated into an ampicillin resistant plasmid backbone.
-
To do this we compose a plasmid containing a promoter, which should either be constitutive or inducible. After the promoter sequence we have a RBS, and then our RIP sequence, which we composted from the amino acid sequence of the protein and made in PCR via two costumed primers. We are working with a clean RIP sequence and a RIP sequence with an export sequence on. After the RIP sequence we have a terminator. It all has to be incorporated into an ampicillin resistant plasmid backbone.
+
We designed our system with two different promotors, since we didn't know whether a high concentration of ''RIP'' will quorum quench the ''E. coli'' itself. It will therefore be practical for us to control the rate of transcription - hence the inducible promoter.
-
We are trying with the two different promotors, because we don’t know whether a high concentration of RIP will quorum quench the E. Coli it self and it will there for be practical for us to control the rate of transcription. On the other hand we know that a higher concentration of RIP is more efficient at quorum quenching S. Aureus, and it will therefore be more efficient if the plasmid is transcribed at all times. Furthermore if the export of the protein out of the cell is weak, an overproduction of the protein might puncture the cell so RIP will leak out. This will of course kill the cell, but they could be replaced.
+
On the other hand we know that a higher concentration of ''RIP'' is more efficient in quorum-quenching ''S. aureus'', and it will therefore be more efficient if the plasmid is transcribed at all times. Furthermore if the export of the protein out of the cell is weak, an overproduction of the protein might puncture the cell and ''RIP'' will leak out. This will of course kill the cells, but we don't see this as a big problem as they easily can be replaced. Our goal is to get as much ''RIP'' exported from the bandage to the wound one way or another.
=Methods=
=Methods=
-
As seen in the flow chart, the parts RIP and sRIP are the first to be produce and ligated into backbone. Afterwards RIP and sRIP is ligated with a terminator resulting in a  two brick. We are using a constitutive promoter that is already assembled with a terminator [http://partsregistry.org/wiki/index.php?title=Part:BBa_J13002 BBa_J13002] and a inducible promoter [http://partsregistry.org/wiki/index.php?title=Part:BBa_R0011 BBa_R0011] that we assemble with a RBS binding site [http://partsregistry.org/wiki/index.php?title=Part:BBa_B0034 BBa_B0034]
 
-
Finally the 4-bricks is constructed.
 
