Team:Newcastle/Metals

From 2009.igem.org

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__NOTOC__
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=Metal Sequester=
=Metal Sequester=
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In our system, the team have used the metallothionein SmtA (which usually mops up zinc ions) and have linked it to the CotC spore coat protein - this means that, should the stochastic switch decide, any cadmium mopped up could be sequestered into spores thereby making it unavailable. Please click on the following links to learn more:
 +
<br>
 +
*[[#Introduction|Introduction]]
 +
*[[#Novelty in this sub-project|Novelty in this sub-project]]
 +
*[[#BioBrick constructs|BioBrick constructs]]
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*[[#Lab Work Strategies|Lab Work Strategies]]
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*[[#Lab Work Done|Lab Work Done]]
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*[[#References|References]]
==Introduction==
==Introduction==
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In order to take up and keep the cadmium from the soil efficiently, we needed to think about a way to cross-link the metal ions to intra-cellular proteins which would end up for the most of it in the spore. If the heavy metal ions were not cross linked to a "sponge protein", it could be lethal to the cell at lower concentration and the cell could end up sporulating too early, or even bursting in the soil, releasing all the heavy metal it has taken up.
In order to take up and keep the cadmium from the soil efficiently, we needed to think about a way to cross-link the metal ions to intra-cellular proteins which would end up for the most of it in the spore. If the heavy metal ions were not cross linked to a "sponge protein", it could be lethal to the cell at lower concentration and the cell could end up sporulating too early, or even bursting in the soil, releasing all the heavy metal it has taken up.
<br>
<br>
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<br>
<br>
<br>
<br>
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It has been shown that in ''B.subtilis'', in order to express a specific protein in the spore coat, it is possible to make a fusion protein with a spore coat protein called ''CotC'', and a group have successfully expressed antigen proteins which are about the same size as our ''smtA'' metallothionein in order to make a vaccine[4]. By fusing CotC spore coat protein from ''Bacillus subtilis'', our ''smtA'' metallothionein can be localized to the spore coat, hence we can successfully trap most of the metals ions into the bacterial spores.  
+
It has been shown that in ''B. subtilis'', in order to express a specific protein in the spore coat, it is possible to make a fusion protein with a spore coat protein called ''CotC'', and a group have successfully expressed antigen proteins which are about the same size as our ''smtA'' metallothionein in order to make a vaccine[4]. By fusing CotC spore coat protein from ''Bacillus subtilis'', our ''smtA'' metallothionein can be localized to the spore coat, hence we hoped to successfully trap most of the metals ions into the bacterial spores.  
<br>
<br>
-
<br>It is also fused with GFP reporter gene in order to detect the expression of the fusion protein into the spores using a fluorescence microscopy.  
+
<br>CotC was also fused with GFP reporter gene in order to detect the expression of the fusion protein into the spores using a fluorescence microscopy.  
<br>
<br>
<br>
<br>
-
Because we want most of the metals to go into the spore rather than the vegetative cell, we designed our fusion protein so that it is controlled by the native ''CotC'' promoter sigK which is activated in sporulation conditions. Therefore, our ''smtA'' metal sequester will only be expressed once the cell have made the decision to become a metal container and sporulate, and it will only be expressed in the spore.
+
Because we want most of the metals to go into the spore rather than the vegetative cell, we designed our fusion protein so that it is controlled by the native ''cotC'' promoter sigK which is activated in sporulation conditions. Therefore, our ''smtA'' metal sequester would only be expressed once the cell have made the decision to become a metal container and sporulate, and only be expressed in the spore.
 +
<br>
 +
<br>
 +
Finally, our construct integrated the ''B. subtilis'' genome through homologous recombination at the native ''CotC'' gene. However, as we will be using pMutin4 integration vector, there will be two different copies of the ''cotC'' gene in our engineered ''B.subtilis'' genome: a native copy of ''cotC'' and our engineered ''CotC-GFP-smtA'' fusion copy. We chose not to knock-out the native ''CotC'' gene because the lack of native CotC might lead to defects in spore coat formation.
==BioBrick constructs==
==BioBrick constructs==
 +
[[Image:Newcastle SmtA-construct.png|center|500px]]
-
==Lab Work Strategies==
+
In the parts registry, BBa_K174008:
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<br>
+
-
===Construction===
+
-
<br>
+
 +
[[Image:Newcastle Metal sequester7.JPG|center|500px]]
 +
 +
