Difference between revisions of "Part:BBa K404122"

 
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__NOTOC__
 
__NOTOC__
 
<partinfo>BBa_K404122 short</partinfo>
 
<partinfo>BBa_K404122 short</partinfo>
 +
{| style="color:black; margin: 0px 0px 5px 20px;" cellpadding="6" cellspacing="1" border="2" align="center"
 +
! colspan="2" style="background:#66bbff;"|[https://parts.igem.org/Part:BBa_K404122 AAV2-left-ITR_pCMV_betaglobin_mGMK_TK30_hGH_AAV2-right-ITR]
 +
|-
 +
|'''BioBrick Nr.'''
 +
|[https://parts.igem.org/Part:BBa_K404122 BBa_K404122]
 +
|-
 +
|'''RFC standard'''
 +
|[https://parts.igem.org/Help:Assembly_standard_10 RFC 10]
 +
|-
 +
|'''Requirement'''
 +
|pSB1C3<br>
 +
|-
 +
|'''Source'''
 +
|
 +
|-
 +
|'''Submitted by'''
 +
|[http://2010.igem.org/Team:Freiburg_Bioware FreiGEM 2010]
 +
|}
  
 +
 +
<html>
 +
<h2>Contents</h2>
 +
 +
<p class="MsoToc2"><a href="#_Toc275981841"><span lang="EN-US">Functional Composite Part for Successful Tumor Cell Ablation</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">1</span></a></p>
 +
 +
<p class="MsoToc3"><a href="#_Toc275981842"><span lang="EN-US">Introduction</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">1</span></a></p>
 +
 +
<p class="MsoToc3"><a href="#_Toc275981843"><span lang="EN-US">Successful Assembly
 +
of Vector Plasmids Carrying Suicide Genes via Cloning</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">1</span></a></p>
 +
 +
<p class="MsoToc3"><a href="#_Toc275981844"><span lang="EN-US">Monitoring Efficient
 +
Tumor Killing by Phase-Contrast Microscopy</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">4</span></a></p>
 +
 +
<p class="MsoToc3"><a href="#_Toc275981845"><span lang="EN-US">Quantitative
 +
Analysis of Cell Death by Flow Cytometry</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">6</span></a></p>
 +
 +
<p class="MsoToc3"><a href="#_Toc275981846"><span lang="EN-US">Titrating
 +
Ganciclovir Concentrations for Efficient Cell Killing by Cytotoxicity Assays</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">8</span></a></p>
 +
 +
 +
<p class="MsoToc3"><a href="#_Toc275981848"><span lang="EN-US">Conclusions</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">16</span></a></p>
 +
 +
<p class="MsoToc3"><a href="#_Toc275981849"><span lang="EN-US">References</span><span style="color: windowtext; display: none; text-decoration: none;">. </span><span style="color: windowtext; display: none; text-decoration: none;">16</span></a></p>
 +
 +
<p class="MsoNormal">&nbsp;</p>
 +
 +
<h2><a name="_Toc275981841"><span lang="EN-US">Functional Composite Part for Successful Tumor Cell Ablation</span></a></h2>
 +
 +
<h3><a name="_Toc275981842"><span lang="EN-US">Introduction</span></a></h3>
 +
 +
<p class="MsoNormal"><span lang="EN-US">Gene delivery using viral vectors to
 +
specifically target tumor cells gained increasing attention in the last years
 +
being efficient in combination with suicide gene approaches </span><span lang="EN-US">(Willmon et al. 2006)</span><span lang="EN-US">. Several prodrug/enzyme
 +
combinations have been reported. Two systems - ganciclovir (GCV)/herpes simplex
 +
virus thymidine kinase (HSV-TK) </span><span lang="EN-US">(Ardiani et al. 2010)</span><span lang="EN-US"> and
 +
5-fluorocytosine/cytosine deaminase (CD) </span><span lang="EN-US">(Fuchita et al. 2009a)</span><span lang="EN-US"> – have been widely
 +
used and their therapeutic benefit was demonstrated in preclinical studies </span><span lang="EN-US">(Greco &amp; Dachs 2001)</span><span lang="EN-US">. Adeno-associated
 +
viruses (AAV) as delivery vectors are commonly used in suicide gene therapy. The
 +
suicide gene flanked by the inverted terminal repeats (ITRs) is encapsulated into
 +
the virus particles and delivered to the target cells where suicide gene
 +
expression is mediated by cellular proteins.</span></p>
 +
 +
<p class="MsoNormal"><span lang="EN-US">The iGEM team Freiburg_Bioware 2010 provides
 +
both the cytosine deaminase (CD, BBa_K404112) and an improved guanylate kinase -
 +
thymidine kinase fusion gene (mGMK_TK, <a href = "https://parts.igem.org/Part:BBa_K404113" target="blank" > BBa_K404113</a>) within the Virus
 +
Construction Kit as effective suicide genes. We demonstrate efficient and
 +
specific killing of tumor cells by enzymatic cytotoxicity assays, flow
 +
cytometry, as well as phase contrast microscopy. HT1080 cancer cell lines were
 +
transduced with directed viral particles containing the suicide genes packaged
 +
into the viral capsids. </span></p>
 +
 +
<h3><a name="_Toc275981843"><span lang="EN-US">Successful Assembly of Vector Plasmids
 +
Carrying Suicide Genes via Cloning</span></a></h3>
 +
 +
<p class="MsoNormal"><span lang="EN-US">To create the functional vector plasmids, assembly
 +
of the constructs carrying the suicide genes was performed following the
 +
BioBrick Standard Assembly. All plasmids contain the enhancer-element human <i>beta-globin</i>
 +
intron (<a href = "https://parts.igem.org/Part:BBa_K404107" target="blank" > BBa_K404107</a>) and the <i>human growth hormone</i> terminator signal (hGH,
 +
<a href = "https://parts.igem.org/Part:BBa_K404108" target="blank" > BBa_K404108</a>) flanked by the inverted terminal repeats (ITRs, <a href = "https://parts.igem.org/Part:BBa_K404100" target="blank" > BBa_K404100</a> and
 +
<a href = "https://parts.igem.org/Part:BBa_K404101" target="blank" > BBa_K404101</a>). Assembled suicide genes are either under the control of the CMV
 +
promoter (<a href = "https://parts.igem.org/Part:BBa_J52034" target="blank" > BBa_J52034</a>) or the tumor-specific telomerase promoter phTERT (<a href = "https://parts.igem.org/Part:BBa_K404106" target="blank" > BBa_K404106</a>).
 +
</span></p>
 +
 +
<div align="center">
 +
 +
<table class="MsoTableGrid" style="border: medium none ; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0">
 +
<tbody><tr style="height: 343.9pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 435.8pt; height: 343.9pt;" valign="top" width="581">
 +
  <p class="MsoNormal" style="text-indent: 0cm; page-break-after: avoid;"><img style="width: 581px; height: 394px;" alt="" id="Grafik 9" src="https://static.igem.org/mediawiki/2010/9/9b/Freiburg10_BBA_overview_suicide.png"></p>
 +
  <p class="MsoCaption"><a name="_Ref275976895"><span lang="EN-US">Figure </span></a><span lang="EN-US">1</span><span lang="EN-US">: BioBrick-compatible assembly of functional
 +
  vector plasmids containing the suicide genes. The schematic figure shows the
 +
  cloning strategy of the guanylate kinase – thymidine kinase fusion gene
 +
  (mGMK_TK30).</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 +
</html>
 
[[Image:Freiburg10_Vectorplasmid composite 4.png|thumb|center|480px]]<br>
 
[[Image:Freiburg10_Vectorplasmid composite 4.png|thumb|center|480px]]<br>
<h2>ITRs</h2><br>
+
<html>
 +
 
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">To enable modularization of the thymidine
 +
kinase mutants TK30 and SR39 (<a href = "https://parts.igem.org/Part:BBa_K404109" target="blank" > BBa_K404109</a> and <a href = "https://parts.igem.org/Part:BBa_K404110" target="blank" > BBa_K404110</a>) according to the
 +
BioBrick standard, the fusion genes mGMK_TK30 and mGMK_SR39 (<a href = "https://parts.igem.org/Part:BBa_K404113" target="blank" > BBa_K404113</a> and </span><span style="line-height: 200%; color: black;" lang="EN-US"><a href = "https://parts.igem.org/Part:BBa_K404315" target="blank" > BBa_K404315</a></span><span lang="EN-US">) and CD (</span><span style="line-height: 200%; color: black;" lang="EN-US"><a href = "https://parts.igem.org/Part:BBa_K404112" target="blank" > BBa_K404112</a></span><span lang="EN-US">) were modified using the QuikChange
 +
Lightning Site-Directed Mutagenesis Kit (Stratagene) for deletion of iGEM RFC10
 +
pre- and suffix restriction sites. </span><span lang="EN-US">Figure 2</span><span lang="EN-US"> demonstrates one example of
 +
successful deletion of a PstI restriction site located within the mGMK_TK30
 +
sequence at position 3109. A point mutation was introduced replacing the
 +
nucleotide G by A, resulting in the deletion of the restriction site while
 +
maintaining the encoded amino acid glutamine. Exchange of guanine to adenine
 +
was confirmed by sequencing (</span><span lang="EN-US">Figure 2</span><span lang="EN-US">). </span></p>
 +
 
