Latest revision as of 18:54, 20 November 2015

Basic Parts

Heroin Esterase BBa_K1615045

Heroin esterase, an acetylmorphine carboxylesterase, was isolated from Rhodococcus erythropolis strain H1 in 1994 from the garden soil at Cambridge and is able to use heroin as its sole carbon and energy source by deacetylating the C-3 and C-6 groups to form morphine¹. The gene her encodes this enzyme and can be expressed in the chassis Escherichia coli². The pH optimum for this enzyme is pH8.5 in bicine buffer¹.

The activity of heroin esterase can be tested using 4-nitrophenyl acetate which is hydrolysed by heroin esterase to form 4-nitrophenol and acetate³. This produces a yellow colour which can be read at 410 nm.

Design: The sequence for our enzyme used the original sequence from Rathbone, et al.², which was then codon optimised for E. coli. The RFC25 prefix and suffix were added which required all illegal sites (EcoRI, SpeI, AgeI, NotI, NgoMIV and XbaI) to be removed. As this was a difficult sequence to make as a gBlock, it was ordered as a gene in an ampicillin backbone where it was then digested and ligated into the pSB1C3 backbone.

¹Cameron, G. W., Jordan, K. N., Holt, P. J., Baker, P. B., Lowe, C. R., & Bruce, N. C. (1994). Identification of a heroin esterase in Rhodococcus sp. strain H1. Applied and environmental microbiology, 60(10), 3881-3883.

²Rathbone, D. A., Holt, P. J., Lowe, C. R., & Bruce, N. C. (1997). Molecular analysis of the Rhodococcus sp. strain H1 her gene and characterization of its product, a heroin esterase, expressed in Escherichia coli. Applied and environmental microbiology, 63(5), 2062-2066.

³Sigma-aldrich. 4-nitrophenyl acetate product information.

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Morphine-6-Dehydrogenase BBa_K1615000

The structural gene morphine-6-dehydrogenase (morA) was first isolated from Pseudomonas putida M10 as it is capable of growth with morphine as its sole carbon source¹. Morphine dehydrogenase (MDH) catalyses the oxidation of both morphine and codeine to produce morphinone and codeinone respectively. During this process NADP⁺ is reduced to NADPH which means that this enzyme is frequently used to detect morphine and codeine².

To test the morphine dehydrogenase activity it can be coupled with morphine and NADP⁺ to produce morphinone and NADPH. The amount of NADPH produced can be measured at 340nm. Morphine dehydrogenase with t7 promoter characterised by Edinburgh iGEM team was provided by Prof Chris French. Michealis Menten kinetic analysis was performed giving values of Vmax and Km, 61.22 and 140.5 uM respectively.

Following table summarises the kinetic analysis and statistics of the measurment.

Design: To make this gene standardised it was codon optimised for the chassis Escherichia coli as well as making it RFC25 compatible which required removing all illegal restriction sites in the gene sequence.

¹Bruce, N. C., Wilmot, C. J., Jordan, K. N., Trebilcock, A. E., Stephens, L. D. G., & Lowe, C. R. (1990). Microbial degradation of the morphine alkaloids: identification of morphinone as an intermediate in the metabolism of morphine by Pseudomonas putida M10. Archives of microbiology, 154(5), 465-470.
²Rathbone, D. A., Holt, P. J., Lowe, C. R., & Bruce, N. C. (1997). Molecular analysis of the Rhodococcus sp. strain H1 her gene and characterization of its product, a heroin esterase, expressed in Escherichia coli. Applied and environmental microbiology, 63(5), 2062-2066.
²WALKER, E., et al. "Mechanistic studies of morphine dehydrogenase and stabilization against covalent inactivation." Biochem. J 345 (2000): 687-692.

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Monoamine oxidase A BBa_K1615022

Monoamine oxidase A is coded by the gene maoA and is subject to catabolite and ammonium ion repression¹. Amine oxidases that contain copper/topaquinone (TPQ), like monoamine oxidase A, convert primary amines into their corresponding aldehydes, hydrogen peroxide and ammonia².

To test the activity of monoamine oxidase A, tyramine can be used as a substrate and its corresponding aldehyde as well as ammonia and hydrogen peroxide will be produced. When the hydrogen peroxide is coupled with horseradish peroxidase and Amplex red, resorufin, a red colour, will be produced.