==Lab Work Strategies==
 +
====a) Construction====
Synthesised by GeneArt, fragment:  1385 bp DNA
Synthesised by GeneArt, fragment:  1385 bp DNA
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[[Image:Newcastle Metal sequester21.JPG|center|500px]]
[[Image:Newcastle Metal sequester21.JPG|center|500px]]
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+
====b) Cloning and Integration====
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===Cloning and Integration===
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GeneArt cloned the vector into a standard biobrick vector. We sent them Plasmid pSB1AT3 with part BBa_J04450 (mCherry).
-
GeneArt will clone the vector into a standard biobrick vector. We will send them Plasmid pSB1AT3 with part BBa_J04450 (mCherry).
+
BBa_J04450 in pSB1AT3 Clone Manager plamid map:
BBa_J04450 in pSB1AT3 Clone Manager plamid map:
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[[Image:Newcastle Metal sequester3.JPG|center|500px]]
[[Image:Newcastle Metal sequester3.JPG|center|500px]]
-
Once we receive this fragment cloned in pSBAT3 we will amplify the part by PCR. Primer 1 will incorporate a HinDIII site and primer 2 will incorporate a BamHI. Checked that these enzymes don’t cut the fragment:
+
Once we received this fragment cloned in pSBAT3 we amplified the part by PCR. Primer 1 will incorporate a HinDIII site and primer 2 will incorporate a BamHI. Checked that these enzymes don’t cut the fragment:
[[Image:Newcastle Metal sequester4.JPG|center|500px]]
[[Image:Newcastle Metal sequester4.JPG|center|500px]]
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We then integrate into the 168 chromosome using homology between our cotC fusion and the native copy of cotC.
We then integrate into the 168 chromosome using homology between our cotC fusion and the native copy of cotC.
-
===Testing and Characterisation===
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====c) Testing and Characterisation====
Once transformed the spores of the mutant will need to be tested for fluorescence.
Once transformed the spores of the mutant will need to be tested for fluorescence.
Two obvious methods:
Two obvious methods:
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3) We would also test whether the strain is able to absorb cadmium in the spores when compared to the wild-type.
3) We would also test whether the strain is able to absorb cadmium in the spores when compared to the wild-type.
<br>
<br>
 +
 +
<br>
 +
==Lab Work Done==
==Lab Work Done==
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{| border="1"
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{| class=wikitable border="1"
|-
|-
! colspan="2" | Summary of Lab Sessions for Metal Sequestering
! colspan="2" | Summary of Lab Sessions for Metal Sequestering
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| <center>'''Description'''</center>           
| <center>'''Description'''</center>           
|-
|-
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| '''[https://2009.igem.org/Team:Newcastle/Labwork/4_August_2009#Sporulation_Tuning.2FChassis_Team 04/08/09]'''
+
| '''[https://2009.igem.org/Team:Newcastle/Labwork/9_September_2009#Metal_Sensor_Team 9th September 2009]'''
-
| Arrival of the non-germination spores. Preparation of the buffer solution required for the treatment of the spores
+
| Arrival of ''cotC-GFP-smtA'' BioBrick - transformed this into ''DH5-alpha E. coli'' cells
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/10_September_2009#Metal_Sensor_Team 10th September 2009]'''
 +
| Used colonies of ''cotC-GFP-smtA'' transformants to inoculate LB media in preparation for mini and midi-preps
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/11_September_2009#Metal_Sensor_Team 11th September 2009]'''
 +
| Mini and midi-prepped ''cotC'' BioBrick and PCR amplified ''cotC'' BioBrick, giving it restriction ends;
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/14_September_2009#Metal_Sensor_Team 14th September 2009]'''
 +
| Ligated ''cotC'' into ''pMUTIN4'' plasmid and attempted ''E. coli'' transformation
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/15_September_2009#Metal_Sensor_Team 15th September 2009]'''
 +
| Transformations seemed to have work; picked 12 colonies from 200ul plate and inoculated 12 tubes of 5ml LB + ampicillin
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/16_September_2009#Metal_Sensor_Team 16th September 2009]'''
 +
|Mini-preps of 12 picked colonies and restriction enzyme digest analysis - gel showed consistent bands so prepared midi-prep cultures
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/17_September_2009#Metal_Sensor_Team 17th September 2009]'''
 +
| Midi-prepped potential ''cotC-GFP-smtA'' transformant ''E. coli'' culture and digested with ''BamHI'' and ''HindIII''
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/21_September_2009#Metal_Sensor_Team 21st September 2009]'''
 +
|
 +
|-
 +
|'''[https://2009.igem.org/Team:Newcastle/Labwork/22_September_2009#Metal_Sensor_Team 22nd September 2009]'''
 +
|
 +
|-
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|'''[https://2009.igem.org/Team:Newcastle/Labwork/24_September_2009#Metal_Sensor_Team 24th September 2009]'''
