Difference between revisions of "Team:Munich/Amplification"

 
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<div class="popup" id="RPA_TEV_Popup">
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<img  src="https://static.igem.org/mediawiki/2017/8/85/T--Munich--RPAPagePicture_gel1.png">
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<div class="popup" id="RPA_Benchmark_Popup">
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<tr>
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<td style="background-color: #51a7f9;" colspan = 6 align="left">
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<ul class="menuList" id="menu">
 +
  <li><a href="/Team:Munich/Results">Overview</a></li>
 +
  <li><a href="/Team:Munich/Cas13a">Cas13a</a></li>
 +
  <li><a href="/Team:Munich/Readouts">Readouts</a></li>
 +
  <li><a href="/Team:Munich/Targets">Targets</a></li>
 +
  <li><a href="/Team:Munich/DetectionOnChip">Detection Chip</a></li>
 +
  <li><a href="/Team:Munich/Amplification">Amplification</a></li>
 +
</ul> 
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</td>
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</tr>
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<tr><td colspan=6 align=left valign=center>
 
<tr><td colspan=6 align=left valign=center>
<font size=7 color=#51a7f9><b style="color: #51a7f9">Amplification Methods</b></font>
+
<div style="margin-top: 40px;"><font size=7 color=#51a7f9><b style="color: #51a7f9">Results: Amplification</b></font></div>
 
</td>
 
</td>
 
</tr>
 
</tr>
 +
<tr>
 +
<td width="900%">
 +
<h3>What worked:</h3>
 +
  <ul class="listResults">
 +
          <li>We used RPA to  <a class="myLink" href="https://2017.igem.org/Team:Munich/Amplification#heatlysed">amplify DNA</a> from heat lysed <i>E. coli</i>.</li>
 +
          <li>We conducted RPA and transcription from an in vitro DNA <a class="myLink" href="https://2017.igem.org/Team:Munich/Amplification#onpaper">on paper</a>.</li>
 +
          <li>We amplified and transcribed an in vitro DNA target to RNA concentrations <a class="myLink" href="https://2017.igem.org/Team:Munich/Amplification#transcriptionreadout">detectable by our readout circuit</a>.</li> 
 +
  </ul>
 +
</td>
 +
</tr>
 +
 +
<tr>
 +
<td width="900%">
 +
<h3>What presented issues:</h3>
 +
  <ul class="listResults">
 +
          <li>Amplifying long sequences with RPA.</li> 
 +
  </ul>
 +
</td>
 +
</tr>
 +
 
<tr class="lastRow">
 
<tr class="lastRow">
 
<td  colspan = 6 align="left">
 
<td  colspan = 6 align="left">
 
<p class="introduction">
 
<p class="introduction">
Since real-world patient's sample contain only traces of pathogens, detection with any
+
Since real-world patient samples contain only traces of pathogens (attomolar at the lowest), any detection method relying on binding affinity (such as Cas13a with target RNA) needs prior amplification of the detected molecule to concentrations within the range of the K<sub>d</sub>.
kind of read-out system will be difficult without prior amplification of the detected substance.
+
After we confirmed that the detection limit of Cas13a is in the nanomolar region, we had to tackle the problem
After we saw that the detection limit of Cas13a is in the nM region, we had to tackle the problem
+
 
of low target concentrations in medical samples.   
 