Design: This monoamine oxidase A sequence was found in Klebsiella pneumoniae³ and was codon optimised for the chassis Escherichia coli as well as made RFC25 compatible with the corresponding prefix and suffix and illegal restriction sites were removed.

¹Oka, M., Murooka, Y., & Harada, T. (1980). Genetic control of tyramine oxidase, which is involved in derepressed synthesis of arylsulfatase in Klebsiella aerogenes. Journal of bacteriology, 143(1), 321-327.
²McIntire, W. S., & Hartmann, C. (1993). Copper-containing amine oxidases. Principles and applications of quinoproteins, 97-171.
³Sugino, H., Sasaki, M., Azakami, H., Yamashita, M., & Murooka, Y. (1992). A monoamine-regulated Klebsiella aerogenes operon containing the monoamine oxidase structural gene (maoA) and the maoC gene. Journal of bacteriology, 174(8), 2485-2492.

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                  <h1 class="brand-heading">Basic Parts</h1>
                  <p class="intro-text">
-<br>
-<br>
-<br>
                  </p>
+                <div align="center">
+                    <a href="#accordion">
+                         <span class="arrowtext">Scroll down to read more</span>
+                         <img src="https://static.igem.org/mediawiki/2014/3/3e/Aalto_Helsinki_Nuoli.png" class="arrow">
+                    </a>
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-    <h3 class="panel-title">Panel title</h3>
-  </div>
-</div>
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-% Agarose Gel
+               Heroin Esterase BBa_K1615045
              </a>
            </h4>
          </div>
-         <div id="collapseOne" class="panel-collapse collapse in" role="tabpanel" aria-labelledby="headingOne">
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            <div class="panel-body">
-            <div class="col-md-6">
                <p style="color: black;">
-              <h2>Materials</h2>
+             Heroin esterase, an acetylmorphine carboxylesterase,  was isolated from <i>Rhodococcus erythropolis</i> strain H1 in 1994 from the garden soil at Cambridge and is able to use heroin as its sole carbon and energy source by deacetylating the C-3 and C-6 groups to form morphine<sup>1</sup>. The gene <i>her</i> encodes this enzyme and can be expressed in the chassis <i>Escherichia coli</i><sup>2</sup>. The pH optimum for this enzyme is pH8.5 in bicine buffer<sup>1</sup>.
-              <ul>
+<br>
-                <li>1g Agarose
+<br>
-                <li>100ml 1X TAE buffer
+<img src="https://static.igem.org/mediawiki/2015/b/b1/Edigem15_bparts_her1.jpg" class="img-responsive">
-                <li>5µl GelRed stain
+<br>
-              </ul>
+<br>
-            </p>
+The activity of heroin esterase can be tested using 4-nitrophenyl acetate which is hydrolysed by heroin esterase to form 4-nitrophenol and acetate<sup>3</sup>. This produces a yellow colour which can be read at 410 nm.
-            </div>
+<br>
-            <div class="col-md-6">
+<img src="https://static.igem.org/mediawiki/2015/c/cc/Edigem15_bparts_her2.jpg" class="img-responsive">
-              <p class="text-muted">
+<br>
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Mix the agarose with the 1X TAE buffer in a flask.
-                <li>2. Heat the mixture until all the agarose is dissolved.
-                <li>3. Swirl the flask under cold running water to cool the mixture.
-                <li> 4. Add the gel stain.
-                <li>5. Pour into an assembled gel tray and let it cool.
-              </uL>
-            </p>
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-            <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseTwo" aria-expanded="false" aria-controls="collapseTwo">
-             Agarose Gel Electrophoresis
-            </a>
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-            <div class="col-md-6">
-              <p>
-              <h2>Materials</h2>
-              <ul>
-                <li>1% Agarose
-                <li>1X TAE buffer
-                <li>5X loading dye
-                <li>DNA ladder
-                <li>DNA samples
-              </ul>
-            </p>
-            </div>
-            <div class="col-md-6">
-              <p>
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Place gel tray into the electrophoresis apparatus.
-                <li>2. Pour 1X TAE so that the gel is covered by buffer.