 +
|
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/7_August_2009#Sporulation_Tuning.2F_Chassis_Team 07/08/09]'''
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|'''[https://2009.igem.org/Team:Newcastle/Labwork/18_September_2009#Metal_Sensor_Team 18th September 2009]'''
-
| Preparation of the lysozyme stock solution required for treatment of the spores
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|Analysed digested midi-prep sample through DNA gel electrophoresis - negative results
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/10_August_2009#Sporulation_Tuning.2F_Chassis_team 10/08/09]'''
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/28_September_2009 28th September 2009]'''
-
| Re-preparation of the buffer solution required for the treatment of the spores. Pouring of agar plates with the appropriate antibiotics.
+
|Picked 10 colonies of potential ''cotC'' in ''pMUTIN4'' ''E. coli'' transformants and inoculated 10 tubes of LB + amp with them
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/11_August_2009#Sporulation_Tuning.2F_Chassis_team 11/08/09]'''
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/29_September_2009 29th September 2009]'''
-
| Re-pouring the agar plates with the appropriate antibiotics
+
|Conducted mini-preps of 10 cultures of potential transformants and analysed them through restriction digests and gel electrophoresis - did not work
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/12_August_2009#Sporulation_Tuning.2FChassis_Team 12/08/09]'''
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|'''[https://2009.igem.org/Team:Newcastle/Labwork/1_October_2009#Ligations 1st October 2009]'''
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| Treatment of the non-germinating <i>cwlD</i> spores using Method A
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|Checked ''pMUTIN4'' and ''cotC'' on gel; carried out another ligation
-
|-
+
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/13_August_2009#Sporulation_Tuning.2FChassis_Team 13/08/09]'''
+
-
| Results for the treatment of the <i>cwlD</i> spores using Method A
+
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/17_August_2009#Sporulation_Tuning.2F_Chassis_Team 17/08/09]'''
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|'''[https://2009.igem.org/Team:Newcastle/Labwork/2_October_2009 2nd October 2009]'''
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| Repeat experiment for the treatment of the <i>cwlD</i> spores using Method A
+
|Used ligation products to transform more ''E. coli'' cells
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/18_August_2009#Sporulation_Tuning.2F_Chassis_Team 18/08/09]'''
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/5_October_2009 5th October 2009]'''
-
| Successful results for the treatment of the cwlD spores using Method A. Performed treatment for the double-knockout mutants <i>sleB</i> and <i>cwlJ</i> spores using Method A
+
|Attempted transformations failed
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/19_August_2009#Sporulation_Tuning.2F_Chassis_Team 19/08/09]'''
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/6_October_2009#Formal_Lab_Session_-_6th_October_2009 6th October 2009]'''
-
| Successful results for the treatment of the double-knockout mutants <i>sleB</i> and <i>cwlJ</i> spores using Method A
+
|Conducted ''pMUTIN4'' midi-prep again and transformed ''E. coli'' with ''cotC'' in ''pSB1AT3'' (newly arrived from GeneArt)
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/25_August_2009#Chassis.2FSporulation_Team 25/08/09]'''
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/7_October_2009 7th October 2009]'''
-
| Freezing down of the treated non-germinating spores, <i>cwlD</i>, and <i>sleB</i> and <i>cwlJ</i>.
+
| Transformations of ''E. coli'' with ''cotC'' in ''pSB1AT3'' worked - inoculated LB with these colonies for mini and midi-preps. Also PCR amplified the ''cotC'' BioBrick with restriction sites.
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/2_September_2009#Chassis_team 02/09/09]'''
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/8_October_2009 8th October 2009]'''
-
| PCR-ing of gene <i>sleB</i> and <i>cwlJ</i> using primers previously designed and ordered.
+
|Digested newly midi-prepped ''pMUTIN4'' and also midi-prepped ''cotC'' in ''pSB1AT3'' (from GeneArt)
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/3_September_2009#Formal_Lab_Session_-_3rd_September_2009 03/09/09]
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/9_October_2009 9th October 2009]'''
-
| Attempt to PCR-ing of gene <i>sleB</i> and <i>cwlJ</i> using primers previously designed and ordered again.
+
|Ran digested ''cotC'' PCR product (made on 07/10/09) on gel and excised band.
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/4_September_2009#Chassis_team 04/09/09]
+
|'''[https://2009.igem.org/Team:Newcastle/Labwork/12_October_2009 12th October 2009]'''
-
| Redesign PCR primers
+
|Because the ''cotC-GFP-smtA'' + ''pMUTIN4'' digests haven't been working, the team plated out some new ''E. coli'' + ''pMUTIN4'' cells.
|-
|-
-
| '''[https://2009.igem.org/Team:Newcastle/Labwork/8_September_2009 08/09/09]
 
