Difference between revisions of "Team:Dundee/Forensic Toolkit/Chromate Fiona"

 
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<h1>Introduction</h1>
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<h2>Background</h2>
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        <h2>Background</h2>
 
                 <p>Stainless steel is an alloy of different metals and apart from the base material, iron, contains a large proportion >11% of chromium. There is a wide range of stainless steels for a variety of different applications, ranging from surgical steel to alloys used in the aeronautic industry. For our application we assumed stainless steels that are used in bulk production of standard kitchen knives with a chromium content between 12% and 14%. We also utilise the fact that chromate is a salt containing chromium. Bone incisions and kerfmarks, distinctive marks left behind, are current indicators for different types of weapons such as saws <a href="#chrome_ref1">(1)</a> or knifes.</p>
 
                 <p>Stainless steel is an alloy of different metals and apart from the base material, iron, contains a large proportion >11% of chromium. There is a wide range of stainless steels for a variety of different applications, ranging from surgical steel to alloys used in the aeronautic industry. For our application we assumed stainless steels that are used in bulk production of standard kitchen knives with a chromium content between 12% and 14%. We also utilise the fact that chromate is a salt containing chromium. Bone incisions and kerfmarks, distinctive marks left behind, are current indicators for different types of weapons such as saws <a href="#chrome_ref1">(1)</a> or knifes.</p>
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<img src="https://static.igem.org/mediawiki/2015/7/7d/TeamDundee_knife_upright_tiny.png"  />
 
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<figcaption>We will use pig bones to investigate incisions by stainless steel.</figcaption></figure>
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<figcaption> We used pig bones to investigate incisions by stainless steel tools.</figcaption></figure1>
 
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<h2>Initial Ideas</h2>
 
<h2>Initial Ideas</h2>
 
                 <p>At the beginning of the project we met with Dr. Lucina Hackman, an expert in dismemberment cases at the University of Dundee. In dismemberment cases it is obvious enough that a body has been dismembered. However, if the body is not found for a long time and the only remains are bones, it is hard to tell if a person has been stabbed or if an animal was chewing on the bone. This is where a chromate biosensor would be useful. By detecting minute amounts of chromate on a bone, the use of a weapon may be inferred which will justify searching for trace evidence.</p>
 