 +
[[Image:SDU-Denmark-flowchart.jpg|350px|thumb|right|Flowchart detailing our project.]]
-
The steps was as following:
+
==Finding parts==
-
'''Interting parts into backbone:'''
+
We used the [http://partsregistry.org Registry of Standard Biological Parts] (Parts Registry in short) to find a suitable [http://partsregistry.org/Part:pSB1A2 backbone], [http://partsregistry.org/wiki/index.php?title=Part:BBa_J13002 promoter, RBS] and [http://partsregistry.org/Part:BBa_B0015 terminators]. All the parts where checked for compatibility with the standard BioBrick assembly method ([http://partsregistry.org/Assembly:Standard_assembly RFC 10]).
-
1. amplification by PCR using VF2G01010 and a modified VR2 primer. ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_Primer_PCR See protocol])
+
-
To skip a bacerial growth step, and thereby save some time, our parts where amplified by PCR, as suggested by the ginkogobioworks assembly manual [http://ginkgobioworks.com/support/BioBrick_Assembly_Manual.pdf assembly manual]
+
We also wanted to test our system with an [http://partsregistry.org/wiki/index.php?title=Part:BBa_R0011 inducible promoter], but sadly never had the time.
-
+
-
2. Digesting with fast digest restriction enzymes EcoRI-HF™ and PstI ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Restriction_digest_-_Protocol_2 See protocol])
+
-
We experienced that digesting with slow digest buffers was ineffective and slow, why we replaced these with fast digest enzymes.
+
==Ligations==
-
3. Ligate with T4 DNA Ligase ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Ligation_-_Protocol_1 See protocol])
+
We ligated our parts together using a slightly different [https://2009.igem.org/Team:SDU-Denmark/Protocols#Ligation_-_Protocol_3 protocol] then suggested in the [http://partsregistry.org/Help:BioBrick_Assembly Parts Registry help pages], before inserting them into our backbone:
-
4. Transformation into competent E.coli ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Electroporation See protocol])
+
1. Amplification by PCR using [http://partsregistry.org/Part:BBa_G00100 VF2] and our modified [http://partsregistry.org/Part:BBa_K237007 VR] primer ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_Primer_PCR Protocol]).
-
4. Testing length by colony-PCR ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_colony_PCR See protocol])
+
2. Digest with fast digest restriction enzymes, upstream part with SpeI and downstream part with XbaI ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Restriction_digest_-_Protocol_2 Protocol]).
-
5. sequencing.
+
3. Ligate with T4 DNA Ligase, resulting in a mixed site ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Ligation_-_Protocol_1 Protocol]), of either 6 or 8 bp length.
-
'''Ligation of parts:'''
+
==Inserting parts in backbone==
-
1. amplification by PCR using VF2G01010 and a modified VR2 primer. ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_Primer_PCR See protocol])
+
The steps was as follows:
-
2. Digesting with fast digest restriction enzymes, upstream part with SpeI and downstream part with XbaI ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Restriction_digest_-_Protocol_2 See protocol])
+
To skip a bacerial growth step, and thereby save some time, our parts where amplified by PCR, as suggested in [http://ginkgobioworks.com/support/BioBrick_Assembly_Manual.pdf  Ginkgo Bioworks assembly manual].
-
3. Ligate with T4 DNA Ligase, resulting in a mixed site. ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Ligation_-_Protocol_1 See protocol])
+
1. Amplification the ligated products by PCR using [http://partsregistry.org/Part:BBa_G00100 VF2 primer] and our modified [http://partsregistry.org/Part:BBa_K237007 VR2 primer] ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_Primer_PCR Protocol]).
-
4. Interting parts into backbone
+
2. Digesting with fast digest restriction enzymes EcoRI-HF™ and PstI ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Restriction_digest_-_Protocol_2 Protocol]).
-
'''Test of quorum quenching mechanism'''
+
We used fast digest enzymes, since normal enzymes where either slow or ineffective in cutting our bricks.
-
To test if our 4-brick inserted into E.coli it functioning and RIP is secreted out of the cell, we are designing a quorum quenching test system.  
+
3. Ligated with T4 DNA Ligase ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Ligation_-_Protocol_1 Protocol]).
-
The system is being made on a 4*6-well plade. Different ''S.aureus'' strains is growing in the wells making biofilms. Inhibition of biofilm formation is tested with different ''E.coli'' components added to the different wells: supernatant, crushed pellet and living'' E.coli''. After one day of growing the wells are washed three times with sterile 1xPBS to remove planktonic bacteria. Cells remaining adhered to the wells are subsequently stained with violet blue, the solution stands for 15 minutes and is again washed twice. A mixture of ethyl alcohol and acetone is added to each stained well to losen the biofilm, the biofilm is tested by measuring the absorbance by transfering the crystal violet/ethanol solution from each well to a cuvette, and measure the optical density (OD) of each of these samples at a wavelength of 595 nm.
+
 
 +
4. Transformation into competent ''E.coli'' ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Electroporation Protocol]).
 +
 
 +
==Testing==
 +
 
 +
[[Image:SDU-Denmark-flowchart03.jpg|250px|thumb|right|Flowchart concerning our testing phase.]]
 +
 
 +
To test if our 4 part brick was actually inserted into ''E.coli'' and functional, we prepared three different test systems: gene transcription by measuring ''RIP'' mRNA expression (Northern Blot), MALDI to measure protein expression and a actual test of quorum-quenching. 
 +
 
 +
===Colony PCR===
 +
 
 +
[[Image:SDU-Denmark-rip-pcr-produkt.jpg|50px|thumb|right|Gel picture of Colony PCR.]]
 +
 
 +
We started by checking our part lengths by colony PCR ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_colony_PCR Protocol]).
 +
 
