Team:UQ-Australia/Project

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'''Electroporation'''
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1uL of plasmid DNA added to a gene pulse cuvette with 50uL of defrosted electrocompetent E.coli and placed in electroporator at 2500V (2mm cuvette). 0.9mL of sterile SOC medium added in order to dilute the transformants and placed into the incubator at 180rpm for one hour at 37deg C. Agar plates loaded with the appropriate antibiotic warmed in incubator and 300-500uL transformed bacteria spread on plates.
1uL of plasmid DNA added to a gene pulse cuvette with 50uL of defrosted electrocompetent E.coli and placed in electroporator at 2500V (2mm cuvette). 0.9mL of sterile SOC medium added in order to dilute the transformants and placed into the incubator at 180rpm for one hour at 37deg C. Agar plates loaded with the appropriate antibiotic warmed in incubator and 300-500uL transformed bacteria spread on plates.
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'''Heat-shock'''
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2uL of plasmid DNA added to 100uL of chemically competent E. coli and incubated on ice for 30 minutes. Bacteria were heat shocked for 30 seconds at 42deg C then incubated on ice for a further 2 minutes. Transformants were then shaken at 225rpm and 37deg C for one hour. 300-500uL of sample added to the agar plates loaded with the approporiate antibiotic and left to grow overnight at 37deg C.
2uL of plasmid DNA added to 100uL of chemically competent E. coli and incubated on ice for 30 minutes. Bacteria were heat shocked for 30 seconds at 42deg C then incubated on ice for a further 2 minutes. Transformants were then shaken at 225rpm and 37deg C for one hour. 300-500uL of sample added to the agar plates loaded with the approporiate antibiotic and left to grow overnight at 37deg C.

Revision as of 23:31, 21 October 2009



Contents

Mercury sequestration using a Multicomponent Operon and Bioprecipitation using P.syringae

Project Abstract

Microbes such as Escherichia coli and Cuprivadis metallidurans have an endogenous multicomponent mercury (Hg2+) uptake and reduction operon, under the control of a metal responsive transcription factor, MerR. By utilising elements of this pathway, with a novel recovery mechanism, mercury can be accumulated intracellularly and efficiently removed from the environment. The presence of mercury activates MerR, driving the expression of Antigen 43 (Ag43), a self-adhering surface protein. Coupling a mercury sensitive promoter to the expression of Ag43 enables cells to accumulate mercury then aggregate in solution.


P. syringae is a ubiquitous airborne bacterium which expresses a unique protein, InaZ. This protein acts as a scaffold for ice nucleation, inducing precipitation. Optimal growth of P. syringae occurs at 22oC. By introducing five heat-shock genes, the tolerance range will be increased to better suit the Australian climate. This modification has the potential to increase the availability of Australia’s most precious resource; water.

Bioaccumulation (Mercury) Project

Project Outline

Escherichia coli.

Water contamination is a key environmental issue for many countries around the world, both developed and developing. In Queensland, Australia we have a particular problem with Mercury (Hg2+) contamination of water supplies around the major mining town of Mt Isa, and also from Airforce bases. After searching through the iGEM projects from previous years, the arsenic detection system inspired us. As the UQ 09' team, we wish to take this idea one step further and completely remove the offending heavy metal from water systems.

To do this we will be utilizing a strain of Escherichia coli, with their already established mercury uptake, reduction and efflux system and making a few modifications. One of our aims is to couple the detection of Mercury to the expression of a native bacterial protein, Antigen 43 (AG43). This protein, when expressed, causes the bacteria to stick to one another. As the bacteria aggregate in clumps, they will fall to the bottom of the sample. Our idea is for the bacteria to take up the mercury, activating Ag43 expression, resulting in aggregation, and the Mercury-filled bacteria will fall to the bottom leaving clean water.

There are a number of parts that we hope to add to the registry. The first is Ag43 as a protein coding sequence and the MerR promoter sequence. We will also add the completed mercury uptake and aggregation system as an operon.