                 <p>At the beginning of the project we met with Dr. Lucina Hackman, an expert in dismemberment cases at the University of Dundee. In dismemberment cases it is obvious enough that a body has been dismembered. However, if the body is not found for a long time and the only remains are bones, it is hard to tell if a person has been stabbed or if an animal was chewing on the bone. This is where a chromate biosensor would be useful. By detecting minute amounts of chromate on a bone, the use of a weapon may be inferred which will justify searching for trace evidence.</p>
<p>We found that a chromate detector had already been submitted by the Beijing Institute of Technology 2013 iGEM team, where they had created a biobrick for this <a href="http://parts.igem.org/Part:BBa_K1058008"><u><b>(BBa_K1058008)</b></u></a>. The biobrick is a modified version of a chromate resistance operon of ochrobactrum tritici 5bvl1(<a href="#chrome_ref2">2</a>,<a href="#chrome_ref3">3</a>).</p><p>The science behind Chromate resistance:
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<p>We found that a chromate detector had already been submitted by the Beijing Institute of Technology 2013 iGEM team, where they had created a biobrick for this <a href="http://parts.igem.org/Part:BBa_K1058008"><u>BBa_K1058008</u></a> (Fig. 1). The biobrick is a modified version of a highly sensitive chromate resistance operon of ochrobactrum tritici 5bvl1(<a href="#chrome_ref2">2</a>,<a href="#chrome_ref3">3</a>), containing a promoter, P<i>chr</i>, a coding region for a chromate responsive repressor of this promoter, <i>chrB</i>, fused to the sequence of the fluorescent reporter GFP.</p><p>
Ochrobactrum tritici 5bvl1 was discovered in 2004 in a chromate contaminated wastewater treatment facility. A specific characteristic of this strain was that it could both, reduce Cr(VI) and be resistant to it at the same time. Previously characterised strains were either resistant or could reduce <a href="#chrome_ref2">(2)</a>. Over the last 10 years the group that discovered it started working out the underlying mechanisms of this set of characteristics. A transposon located set of genes that lead to chromate resistance (TnOtChr) was uncovered. This operon, expressed from the pChr promoter led to the expression of the genes ChrA, ChrB, ChrC, and ChrF. ChrA was found to express and efflux pump, whereas ChrB was identified as being a chromate-inducible regulator of pChr. Additionally, ChrC and ChrF were found to confer tolerance to superoxides. Deleting ChrC and ChrF was shown to have no significant effect on chromate resistance which at first seemed unusual, but considering that Cr(VI) is often reduced via Cr(V) and Cr(IV) intermediates which can lead to the generation of superoxides, these 2 genes are suspected to act as a second line of defense <a href="#chrome_ref4">(4)</a>.</p>
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<h2>The Science behind Chromate resistance</h2>
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<p>Ochrobactrum tritici 5bvl1 was discovered in 2004 in a chromate contaminated wastewater treatment facility. A specific characteristic of this strain was that it could both, reduce Cr(VI) and be resistant to it at the same time. Previously characterised strains were either resistant or could reduce chromate <a href="#chrome_ref2">(2)</a>. Over the last 10 years the group that discovered it started working out the underlying mechanisms of this set of characteristics. A transposon located set of genes that lead to chromate resistance (<i>TnOtChr</i>) was uncovered. This operon, expressed from the P<i>chr</i> - promoter led to the expression of the downstream genes <i>chrA, chrB, chrC</i>, and <i>chrF</i>. <i>chrA</i> was found to express and efflux pump, whereas the gene product of <i>chrB</i> was identified as being a chromate-inducible regulator of P<i>chr</i>. Additionally, <i>chrC</i> and <i>chrF</i> were found to confer tolerance to superoxides. Deleting <i>chrC</i> and <i>chrF</i> was shown to have no significant effect on chromate resistance which at first seemed unusual, but considering that Cr(VI) is often reduced via Cr(V) and Cr(IV) intermediates which can lead to the generation of superoxides, these 2 genes are suspected to act as a second line of defense <a href="#chrome_ref4">(4)</a>.</p></p>
  
 
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<figcaption>Plasmid map of the original biobrick system, <a href="http://parts.igem.org/Part:BBa_K1058008"><u><b>(BBa_K1058008)</b></u></a>.</figcaption></figure1>
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<figcaption>Figure 1: Plasmid map of the original biobrick system, <a href="http://parts.igem.org/Part:BBa_K1058008"><u><b>(BBa_K1058008)</b></u></a>.</figcaption></figure1>
 
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<p>We aimed to modify and improve this existing biobrick by taking the brick apart and use its constituent parts in a new arrangement. This should have the advantage that each part can be modified individually and the level of GFP and/or the repressor can be modulated more easily by simply cloning it into a higher or lower copy number plasmid.  
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<p>To make the system more modular, we aimed to modify and improve this existing biobrick by taking it apart and using its constituent parts in a new arrangement (Fig. 2). This has the advantage that each part can be modified individually and the level of the reporter, GFP, and/or the repressor can be modulated more easily by subcloning either of them.  
 
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<img src="https://static.igem.org/mediawiki/2015/6/64/TeamDundee_plasmid_md_tiny.png"  height="auto" width="40%" />
 
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<figcaption>Plasmid map of the modified biobrick system, <a href="http://parts.igem.org/Part:BBa_K1590003"><u><b>(BBa_K1590003</b></u></a>, <a href="http://parts.igem.org/Part:BBa_K1590004"><u><b>BBa_K1590004)</b></u></a>.</figcaption></figure>
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<figcaption>Figure 2: Plasmid map of the modified biobrick system, (submitted to registry under <a href="http://parts.igem.org/Part:BBa_K1590003"><u>BBa_K1590003</u></a>, and <a href="http://parts.igem.org/Part:BBa_K1590004"><u>BBa_K1590004</u></a>.</figcaption></figure>
 
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<h1>What did we do?</h1>
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<h1>How did we test it?</h1>
 