 +
<div align="center">
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; width: 479.55pt; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0" width="639">
 +
<tbody><tr style="height: 179.55pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 479.55pt; height: 179.55pt;" valign="top" width="639">
 +
  <p class="MsoNormal" style="text-indent: 0cm; page-break-after: avoid;"><img style="width: 635px; height: 328px;" alt="" id="Grafik 81" src="https://static.igem.org/mediawiki/2010/3/32/Freiburg10_SDM_mGMK_TK30.png"></p>
 +
  <p class="MsoCaption"><a name="_Ref275976917"><span lang="EN-US">Figure </span></a><span lang="EN-US">2</span><span lang="EN-US">: Cytosine to guanine exchange by
 +
  site-directed mutagenesis using QuikChange Lightning Kit provided by
 +
  Stratagene was successful as demonstrated by (A) test digestion linearizing
 +
  the plasmid with PstI and (B) by sequencing.</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Furthermore, assembly of BioBrick-compatible
 +
vector plasmids was performed. An example for the last assembly step of
 +
mGMK_TK30 and hGH_rITR is shown in </span><span lang="EN-US">Figure 3</span><span lang="EN-US">. The plasmids were digested with
 +
both XbaI and PstI (New England Biolabs, Insert: <a href = "https://parts.igem.org/Part:BBa_K404116" target="blank" > BBa_K404116</a>: hGH_rITR) or SpeI
 +
and PstI (Vector) and loaded on an agarose gel. As demonstrated in the preparative
 +
gel in </span><span lang="EN-US">Figure 3</span><span lang="EN-US">, the expected
 +
bands were detected under UV light and the extracted, subsequently purified DNA
 +
was successfully ligated and transformed into <i>E. coli</i>. Each assembly
 +
step for producing the BioBricks was conducted following the iGEM BioBrick
 +
standard.</span></p>
 +
 
 +
<div align="center">
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; width: 387.35pt; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0" width="516">
 +
<tbody><tr style="height: 125.95pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 387.35pt; height: 125.95pt;" valign="top" width="516">
 +
  <p class="MsoNormal" style="text-indent: 0cm; page-break-after: avoid;"><img style="width: 519px; height: 189px;" alt="" id="Grafik 28" src="https://static.igem.org/mediawiki/2010/f/f2/Freiburg10_Cloning_mGMK_TK30_Arming.png"></p>
 +
  <p class="MsoCaption"><a name="_Ref275976959"><span lang="EN-US">Figure </span></a><span lang="EN-US">3</span><span lang="EN-US">: Assembly of mGMK_TK30 (vector molecule, in
 +
  pSB1C3) and hGH-terminator_rightITR (insert molecule). The digested fragments
 +
  were visualized under UV-light and correspond to the expected sizes.</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<h3><a name="_Toc275981844"><span lang="EN-US">Monitoring Efficient Tumor Killing
 +
by Phase-Contrast Microscopy</span></a></h3>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Tumor cells, transduced with viral
 +
particles encapsidating the effector constructs containing the mGMK_TK30 driven
 +
by the CMV promoter, were cultured both in presence and absence of ganciclovir
 +
(Roche). Morphological changes were monitored via phase-contrast microscopy for
 +
48 hours post infection. As it can be seen in </span><span lang="EN-US">Figure 4</span><span lang="EN-US">, non-transduced tumor cells treated
 +
with ganciclovir and transduced cells without ganciclovir did not show
 +
significant cell ablation. In contrast, transduced cells expressing the
 +
guanylate kinase - thymidine kinase fusion protein showed significant cell
 +
death after incubation with ganciclovir for 48 hours post infection. </span></p>
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; width: 491pt; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0" width="655">
 +
<tbody><tr style="height: 188.8pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 247.35pt; height: 188.8pt;" width="330">
 +
  <p class="MsoNoSpacing"><b><span lang="EN-US">A</span></b><span lang="EN-US"> </span><img style="width: 318px; height: 238px;" id="Grafik 1" src="https://static.igem.org/mediawiki/2010/4/4f/Freiburg10_Microscopy_Arming_A.png" alt="Beschreibung: https://static.igem.org/mediawiki/2010/3/3e/HT_negativ_control_ganciclovir_only.jpg"></p>
 +
  </td>
 +
  <td style="padding: 0cm 5.4pt; width: 243.65pt; height: 188.8pt;" width="325">
 +
  <p class="MsoNoSpacing"><b><span lang="EN-US">B</span></b><span lang="EN-US"> </span><img style="width: 318px; height: 238px;" id="Grafik 2" src="https://static.igem.org/mediawiki/2010/e/e8/Freiburg10_Microscopy_Arming_B.png" alt="Beschreibung: https://static.igem.org/mediawiki/2010/f/f0/HT_TKGMK_clone_1_ohne_Ganciclovir_300%C2%B5l.jpg"></p>
 +
  </td>
 +
</tr>
 +
<tr style="height: 188.8pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 247.35pt; height: 188.8pt;" width="330">
 +
  <p class="MsoNoSpacing"><b><span lang="EN-US">C</span></b><span lang="EN-US"> </span></p>
 +
  <p class="MsoNoSpacing" style="page-break-after: avoid;"><img style="width: 318px; height: 239px;" id="Grafik 3" src="https://static.igem.org/mediawiki/2010/a/ac/Freiburg10_Microscopy_Arming_C.png" alt="Beschreibung: https://static.igem.org/mediawiki/2010/c/c3/HT_TKGMK_clone_1_with_ganciclovir_300%C2%B5l.jpg"></p>
 +
  </td>
 +
  <td style="padding: 0cm 5.4pt; width: 243.65pt; height: 188.8pt;" width="325">
 +
  <p class="MsoNoSpacing"><b><span lang="EN-US">D</span></b><span lang="EN-US"> </span><img style="width: 318px; height: 238px;" id="Grafik 4" src="https://static.igem.org/mediawiki/2010/d/df/Freiburg10_Microscopy_Arming_D.png" alt="Beschreibung: https://static.igem.org/mediawiki/2010/7/73/HT_TKGMK_clone_1_with_ganciclovir_600%C2%B5l_well_2.jpg"></p>
 +
  </td>
 +
</tr>
 +
<tr style="height: 34.2pt;">
 +
  <td colspan="2" style="padding: 0cm 5.4pt; width: 491pt; height: 34.2pt;" width="655">
 +
  <p class="MsoCaption"><a name="_Ref275976998"><span lang="EN-US">Figure </span></a><span lang="EN-US">4</span><span lang="EN-US">: Qualitative analysis of cell death induced
 +
  by conversion of ganciclovir to ganciclovir-triphosphate by virus-delivered
 +
  guanylate - thymidine kinase (mGMK_TK30). A: Non-transduced HT1080 cells
 +
  incubated in the presence of ganciclovir not exhibiting cell death. B: Untreated
 +
  transduced HT1080 cells showing a high survival rate. C: HT1080 cells
 +
  transduced with 300 µL viral particles and incubated with ganciclovir leading
 +
  to tumor cell ablation. D: HT1080 cells transduced with 600 µL viral
 +
  particles and incubated with ganciclovir leading to ablation of tumor cells. </span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Suicide gene therapy is based on the localized
 +
conversion of non-toxic prodrugs to toxic substances </span><span lang="EN-US">(Greco &amp; Dachs 2001)</span><span lang="EN-US">, promoting cell
 +
death in the tumor tissue (</span><span lang="EN-US">Figure 5</span><span lang="EN-US">). Directed gene delivery is achieved by using recombinant viral
 +
vectors as provided by the iGEM team Freiburg_Bioware 2010 within the Virus
 +
Construction Kit.</span></p>
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; border-collapse: collapse; margin-left: 4.8pt; margin-right: 4.8pt;" align="left" border="0" cellpadding="0" cellspacing="0">
 +
<tbody><tr style="height: 174.85pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 447.8pt; height: 174.85pt;" valign="top" width="597">
 +
  <p class="MsoNormal" style="text-indent: 0cm; page-break-after: avoid;"><span style="position: relative; z-index: 251659264; left: -1px; top: 0px; width: 583px; height: 271px;"><img style="width: 597px; height: 279px;" alt="" src="https://static.igem.org/mediawiki/2010/a/a4/Freiburg10_overview_GDEPT.png"></span><br clear="all">
 +
  </p>
 +
  <p class="MsoCaption"><a name="_Ref275977093"><span lang="EN-US">Figure </span></a><span lang="EN-US">5</span><span lang="EN-US">: Overview of the suicide gene therapy
 +
  approach. Non-toxic prodrugs are converted into toxic effector molecules
 +
  leading to cell death of the tumor cells. </span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Non-transduced cells can survive in the
 +
presence of ganciclovir since the prodrug is not toxic for these cells (</span><span lang="EN-US">Figure 4</span><span lang="EN-US">A). </span>The demonstration that
 +
transduced cells are viable in the absence of ganciclovir confirms that cell
 +
killing is indeed induced by combination of the delivered thymidine kinase and
 +
treatment with ganciclovir. Viral particles encapsidating the suicide construct
 +
mGMK_TK30 are efficient in directed gene delivery, thus leading to cell death
 +
of transduced cells due to overexpression of mGMK_TK30 and prodrug conversion. The
 +
cell-toxic ganciclovir-triphosphate is incorporated into the<span lang="EN-US">
 +
nascent DNA chain leading to replication termination and finally resulting in
 +
death of dividing cells. </span></p>
 +
<br />
 +
<br />
 +
<br />
 +
<br />
 +
<h3><a name="_Toc275981845"><span lang="EN-US">Quantitative Analysis of Cell
 +
Death by Flow Cytometry</span></a></h3>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Quantitative analysis of the cytotoxic
 +
effect induced by mGMK_TK30 was first conducted by flow cytometry analysis 72 hours
 +
post transduction. HT1080 cells were stained with 7-AAD and Annexin V. 7-AAD intercalates
 +
in double-stranded DNA after penetrating cell membranes of dead cells, whereas
 +
Annexin V specifically binds phosphatidylserine which is only accessible during
 +
apoptosis. </span><span lang="EN-US">Figure 6</span><span lang="EN-US"> demonstrates
 +
the relation between cell death and ganciclovir concentration.</span></p>
 +
 