 +
===Sequencing===
 +
 
 +
We sent our parts to sequencing to be sure that we had exactly the right DNA in our bacteria. We used the Plasmid editor [[Team:SDU-Denmark/Tools|APE]], to see our sequencing data.
 +
 
 +
===RNA expression===
 +
 
 +
To measure if RNA was being expressed, we used northern blotting ([https://2009.igem.org/Team:SDU-Denmark/Protocols#Protocol_for_Northern_Blotting Protocol]). We used a radioactive probe (32P) that binds to ''RIP'' mRNA and ran it through a membrane, to separate mRNA's into different sizes. The membrane was then put on a film, and scanned so we could visualize if there was any ''RIP'' mRNA in our cells.
 +
 
 +
===Biofilm assay===
 +
 
 +
[[Image:SDU-Denmark-cristal violet.jpg|200px|thumb|left|Biofilm assay.]]
 +
 
 +
To test whether or not our ''RIP'' part was being secreted out of our ''E. coli'' biomachine, we designed a biofilm assay.
 +
 
 +
The assay was made on a 4*6-well plate. ''S.aureus'' were grown in the wells, thereby making biofilms.  
 +
 
 +
We then added different ''E. coli'' components to the wells: supernatant, crushed pellet and living ''E. coli''. After 24 hours the wells were washed three times with sterile 1x PBS solution to remove planctonic bacteria. Cells remaining adhered to the wells are subsequently stained with violet blue, the solution stands for 15 minutes and was washed twice.
 +
 
 +
1 ml of 96% ethanol was added to each stained well to loosen the biofilm. The biofilm was tested by measuring the absorbance by transferring the crystal violet/ethanol solution from each well to a cuvette, and measure the optical density (OD) of each of these samples at a wavelength of 595 nm.
 +
 
 +
===MALDI===
 +
 
 +
Matrix-assisted laser desorption/ionization (MALDI) is a technique used in mass spectrometry, allowing the analysis of for example proteins.
 +
 