of low target concentrations in medical samples.   
This is why we explored different amplification methods. Our main idea was to keep things simple,
+
We debated different amplification methods that would be simple and stable on our portable platform. Traditional PCR, using a proper thermocycler and well-defined cycling times, also requires a trained personnel to use them, which dioes not fit to our goal of a distributable diagnostic device. We therefore chose to explore isothermal amplification reactions, to facilitate hardware design, leading to decreased production and development costs.  
transportable and stable by incorporating isothermal reactions on paper with lyophilized reaction mixes.
+
While Cas13a detects RNA, rather than DNA, we would eventually need to be able to detect both DNA and RNA samples. We therefore chose a combination of <b>reverse-transcriptase</b>-coupled isothermal <b>recombinase polymerase amplification</b> and subsequent <b> <i>in vitro</i> transcription </b> for amplification. We term this cascade of amplification reactions <b>RT-RPA-TX</b>. For detection of DNA samples, the RT step can be omitted. Finally, we  lyophilize the reaction mixture on paper, to stabilize the sensitive enzymes for transport.
Therefore, we explored <i> isothermal PCR </i> methods coupled to <i> In-Vitro Transcription </i>.
+
The final idea was to be able to detect both DNA and RNA samples by using either a  
+
<i>Reverse Transcriptase </i> coupled <i>Recombinase Polymerase Amplification </i> and subsequent  
+
<i> In-Vitro Transcription </i> for RNA targets or leaving out the step of reverse transcription for DNA targets.
+
 
                 </p>
 
                 </p>
</td>
 
</tr>
 
  
 
+
<div class="captionPicture">
 
+
<img alt="Cascade_1" src="https://static.igem.org/mediawiki/2017/a/a6/Cascade_1.svg" width="1000">
 
+
<p>
 
+
Our amplification cascade consisting of RT-RPA-TX can be coupled to the Cas13a-based readout circuit to improve the sensitivity of CascAID.
 
+
<tr class="lastRow"><td colspan=6 align=center valign=center>
+
<h1>Why isothermal PCR?</h1>
+
<br>
+
<p>
+
Classical Polymerase Chain Reactions
+
We chose to explore isothermal methods for signal amplification since isothermal techniques
+
come with the potential of simplified hardware design which would lead to decreased production and development costs.  
+
 
</p>
 
</p>
 +
 +
</div>
 +
</td>
 
</tr>
 
</tr>
  
 
<tr class="lastRow">
 
<tr class="lastRow">
 
<td colspan=4>
 
<td colspan=4>
<h3> Recombinase Polymerase Amplification </h3>
+
<h3 id="heatlysed">Recombinase Polymerase Amplification</h3>
<br>
+
 
<p>
 
<p>
The Recombinase Polymerase Amplification (RPA) developed by TwistDx is an isothermal amplification method for DNA.  
+
The <b>Recombinase Polymerase Amplification</b> (RPA) developed by TwistDx is an isothermal amplification method for DNA.  
 
Rather than melting the double strand and annealing the primers through temperature cycles, it uses a recombinase
 
Rather than melting the double strand and annealing the primers through temperature cycles, it uses a recombinase
that binds the primers and assists them in the annealing process. Another protein, single-strand DNA binding protein (SSB)  
+
that binds the primers and assists in the annealing process. Another protein, single-strand DNA binding protein (SSB),
 
promotes the binding of the primers to the recombinase in this process.
 