 +
<div align="center">
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; width: 477.6pt; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0" width="637">
 +
<tbody><tr style="height: 248.5pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 241.8pt; height: 248.5pt;" valign="top" width="322">
 +
  <p class="MsoNormal" style="text-indent: 0cm; page-break-after: avoid;"><img style="width: 341px; height: 321px;" alt="" id="Grafik 24" src="https://static.igem.org/mediawiki/2010/9/9d/Freiburg10_FACS_A_D.png"></p>
 +
  </td>
 +
  <td style="padding: 0cm 5.4pt; width: 235.8pt; height: 248.5pt;" valign="top" width="314">
 +
  <p class="MsoNormal" style="text-indent: 0cm; page-break-after: avoid;"><img style="width: 300px; height: 326px;" alt="" id="Grafik 36" src="https://static.igem.org/mediawiki/2010/0/0b/Freiburg10_FACS_E_H.png"></p>
 +
  <p class="MsoCaption">&nbsp;</p>
 +
  </td>
 +
</tr>
 +
<tr style="height: 38pt;">
 +
  <td colspan="2" style="padding: 0cm 5.4pt; width: 477.6pt; height: 38pt;" valign="top" width="637">
 +
  <p class="MsoCaption" style="text-indent: 0cm;"><a name="_Ref275977177"><span lang="EN-US">Figure </span></a><span lang="EN-US">6</span><span lang="EN-US">: Flow
 +
  cytometry data analysis. </span><span lang="EN-US">A: Gating non-transduced
 +
  HT1080 cells (control). B: Non-transduced cells without staining plotted
 +
  against 7-AAD. C: Gating non-transduced cells stained with 7-AAD. D:
 +
  Non-transduced, 7-AAD-stained cells plotted against 7-AAD. E: Gating
 +
  transduced cells (GOI: mGMK_TK30) treated with 485 µM ganciclovir. F: Gated,
 +
  Annexin-V stained cells plotted against AnnV-2 Log.&nbsp; G: Gated cells&nbsp; plotted
 +
  against 7-AAD H: Gated, 7-AAD and Annexin-V stained cells plotted against
 +
  7-AAD and Annexin-V. Gate R19 comprised Annexin-V and 7-AAD positive cells.</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal" style="text-align: center; text-indent: 0cm;" align="center"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<div align="center">
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0">
 +
<tbody><tr>
 +
  <td style="padding: 0cm 5.4pt; width: 460.6pt;" valign="top" width="614">
 +
  <p class="MsoNormal" style="text-align: center; text-indent: 0cm; page-break-after: avoid;" align="center"><img style="width: 614px; height: 424px;" alt="" id="Diagramm 8" src="https://static.igem.org/mediawiki/2010/2/29/Freiburg10_Diagram_mGMK_effectFACS.png"></p>
 +
  <p class="MsoCaption"><a name="_Ref275977227"><span lang="EN-US">Figure </span></a><span lang="EN-US">7</span><span lang="EN-US">: Quantification of flow cytometry data
 +
  provided in </span><span lang="EN-US">Figure 6</span><span lang="EN-US">. With
 +
  increasing ganciclovir concentration, the survival rate of cells decreases. 60
 +
  % of HT1080 cells treated with 4.85 mM ganciclovir show tumor ablation,
 +
  however even lower amounts of ganciclovir lead to significant cell death.</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-align: center; text-indent: 0cm;" align="center"><span lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">The effect of different ganciclovir
 +
concentrations on transduced HT1080 sarcoma cells was investigated.
 +
Transduction was performed with recombinant viral particles encapsidating the
 +
mGMK_TK30 prodrug gene. 72 hours post infection, cells were stained with 7-AAD
 +
and Annexin V. As </span><span lang="EN-US">Figure 7</span><span lang="EN-US"> shows,
 +
the fraction of killed transduced cells is proportional to the applied ganciclovir
 +
concentration.</span></p>
 +
 
 +
<h3><a name="_Toc275981846"><span lang="EN-US">Titrating Ganciclovir
 +
Concentrations for Efficient Cell Killing by Cytotoxicity Assays</span></a></h3>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Further analysis of the cytotoxic effect
 +
induced by thymidine kinase converting ganciclovir to the toxic anti-metabolite
 +
has been performed using MTT assays. 3-(4,5-Dimethylthiazol-2-yl)-2,5diphenyltetrazolium
 +
bromide), also known as MTT, is a yellow-colored tetrazole, which is reduced to
 +
purple insoluble formazan in the presence of NADH and NADPH </span><span lang="EN-US">(Roche n.d.)</span><span lang="EN-US">. Colorimetric analysis can be
 +
carried out via spectrometry. Different tumor cell lines, HT1080 and A431, were
 +
transduced with the recombinant viruses carrying the linear DNA construct
 +
coding for mGMK-TK30 regulated by the CMV promoter and subsequently treated
 +
with ganciclovir. 48 and 72 hours post infection, cells were incubated with MTT
 +
and fresh DMEM. After cell lysis by DMSO, absorbance of formazan at 570 nm was
 +
quantified using a Tecan Sunrise plate reader. </span></p>
 +
 
 +
<div align="center">
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; width: 451.05pt; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0" width="601">
 +
<tbody><tr style="height: 176.7pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 451.05pt; height: 176.7pt;" valign="top" width="601">
 +
  <p class="MsoNormal" style="text-indent: 0cm;"><b><span lang="EN-US">A</span></b><img style="width: 588px; height: 413px;" alt="" id="Diagramm 95" src="https://static.igem.org/mediawiki/2010/8/86/Freiburg10_MTT_72h_2d.png"></p>
 +
  </td>
 +
</tr>
 +
<tr style="height: 176.7pt;">
 +
  <td style="padding: 0cm 3.5pt; width: 451.05pt; height: 176.7pt;" valign="top" width="601">
 +
  <p class="MsoNormal" style="text-indent: 0cm;"><b>B</b> </p>
 +
  <p class="MsoNormal" style="text-align: center; text-indent: 0cm; page-break-after: avoid;" align="center"><img style="width: 593px; height: 409px;" alt="" id="Diagramm 10" src="https://static.igem.org/mediawiki/2010/7/76/Freiburg10_MTT_72h_3d.png"></p>
 +
  <p class="MsoCaption"><a name="_Ref275977309"><span lang="EN-US">Figure </span></a><span lang="EN-US">8</span><span lang="EN-US">: Effect of ganciclovir on HT1080 cell survival
 +
  72 hours post infection as (A) two dimensional plot of survival of cells and
 +
  (B) three-dimensional plot of ganciclovir, virus particles and cell survival.</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span style="font-size: 8pt; line-height: 200%;" lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span style="font-size: 8pt; line-height: 200%;" lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span style="font-size: 8pt; line-height: 200%;" lang="EN-US">&nbsp;</span></p>
 +
 