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                 <p>To ensure that the modified system was valid we used mathematical modelling to compare the original biobrick and our modified system. We also looked at GFP production with varying levels of chromate added to the system. The models of both the original and modified pathways revealed two key points; the modified pathway is just as reliable as the original pathway and the level of GFP produced will not be changed. However the response will be faster for increasing levels of chromate added to the system. </p>
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                 <p>To ensure that the modified system was valid we used mathematical modelling to compare the original biobrick and our modified system (Fig. 3). We also looked at GFP production with varying levels of chromate added to the system (Fig. 4). The models of both the original and modified pathways revealed two key points; the modified pathway is just as reliable as the original pathway, and the level of GFP produced does not change. However the response will be faster for increasing levels of chromate added to the system. </p>
 
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     <img  src="https://static.igem.org/mediawiki/2015/a/a4/TeamDundee_Chrom_fig7_tiny.png" />
 
     <img  src="https://static.igem.org/mediawiki/2015/a/a4/TeamDundee_Chrom_fig7_tiny.png" />
  <figcaption>Comparing the likelihood of false positives of both systems.</figcaption></figure>
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  <figcaption>Figure 3: Comparing the likelihood of false positives, in terms of leakiness, of both systems in the case of GFP output. The figure shows that both systems are equally reliable.</figcaption></figure>
 
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  <img  src="https://static.igem.org/mediawiki/2015/d/d7/TeamDundee_Chrom_fig3_tiny.png" />  
 
  <img  src="https://static.igem.org/mediawiki/2015/d/d7/TeamDundee_Chrom_fig3_tiny.png" />  
 
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  <figcaption>GFP production with varying levels of chromate present.</figcaption>
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  <figcaption>Figure 4: GFP production with varying levels of chromate present showing that the more GFP the faster the response.</figcaption>
 
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                 <p>The models allowed us to ensure that it will be valid to use our modified system. In the lab to test the system we used the two compounds potassium chromate and potassium dichromate, as well as the two controls, Chromium(III)Chloride and the isostructural potassium sulphate and observed if it had any influence on the level of fluorescence. We tested concentrations between 10nM and 100µM as recommended by literature <a href="#chrome_ref5">(5)</a>. Our cloning strategy focused on taking this brick apart and use its constituent parts in a new arrangement.</p>
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                 <p>The models allowed us to ensure that it will be valid to use our modified system. Our cloning strategy hence focused on taking this brick apart and using its constituent parts in a new arrangement (Fig. 2). To test our system, we used the two compounds potassium chromate, and potassium dichromate. We also used two control substances, chromium(III)chloride and the isostructural potassium sulphate and observed if it had any influence on the level of fluorescence. Chromium(III)chloride was chosen to probe the system's specificity for Cr(VI), and potassium sulphate was chosen in order to test the structural selectivity for Cr(VI). All additives were tested at concentrations between 10nM and 100µM as recommended in the literature. <a href="#chrome_ref5">(5)</a>.</p>
<p> The newly arranged system was then investigated by firstly comparing the GFP output for different concentrations of chromate. Cell density over time was also considered using chromate and other similar substances in response to the system. From these experiments it was seen that at a specific time both fluorescence and cell density increased, when the cell density reached exponential growth. this inferred that fluorescence only increased once the cell density increased, further experiments would have to be done to try and disconnect these two variables. After these experiments we then wanted to compare the original biobrick and the modified two plasmid system.</p>
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                <p>Before testing the complete system, we first checked if we can detect both individual parts of it. For this purpose, western blots against both, GFP, and His-6 - ChrB were done (Fig. 5 and 6).</p>
  
  
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<figcaption>Figure 5. Top: anti-GFP: Single colonies of JM110 + pSB1C3-P<i>chr-gfp</i> (A) and MC1061 + pSB1C3-P<i>chr-gfp</i> (B) were prepared for western blotting against GFP. pSB1C3 was included as a negative control, and P<i>manA-gfp</i> as a positive control.
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<figcaption>Figure 6. Top: anti-GFP: Single colonies of anti-6-His - ChrB: JM110 pUniprom-<i>chrB</i> and JM110 pUniprom-<i>chrB</i> (opt) were prepared for western blotting against 6-His - ChrB. pUniprom was included as a negative control, and <i>hydA - 6-His</i> as a positive control.</figcaption>
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                <p>The newly designed system was investigated firstly by comparing the GFP output for the different concentrations of the respective additive. At the same time the results were compared to the original biobrick. Furthermore, the cell density was measured at the same time (Fig. 7). While in both cases an increase in fluorescence could be observed, this increase coincided in timing with the exponential increase of growth, suggesting that a higher level of fluorescence was observed due to more cells being present in the medium. Further experiments will have to be done in order to disconnect these 2 variables.</p>
  