Project Background

Many bacteria carry heavy metal resistance systems, either encoded on a plasmid or within their genome. For example, the bacterium Cupriavidis metallidurans, first isolated from a sludge tank contaminated with high levels of heavy metals, contains genes which encode for reistance systems to Ag(I), Cd(II), Co(II), Cr(IV), Hg(II), Ni(II), Pb(II), and Zn(II) [http://jb.asm.org/cgi/content/full/189/20/7417?view=long&pmid=17675385]. These systems commonly contain a metal transporter, a metal binding protein, a reduction mechanism, and a metal responsive promoter. In the case of Hg(II), the currently accepted general system is outlined below. [http://www.sciencedirect.com.ezproxy.library.uq.edu.au/science?_ob=ArticleURL&_udi=B6T37-48GFVCN-1&_user=331728&_rdoc=1&_fmt=&_orig=search&_sort=d&_docanchor=&view=c&_acct=C000016898&_version=1&_urlVersion=0&_userid=331728&md5=6382dc0a7b36b391d954a54651c2ff72]

UQ-Figure1.JPG

This system facilitates the transportation of Hg(II) into the cell, where MerA acts a reductase, producing Hg(0), which then diffuses out of the cell. However, our project focuses on the accumulation of mercury within the cell, so many elements of this pathway are unsuitable for our purpose. We envisage a system of two plasmids, one containing mercury resistance genes (mer genes).

Plasmid 1

This plasmid will allow for the transport of Hg(II) into the cell, where the protein metallothionien aids in intracellular accumulation. Once Hg(II) enters the cell, it activates MerR, a transcriptional regulator. When active, MerR will initiate the transcription of Antigen43 (Ag43).

Plasmid 2
A. DNA twisted conformation and transcription unable to occur B.Conformational change in MerR when Hg binds - transcription goes ahead C. Hypothetical situation in which MerD (in the endogenous system) binds preferentially to stop transcription [http://www.ncbi.nlm.nih.gov/pubmed/12829265 (4)].

Ag43 is a surface expressed autotransporter [http://jb.asm.org/cgi/content/full/182/17/4789?view=long&pmid=10940019]. This means all the information for suface targeting of the plasma membrane is contained within the protein. Since Ag43 is a native protein to E. Coli (specifically K12 strain), it must first be removed from the genome, then re-inserted as a plasmid so that its expression can be controlled. We were able to obtain a flu- E. coli strain, kindly donated by Associate Professor Mark Schembri from the University of Queensland. When two E. coli cells express Ag43, they aggregate together. Once enough of these cells aggregate, they will fall to the bottom of solution. This autoaggregation can be easily measured using a spectrophotometer.

UQ-Figure4.JPG

Methods

Transformation

Electroporation

1uL of plasmid DNA added to a gene pulse cuvette with 50uL of defrosted electrocompetent E.coli and placed in electroporator at 2500V (2mm cuvette). 0.9mL of sterile SOC medium added in order to dilute the transformants and placed into the incubator at 180rpm for one hour at 37deg C. Agar plates loaded with the appropriate antibiotic warmed in incubator and 300-500uL transformed bacteria spread on plates.

Heat-shock

2uL of plasmid DNA added to 100uL of chemically competent E. coli and incubated on ice for 30 minutes. Bacteria were heat shocked for 30 seconds at 42deg C then incubated on ice for a further 2 minutes. Transformants were then shaken at 225rpm and 37deg C for one hour. 300-500uL of sample added to the agar plates loaded with the approporiate antibiotic and left to grow overnight at 37deg C.

Picking Colonies

Positive colonies were picked from plates, and cultured in 3mL of either LB broth or S.O.C media, supplemented with the appropriate antibiotic. These cultures were incubated overnight at 37deg C in a shaking incubator.