-                <li>3. Prepare the samples by adding the appropriate amount of loading dye.
-                <li>4. Load samples and DNA ladder into wells on the gel.
-                <li>5. Run the gel at roughly 100V for around an hour
-              </uL>
+<img src="https://static.igem.org/mediawiki/2015/c/c1/Hertab1.png" class="img-responsive">
-            </p>
+<br>
-            </div>
+<img src="https://static.igem.org/mediawiki/2015/0/07/Hertab2.png" class="img-responsive">
-          </div>
+<br>
-        </div>
+<img src="https://static.igem.org/mediawiki/2015/9/96/Herest1.jpg" class="img-responsive">
-      </div>
+<br>
-      <div class="panel panel-default">
+<b>Design:</b> The sequence for our enzyme used the original sequence from Rathbone, et al.<sup>2</sup>, which was then codon optimised for <i>E. coli</i>. The RFC25 prefix and suffix were added which required all illegal sites (EcoRI, SpeI, AgeI, NotI, NgoMIV and XbaI) to be removed. As this was a difficult sequence to make as a gBlock, it was ordered as a gene in an ampicillin backbone where it was then digested and ligated into the pSB1C3 backbone.
-        <div class="panel-heading" role="tab" id="headingThree">
+<br>
-          <h4 class="panel-title">
+<br>
-            <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseThree" aria-expanded="false" aria-controls="collapseThree">
+<br>
-              Culture
+<br>
-            </a>
+<sup>1</sup>Cameron, G. W., Jordan, K. N., Holt, P. J., Baker, P. B., Lowe, C. R., & Bruce, N. C. (1994). Identification of a heroin esterase in Rhodococcus sp. strain H1. Applied and environmental microbiology, 60(10), 3881-3883.
-          </h4>
+<br>
-        </div>
+<br><sup>2</sup>Rathbone, D. A., Holt, P. J., Lowe, C. R., & Bruce, N. C. (1997). Molecular analysis of the Rhodococcus sp. strain H1 her gene and characterization of its product, a heroin esterase, expressed in Escherichia coli. <i>Applied and environmental microbiology</i>, 63(5), 2062-2066.
-        <div id="collapseThree" class="panel-collapse collapse" role="tabpanel" aria-labelledby="headingThree">
+<br>
-          <div class="panel-body">
+<br>
-           <div class="col-md-6">
+<sup>3</sup>Sigma-aldrich. 4-nitrophenyl acetate product information.
-              <p>
-              <h2>Materials</h2>
-              <ul>
-                <li>10ml Luria Broth (LB)
-                <li>10µl Specific Antibiotic at 1000x (Chloramphenicol, Ampicillin or Kanamycin)
-                <li>Loop (for picking colony)
-                <li>Ethanol
-              </ul>
-            </p>
-            </div>
-            <div class="col-md-6">
-              <p>
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Pour 10ml of LB into a 50ml Falcon tube.
-                <li>2. Pipette 10µl of antibiotic into the broth.
-                <li>3. Dip loop in ethanol and flame to sterilise. Once it is cool, pick colony and transfer to a 50ml Falcon tube.
-                <li>4. Incubate at 37°C overnight in a shaking incubator.
-              </uL>
-            </p>
-            </div>
-          </div>
-        </div>
-      </div>
-    </div>
-  </div>
-<div class="panel panel-default">
-  <div class="panel-heading">
-    <h3 class="panel-title">Panel title</h3>
-  </div>
-</div>
-    <div class="panel-group" id="accordion" role="tablist" aria-multiselectable="true">
-      <div class="panel panel-default">
-        <div class="panel-heading" role="tab" id="headingOne">
-          <h4 class="panel-title">
-            <a role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseOne" aria-expanded="false" aria-controls="collapseOne">
-% Agarose Gel
-            </a>
-          </h4>
-        </div>
-        <div id="collapseOne" class="panel-collapse collapse in" role="tabpanel" aria-labelledby="headingOne">
-          <div class="panel-body">
-            <div class="col-md-6">
-              <p style="color: black;">
-              <h2>Materials</h2>
-              <ul>
-                <li>1g Agarose
-                <li>100ml 1X TAE buffer
-                <li>5µl GelRed stain
-              </ul>
-            </p>
-            </div>
-            <div class="col-md-6">
-              <p class="text-muted">
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Mix the agarose with the 1X TAE buffer in a flask.
-                <li>2. Heat the mixture until all the agarose is dissolved.