 
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  <figcaption>GFP output over time for different concentrations of chromate.</figcaption>
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  <figcaption>Figure 7: Top: Comparison of relative fluorescence (left) and cell density (right) of MG1655 + pSB1C3-P<i>chr-gfp</i> (A) + pUniprom-<i>chrB</i> (opt). Botton: Comparison of relative fluorescence (left) and cell density (right) of MG1655 + <a href="http://parts.igem.org/Part:BBa_K1058008" target="_blank">BBa_K1058008</a>. In both cases, an increase of both values can be observed at the same time, independently of the additive or the concentration thereof.</figcaption>
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<figcaption>Cell density over time for chromate and other similar substances.</figcaption>
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<p>The original biobrick and our modified two plasmid system were compared by looking at the differences in GFP output. Different concentrations of the biobrick and the modified system were loaded onto a gel and blotted against GFP. It was found that GFP was produced in the absence of chromate for both systems. This is perhaps due to an error in the original biobrick. This result was unexpected and further investigation into why this occurred is required.
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<p>The original biobrick and our modified two plasmid system were furthermore compared by western blotting (Fig. 9 and 10). It was found that GFP was produced in the absence of chromate for both systems. This reason for these unexpected results could not be discerned, and further experiments are required to understand those. At this stage of the project the results indicate that ChrB might not be a repressor.
  
 
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<figcaption>Western blot showing GFP production.</figcaption></figure>
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<figcaption>Figure 9: Comparison of presence of GFP in MG1655 + <a href="http://parts.igem.org/Part:BBa_K1058008" target="_blank">BBa_K1058008</a>, MG1655 + pSB1C3-P<i>chr-gfp</i> (A) + pUniprom-<i>chrB</i>, and MG1655 + pSB1C3-P<i>chr-gfp</i> (A) + pUniprom-<i>chrB</i> (opt). All samples were prepared and diluted to a suitable concentration for western blotting against GFP. P<i>manA-gfp</i> was included as a positive control.</figcaption></figure>
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<figcaption>Figure 10: Comparison of presence of GFP in MG1655, containing all 4 combinations, pUniprom-<i>chrB</i> - pSB1C3-P<i>chr-gfp</i> (A), pUniprom-<i>chrB</i> - pSB1C3-P<i>chr-gfp</i> (B), pUniprom-<i>chrB</i> (opt) - pSB1C3-P<i>chr-gfp</i> (A), and pUniprom-<i>chrB</i> (opt) - pSB1C3-P<i>chr-gfp</i> (B). All samples were prepared and diluted to a suitable concentration for western blotting against GFP. pSB1C3, and pUniprom were included as a negative control, and P<i>manA-gfp</i> as a positive control.</figcaption>
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                 <p>To complement our chromate biosensor, we originally aimed to find out how much chromate would be left on an incision in a bone from a stab of a certain force. However this was quickly turned around to measure the wear of bone instead of stainless steel. By calculating the force required to make the incision, this could potentially indicate the size or strength of a possible suspect, while the sliding distance would correspond to the length of the blade. The bone incision experiments allowed us to create a relationship between the applied force, sliding distance and wear volume when a stainless steel knife collides with bone. The results showed that the volume will increase as the length of the blade or the force increases. However some irregularities were noticed and could be due to experimental error. You can see Hannah demonstrating the method used in our <a href="https://2015.igem.org/Team:Dundee/Media#video"><u><b>STV appearance</b></u></a>.</p>
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                 <p>To complement our chromate biosensor, we originally aimed to find out how much chromate would be left on an incision in a bone from a stab of a certain force. However this was quickly turned around to measure the wear of bone instead of stainless steel. By calculating the force required to make the incision, this could potentially indicate the size or strength of a possible suspect, while the sliding distance would correspond to the length of the blade. The bone incision experiments allowed us to create a relationship between the applied force, sliding distance and wear volume when a stainless steel knife collides with bone. The results showed that the volume will increase as the length of the blade or the force increases (Fig. 11). However some irregularities were noticed and are likely due to experimental error with the equipment shown in Fig. 12. You can see Hannah demonstrating the method used in our <a href="https://2015.igem.org/Team:Dundee/Media#video"><u><b>STV appearance</b></u></a>.</p>
 