Miniprep

3mL of overnight culture was pelleted, and processed using an Invitrogen PureLinkQuick Plasmid Miniprep Kit.
1. Pellet resuspended in 250uL Resuspension Buffer with RNase A.
2. 250uL Lysis Buffer added to lyse cells.
3. Tubes incubated at room temperature for 5 minutes.
4. 350uL Precipitation Buffer added then centrifuged at 12000g for 10 minutes.
5. Supernatant extracted into a spin column then centrifuged once more at 12000g for one minute.
6. 700uL Wash Buffer with ethanol added to the column and incubated for 1 minute then centrifuged at 12000g for one minute.
7. Flow through discarded then spin column placed into a fresh 1.5mL recovery tube.
8. 75uL of pre-heated TE buffer added to column before incubation at room temperature for one minute.
9. Centrifugation of sample at 12000g for 2 minutes.
10. Recovery tube now contains purified plasmid DNA!
Product was Nanodropped to determine concentration, then stored at -20deg C.

Glycerol Stock

Glycerol stock solution was created by initially grown the original sample strain on an agarose gel plate overnight. Colonies grown overnight were then picked and placed into LB broth solution containing ampicillin and grown overnight at 37 deg C on the shaker. The cells were formed into a pellet and resuspended in a 50:50 glycerol and LB stock solution mixture. Cells were then stored for later use in a -80 deg C freezer.

Digestions

Samples contained a mixture of water, buffer plasmid and appropriate enzymes. Samples were incubated at 37deg C with NEB or Promega restriction enzymes for at least 3 hours to ensure complete digestion. Samples were then run on a 1% gel to determine the band size and if the digest had occurred.

Agarose Gel

DNA grade agarose powder was mixed into 1x TAE and heated until fully dissolved to create either a 1% or 2% gel depending on the experimental parameters. The heated mixure is then poured into a mold and allowed to set. Gels were post-stained using Ethidium Bromide, then visualized with a UV transilluminator. All gels were run with an appropriate ladder depending on the size of the fragments.

In-gel extraction

Bands were excised with a scalpel blade viewed using a UV box removing all of the band with as little of the agarose from the gel. These pieces were then placed into pre-weighed eppendorf tubes and re-weighed after to determine the mass of the excised piece of agarose. In-gel extraction was performed as per protocol from Invitrogen Purelink Gel Extraction Kit.
1. 3 volumes of Gel Solubilisation Buffer added to each volume of gel (preweighed).
2. Tube containing gel + buffer incubated in 50deg C waterbath for 10-15 minutes and inverted every 3 minutes to dissolve all gel.
3. 1 gel volume of isopropanol added for optimal DNA yields.
4. Dissolved gel mixture added to a Gel Extraction Column inside a wash tube.
5. Sample centrifuged at 12000g for one minute. Flow-through discarded.
6. 600uL Wash Buffer with ethanol added then centrifuged again for one minute at 12000g. Wash tube discarded and replaces with a Recovery tube.
7. 50uL Elution Buffer added and incubated at room temperature for one minute.
8. Purified DNA recovered from recovery tube after centrifugation at 12000g for one minute.

Product was Nanodropped to the determine concentration.

PCR

De-phosphorylation

10uL vector was incubated with 0.5uL Promega Shrimp Alkaline Phosphatase and 3uL 10XSAP reaction buffer at 37deg C overnight.

Ligation

Insert and de-phosphorylated vector were incubated at room temperature with NEB T4 DNA ligase for at least one hour before transformation.

Sequencing

Whole plasmid samples with appropriate primers were submitted to the Australian Genome Research Facility within the University of Queensland for sequencing.

Results

Isolation of Ag43 gene

Samples of E. coli MS427 containing either pBAD (empty vector) or pKKJ143 (Ag43+) were kindly donated by Associate Professor Mark Schembri, of The University of Queensland.
UQ-Fig1.jpg
Figure 1 | Plasmid DNA was extracted from cultures, and run on a 1% agarose gel. Bands were observed which corresponded to the expected size of pBAD (4,210bp) and pKKJ143 (7,205bp)

Creation of BBa_I716101 Plasmid Stock, and Restriction Site Checking

Plasmid backbone BBa_I716101 with part BBa_J04450 was obtained from the Spring parts distribution (Plate 1, Well 1C). This plasmid was transformed into E. coli, and red colonies were observed, indicating a positive result. Five clones were cultured further, then plasmid DNA extracted using a miniprep kit.