-
| Cloning of sleB
 
|}
|}

Latest revision as of 03:56, 22 October 2009


Metal Sequester

In our system, the team have used the metallothionein SmtA (which usually mops up zinc ions) and have linked it to the CotC spore coat protein - this means that, should the stochastic switch decide, any cadmium mopped up could be sequestered into spores thereby making it unavailable. Please click on the following links to learn more:

Introduction

In order to take up and keep the cadmium from the soil efficiently, we needed to think about a way to cross-link the metal ions to intra-cellular proteins which would end up for the most of it in the spore. If the heavy metal ions were not cross linked to a "sponge protein", it could be lethal to the cell at lower concentration and the cell could end up sporulating too early, or even bursting in the soil, releasing all the heavy metal it has taken up.
From our meeting with Prof. Nigel Robinson on the 18th of March 2009, it was evident that the best way of getting cadmium into the spore is to express a metallothionein, which would 'soak up' the cadmium, which in turn would be trapped within the protein in the spore.

Novelty in this sub-project

To increase the efficiency of our system in sequestering the heavy metal cadmium from the soil, we divised a plan to make sure that most of the metal ions that have been taken in our B.subtilis cell is then rendered bio-unavailable by incorporating it into smtA metallothionein.

SmtA metallothionein protein from E. coli can bind to heavy metals [1,2,3]. They have a tendency to bind to cationic metal ions such as cadmium, copper, arsenic, mercury, silver.

It has been shown that in B. subtilis, in order to express a specific protein in the spore coat, it is possible to make a fusion protein with a spore coat protein called CotC, and a group have successfully expressed antigen proteins which are about the same size as our smtA metallothionein in order to make a vaccine[4]. By fusing CotC spore coat protein from Bacillus subtilis, our smtA metallothionein can be localized to the spore coat, hence we hoped to successfully trap most of the metals ions into the bacterial spores.

CotC was also fused with GFP reporter gene in order to detect the expression of the fusion protein into the spores using a fluorescence microscopy.

Because we want most of the metals to go into the spore rather than the vegetative cell, we designed our fusion protein so that it is controlled by the native cotC promoter sigK which is activated in sporulation conditions. Therefore, our smtA metal sequester would only be expressed once the cell have made the decision to become a metal container and sporulate, and only be expressed in the spore.

Finally, our construct integrated the B. subtilis genome through homologous recombination at the native CotC gene. However, as we will be using pMutin4 integration vector, there will be two different copies of the cotC gene in our engineered B.subtilis genome: a native copy of cotC and our engineered CotC-GFP-smtA fusion copy. We chose not to knock-out the native CotC gene because the lack of native CotC might lead to defects in spore coat formation.

BioBrick constructs

Newcastle SmtA-construct.png

In the parts registry, BBa_K174008:

Newcastle Metal sequester7.JPG

Lab Work Strategies

a) Construction

Synthesised by GeneArt, fragment: 1385 bp DNA

Clone Manager construct and cut map:

Newcastle Metal sequester1.JPG

Sequencher construct:

Newcastle Metal sequester21.JPG

b) Cloning and Integration

GeneArt cloned the vector into a standard biobrick vector. We sent them Plasmid pSB1AT3 with part BBa_J04450 (mCherry).