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<figcaption> The Intron 4204 with the knife attached and bone placed on stand below.</figcaption>
 
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<figcaption> A graph showing the relationship between the volume of a bone incision, length of the blade and force of stabbing. </figcaption></figure>
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<figcaption>Figure 11: A graph showing the relationship between the volume of a bone incision, length of the blade and force of stabbing. </figcaption></figure>
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<figcaption>Figure 12: The Instron 4204 compression tested with the knife attached and bone placed on stand below.</figcaption>
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<h1>What next?</h1>
 
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                 <p>Since most of the parameters were assumed in the mathematical models then there is room for error. Practical experiments could be done to produce values for the kinetic parameters or sensitivity analysis done to compare varying kinetic parameter values. Probing the concentration range for detecting different chromate salts will be essential to feed back into the modelling which is currently largely based on assumptions. This would ensure that the models are more realistic and therefore give a more valid description of the systems.</p>
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                 <p>Since most of the parameters were assumed in the mathematical models, there is room for error. Practical experiments could be done to produce values for the kinetic parameters or sensitivity analysis to compare varying kinetic parameter values. Probing the concentration range for detecting different chromate salts will be essential to feed back into the modelling which is currently largely based on assumptions. This would ensure that the models are more realistic and therefore give a more valid description of the systems.</p>
 
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  <figcaption>Further work would include testing and validation of our methods.</figcaption>
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  <figcaption>Figure 13: Further work would include testing and validation of our methods.</figcaption>
 
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<p>The next step for this project is to find an ideal concentration of ChrB in relation to pChrGFP to work in a balance way of expression/repression. This involves finding plasmids with an appropriate copy number and promoters of appropriate strength. The modularity of this system makes this process easier. Once a concentration range has been established, we can test the system by using actual shavings of stainless steel. A problem that might occur is that the chromium contained in the alloy is in the wrong oxidation state. Oxidising chromium to yield Cr(VI) can be done by subjecting it to a strong acid. The solution will have to be neutralised again to be used as an additive for an experiment. The question is then if the concentration is still high enough to induce expression of GFP in our system. Good insights into the amount of steel retained after sharp-force trauma and blunt-force trauma on bones can be found in a series of papers (<a href="#chrome_ref6">6</a>,<a href="#chrome_ref7">7</a>).
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<p>The next step for this project is to find an ideal concentration of ChrB in relation to P<i>chr-gfp</i> to work in a balance way of expression/repression. This involves finding plasmids with an appropriate copy number and promoters of appropriate strength. The modularity of this system makes this process easier. Once a concentration range has been established, we can test the system by using actual shavings of stainless steel. A problem that might occur is that the chromium contained in the alloy is in the wrong oxidation state. Oxidising chromium to yield Cr(VI) can be done by subjecting it to a strong acid. The solution will have to be neutralised again to be used as an additive for an experiment. The question is then if the concentration is still high enough to induce expression of GFP in our system. Good insights into the amount of steel retained after sharp-force trauma and blunt-force trauma on bones can be found in a series of papers (<a href="#chrome_ref6">6</a>,<a href="#chrome_ref7">7</a>).
Of great importance will also be potential contaminants. Hence testing the system with similar compounds will be one test. Checking for the prevalence of inducing compounds in or around bones is essential to see how prone the test is to leading to false negatives.
+
Potential contaminants will also be of great importance. Hence testing the system with similar compounds will be one test. Checking for the prevalence of inducing compounds in or around bones is essential to see how prone the test is to leading to false negatives.
 