UQ-Fig2.jpg
Figure 2 | DNA of five clones was digested overnight with either XhoI, BamHI, EcoRI or BglII. Only EcoRI appears to have been effective at cutting the plasmid. Lanes 1-5: Clones A->E, EcoRI. Lanes 6-10: Clones A->E, BglII. Lanes 11-15: Clones A->E, XhoI. Lanes 16-19: Clones B->E, BamHI.

UQ-Fig3.jpg
Figure 3| repeat digestion using XhoI, BamHI, EcoRI or BglII was performed, with known control digests (pGfa2cLacZ - from Thomas lab). Again, only EcoRI appears to digest BBa_I716101. Lane 1: pGfa2cLacZ, EcoRI. Lane 2: BBa_I716101 clone A, EcoRI. Lane 3: pGfa2cLacZ, BglII. Lane 4: BBa_I716101, BglII. Lane 5: pGfa2cLacZ, XhoI. Lane 6: BBa_I716101 XhoI. Lane 7:pGfa2cLacZ, BamHI. Lane 8: BBa_I716101, BamHI. Lane 9: pGfa2cLacZ, undigested. Lane 10: BBa_I716101, undigested.

UQ-Fig7.jpg
Figure 4| Digestion of BBa_J63010 A with PstI. Lane 1: BBa_J63010, undigested. Lane 2: BBa_J63010, PstI.

Preparation of Ag43 gene for compatability with BioBrick Standard 21

The sequence of Ag43 was analysed for incompatible restriction sites, and primers designed to add the appropriate restriction sites to allow Ag43 to be cloned into BBa_I716101.
Uq-Fig4.jpg
Figure 5 | Primer sequences for addition of restriction sites to Ag43 gene. Green nucleotides are part of the known sequence, red nucleotides are new nucleotides to be added to the gene. Italic nucleotides are the prefix and suffix for Standard 21.

UQ-Fig5.jpg
Figure 6 | Gel of PCR product; Lane 1 - AG43 with Standard 21 prefix and suffix attached (3,176bp).

Creation of BBa_J63010 Plasmid Stock, and Restriction Site Checking

Plasmid backbone BBa_J63010 with part BBa_J04450 was obtained from the Spring parts distribution (Plate 1, Well 3C). This plasmid was transformed into E. coli, and red colonies were observed, indicating a positive result. Five clones were cultured further, then plasmid DNA extracted using a miniprep kit.

UQ-Fig6.jpg
Figure 7 | Agarose gel of BBa_J63010 clones. Lanes 1-5: BBa_J63010 clones A-E.

UQ-Fig8.jpg
Figure 8 | Digestion of BBa_J63010 with EcoRI, XbaI, SpeI, PstI. Lane 1: Control 1, undigested. Lane 2: Control 1, EcoRI. Lane 3: Control 1, XbaI. Lane 4: Control 2, undigested. Lane 5: Control 2, SpeI. Lane 6: Control 2, PstI. Lanes 7-11: BBa_J63010 A; undigested, EcoRI, XbaI, SpeI, PstI. Lanes 12-16: BBa_J63010 B; undigested, EcoRI, XbaI, SpeI, PstI. Lanes 17-21: BBa_J63010 C; undigested, EcoRI, XbaI, SpeI, PstI. Lanes 22-26: BBa_J63010 D; undigested, EcoRI, XbaI, SpeI, PstI. Lanes 27-31: BBa_J63010 E; undigested, EcoRI, XbaI, SpeI, PstI.