 +
We did a MALDI on the supernatant of our 4 part brick, to see whether or not ''RIP'' was being exported out of the bacteria.
=Results=
=Results=
 +
 +
[[Image:SDU-Denmark-4part-sequence.jpg|200px|thumb|right|Sequencing confirmed that we have the right DNA in our bacteria. The red parts are restriction-sites, green is the composite promoter and RBS, blue is ''RIP'' and orange is our double terminator.]]
 +
 +
===New parts and primers===
 +
 +
We have successfully constructed the ''RIP'' and ''sRIP''
 +
[[Team:SDU-Denmark/Parts|parts]], and used these with older parts, all of which have been added to the registry. We have also added a slightly modified VR primer to the registry.
 +
 +
===''RIP'' expression in ''E. coli''===
 +
 +
[[Image:SDU-Denmark-Nothern-Blot-RIP.jpg|200px|thumb|right|Northern blot of our 4 brick part (<partinfo>K237002</partinfo>) and our RIP-Terminator part (<partinfo>S04235</partinfo>). As seen here only the 4 brick part (left) is transcribed into mRNA and hopefully further translated into peptide.]]
 +
 +
We have successfully assembled a 4 brick part containing a constitutive promotor with RBS, our novel ''RIP'' part and a terminator.
 +
 +
Sequencing confirmed the 4 brick part DNA sequence and a northern blot analysis confirmed that our ''E. coli'' indeed transcribes the ''RIP'' gene. To our knowledge this is the first recombinant organism to harbour and transcribe the ''RIP'' gene.
 +
 +
[[Image:SDU-Denmark-MALDI.jpg|200px|thumb|right|Mass spectrometry of supernatant from our 4 part ''RIP'' colony (A and C) compared with a reference colony (B and D). No conclusive results could be gathered from this analysis.]]
 +
 +
We also did protein MALDI mass spectrometry, which didn't show anything conclusive, perhaps as a consequence of the ''RIP'' peptides small size, which makes it hard to distinguish from fragmentation peaks of larger proteins. Another possible explanation could be that our bacteria is not transporting ''RIP'' out of the cell.
 +
 +
===Quorum-quenching and biofilm inhibition===
 +
 +
We are currently testing the quorum-quenching effect on ''S. aureus'' biofilm formation and the results are promising. The big question is whether or not, ''RIP'' gets exported out of ''E. coli'' and past the peptideglycan layer and capsule. The final results will be presented at the Jamboree.
 +
 +
===Problems===
 +
 +
Throughout most of the summer, we've had problems getting our ligations product sizes to match. What ever we tried nothing seemed to work, since it was always the wrong size. Then a few weeks ago, it was discovered, that the [[Team:SDU-Denmark/Parts/backbone_troubles|problem]] was with our backbone (1K from plate 1, 2009 spring distribution), not our work. 1K was suppose to be <partinfo>pSB1A3</partinfo>, but instead it was <partinfo>pSB1A2</partinfo>.
 +
 +
Sadly we didn't discover this till the very last week, and so we didn't get to do all the experiments we wanted, including one with an inducible promoter and one with our signaling peptide coupled with ''RIP''.
 +
 +
<div style="clear:both;"></div>
 +
 +
=Implications=
 +
 +
If indeed our ''E. coli'' can inhibit biofilm formation by producing ''RIP'', this generates many different opportunities for further development.
 +
 +
Our machine opens up for the possibility to combat infections more intelligently.
 +
 +
As mentioned earlier we considered using a inducible promotor to control the expression of ''RIP''. Optimally the promotor should react to the level of autoinducers in the environment by use of quorum-signaling receptors.
 +
The concept could also be implicated on other strains of bacteria performing quorum sensing with other types of autoinducers.
 +
 +
A logical next step would be to couple several kinds of quorum-quenching molecules to our machine, together with different quorum-signaling receptors. This would allow for inhibition of only the specific bacteria that are currently infecting the wound.
 +
 +
Essentially the Bacto-Bandage would sense if any kind of bacteria was trying to colonize the wound and inhibit this by means of producing the most effective quorum-quenching molecules.
 +
 +
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<div id="rightcontent">
<div id="rightcontent">
 +
 +
==Our project in 1 minute==
 +
 +
[[Image:SDU-Denmark-Clock-Icon.gif|20px|right]]
 +
 +
We want to fight hospital infections, using a biological machine.
 +
 +
For this purpose we have constructed a recombinant ''E. coli'', which produces the ''RIP'' peptide. ''RIP'' inhibits biofilm formation in the bacteria ''S. aureus''.
 +
 +
This peptide will make it easier to fight infections and kill ''S. aureus'' with conventional antibiotics.
 +
 +
==Other stuff==
 +
 +
* Check out all our [[Team:SDU-Denmark/Protocols|protocols]].
 +
 +
* See what [[Team:SDU-Denmark/Tools|tools]] we used.
 +
 +
* Read our [[Team:SDU-Denmark/Safety|safety]] page.
 +
 +
==Content==
__TOC__
__TOC__

Latest revision as of 00:14, 22 October 2009







Concept

Bacto-Bandage

Different kinds of plastic adhesive drapes are already in use today.

The main goal of our project was to assemble biobricks in to a plasmid and in this way make E. coli produce and excrete the quorum-quenching protein RIP.

We propose making a bandage that contains our engineered bacteria behind a semipermeable membrane, allowing only small peptides such as RIP to pass through, into the wound.

We have reason to hope that this will weaken the biofilm formation, thereby making multiresistant bacteria easier to treat with conventional antibiotics. This should also increase the effectiveness of the antibiotics and thereby decrease the amount and range of antibiotics that are needed today, to fight the infections.

Since our system doesn't kill S. aureus but only prevents it from becoming pathogenic, it is less likely to promote the development of resistant strains.

Parts

Our biological machine, composed of a [http://partsregistry.org/wiki/index.php?title=Part:BBa_J13002 promoter and RBS], our novel [http://partsregistry.org/Part:BBa_K237002 RIP] part and a [http://partsregistry.org/wiki/index.php?title=Part:BBa_B0015 double terminator].