</p>
 
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Latest revision as of 12:30, 18 September 2015

Chromate Biosensor


Summary

Introduction

Background

Stainless steel is an alloy of different metals and apart from the base material, iron, contains a large proportion >11% of chromium. There is a wide range of stainless steels for a variety of different applications, ranging from surgical steel to alloys used in the aeronautic industry. For our application we assumed stainless steels that are used in bulk production of standard kitchen knives with a chromium content between 12% and 14%. We also utilise the fact that chromate is a salt containing chromium. Bone incisions and kerfmarks, distinctive marks left behind, are current indicators for different types of weapons such as saws (1) or knifes.

We used pig bones to investigate incisions by stainless steel tools.

Initial Ideas

At the beginning of the project we met with Dr. Lucina Hackman, an expert in dismemberment cases at the University of Dundee. In dismemberment cases it is obvious enough that a body has been dismembered. However, if the body is not found for a long time and the only remains are bones, it is hard to tell if a person has been stabbed or if an animal was chewing on the bone. This is where a chromate biosensor would be useful. By detecting minute amounts of chromate on a bone, the use of a weapon may be inferred which will justify searching for trace evidence.

We found that a chromate detector had already been submitted by the Beijing Institute of Technology 2013 iGEM team, where they had created a biobrick for this BBa_K1058008 (Fig. 1). The biobrick is a modified version of a highly sensitive chromate resistance operon of ochrobactrum tritici 5bvl1(2,3), containing a promoter, Pchr, a coding region for a chromate responsive repressor of this promoter, chrB, fused to the sequence of the fluorescent reporter GFP.

The Science behind Chromate resistance

Ochrobactrum tritici 5bvl1 was discovered in 2004 in a chromate contaminated wastewater treatment facility. A specific characteristic of this strain was that it could both, reduce Cr(VI) and be resistant to it at the same time. Previously characterised strains were either resistant or could reduce chromate (2). Over the last 10 years the group that discovered it started working out the underlying mechanisms of this set of characteristics. A transposon located set of genes that lead to chromate resistance (TnOtChr) was uncovered. This operon, expressed from the Pchr - promoter led to the expression of the downstream genes chrA, chrB, chrC, and chrF. chrA was found to express and efflux pump, whereas the gene product of chrB was identified as being a chromate-inducible regulator of Pchr. Additionally, chrC and chrF were found to confer tolerance to superoxides. Deleting chrC and chrF was shown to have no significant effect on chromate resistance which at first seemed unusual, but considering that Cr(VI) is often reduced via Cr(V) and Cr(IV) intermediates which can lead to the generation of superoxides, these 2 genes are suspected to act as a second line of defense (4).

Figure 1: Plasmid map of the original biobrick system, (BBa_K1058008).

To make the system more modular, we aimed to modify and improve this existing biobrick by taking it apart and using its constituent parts in a new arrangement (Fig. 2). This has the advantage that each part can be modified individually and the level of the reporter, GFP, and/or the repressor can be modulated more easily by subcloning either of them.

Figure 2: Plasmid map of the modified biobrick system, (submitted to registry under BBa_K1590003, and BBa_K1590004.

How did we test it?

To ensure that the modified system was valid we used mathematical modelling to compare the original biobrick and our modified system (Fig. 3). We also looked at GFP production with varying levels of chromate added to the system (Fig. 4). The models of both the original and modified pathways revealed two key points; the modified pathway is just as reliable as the original pathway, and the level of GFP produced does not change. However the response will be faster for increasing levels of chromate added to the system.

Figure 3: Comparing the likelihood of false positives, in terms of leakiness, of both systems in the case of GFP output. The figure shows that both systems are equally reliable.

Figure 4: GFP production with varying levels of chromate present showing that the more GFP the faster the response.

The models allowed us to ensure that it will be valid to use our modified system. Our cloning strategy hence focused on taking this brick apart and using its constituent parts in a new arrangement (Fig. 2). To test our system, we used the two compounds potassium chromate, and potassium dichromate. We also used two control substances, chromium(III)chloride and the isostructural potassium sulphate and observed if it had any influence on the level of fluorescence. Chromium(III)chloride was chosen to probe the system's specificity for Cr(VI), and potassium sulphate was chosen in order to test the structural selectivity for Cr(VI). All additives were tested at concentrations between 10nM and 100µM as recommended in the literature. (5).