BBa_J04450 in pSB1AT3 Clone Manager plamid map:

Newcastle Metal sequester3.JPG

Once we received this fragment cloned in pSBAT3 we amplified the part by PCR. Primer 1 will incorporate a HinDIII site and primer 2 will incorporate a BamHI. Checked that these enzymes don’t cut the fragment:

Newcastle Metal sequester4.JPG

We cut the PCR fragment and clone into pMutin4 cut with the same enzymes (diagram below is pMutin2 but this is essentially the same)

Newcastle Metal sequester5.JPG

We then integrate into the 168 chromosome using homology between our cotC fusion and the native copy of cotC.

c) Testing and Characterisation

Once transformed the spores of the mutant will need to be tested for fluorescence. Two obvious methods:

1) Fluorescence microscopy: grow the cells in sporulation medium and look under the microscope for fluorescent spores.
2) Purify spores and measure their fluorescence in a fluorescence plate reader.
3) We would also test whether the strain is able to absorb cadmium in the spores when compared to the wild-type.


Lab Work Done

Summary of Lab Sessions for Metal Sequestering
Date
Description
9th September 2009 Arrival of cotC-GFP-smtA BioBrick - transformed this into DH5-alpha E. coli cells
10th September 2009 Used colonies of cotC-GFP-smtA transformants to inoculate LB media in preparation for mini and midi-preps
11th September 2009 Mini and midi-prepped cotC BioBrick and PCR amplified cotC BioBrick, giving it restriction ends;
14th September 2009 Ligated cotC into pMUTIN4 plasmid and attempted E. coli transformation
15th September 2009 Transformations seemed to have work; picked 12 colonies from 200ul plate and inoculated 12 tubes of 5ml LB + ampicillin
16th September 2009 Mini-preps of 12 picked colonies and restriction enzyme digest analysis - gel showed consistent bands so prepared midi-prep cultures
17th September 2009 Midi-prepped potential cotC-GFP-smtA transformant E. coli culture and digested with BamHI and HindIII
21st September 2009
22nd September 2009
24th September 2009
18th September 2009 Analysed digested midi-prep sample through DNA gel electrophoresis - negative results
28th September 2009 Picked 10 colonies of potential cotC in pMUTIN4 E. coli transformants and inoculated 10 tubes of LB + amp with them
29th September 2009 Conducted mini-preps of 10 cultures of potential transformants and analysed them through restriction digests and gel electrophoresis - did not work
1st October 2009 Checked pMUTIN4 and cotC on gel; carried out another ligation
2nd October 2009 Used ligation products to transform more E. coli cells
5th October 2009 Attempted transformations failed
6th October 2009 Conducted pMUTIN4 midi-prep again and transformed E. coli with cotC in pSB1AT3 (newly arrived from GeneArt)
7th October 2009 Transformations of E. coli with cotC in pSB1AT3 worked - inoculated LB with these colonies for mini and midi-preps. Also PCR amplified the cotC BioBrick with restriction sites.
8th October 2009 Digested newly midi-prepped pMUTIN4 and also midi-prepped cotC in pSB1AT3 (from GeneArt)
9th October 2009 Ran digested cotC PCR product (made on 07/10/09) on gel and excised band.
12th October 2009 Because the cotC-GFP-smtA + pMUTIN4 digests haven't been working, the team plated out some new E. coli + pMUTIN4 cells.

References

1- Cretì, P., F. Trinchella, et al. "Heavy metal bioaccumulation and metallothionein content in tissues of the sea bream Sparus aurata from three different fish farming systems." Environmental Monitoring and Assessment.

2- Morby, A. P., J. S. Turner, et al. (1993). SmtB is a metal-dependent repressor of the cyanobacterial metallothionein gene smtA: identification of a Zn inhibited DNA-protein complex. 21: 921-925.

3- Waldron, K. J. and N. J. Robinson (2009). "How do bacterial cells ensure that metalloproteins get the correct metal?" Nat Rev Micro 7(1): 25-35.

4- Mauriello, E. M. F., L. H. Duc, et al. (2004). "Display of heterologous antigens on the Bacillus subtilis spore coat using CotC as a fusion partner." Vaccine 22(9-10): 1177-1187.




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