Our idea is to compose a plasmid containing a promoter, which should either be constitutive or inducible. After the promoter sequence we have a RBS, and then our RIP sequence, which we based on the amino acid sequence of the protein and made in PCR via two flanking primers. We are working with a clean RIP sequence and a RIP sequence with an export sequence on it, called sRIP. Following the RIP sequence we have a terminator.

All the four parts were incorporated into an ampicillin resistant plasmid backbone.

We designed our system with two different promotors, since we didn't know whether a high concentration of RIP will quorum quench the E. coli itself. It will therefore be practical for us to control the rate of transcription - hence the inducible promoter.

On the other hand we know that a higher concentration of RIP is more efficient in quorum-quenching S. aureus, and it will therefore be more efficient if the plasmid is transcribed at all times. Furthermore if the export of the protein out of the cell is weak, an overproduction of the protein might puncture the cell and RIP will leak out. This will of course kill the cells, but we don't see this as a big problem as they easily can be replaced. Our goal is to get as much RIP exported from the bandage to the wound one way or another.

Methods

Flowchart detailing our project.

Finding parts

We used the [http://partsregistry.org Registry of Standard Biological Parts] (Parts Registry in short) to find a suitable [http://partsregistry.org/Part:pSB1A2 backbone], [http://partsregistry.org/wiki/index.php?title=Part:BBa_J13002 promoter, RBS] and [http://partsregistry.org/Part:BBa_B0015 terminators]. All the parts where checked for compatibility with the standard BioBrick assembly method ([http://partsregistry.org/Assembly:Standard_assembly RFC 10]).

We also wanted to test our system with an [http://partsregistry.org/wiki/index.php?title=Part:BBa_R0011 inducible promoter], but sadly never had the time.

Ligations

We ligated our parts together using a slightly different protocol then suggested in the [http://partsregistry.org/Help:BioBrick_Assembly Parts Registry help pages], before inserting them into our backbone:

1. Amplification by PCR using [http://partsregistry.org/Part:BBa_G00100 VF2] and our modified [http://partsregistry.org/Part:BBa_K237007 VR] primer (Protocol).

2. Digest with fast digest restriction enzymes, upstream part with SpeI and downstream part with XbaI (Protocol).

3. Ligate with T4 DNA Ligase, resulting in a mixed site (Protocol), of either 6 or 8 bp length.

Inserting parts in backbone

The steps was as follows:

To skip a bacerial growth step, and thereby save some time, our parts where amplified by PCR, as suggested in [http://ginkgobioworks.com/support/BioBrick_Assembly_Manual.pdf Ginkgo Bioworks assembly manual].

1. Amplification the ligated products by PCR using [http://partsregistry.org/Part:BBa_G00100 VF2 primer] and our modified [http://partsregistry.org/Part:BBa_K237007 VR2 primer] (Protocol).

2. Digesting with fast digest restriction enzymes EcoRI-HF™ and PstI (Protocol).

We used fast digest enzymes, since normal enzymes where either slow or ineffective in cutting our bricks.

3. Ligated with T4 DNA Ligase (Protocol).

4. Transformation into competent E.coli (Protocol).

Testing

Flowchart concerning our testing phase.

To test if our 4 part brick was actually inserted into E.coli and functional, we prepared three different test systems: gene transcription by measuring RIP mRNA expression (Northern Blot), MALDI to measure protein expression and a actual test of quorum-quenching.

Colony PCR

Gel picture of Colony PCR.

We started by checking our part lengths by colony PCR (Protocol).

Sequencing

We sent our parts to sequencing to be sure that we had exactly the right DNA in our bacteria. We used the Plasmid editor APE, to see our sequencing data.

RNA expression

To measure if RNA was being expressed, we used northern blotting (Protocol). We used a radioactive probe (32P) that binds to RIP mRNA and ran it through a membrane, to separate mRNA's into different sizes. The membrane was then put on a film, and scanned so we could visualize if there was any RIP mRNA in our cells.

Biofilm assay

Biofilm assay.

To test whether or not our RIP part was being secreted out of our E. coli biomachine, we designed a biofilm assay.

The assay was made on a 4*6-well plate. S.aureus were grown in the wells, thereby making biofilms.