Before testing the complete system, we first checked if we can detect both individual parts of it. For this purpose, western blots against both, GFP, and His-6 - ChrB were done (Fig. 5 and 6).

Figure 5. Top: anti-GFP: Single colonies of JM110 + pSB1C3-Pchr-gfp (A) and MC1061 + pSB1C3-Pchr-gfp (B) were prepared for western blotting against GFP. pSB1C3 was included as a negative control, and PmanA-gfp as a positive control.

Figure 6. Top: anti-GFP: Single colonies of anti-6-His - ChrB: JM110 pUniprom-chrB and JM110 pUniprom-chrB (opt) were prepared for western blotting against 6-His - ChrB. pUniprom was included as a negative control, and hydA - 6-His as a positive control.

The newly designed system was investigated firstly by comparing the GFP output for the different concentrations of the respective additive. At the same time the results were compared to the original biobrick. Furthermore, the cell density was measured at the same time (Fig. 7). While in both cases an increase in fluorescence could be observed, this increase coincided in timing with the exponential increase of growth, suggesting that a higher level of fluorescence was observed due to more cells being present in the medium. Further experiments will have to be done in order to disconnect these 2 variables.

Figure 7: Top: Comparison of relative fluorescence (left) and cell density (right) of MG1655 + pSB1C3-Pchr-gfp (A) + pUniprom-chrB (opt). Botton: Comparison of relative fluorescence (left) and cell density (right) of MG1655 + BBa_K1058008. In both cases, an increase of both values can be observed at the same time, independently of the additive or the concentration thereof.

The original biobrick and our modified two plasmid system were furthermore compared by western blotting (Fig. 9 and 10). It was found that GFP was produced in the absence of chromate for both systems. This reason for these unexpected results could not be discerned, and further experiments are required to understand those. At this stage of the project the results indicate that ChrB might not be a repressor.

Figure 9: Comparison of presence of GFP in MG1655 + BBa_K1058008, MG1655 + pSB1C3-Pchr-gfp (A) + pUniprom-chrB, and MG1655 + pSB1C3-Pchr-gfp (A) + pUniprom-chrB (opt). All samples were prepared and diluted to a suitable concentration for western blotting against GFP. PmanA-gfp was included as a positive control.

Figure 10: Comparison of presence of GFP in MG1655, containing all 4 combinations, pUniprom-chrB - pSB1C3-Pchr-gfp (A), pUniprom-chrB - pSB1C3-Pchr-gfp (B), pUniprom-chrB (opt) - pSB1C3-Pchr-gfp (A), and pUniprom-chrB (opt) - pSB1C3-Pchr-gfp (B). All samples were prepared and diluted to a suitable concentration for western blotting against GFP. pSB1C3, and pUniprom were included as a negative control, and PmanA-gfp as a positive control.

To complement our chromate biosensor, we originally aimed to find out how much chromate would be left on an incision in a bone from a stab of a certain force. However this was quickly turned around to measure the wear of bone instead of stainless steel. By calculating the force required to make the incision, this could potentially indicate the size or strength of a possible suspect, while the sliding distance would correspond to the length of the blade. The bone incision experiments allowed us to create a relationship between the applied force, sliding distance and wear volume when a stainless steel knife collides with bone. The results showed that the volume will increase as the length of the blade or the force increases (Fig. 11). However some irregularities were noticed and are likely due to experimental error with the equipment shown in Fig. 12. You can see Hannah demonstrating the method used in our STV appearance.

Figure 11: A graph showing the relationship between the volume of a bone incision, length of the blade and force of stabbing.
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Figure 12: The Instron 4204 compression tested with the knife attached and bone placed on stand below.

What next?

Since most of the parameters were assumed in the mathematical models, there is room for error. Practical experiments could be done to produce values for the kinetic parameters or sensitivity analysis to compare varying kinetic parameter values. Probing the concentration range for detecting different chromate salts will be essential to feed back into the modelling which is currently largely based on assumptions. This would ensure that the models are more realistic and therefore give a more valid description of the systems.