 +
<div align="center">
 +
 
 +
<table class="MsoTableGrid" style="border: medium none ; width: 415pt; border-collapse: collapse;" border="0" cellpadding="0" cellspacing="0" width="553">
 +
<tbody><tr style="height: 176.7pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 415pt; height: 176.7pt;" valign="top" width="553">
 +
  <p class="MsoNormal" style="text-indent: 0cm;"><b><span lang="EN-US">A </span></b><span lang="EN-US">&nbsp;</span></p>
 +
  <p class="MsoNormal" style="text-align: center; text-indent: 0cm;" align="center"><img style="width: 607px; height: 427px;" alt="" id="Diagramm 1154" src="https://static.igem.org/mediawiki/2010/2/2a/Freiburg10_MTT_96h_2d.png"></p>
 +
  </td>
 +
</tr>
 +
<tr style="height: 176.7pt;">
 +
  <td style="padding: 0cm 5.4pt; width: 415pt; height: 176.7pt;" valign="top" width="553">
 +
  <p class="MsoNormal" style="text-indent: 0cm;"><b>B</b></p>
 +
  <p class="MsoNormal" style="text-align: center; text-indent: 0cm; page-break-after: avoid;" align="center"><img style="width: 607px; height: 481px;" alt="" id="Diagramm 1156" src="https://static.igem.org/mediawiki/2010/0/0a/Freiburg10_MTT_96h_3d.png"></p>
 +
  <p class="MsoCaption"><a name="_Ref275977314"><span lang="EN-US">Figure </span></a><span lang="EN-US">9</span><span lang="EN-US">: Effect of ganciclovir on HT1080 cell survival
 +
  96 hours post infection. (A) two dimensional plot of cell survival&nbsp; (B)
 +
  three-dimensional plot of ganciclovir, virus particles and cell survival.</span></p>
 +
  </td>
 +
</tr>
 +
</tbody></table>
 +
 
 +
</div>
 +
 
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span style="font-size: 8pt; line-height: 200%;" lang="EN-US">&nbsp;</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Data of MTT assay quantification are shown
 +
in </span><span lang="EN-US">Figure 8</span><span lang="EN-US"> and </span><span lang="EN-US">Figure 9</span><span lang="EN-US">. HT1080 cells were infected with
 +
viral particles containing the mGMK_TK30 transgene. &nbsp;72 h- and 96 h post
 +
infection and addition of ganciclovir, cells were incubated with MTT. Changes
 +
in absorbance were measured and survival of cells plotted against ganciclovir
 +
concentration. </span><span lang="EN-US">Figure 8</span><span lang="EN-US">A
 +
demonstrates the correlation between increasing ganciclovir concentrations and
 +
percentage of cell survival. Furthermore, different virus particle
 +
concentrations were used for transduction. </span><span lang="EN-US">Figure 8</span><span lang="EN-US">B shows that the highest amount of
 +
viral particles combined with the highest ganciclovir concentration led to
 +
significant HT1080 apoptosis 72 hours post transduction.</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Additionally, 96 hours post infection cells
 +
were incubated with MTT and absorbance was quantified via spectrometry (</span><span lang="EN-US">Figure 9</span><span lang="EN-US">). Again, survival of HT1080 cells
 +
was plotted against increasing ganciclovir concentrations. </span></p>
 +
 
 +
 
 +
<h3><a name="_Toc275981848"><span lang="EN-US">Conclusions</span></a></h3>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">Efficient and tissue-specific tumor killing
 +
is one major challenge in cancer therapy </span><span lang="EN-US">(Black et al. 1996)</span><span lang="EN-US">. Gene-directed enzyme
 +
prodrug therapy (GDEPT) is based on the conversion of non-toxic substances into
 +
toxic drugs resulting in tumor cell death. The iGEM team Freiburg_Bioware 2010
 +
provides several functional suicide genes within the Virus Construction Kit, thus
 +
offering a feasible and modular tool to the growing field of personalized
 +
medicine and the iGEM community. We successfully demonstrated cancer cell death
 +
caused by the introduction of modified fusion genes
 +
consisting of guanylate and thymidine kinases.</span></p>
 +
 
 +
<p class="MsoNormal"><span lang="EN-US">&nbsp;To prevent systemic toxic side effects of
 +
conventional chemotherapy, the iGEM team Freiburg_Bioware 2010 took a leap and
 +
efficiently retargeted the viral vector for directed suicide gene delivery
 +
towards tumor cells. Capsid engineering was successfully demonstrated by the
 +
iGEM team Freiburg_Bioware 2010. Further details can be found under  <a href="http://2010.igem.org/Team:Freiburg_Bioware/Project/Results#targeting">iGEM wiki Freiburg_Bioware 2010 - Results - Targeting</a>
 +
</span></p>
 +
 
 +
 
 +
 
 +
<p><span lang="EN-US">&nbsp;</span></p>
 +
</html>
 +
<h2>Individual components of the assembled vector plasmid </h2>
 +
<h3>ITRs</h3><br>
 
<html>
 
<html>
 
<center>
 
<center>
 
<img src=https://static.igem.org/mediawiki/2010/8/88/Freiburg10_organization_ITRs.png width=400>
 
<img src=https://static.igem.org/mediawiki/2010/8/88/Freiburg10_organization_ITRs.png width=400>
 +
<p>Figure 10: ITR details </p>
 
</center>
 
</center>
 
</html><br>
 
</html><br>
 
The inverted terminal repeat structures can be subdivided into several palindromic motives: A and A’ form a stem loop which encases B and B’ as well as C and C’. Those motives form both arms of the T-shaped structure. The functional motives on the ITR are two regions that bind Rep 68/78, called Rep-binding elements (RBE on the stem and RBE’ on the B arm) and the terminal resolution site (trs) in which the rep proteins introduce single-stranded nicks. The 3’ OH end of the A motive acts as a primer for DNA replication (Im & Muzyczka, 1990) (Lusby, Fife, & Berns, 1980).
 
The inverted terminal repeat structures can be subdivided into several palindromic motives: A and A’ form a stem loop which encases B and B’ as well as C and C’. Those motives form both arms of the T-shaped structure. The functional motives on the ITR are two regions that bind Rep 68/78, called Rep-binding elements (RBE on the stem and RBE’ on the B arm) and the terminal resolution site (trs) in which the rep proteins introduce single-stranded nicks. The 3’ OH end of the A motive acts as a primer for DNA replication (Im & Muzyczka, 1990) (Lusby, Fife, & Berns, 1980).
<h2>CMV promoter</h2><br>
 
 
<h2>Beta-globin-intron</h2><br>
 
<h2>Beta-globin-intron</h2><br>
 
<html>
 
<html>
 
<center>
 
<center>
 
<img src=https://static.igem.org/mediawiki/2010/7/7c/Freiburg10_FACS_betaglobin.png width=400>
 
<img src=https://static.igem.org/mediawiki/2010/7/7c/Freiburg10_FACS_betaglobin.png width=400>
 +
<p>Figure 11 A: FACS data </p>
 
</center>
 
</center>
 
</html><br>
 
</html><br>
Line 20: Line 439:
 
<center>
 
<center>
 
<img src=https://static.igem.org/mediawiki/2010/2/26/Freiburg10_Diagram_betaglobin.png.png width=400>
 
<img src=https://static.igem.org/mediawiki/2010/2/26/Freiburg10_Diagram_betaglobin.png.png width=400>
 +
<p>Figure 11 B: Calculated percentage of mVenus expressing cells</p>
 
</center>
 
</center>
 
</html><br>
 
</html><br>
  
The beta-globin intron BioBrick consists of a partial chimeric CMV promoter followed by the intron II of the beta-globin gene. The 3´end of the intron is fused to the first 25 bases of human beta globin gene exon 3. The beta globin intron BioBrick is assumed to enhance eukaryotic gene expression (Nott, Meislin, & Moore, 2003). As shown in Figure 9 and Figure 10 the vectorplasmid missing the beta-globin intron showed a negligible difference in mVenus expression compared to viral genomes containing the beta-globin intron. Considering these results and taking into account that a constant volume of viral particles has been used for transduction, the difference between the construct containing and lacking the beta-globin intron is minimal. Since packaging efficiency of the AAV-2 decreases with increasing sizes of the insert (Dong, Fan, & Frizzell, 1996), the iGEM team Freiburg_Bioware suggests using the beta-globin intron in dependence on the size of your transgene.
+
The beta-globin intron BioBrick consists of a partial chimeric CMV promoter followed by the intron II of the beta-globin gene. The 3´end of the intron is fused to the first 25 bases of human beta globin gene exon 3. The beta globin intron BioBrick is assumed to enhance eukaryotic gene expression (Nott, Meislin, & Moore, 2003). As shown in Figure 11 A and B the vectorplasmid missing the beta-globin intron showed a negligible difference in mVenus expression compared to viral genomes containing the beta-globin intron. Considering these results and taking into account that a constant volume of viral particles has been used for transduction, the difference between the construct containing and lacking the beta-globin intron is minimal. Since packaging efficiency of the AAV-2 decreases with increasing sizes of the insert (Dong, Fan, & Frizzell, 1996), the iGEM team Freiburg_Bioware suggests using the beta-globin intron in dependence on the size of your transgene.
 