We then added different E. coli components to the wells: supernatant, crushed pellet and living E. coli. After 24 hours the wells were washed three times with sterile 1x PBS solution to remove planctonic bacteria. Cells remaining adhered to the wells are subsequently stained with violet blue, the solution stands for 15 minutes and was washed twice.

1 ml of 96% ethanol was added to each stained well to loosen the biofilm. The biofilm was tested by measuring the absorbance by transferring the crystal violet/ethanol solution from each well to a cuvette, and measure the optical density (OD) of each of these samples at a wavelength of 595 nm.

MALDI

Matrix-assisted laser desorption/ionization (MALDI) is a technique used in mass spectrometry, allowing the analysis of for example proteins.

We did a MALDI on the supernatant of our 4 part brick, to see whether or not RIP was being exported out of the bacteria.

Results

Sequencing confirmed that we have the right DNA in our bacteria. The red parts are restriction-sites, green is the composite promoter and RBS, blue is RIP and orange is our double terminator.

New parts and primers

We have successfully constructed the RIP and sRIP parts, and used these with older parts, all of which have been added to the registry. We have also added a slightly modified VR primer to the registry.

RIP expression in E. coli

Northern blot of our 4 brick part () and our RIP-Terminator part (). As seen here only the 4 brick part (left) is transcribed into mRNA and hopefully further translated into peptide.

We have successfully assembled a 4 brick part containing a constitutive promotor with RBS, our novel RIP part and a terminator.

Sequencing confirmed the 4 brick part DNA sequence and a northern blot analysis confirmed that our E. coli indeed transcribes the RIP gene. To our knowledge this is the first recombinant organism to harbour and transcribe the RIP gene.

Mass spectrometry of supernatant from our 4 part RIP colony (A and C) compared with a reference colony (B and D). No conclusive results could be gathered from this analysis.

We also did protein MALDI mass spectrometry, which didn't show anything conclusive, perhaps as a consequence of the RIP peptides small size, which makes it hard to distinguish from fragmentation peaks of larger proteins. Another possible explanation could be that our bacteria is not transporting RIP out of the cell.

Quorum-quenching and biofilm inhibition

We are currently testing the quorum-quenching effect on S. aureus biofilm formation and the results are promising. The big question is whether or not, RIP gets exported out of E. coli and past the peptideglycan layer and capsule. The final results will be presented at the Jamboree.

Problems

Throughout most of the summer, we've had problems getting our ligations product sizes to match. What ever we tried nothing seemed to work, since it was always the wrong size. Then a few weeks ago, it was discovered, that the problem was with our backbone (1K from plate 1, 2009 spring distribution), not our work. 1K was suppose to be , but instead it was .

Sadly we didn't discover this till the very last week, and so we didn't get to do all the experiments we wanted, including one with an inducible promoter and one with our signaling peptide coupled with RIP.

Implications

If indeed our E. coli can inhibit biofilm formation by producing RIP, this generates many different opportunities for further development.

Our machine opens up for the possibility to combat infections more intelligently.

As mentioned earlier we considered using a inducible promotor to control the expression of RIP. Optimally the promotor should react to the level of autoinducers in the environment by use of quorum-signaling receptors. The concept could also be implicated on other strains of bacteria performing quorum sensing with other types of autoinducers.

A logical next step would be to couple several kinds of quorum-quenching molecules to our machine, together with different quorum-signaling receptors. This would allow for inhibition of only the specific bacteria that are currently infecting the wound.

Essentially the Bacto-Bandage would sense if any kind of bacteria was trying to colonize the wound and inhibit this by means of producing the most effective quorum-quenching molecules.


Our project in 1 minute

SDU-Denmark-Clock-Icon.gif

We want to fight hospital infections, using a biological machine.

For this purpose we have constructed a recombinant E. coli, which produces the RIP peptide. RIP inhibits biofilm formation in the bacteria S. aureus.

This peptide will make it easier to fight infections and kill S. aureus with conventional antibiotics.

Other stuff

  • See what tools we used.

Content

Contents