-                <li>3. Swirl the flask under cold running water to cool the mixture.
-                <li> 4. Add the gel stain.
-                <li>5. Pour into an assembled gel tray and let it cool.
-              </uL>
-            </p>
-            </div>
-          </div>
-        </div>
-      </div>
-      <div class="panel panel-default">
-        <div class="panel-heading" role="tab" id="headingTwo">
-          <h4 class="panel-title">
-            <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseTwo" aria-expanded="false" aria-controls="collapseTwo">
-             Agarose Gel Electrophoresis
-            </a>
-          </h4>
-        </div>
-        <div id="collapseTwo" class="panel-collapse collapse" role="tabpanel" aria-labelledby="headingTwo">
-          <div class="panel-body">
-            <div class="col-md-6">
-              <p>
-              <h2>Materials</h2>
-              <ul>
-                <li>1% Agarose
-                <li>1X TAE buffer
-                <li>5X loading dye
-                <li>DNA ladder
-                <li>DNA samples
-              </ul>
-            </p>
-            </div>
-            <div class="col-md-6">
-              <p>
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Place gel tray into the electrophoresis apparatus.
-                <li>2. Pour 1X TAE so that the gel is covered by buffer.
-                <li>3. Prepare the samples by adding the appropriate amount of loading dye.
-                <li>4. Load samples and DNA ladder into wells on the gel.
-                <li>5. Run the gel at roughly 100V for around an hour
-              </uL>
-            </p>
-            </div>
-          </div>
-        </div>
-      </div>
-      <div class="panel panel-default">
-        <div class="panel-heading" role="tab" id="headingThree">
-          <h4 class="panel-title">
-            <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseThree" aria-expanded="false" aria-controls="collapseThree">
-              Culture
-            </a>
-          </h4>
-        </div>
-        <div id="collapseThree" class="panel-collapse collapse" role="tabpanel" aria-labelledby="headingThree">
-          <div class="panel-body">
-           <div class="col-md-6">
-              <p>
-              <h2>Materials</h2>
-              <ul>
-                <li>10ml Luria Broth (LB)
-                <li>10µl Specific Antibiotic at 1000x (Chloramphenicol, Ampicillin or Kanamycin)
-                <li>Loop (for picking colony)
-                <li>Ethanol
                </ul>
              </p>
-            </div>
-            <div class="col-md-6">
-              <p>
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Pour 10ml of LB into a 50ml Falcon tube.
-                <li>2. Pipette 10µl of antibiotic into the broth.
-                <li>3. Dip loop in ethanol and flame to sterilise. Once it is cool, pick colony and transfer to a 50ml Falcon tube.
-                <li>4. Incubate at 37°C overnight in a shaking incubator.
-              </uL>
-            </p>
-            </div>
-          </div>
-        </div>
-      </div>
-       <div class="panel panel-default">
-        <div class="panel-heading" role="tab" id="headingFour">
-          <h4 class="panel-title">
-            <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseFour" aria-expanded="false" aria-controls="collapseFour">
-             Gel Purification using QIAquick Gel Extraction Kit
-            </a>
-          </h4>
-        </div>
-      </div>
-    </div>
-  </div>
-<div class="panel panel-default">
+             <div align="center">
-  <div class="panel-heading">
+                 <a href="#" class="btn btn-primary btn-lg outline" role="button">Check it out in the registry</a>
-    <h3 class="panel-title">Panel title</h3>
+             </div>
-  </div>
-</div>
-    <div class="panel-group" id="accordion" role="tablist" aria-multiselectable="true">
-      <div class="panel panel-default">
-        <div class="panel-heading" role="tab" id="headingOne">
-          <h4 class="panel-title">
-            <a role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseOne" aria-expanded="false" aria-controls="collapseOne">
-% Agarose Gel
-            </a>
-          </h4>
-        </div>
-        <div id="collapseOne" class="panel-collapse collapse in" role="tabpanel" aria-labelledby="headingOne">
-          <div class="panel-body">