<h2>mGMK_TK30 fusion protein</h2><br>
 
<h2>mGMK_TK30 fusion protein</h2><br>
 
The thymidine kinase mutant TK30 contains six modified amino acids (Black, Newcomb, Wilson, & Loeb, 1996) created in a first screening showing enhanced affinity for gancivlocir and acyclovir, but reduced specificity for its natural substrate thymidine.<br><br>
 
The thymidine kinase mutant TK30 contains six modified amino acids (Black, Newcomb, Wilson, & Loeb, 1996) created in a first screening showing enhanced affinity for gancivlocir and acyclovir, but reduced specificity for its natural substrate thymidine.<br><br>
 
As efficient tumor killing and therefore ganciclovir activation is essential for successful tumor ablation, further improvements were conducted. Overexpression of transgenic thymidine kinase leads to accumulation of non-toxic intermediates, which cannot be phosphorylated sufficiently by endogenous guanylate kinase, the second enzyme in the salvage pathway of nucleotides. <br>
 
As efficient tumor killing and therefore ganciclovir activation is essential for successful tumor ablation, further improvements were conducted. Overexpression of transgenic thymidine kinase leads to accumulation of non-toxic intermediates, which cannot be phosphorylated sufficiently by endogenous guanylate kinase, the second enzyme in the salvage pathway of nucleotides. <br>
 
Overcoming this bottleneck was accomplished by fusing the mouse guanylate kinase (mGMK) to the N-terminus of TK30 mutant creating a fusion protein (mGMK_TK30) with enhanced GCV/ACV sensitivity in vitro and in vivo (Ardiani, Sanchez-Bonilla, & Black, 2010) and improved bystander activity. The effect of non-transfected tumor cell killing upon transfer of toxic metabolites through gap junctional intercellular communication (GJIC) or immune-mediated tumor ablation is essential in suicide gene therapy (Pope, 1997). GCV-triphosphate is mainly transported through the central pore formed between connexin proteins from neighboring cells (Gentry, Im, Boucher, Ruch, & Shewach, 2005), but immune-induced bystander effect seems to be likely as well (Grignet-Debrus, Cool, Baudson, Velu, & Calberg-Bacq, 2000). <br>
 
Overcoming this bottleneck was accomplished by fusing the mouse guanylate kinase (mGMK) to the N-terminus of TK30 mutant creating a fusion protein (mGMK_TK30) with enhanced GCV/ACV sensitivity in vitro and in vivo (Ardiani, Sanchez-Bonilla, & Black, 2010) and improved bystander activity. The effect of non-transfected tumor cell killing upon transfer of toxic metabolites through gap junctional intercellular communication (GJIC) or immune-mediated tumor ablation is essential in suicide gene therapy (Pope, 1997). GCV-triphosphate is mainly transported through the central pore formed between connexin proteins from neighboring cells (Gentry, Im, Boucher, Ruch, & Shewach, 2005), but immune-induced bystander effect seems to be likely as well (Grignet-Debrus, Cool, Baudson, Velu, & Calberg-Bacq, 2000). <br>
<h2>hGH</h2><br>
 
  
 +
 +
<html>
 +
<h3> hGH termination signal</h3>
 +
<p style="margin-right:100px" align="justify">
 +
Recombinant AAV genomes were engineered containing the inverted terminal repeats (ITRs), a strong eukaryotic promoter and mVenus as gene of interest with and without the hGH terminator signal. Transduction of HT1080 cells with viral particles containing the rAAV genomes and measuring mVenus expression 24-hours post infection by flow cytometry demonstrated that transgene expression of the constructs lacking the hGH termination signal is significantly reduced. The iGEM team Freiburg_Bioware 2010 therefore suggests using the provided hGH termination signal within the Virus Construction Kit for optimal gene expression.
 +
</p>
 +
<p class="MsoNormal" style="text-indent: 0cm;"><span lang="EN-US">&nbsp;</span></p>
 +
<p class="MsoNormal" style="text-align:justify;"><span lang="EN-US">Since cloning does not confirm
 +
biological
 +
activity, we analyzed the plasmids and their functional components, hGH
 +
terminator and <i>beta-globin</i> intron, in cell culture. Assembled
 +
plasmids
 +
have been cotransfected, using AAV-293 cells, which provide the stable
 +
integrated E1A and E1B genes, with helper plasmids required for capsid
 +
assembly and genome encapsidation (pRC and pHelper) in a molar ratio of
 +
1:1:1
 +
(pGOI:pRC:pHelper). Virus particles containing the single stranded DNA
 +
were
 +
harvested 72-hours post transfection and HT1080 cells transduced with
 +
constant
 +
volumes of viral vectors. 48-hours post infection; transduced cells
 +
expressing
 +
the gene of interest were analyzed by flow cytometry.</span></p>
 +
 +
</span><p style="text-align:justify;">
 +
Recombinant vectorplasmids
 +
were engineered containing the inverted terminal repeats (ITRs), a
 +
strong
 +
eukaryotic promoter (CMV promoter: BBa_K404102) and mVenus as gene of
 +
interest
 +
with and without the hGH terminator signal. Transduction of HT1080
 +
cells with constant
 +
volume of viral particles containing the vectorplasmids and measuring
 +
mVenus
 +
expression 24-hours post infection by flow cytometry demonstrated that
 +
transgene expression of the constructs lacking the hGH termination
 +
signal is
 +
significantly reduced as shown in </span>
 +
<span
 +
lang="EN-US"> confirming the expected results
 +
that hGH is essential for mRNA processing. The iGEM team
 +
Freiburg_Bioware 2010
 +
therefore suggests using the provided hGH termination signal within the
 +
Virus
 +
Construction Kit for optimal gene expression.</p>
 +
<table class="MsoTableGrid"
 +
style="border: medium none ; border-collapse: collapse;" border="0"
 +
cellpadding="0" cellspacing="0">
 +
</p>
 +
 +
 +
<table>
 +
<tr>
 +
<td style="width: 400px; height: auto;"><img src="https://static.igem.org/mediawiki/parts/c/c7/Freiburg10_FACS_woHGH.png" style="width: 400px; height: auto;"/></td>
 +
<td style="width: 400px;"><img src="https://static.igem.org/mediawiki/parts/7/70/Freiburg10_FACS_withHGH.png"  style="width: 400px; height: auto;"/></td>
 +
</tr>
 +
<tr>
 +
<td style="width: 400px; vertical-align: top;">Figure 12: Flow cytometry analysis of vectorplasmid without (left) and with (right) hGH. For viral particle production, AAV-293 cells were transfected with the reassembled vector plasmid (BBa_K404119) or the reference plasmid, respectively.<br />A: Gating non transduced cells (control); subcellular debris and cellular aggreates can be distinguished from single cells by size, estimated forward scatter (FS Lin) and granularity, estimated side scatter (SS Lin) <br />B: Non-transduced cells plotted against cells expressing mVenus (Analytical gate was set such that 1% or fewer of negative control cells fell within the positive region (R5) <br />C: Gating transduced cells (R2 ≙ R14) (plasmids used for transfection: pGOI: pSB1C3_lITR_CMV_beta-globin_mVenus_hGH_rITR (pSB1C3_mVenus: BBa_K404119), pHelper, pRC. <br />D: Transduced cells plotted against cells expressing mVenus. R10 comprises transduced cells detected by mVenus fluorescence. <br />E: Overlay of non-transduced (red) and transduced (green).</td>
 +
<td style="width: 400px; vertical-align: top;">F: Gating non-transduced cells (control). <br />G: Non-transduced cells plotted against cells expressing mVenus (R5). <br />H: Gating transduced cells (R14 ≙ R2) (plasmids used for transfection: pGOI: pAAV_mVenus, pHelper). <br />I: Transduced cells plotted against cells expressing mVenus. R10 comprises transduced cells detected by mVenus fluorescence. <br />J: Overlay of non-transduced (red) and transduced (green) cells plotted against mVenus expression. </td>
 +
</tr>
 +
</table>
 +
 +
<center>
 +
<img src="https://static.igem.org/mediawiki/parts/9/94/Freiburg10_Diagram_hGH.png" style="width: 500px; height: auto; align: center; text-align: center;"/> <p>Figure 13: Calculated percentage of mVenus expressing cells </p>
 +
 +
<p style="align: center; text-align: center;">Flow cytometry analysis of vectorplasmids with and without hGH terminator. YFP expression of viral genomes was determined by flow cytomery after 24-hour post infection. Results demonstrate that mVenus expression of vectorplasmids lacking the hGH terminator is reduced significantly proving that the polyadenylation signal is essential for viral gene expression using recombinant viral vectors engineered by using components of the Virus Construction Kit.</p>
 +
 +
</center>
 +
 +
</html>
 