Figure 13: Further work would include testing and validation of our methods.

The next step for this project is to find an ideal concentration of ChrB in relation to Pchr-gfp to work in a balance way of expression/repression. This involves finding plasmids with an appropriate copy number and promoters of appropriate strength. The modularity of this system makes this process easier. Once a concentration range has been established, we can test the system by using actual shavings of stainless steel. A problem that might occur is that the chromium contained in the alloy is in the wrong oxidation state. Oxidising chromium to yield Cr(VI) can be done by subjecting it to a strong acid. The solution will have to be neutralised again to be used as an additive for an experiment. The question is then if the concentration is still high enough to induce expression of GFP in our system. Good insights into the amount of steel retained after sharp-force trauma and blunt-force trauma on bones can be found in a series of papers (6,7). Potential contaminants will also be of great importance. Hence testing the system with similar compounds will be one test. Checking for the prevalence of inducing compounds in or around bones is essential to see how prone the test is to leading to false negatives.

To remove doubts in the data from the bone incision experiments, due to possible experimental error we should repeat the experiments. This would ensure that the experiments are reproducible and reliable.

References

  1. Saville PA, Hainsworth SV, Rutty GN. Cutting crime: the analysis of the "uniqueness" of saw marks on bone. Int J Legal Med 2007; 121(5): 349-357.
  2. Branco R, Alpoim MC, Morais PV. Ochrobactrum tritici strain 5bvl1 - characterization of a Cr(VI)-resistant and Cr(VI)-reducing strain. Can J Microbiol 2004; 50(9): 697-703.
  3. Branco R, Morais PV. Identification and Characterization of the Transcriptional Regulator ChrB in the Chromate Resistance Determinant of Ochrobactrum tritici 5bvl1. PLoS ONE 2013; 8: 77987.
  4. Branco R, Chung AP, Johnston T, Gurel V, Morais P, Zhitkovich A. The chromate-inducible chrBACF operon from the transposable element TnOtChr confers resistance to chromium(VI) and superoxide. J Bacteriol 2008; 190(21): 6996-7003.
  5. Branco R, Cristovao A, Morais PV. Highly Sensitive, Highly Specific Whole-Cell Bioreporters for the Detection of Chromate in Environmental Samples. PLoS ONE 2013; 8(1): e54005.
  6. Pechníková M, Porta D, Mazzarelli D, Rizzi A, Drozdová E, Gibelli D, Cattaneo C. Detection of metal residues on bone using SEM-EDS. Part I: Blunt force injury. Forensic Sci Int 2012; 223(1): 87-90.
  7. Gibelli D, Mazzarelli D, Porta D, Rizzi A, Cattaneo C. Detection of metal residues on bone using SEM-EDS--part II: Sharp force injury. Forensic Science International 2012; 223(1): 91-96.

Recommended Reading

  • Coelho C, Branco R, Natal-da-Luz T, Sousa JP, Morais PV. Evaluation of bacterial biosensors to determine chromate bioavailability and to assess ecotoxicity of soils. Chemosphere 2015; 128(1): 62-69.
  • Díaz-Pérez C, Cervantes C, Campos-García J, Julián-Sánchez A, Riveros-Rosas H. Phylogenetic analysis of the chromate ion transporter (CHR) superfamily. FEBS J 2007; 274(23): 6215-6227.
  • Hainsworth SV, Delaney RJ, Rutty GN. How sharp is sharp? Towards quantification of the sharpness and penetration ability of kitchen knives used in stabbings. Int J Legal Med. 2008; 122(4): 281-91.
  • Morais PV, Branco R, Francisco R. Chromium resistance strategies and toxicity: what makes Ochrobactrum tritici 5bvl1 a strain highly resistant. Biometals 2011; 24(3): 401-410.
  • Saikia SK, Gupta R, Pant A, Pandey R. Genetic revelation of hexavalent chromium toxicity using Caenorhabditis elegans as a biosensor. Journal of Exposure Science and Environmental Epidemiology 2014; 24(1): 180-184.