-            <div class="col-md-6">
-              <p style="color: black;">
-              <h2>Materials</h2>
-              <ul>
-                <li>1g Agarose
-                <li>100ml 1X TAE buffer
-                <li>5µl GelRed stain
-              </ul>
-            </p>
-            </div>
-            <div class="col-md-6">
-              <p class="text-muted">
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Mix the agarose with the 1X TAE buffer in a flask.
-                <li>2. Heat the mixture until all the agarose is dissolved.
-                <li>3. Swirl the flask under cold running water to cool the mixture.
-                <li> 4. Add the gel stain.
-                <li>5. Pour into an assembled gel tray and let it cool.
-              </uL>
-            </p>
              </div>
            </div>
@@ Line 369: / Line 173: @@
            <h4 class="panel-title">
              <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseTwo" aria-expanded="false" aria-controls="collapseTwo">
-              Agarose Gel Electrophoresis
+              Morphine-6-Dehydrogenase BBa_K1615000
              </a>
            </h4>
@@ Line 375: / Line 179: @@
          <div id="collapseTwo" class="panel-collapse collapse" role="tabpanel" aria-labelledby="headingTwo">
            <div class="panel-body">
-            <div class="col-md-6">
                <p>
-              <h2>Materials</h2>
+               The structural gene morphine-6-dehydrogenase (<i>morA</i>) was first isolated from <i>Pseudomonas putida</i> M10 as it is capable of growth with morphine as its sole carbon source<sup>1</sup>. Morphine dehydrogenase (MDH) catalyses the oxidation of both morphine and codeine to produce morphinone and codeinone respectively. During this process NADP<sup>+</sup> is reduced to NADPH which means that this enzyme is frequently used to detect morphine and codeine<sup>2</sup>.
-              <ul>
+<br>
-                <li>1% Agarose
+<br>
-                <li>1X TAE buffer
+<img src="https://static.igem.org/mediawiki/2015/4/4f/Morphine_dehydrogenase_activity.jpeg" class="img-responsive">
-                <li>5X loading dye
+<br>
-                <li>DNA ladder
+<br>
-                <li>DNA samples
+<br>
-              </ul>
+<br>To test the morphine dehydrogenase activity it can be coupled with morphine and NADP<sup>+</sup> to produce morphinone and NADPH. The amount of NADPH produced can be measured at 340nm. Morphine dehydrogenase with t7 promoter characterised by Edinburgh iGEM team was provided by Prof Chris French. Michealis Menten kinetic analysis was performed giving values of Vmax and Km, 61.22 and 140.5 uM respectively.
-            </p>
+<br>
-            </div>
+<img src="https://static.igem.org/mediawiki/2015/2/2f/Morpg.jpg" class="img-responsive">
-            <div class="col-md-6">
+<br>
-              <p>
+<br>Following table summarises the kinetic analysis and statistics of the measurment.
-              <h2>Procedure</h2>
+<img src="https://static.igem.org/mediawiki/2015/e/e1/Morphgraph.jpg" class="img-responsive">
-              <ul>
+<br>
-                <li>1. Place gel tray into the electrophoresis apparatus.
+<br>
-                <li>2. Pour 1X TAE so that the gel is covered by buffer.
+<b>Design:</b> To make this gene standardised it was codon optimised for the chassis <i>Escherichia coli</i> as well as making it RFC25 compatible which required removing all illegal restriction sites in the gene sequence.
-                <li>3. Prepare the samples by adding the appropriate amount of loading dye.
+<br>
-                <li>4. Load samples and DNA ladder into wells on the gel.
+<br>
-                <li>5. Run the gel at roughly 100V for around an hour
+<br>
+<br>
+<sup>1</sup>Bruce, N. C., Wilmot, C. J., Jordan, K. N., Trebilcock, A. E., Stephens, L. D. G., & Lowe, C. R. (1990). Microbial degradation of the morphine alkaloids: identification of morphinone as an intermediate in the metabolism of morphine by Pseudomonas putida M10. <i>Archives of microbiology</i>, 154(5), 465-470.
+<br><sup>2</sup>Rathbone, D. A., Holt, P. J., Lowe, C. R., & Bruce, N. C. (1997). Molecular analysis of the Rhodococcus sp. strain H1 her gene and characterization of its product, a heroin esterase, expressed in Escherichia coli. <i>Applied and environmental microbiology</i>, 63(5), 2062-2066.