<!-- Add more about the biology of this part here
 
<!-- Add more about the biology of this part here
 
===Usage and Biology===
 
===Usage and Biology===
Line 42: Line 531:
 
<partinfo>BBa_K404122 parameters</partinfo>
 
<partinfo>BBa_K404122 parameters</partinfo>
 
<!-- -->
 
<!-- -->
 +
 +
<html>
 +
<h3><a name="_Toc275981849"><span lang="EN-US">References</span></a></h3>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Ardiani, A., Sanchez-Bonilla, M. &amp;
 +
Black, M.E., 2010. Fusion enzymes containing HSV-1 thymidine kinase mutants and
 +
guanylate kinase enhance prodrug sensitivity in vitro and in vivo. <i>Cancer
 +
gene therapy</i>, 17(2), 86-96. Available at:
 +
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=2808426&amp;tool=pmcentrez&amp;rendertype=abstract.</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Black, M.E. et al., 1996. Creation of
 +
drug-specific herpes simplex virus type 1 thymidine kinase mutants for gene
 +
therapy. <i>Proceedings of the National Academy of Sciences of the United
 +
States of America</i>, 93(8), 3525-9. Available at:
 +
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=39643&amp;tool=pmcentrez&amp;rendertype=abstract.</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Fuchita, M. et al., 2009. Bacterial
 +
cytosine deaminase mutants created by molecular engineering show improved
 +
5-fluorocytosine-mediated cell killing in vitro and in vivo. <i>Cancer research</i>,
 +
69(11), 4791-9. Available at:
 +
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=2765227&amp;tool=pmcentrez&amp;rendertype=abstract.</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Fuchita, M. et al., 2009. Bacterial
 +
cytosine deaminase mutants created by molecular engineering show improved
 +
5-fluorocytosine-mediated cell killing in vitro and in vivo. <i>Cancer research</i>,
 +
69(11), 4791-9. Available at:
 +
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=2765227&amp;tool=pmcentrez&amp;rendertype=abstract.</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;">Greco,
 +
O. &amp; Dachs, G.U., 2001. </span><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Gene directed enzyme/prodrug therapy of
 +
cancer: historical appraisal and future prospectives. <i>Journal of cellular
 +
physiology</i>, 187(1), 22-36. Available at:
 +
http://www.ncbi.nlm.nih.gov/pubmed/11241346.</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;">Huber,
 +
B.E. et al., 1993. </span><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">In vivo antitumor activity of 5-fluorocytosine on human
 +
colorectal carcinoma cells genetically modified to express cytosine deaminase. <i>Cancer
 +
research</i>, 53(19), 4619-26. Available at:
 +
http://www.ncbi.nlm.nih.gov/pubmed/8402637.</span></p>
 +
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Moolten, F.L., 1986. Tumor chemosensitivity
 +
conferred by inserted herpes thymidine kinase genes: paradigm for a prospective
 +
cancer control strategy. <i>Cancer research</i>, 46(10), 5276-81. Available at:
 +
http://www.ncbi.nlm.nih.gov/pubmed/3019523.</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Roche, <i>Apoptosis , Cell Death and Cell
 +
Proliferation</i>,</span></p>
 +
 +
<p style="text-indent: 36pt;"><span style="font-size: 10pt; font-family: &quot;Calibri&quot;,&quot;sans-serif&quot;;" lang="EN-US">Willmon, C.L., Krabbenhoft, E. &amp; Black,
 +
M.E., 2006. A guanylate kinase/HSV-1 thymidine kinase fusion protein enhances
 +
prodrug-mediated cell killing. <i>Gene therapy</i>, 13(17), 1309-12. Available
 +
at: http://www.ncbi.nlm.nih.gov/pubmed/16810197.</span></p>
 +
</html>

Latest revision as of 14:43, 30 October 2010

[AAV2]-left-ITR_pCMV_betaglobin_mGMK_TK30_hGH_[AAV2]-right-ITR

AAV2-left-ITR_pCMV_betaglobin_mGMK_TK30_hGH_AAV2-right-ITR
BioBrick Nr. BBa_K404122
RFC standard RFC 10
Requirement pSB1C3
Source
Submitted by [http://2010.igem.org/Team:Freiburg_Bioware FreiGEM 2010]


Contents

Functional Composite Part for Successful Tumor Cell Ablation. 1

Introduction. 1

Successful Assembly of Vector Plasmids Carrying Suicide Genes via Cloning. 1

Monitoring Efficient Tumor Killing by Phase-Contrast Microscopy. 4

Quantitative Analysis of Cell Death by Flow Cytometry. 6

Titrating Ganciclovir Concentrations for Efficient Cell Killing by Cytotoxicity Assays. 8

Conclusions. 16

References. 16

 

Functional Composite Part for Successful Tumor Cell Ablation

Introduction

Gene delivery using viral vectors to specifically target tumor cells gained increasing attention in the last years being efficient in combination with suicide gene approaches (Willmon et al. 2006). Several prodrug/enzyme combinations have been reported. Two systems - ganciclovir (GCV)/herpes simplex virus thymidine kinase (HSV-TK) (Ardiani et al. 2010) and 5-fluorocytosine/cytosine deaminase (CD) (Fuchita et al. 2009a) – have been widely used and their therapeutic benefit was demonstrated in preclinical studies (Greco & Dachs 2001). Adeno-associated viruses (AAV) as delivery vectors are commonly used in suicide gene therapy. The suicide gene flanked by the inverted terminal repeats (ITRs) is encapsulated into the virus particles and delivered to the target cells where suicide gene expression is mediated by cellular proteins.

The iGEM team Freiburg_Bioware 2010 provides both the cytosine deaminase (CD, BBa_K404112) and an improved guanylate kinase - thymidine kinase fusion gene (mGMK_TK, BBa_K404113) within the Virus Construction Kit as effective suicide genes. We demonstrate efficient and specific killing of tumor cells by enzymatic cytotoxicity assays, flow cytometry, as well as phase contrast microscopy. HT1080 cancer cell lines were transduced with directed viral particles containing the suicide genes packaged into the viral capsids.

Successful Assembly of Vector Plasmids Carrying Suicide Genes via Cloning

To create the functional vector plasmids, assembly of the constructs carrying the suicide genes was performed following the BioBrick Standard Assembly. All plasmids contain the enhancer-element human beta-globin intron ( BBa_K404107) and the human growth hormone terminator signal (hGH, BBa_K404108) flanked by the inverted terminal repeats (ITRs, BBa_K404100 and BBa_K404101). Assembled suicide genes are either under the control of the CMV promoter ( BBa_J52034) or the tumor-specific telomerase promoter phTERT ( BBa_K404106).

Figure 1: BioBrick-compatible assembly of functional vector plasmids containing the suicide genes. The schematic figure shows the cloning strategy of the guanylate kinase – thymidine kinase fusion gene (mGMK_TK30).

Freiburg10 Vectorplasmid composite 4.png

 

To enable modularization of the thymidine kinase mutants TK30 and SR39 ( BBa_K404109 and BBa_K404110) according to the BioBrick standard, the fusion genes mGMK_TK30 and mGMK_SR39 ( BBa_K404113 and BBa_K404315) and CD ( BBa_K404112) were modified using the QuikChange Lightning Site-Directed Mutagenesis Kit (Stratagene) for deletion of iGEM RFC10 pre- and suffix restriction sites. Figure 2 demonstrates one example of successful deletion of a PstI restriction site located within the mGMK_TK30 sequence at position 3109. A point mutation was introduced replacing the nucleotide G by A, resulting in the deletion of the restriction site while maintaining the encoded amino acid glutamine. Exchange of guanine to adenine was confirmed by sequencing (Figure 2).

Figure 2: Cytosine to guanine exchange by site-directed mutagenesis using QuikChange Lightning Kit provided by Stratagene was successful as demonstrated by (A) test digestion linearizing the plasmid with PstI and (B) by sequencing.

 

Furthermore, assembly of BioBrick-compatible vector plasmids was performed. An example for the last assembly step of mGMK_TK30 and hGH_rITR is shown in Figure 3. The plasmids were digested with both XbaI and PstI (New England Biolabs, Insert: BBa_K404116: hGH_rITR) or SpeI and PstI (Vector) and loaded on an agarose gel. As demonstrated in the preparative gel in Figure 3, the expected bands were detected under UV light and the extracted, subsequently purified DNA was successfully ligated and transformed into E. coli. Each assembly step for producing the BioBricks was conducted following the iGEM BioBrick standard.