Mer gene extraction and Standard compatability

E. coli JM109 containing plasmids pSUTp (MerT, MerP), pGmpt (P. sativium Metallothionein)and pSUTp.pG.pmt were kindly donated by Professor David Wilson, from the Department of Molecular Biology and Genetics, Cornell University. Cells were cultured, then plasmid DNA extracted using a miniprep kit.

UQ-Fig9.jpg
Figure 9 | Lane 1: pSUTp.pG.pmt. Lane 2: pGpmt. Lane 3: pSUTp.

Since these plasmids are unsequenced, samples were sent to the AGRF for sequencing. Sequencing of mer genes Primer sequences, proposed sequence. Sequencing data?

UQ-Fig10.jpg
Figure 10 | Primer sequences for addition of restriction sites to MerT and MerP genes. Green nucleotides are part of the gene sequences, red nucleotides are new nucleotides to be added to the gene. Italic nucleotides are the prefix and suffix for Standard 23.

File:UQ-Fig11.jpg


Digest our genes, digest vectors. Picture? Think I cut the gel .... use nanodrop concentrations?

De-phosphorylate Method

Ligate Method

Transform (x2) Positive colonies!

Digest Gel picture

Send off!

Sequence Being done.

Conclusions

Standard 21 isn't standard 21!

Standard 23 is all good.

MerT part is correct.

References

[1] Monchy, S., Benotmane, M. A., Janssen, P., Vallaeys, T., Taghavi, S., van der Lelie, D. and Mergeay, M. (2007). Plasmids pMOL28 and pMOL30 of Cupriavidus metallidurans are specialized in the maximal viable response to heavy metals. J Bacteriol 189, 7417-25.

[2] Barkay, T., Miller, S. M. and Summers, A. O. (2003). Bacterial mercury resistance from atoms to ecosystems. FEMS Microbiol Rev 27, 355-84.

[3] Kjaergaard, K., M. A. Schembri, et al. (2000). Antigen 43 from Escherichia coli induces inter- and intraspecies cell aggregation and changes in colony morphology of Pseudomonas fluorescens. J Bacteriol 182(17): 4789-96.

Bioprecipitation using P.syringae

Project Description

P. syringae

The arid climate of Australia has become notorious for causing widespread problems for agricultural industries. That is, the scarcity of water hinders the production of crops and livestock, as well as forcing restrictions of daily water usage for households. Team UQ Australia aims to solve this problem through the use of a bio-precipitation technique, thus increasing the availability of our most precious resource.

Pseudomonas syringae is a common bacterium, primarily found in colder climates (optimally at 22°C), and is well known for its biological ice nucleation properties, i.e. the formation of rain/snow. This bacteria expresses an ice nucleation protein on its outer membrane (InaZ). InaZ acts as a scaffold for the formation of the ice crystals, this directly assists in the formation of clouds and speeds up the rain cycle. However, the bacteria are unable to survive in environmental temperatures above 28°C. The ideal growing temperatures for syringae are 22°C - 26°C. By introducing heat shock proteins (DnaK, DnaJ, GroEL, and GroES) through plasmid insertion, UQ Australia aims to increase the optimal growth temperature available to P.syringae, thereby allowing bio-precipitation to occur in warmer (and drought stricken) climates. Although syringae already has this proteins encoded within the genome, they are not expressed at levels similar to bacteria which grow at higher temperatures.

The heat shock proteins form two systems. GroEL and GroES form one dimer which acts as a chaperon. Together these proteins assists in lowering the mis-folding of proteins. At higher temperatures proteins become unstable and mis-fold at a higher rate.

Ideally, UQ Australia will be contributing a number of parts to the registry. Firstly, a plasmid with DnaK, DnaJ, as well as an upstream promoter will drive the expression of these two genes. Secondly, an additional plasmid will carry the genes for GroEL and GroES, also complemented by an upstream promoter to drive gene expression.

P. syringae and the rain cycle


Method

By taking measurements during the life cycle of P. syringae it should show a shift in the maximal growth peak. Over a 14 hour growth period absorbance readings were taken of the transformed bacteria.