+<br><sup>2</sup>WALKER, E., et al. "Mechanistic studies of morphine dehydrogenase and stabilization against covalent inactivation." Biochem. J 345 (2000): 687-692.
-              </uL>
              </p>
-            </div>
+             <div align="center">
+                 <a href="#" class="btn btn-primary btn-lg outline" role="button">Check it out in the registry</a>
+             </div>
            </div>
          </div>
@@ Line 407: / Line 216: @@
            <h4 class="panel-title">
              <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseThree" aria-expanded="false" aria-controls="collapseThree">
-               Culture
+               Monoamine oxidase A BBa_K1615022
              </a>
            </h4>
@@ Line 413: / Line 222: @@
          <div id="collapseThree" class="panel-collapse collapse" role="tabpanel" aria-labelledby="headingThree">
            <div class="panel-body">
-           <div class="col-md-6">
                <p>
-              <h2>Materials</h2>
+                Monoamine oxidase A is coded by the gene <i>maoA</i> and is subject to catabolite and ammonium ion repression<sup>1</sup>. Amine oxidases that contain copper/topaquinone (TPQ), like monoamine oxidase A, convert primary amines into their corresponding aldehydes, hydrogen peroxide and ammonia<sup>2</sup>.
-              <ul>
+<br>
-                <li>10ml Luria Broth (LB)
+<br>
-                <li>10µl Specific Antibiotic at 1000x (Chloramphenicol, Ampicillin or Kanamycin)
+To test the activity of monoamine oxidase A, tyramine can be used as a substrate and its corresponding aldehyde as well as ammonia and hydrogen peroxide will be produced. When the hydrogen peroxide is coupled with horseradish peroxidase and Amplex red, resorufin, a red colour, will be produced.
-                <li>Loop (for picking colony)
+<br>
-                <li>Ethanol
+<br>
-              </ul>
+Design: This monoamine oxidase A sequence was found in <i>Klebsiella pneumoniae</i><sup>3</sup> and was codon optimised for the chassis Escherichia coli as well as made RFC25 compatible with the corresponding prefix and suffix and illegal restriction sites were removed.
+<br>
+<br>
+<sup>1</sup>Oka, M., Murooka, Y., & Harada, T. (1980). Genetic control of tyramine oxidase, which is involved in derepressed synthesis of arylsulfatase in Klebsiella aerogenes. <i>Journal of bacteriology</i>, 143(1), 321-327.
+<br><sup>2</sup>McIntire, W. S., & Hartmann, C. (1993). Copper-containing amine oxidases. <i>Principles and applications of quinoproteins</i>, 97-171.
+<br><sup>3</sup>Sugino, H., Sasaki, M., Azakami, H., Yamashita, M., & Murooka, Y. (1992). A monoamine-regulated Klebsiella aerogenes operon containing the monoamine oxidase structural gene (maoA) and the maoC gene. <i>Journal of bacteriology</i>, 174(8), 2485-2492.
              </p>
-            </div>
+             <div align="center">
-            <div class="col-md-6">
+                 <a href="#" class="btn btn-primary btn-lg outline" role="button">Check it out in the registry</a>
-              <p>
+             </div>
-              <h2>Procedure</h2>
-              <ul>
-                <li>1. Pour 10ml of LB into a 50ml Falcon tube.
-                <li>2. Pipette 10µl of antibiotic into the broth.
-                <li>3. Dip loop in ethanol and flame to sterilise. Once it is cool, pick colony and transfer to a 50ml Falcon tube.
-                <li>4. Incubate at 37°C overnight in a shaking incubator.
-              </uL>
-            </p>
-            </div>
            </div>
          </div>
        </div>
-       <div class="panel panel-default">
-        <div class="panel-heading" role="tab" id="headingFour">
-          <h4 class="panel-title">
-            <a class="collapsed" role="button" data-toggle="collapse" data-parent="#accordion" href="#collapseFour" aria-expanded="false" aria-controls="collapseFour">
-             Gel Purification using QIAquick Gel Extraction Kit
-            </a>
-          </h4>
-        </div>
-      </div>
-    </div>
-  </div>
-</div>
-      <footer>
-        <p class="pull-right"><a href="#">Back to top</a></p>
-        <p>&copy; 2015 EdiGEM &middot; <a href="#">Privacy</a> &middot; <a href="#">Terms</a></p>
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Difference between revisions of "Team:Edinburgh/Basic Part"

Latest revision as of 18:54, 20 November 2015

Heroin Esterase BBa_K1615045

Morphine-6-Dehydrogenase BBa_K1615000

Monoamine oxidase A BBa_K1615022