Figure 3: Assembly of mGMK_TK30 (vector molecule, in pSB1C3) and hGH-terminator_rightITR (insert molecule). The digested fragments were visualized under UV-light and correspond to the expected sizes.

 

Monitoring Efficient Tumor Killing by Phase-Contrast Microscopy

Tumor cells, transduced with viral particles encapsidating the effector constructs containing the mGMK_TK30 driven by the CMV promoter, were cultured both in presence and absence of ganciclovir (Roche). Morphological changes were monitored via phase-contrast microscopy for 48 hours post infection. As it can be seen in Figure 4, non-transduced tumor cells treated with ganciclovir and transduced cells without ganciclovir did not show significant cell ablation. In contrast, transduced cells expressing the guanylate kinase - thymidine kinase fusion protein showed significant cell death after incubation with ganciclovir for 48 hours post infection.

A Beschreibung: https://static.igem.org/mediawiki/2010/3/3e/HT_negativ_control_ganciclovir_only.jpg

B Beschreibung: https://static.igem.org/mediawiki/2010/f/f0/HT_TKGMK_clone_1_ohne_Ganciclovir_300%C2%B5l.jpg

C

Beschreibung: https://static.igem.org/mediawiki/2010/c/c3/HT_TKGMK_clone_1_with_ganciclovir_300%C2%B5l.jpg

D Beschreibung: https://static.igem.org/mediawiki/2010/7/73/HT_TKGMK_clone_1_with_ganciclovir_600%C2%B5l_well_2.jpg

Figure 4: Qualitative analysis of cell death induced by conversion of ganciclovir to ganciclovir-triphosphate by virus-delivered guanylate - thymidine kinase (mGMK_TK30). A: Non-transduced HT1080 cells incubated in the presence of ganciclovir not exhibiting cell death. B: Untreated transduced HT1080 cells showing a high survival rate. C: HT1080 cells transduced with 300 µL viral particles and incubated with ganciclovir leading to tumor cell ablation. D: HT1080 cells transduced with 600 µL viral particles and incubated with ganciclovir leading to ablation of tumor cells.

 

Suicide gene therapy is based on the localized conversion of non-toxic prodrugs to toxic substances (Greco & Dachs 2001), promoting cell death in the tumor tissue (Figure 5). Directed gene delivery is achieved by using recombinant viral vectors as provided by the iGEM team Freiburg_Bioware 2010 within the Virus Construction Kit.


Figure 5: Overview of the suicide gene therapy approach. Non-toxic prodrugs are converted into toxic effector molecules leading to cell death of the tumor cells.

Non-transduced cells can survive in the presence of ganciclovir since the prodrug is not toxic for these cells (Figure 4A). The demonstration that transduced cells are viable in the absence of ganciclovir confirms that cell killing is indeed induced by combination of the delivered thymidine kinase and treatment with ganciclovir. Viral particles encapsidating the suicide construct mGMK_TK30 are efficient in directed gene delivery, thus leading to cell death of transduced cells due to overexpression of mGMK_TK30 and prodrug conversion. The cell-toxic ganciclovir-triphosphate is incorporated into the nascent DNA chain leading to replication termination and finally resulting in death of dividing cells.





Quantitative Analysis of Cell Death by Flow Cytometry

Quantitative analysis of the cytotoxic effect induced by mGMK_TK30 was first conducted by flow cytometry analysis 72 hours post transduction. HT1080 cells were stained with 7-AAD and Annexin V. 7-AAD intercalates in double-stranded DNA after penetrating cell membranes of dead cells, whereas Annexin V specifically binds phosphatidylserine which is only accessible during apoptosis. Figure 6 demonstrates the relation between cell death and ganciclovir concentration.

 

Figure 6: Flow cytometry data analysis. A: Gating non-transduced HT1080 cells (control). B: Non-transduced cells without staining plotted against 7-AAD. C: Gating non-transduced cells stained with 7-AAD. D: Non-transduced, 7-AAD-stained cells plotted against 7-AAD. E: Gating transduced cells (GOI: mGMK_TK30) treated with 485 µM ganciclovir. F: Gated, Annexin-V stained cells plotted against AnnV-2 Log.  G: Gated cells  plotted against 7-AAD H: Gated, 7-AAD and Annexin-V stained cells plotted against 7-AAD and Annexin-V. Gate R19 comprised Annexin-V and 7-AAD positive cells.

 

 

Figure 7: Quantification of flow cytometry data provided in Figure 6. With increasing ganciclovir concentration, the survival rate of cells decreases. 60 % of HT1080 cells treated with 4.85 mM ganciclovir show tumor ablation, however even lower amounts of ganciclovir lead to significant cell death.

 

The effect of different ganciclovir concentrations on transduced HT1080 sarcoma cells was investigated. Transduction was performed with recombinant viral particles encapsidating the mGMK_TK30 prodrug gene. 72 hours post infection, cells were stained with 7-AAD and Annexin V. As Figure 7 shows, the fraction of killed transduced cells is proportional to the applied ganciclovir concentration.

Titrating Ganciclovir Concentrations for Efficient Cell Killing by Cytotoxicity Assays

Further analysis of the cytotoxic effect induced by thymidine kinase converting ganciclovir to the toxic anti-metabolite has been performed using MTT assays. 3-(4,5-Dimethylthiazol-2-yl)-2,5diphenyltetrazolium bromide), also known as MTT, is a yellow-colored tetrazole, which is reduced to purple insoluble formazan in the presence of NADH and NADPH (Roche n.d.). Colorimetric analysis can be carried out via spectrometry. Different tumor cell lines, HT1080 and A431, were transduced with the recombinant viruses carrying the linear DNA construct coding for mGMK-TK30 regulated by the CMV promoter and subsequently treated with ganciclovir. 48 and 72 hours post infection, cells were incubated with MTT and fresh DMEM. After cell lysis by DMSO, absorbance of formazan at 570 nm was quantified using a Tecan Sunrise plate reader.

A

B

Figure 8: Effect of ganciclovir on HT1080 cell survival 72 hours post infection as (A) two dimensional plot of survival of cells and (B) three-dimensional plot of ganciclovir, virus particles and cell survival.

 

 

 

A  

B

Figure 9: Effect of ganciclovir on HT1080 cell survival 96 hours post infection. (A) two dimensional plot of cell survival  (B) three-dimensional plot of ganciclovir, virus particles and cell survival.

 

Data of MTT assay quantification are shown in Figure 8 and Figure 9. HT1080 cells were infected with viral particles containing the mGMK_TK30 transgene.  72 h- and 96 h post infection and addition of ganciclovir, cells were incubated with MTT. Changes in absorbance were measured and survival of cells plotted against ganciclovir concentration. Figure 8A demonstrates the correlation between increasing ganciclovir concentrations and percentage of cell survival. Furthermore, different virus particle concentrations were used for transduction. Figure 8B shows that the highest amount of viral particles combined with the highest ganciclovir concentration led to significant HT1080 apoptosis 72 hours post transduction.

Additionally, 96 hours post infection cells were incubated with MTT and absorbance was quantified via spectrometry (Figure 9). Again, survival of HT1080 cells was plotted against increasing ganciclovir concentrations.

Conclusions

Efficient and tissue-specific tumor killing is one major challenge in cancer therapy (Black et al. 1996). Gene-directed enzyme prodrug therapy (GDEPT) is based on the conversion of non-toxic substances into toxic drugs resulting in tumor cell death. The iGEM team Freiburg_Bioware 2010 provides several functional suicide genes within the Virus Construction Kit, thus offering a feasible and modular tool to the growing field of personalized medicine and the iGEM community. We successfully demonstrated cancer cell death caused by the introduction of modified fusion genes consisting of guanylate and thymidine kinases.

 To prevent systemic toxic side effects of conventional chemotherapy, the iGEM team Freiburg_Bioware 2010 took a leap and efficiently retargeted the viral vector for directed suicide gene delivery towards tumor cells. Capsid engineering was successfully demonstrated by the iGEM team Freiburg_Bioware 2010. Further details can be found under iGEM wiki Freiburg_Bioware 2010 - Results - Targeting

 

Individual components of the assembled vector plasmid

ITRs


Figure 10: ITR details


The inverted terminal repeat structures can be subdivided into several palindromic motives: A and A’ form a stem loop which encases B and B’ as well as C and C’. Those motives form both arms of the T-shaped structure. The functional motives on the ITR are two regions that bind Rep 68/78, called Rep-binding elements (RBE on the stem and RBE’ on the B arm) and the terminal resolution site (trs) in which the rep proteins introduce single-stranded nicks. The 3’ OH end of the A motive acts as a primer for DNA replication (Im & Muzyczka, 1990) (Lusby, Fife, & Berns, 1980).

Beta-globin-intron


Figure 11 A: FACS data


Figure 11 B: Calculated percentage of mVenus expressing cells


The beta-globin intron BioBrick consists of a partial chimeric CMV promoter followed by the intron II of the beta-globin gene. The 3´end of the intron is fused to the first 25 bases of human beta globin gene exon 3. The beta globin intron BioBrick is assumed to enhance eukaryotic gene expression (Nott, Meislin, & Moore, 2003). As shown in Figure 11 A and B the vectorplasmid missing the beta-globin intron showed a negligible difference in mVenus expression compared to viral genomes containing the beta-globin intron. Considering these results and taking into account that a constant volume of viral particles has been used for transduction, the difference between the construct containing and lacking the beta-globin intron is minimal. Since packaging efficiency of the AAV-2 decreases with increasing sizes of the insert (Dong, Fan, & Frizzell, 1996), the iGEM team Freiburg_Bioware suggests using the beta-globin intron in dependence on the size of your transgene.

mGMK_TK30 fusion protein


The thymidine kinase mutant TK30 contains six modified amino acids (Black, Newcomb, Wilson, & Loeb, 1996) created in a first screening showing enhanced affinity for gancivlocir and acyclovir, but reduced specificity for its natural substrate thymidine.

As efficient tumor killing and therefore ganciclovir activation is essential for successful tumor ablation, further improvements were conducted. Overexpression of transgenic thymidine kinase leads to accumulation of non-toxic intermediates, which cannot be phosphorylated sufficiently by endogenous guanylate kinase, the second enzyme in the salvage pathway of nucleotides.
Overcoming this bottleneck was accomplished by fusing the mouse guanylate kinase (mGMK) to the N-terminus of TK30 mutant creating a fusion protein (mGMK_TK30) with enhanced GCV/ACV sensitivity in vitro and in vivo (Ardiani, Sanchez-Bonilla, & Black, 2010) and improved bystander activity. The effect of non-transfected tumor cell killing upon transfer of toxic metabolites through gap junctional intercellular communication (GJIC) or immune-mediated tumor ablation is essential in suicide gene therapy (Pope, 1997). GCV-triphosphate is mainly transported through the central pore formed between connexin proteins from neighboring cells (Gentry, Im, Boucher, Ruch, & Shewach, 2005), but immune-induced bystander effect seems to be likely as well (Grignet-Debrus, Cool, Baudson, Velu, & Calberg-Bacq, 2000).


hGH termination signal

Recombinant AAV genomes were engineered containing the inverted terminal repeats (ITRs), a strong eukaryotic promoter and mVenus as gene of interest with and without the hGH terminator signal. Transduction of HT1080 cells with viral particles containing the rAAV genomes and measuring mVenus expression 24-hours post infection by flow cytometry demonstrated that transgene expression of the constructs lacking the hGH termination signal is significantly reduced. The iGEM team Freiburg_Bioware 2010 therefore suggests using the provided hGH termination signal within the Virus Construction Kit for optimal gene expression.

 

Since cloning does not confirm biological activity, we analyzed the plasmids and their functional components, hGH terminator and beta-globin intron, in cell culture. Assembled plasmids have been cotransfected, using AAV-293 cells, which provide the stable integrated E1A and E1B genes, with helper plasmids required for capsid assembly and genome encapsidation (pRC and pHelper) in a molar ratio of 1:1:1 (pGOI:pRC:pHelper). Virus particles containing the single stranded DNA were harvested 72-hours post transfection and HT1080 cells transduced with constant volumes of viral vectors. 48-hours post infection; transduced cells expressing the gene of interest were analyzed by flow cytometry.

Recombinant vectorplasmids were engineered containing the inverted terminal repeats (ITRs), a strong eukaryotic promoter (CMV promoter: BBa_K404102) and mVenus as gene of interest with and without the hGH terminator signal. Transduction of HT1080 cells with constant volume of viral particles containing the vectorplasmids and measuring mVenus expression 24-hours post infection by flow cytometry demonstrated that transgene expression of the constructs lacking the hGH termination signal is significantly reduced as shown in confirming the expected results that hGH is essential for mRNA processing. The iGEM team Freiburg_Bioware 2010 therefore suggests using the provided hGH termination signal within the Virus Construction Kit for optimal gene expression.

Figure 12: Flow cytometry analysis of vectorplasmid without (left) and with (right) hGH. For viral particle production, AAV-293 cells were transfected with the reassembled vector plasmid (BBa_K404119) or the reference plasmid, respectively.
A: Gating non transduced cells (control); subcellular debris and cellular aggreates can be distinguished from single cells by size, estimated forward scatter (FS Lin) and granularity, estimated side scatter (SS Lin)
B: Non-transduced cells plotted against cells expressing mVenus (Analytical gate was set such that 1% or fewer of negative control cells fell within the positive region (R5)
C: Gating transduced cells (R2 ≙ R14) (plasmids used for transfection: pGOI: pSB1C3_lITR_CMV_beta-globin_mVenus_hGH_rITR (pSB1C3_mVenus: BBa_K404119), pHelper, pRC.
D: Transduced cells plotted against cells expressing mVenus. R10 comprises transduced cells detected by mVenus fluorescence.
E: Overlay of non-transduced (red) and transduced (green).
F: Gating non-transduced cells (control).
G: Non-transduced cells plotted against cells expressing mVenus (R5).
H: Gating transduced cells (R14 ≙ R2) (plasmids used for transfection: pGOI: pAAV_mVenus, pHelper).
I: Transduced cells plotted against cells expressing mVenus. R10 comprises transduced cells detected by mVenus fluorescence.
J: Overlay of non-transduced (red) and transduced (green) cells plotted against mVenus expression.

Figure 13: Calculated percentage of mVenus expressing cells

Flow cytometry analysis of vectorplasmids with and without hGH terminator. YFP expression of viral genomes was determined by flow cytomery after 24-hour post infection. Results demonstrate that mVenus expression of vectorplasmids lacking the hGH terminator is reduced significantly proving that the polyadenylation signal is essential for viral gene expression using recombinant viral vectors engineered by using components of the Virus Construction Kit.

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal NgoMIV site found at 1319
    Illegal NgoMIV site found at 1977
    Illegal NgoMIV site found at 2882
    Illegal AgeI site found at 3011
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI site found at 3413
    Illegal SapI.rc site found at 1369


References

Ardiani, A., Sanchez-Bonilla, M. & Black, M.E., 2010. Fusion enzymes containing HSV-1 thymidine kinase mutants and guanylate kinase enhance prodrug sensitivity in vitro and in vivo. Cancer gene therapy, 17(2), 86-96. Available at: http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=2808426&tool=pmcentrez&rendertype=abstract.

Black, M.E. et al., 1996. Creation of drug-specific herpes simplex virus type 1 thymidine kinase mutants for gene therapy. Proceedings of the National Academy of Sciences of the United States of America, 93(8), 3525-9. Available at: http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=39643&tool=pmcentrez&rendertype=abstract.

Fuchita, M. et al., 2009. Bacterial cytosine deaminase mutants created by molecular engineering show improved 5-fluorocytosine-mediated cell killing in vitro and in vivo. Cancer research, 69(11), 4791-9. Available at: http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=2765227&tool=pmcentrez&rendertype=abstract.

Fuchita, M. et al., 2009. Bacterial cytosine deaminase mutants created by molecular engineering show improved 5-fluorocytosine-mediated cell killing in vitro and in vivo. Cancer research, 69(11), 4791-9. Available at: http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=2765227&tool=pmcentrez&rendertype=abstract.

Greco, O. & Dachs, G.U., 2001. Gene directed enzyme/prodrug therapy of cancer: historical appraisal and future prospectives. Journal of cellular physiology, 187(1), 22-36. Available at: http://www.ncbi.nlm.nih.gov/pubmed/11241346.

Huber, B.E. et al., 1993. In vivo antitumor activity of 5-fluorocytosine on human colorectal carcinoma cells genetically modified to express cytosine deaminase. Cancer research, 53(19), 4619-26. Available at: http://www.ncbi.nlm.nih.gov/pubmed/8402637.

Moolten, F.L., 1986. Tumor chemosensitivity conferred by inserted herpes thymidine kinase genes: paradigm for a prospective cancer control strategy. Cancer research, 46(10), 5276-81. Available at: http://www.ncbi.nlm.nih.gov/pubmed/3019523.

Roche, Apoptosis , Cell Death and Cell Proliferation,

Willmon, C.L., Krabbenhoft, E. & Black, M.E., 2006. A guanylate kinase/HSV-1 thymidine kinase fusion protein enhances prodrug-mediated cell killing. Gene therapy, 13(17), 1309-12. Available at: http://www.ncbi.nlm.nih.gov/pubmed/16810197.