promotes the binding of the primers to the recombinase in this process.
Hence, the first step in the development of an isothermal amplification method of an RNA signal via RT-RPA-Tx was testing the  
+
Hence, the first step in the development of an isothermal amplification method of an RNA signal via RT-RPA-TX was testing the RPA itself in bulk. For this, we took our previously cloned His-tagged TEV Protease (<a class="myLink" href="http://parts.igem.org/Part:BBa_K2323002">BBa_K2323002</a> improved from <a class="myLink" href="http://parts.igem.org/Part:BBa_K1319008">BBa_K1319008</a>)
Recombinase Polymerase Amplification (RPA) itself in bulk. For this, we took our previously cloned His-tagged TEV Protease
+
and ran dummy PCR reactions using the TwistDx RPA kit and the universal biobrick primers VF2 (<a class="myLink" href="http://parts.igem.org/Part:BBa_G00100">BBa_G00100</a>) and VR (<a class="myLink" href="http://parts.igem.org/Part:BBa_G00101">BBa_G00101</a>). We ran the provided test reaction of the TwistDx RPA kit as a positive control (<a class="myLink" href="https://www.twistdx.co.uk/en/products/product/twistamp-exo">TwistAmp exo</a>). The results are shown in <b>Figure 1</b>.  
and ran dummy PCR reactions using the TwistDx RPA Kit. We tested this with standard Biobrick primers VF2 and VR and ran
+
The first point to note is that PCR primers and RPA primers have different requirements. Due to the need for affinity of the recombinase to the primers, RPA primers tend to be shorter with a higher GC content. Therefore VF2 and VR might not be ideal primers for RPA. The second point is that RPA's optimum amplification length is 500 bp. For longer amplifications, it is possible that the polymerase falls off the strand. This could explain why we see at maximum a band of 500 bp, and shorter bands, although our amplicon should be 1262 bp. We could therefore see that amplification using RPA was possible in bulk, but that primer design would need to be optimized for our final product.
the provided test reaction of the TwistDx RPA Kit as a positive control. The results are shown in Figure 1.  
+
<br><br>
This approach is connected to some risk, since it is not said that PCR primers will work just as fine in RPA reactions.  
+
To better assess the RPA reaction, we therefore constructed a benchmark pSB1C3 plasmid coding for 3 of our <a class="myLink" href="https://2017.igem.org/Team:Munich/Targets">target sequences</a> (<i>E. coli</i>, <i>B. subtilis</i> and Norovirus) under the control of a T7 promoter. It is flanked by VF2 and VR primer binding sequences, so that it can be amplified similarly to our first His-TEV construct, but the amplicon is only 194 bp. This was a great benchmarking sequence, as the plasmid could be used for amplification from lysed cells, as would be the case with a real sample. The sequence was short enough, could be coupled with transcription and consisted of relevant targets for our readout.<br>
The affinity of Recombinase to the primers is important to get an efficient binding of the primers to the template DNA.
+
 
For this reason PCR primers tend to be longer and have less GC% than RPA primers in general.  
+
<h3 id="onpaper">RPA on Paper</h3>
In addition, the tested construct was approximately 1500 bp long, which is also quite far from RPA's optimum of 500 bp.  
+
<p>
Nevertheless, we could show that product is formed, though only up to the size of 500 bp. After that, it seems that the
+
The next step was to bring the RPA reaction on paper. For this, we lyophilized the reaction mixture provided by TwistDx  
Polymerase falls off the strand and was not able to produce longer amplicons. This is why one can see small bands for  
+
longer constructs, just with a much lower yield.<br><br>
+
The next step was to bring the RPA reaction on paper. For this, we lyophilised the reaction mixture provided by TwistDx  
+
 
on paper and tried to run RPA reactions directly from it by inserting the blotting paper into the PCR tube.  
 
on paper and tried to run RPA reactions directly from it by inserting the blotting paper into the PCR tube.  
Activity could be shown on an agarose gel but first time stability experiments showed that the activity decreases quickly.   
+
Activity could be shown on an agarose gel, but time-stability experiments showed that the activity of the RPA kit decreases quickly.   
In the user's manual, it is stated that after breaking the seal one should use up the reaction mix in the next hour.  
+
In the user's manual, it is stated that after breaking the seal, one should use the reaction mix within one hour.  
 
We can confirm this statement since activity declined rapidly after as little as two hours and was non-existent after  
 
We can confirm this statement since activity declined rapidly after as little as two hours and was non-existent after  
24 hours. <br>
+
24 hours, as is visible in <b>Figure 2</b>.
Furthermore, temperature seems to be a very important factor during amplification using RPA. As observable in Figure 2,
+
Furthermore, temperature seems to be a very important factor during amplification using RPA. The samples incubated at 20°C, though still active, showed dramatically decreased activity compared to the same samples at 37°C.
the sample without any prior storage at a reaction temperature of 20 °C, though still active, showed dramatically decreased activity.
+
 
<br>
 
<br>
 
<br>
 
<br>
 
For usage of RPA on a detection device that does not require purification of the sample, the reaction needs to take
 
For usage of RPA on a detection device that does not require purification of the sample, the reaction needs to take
place in the environment of a lysate with cell debris and released protein from the cell. In order to see whether this
+
place in the environment of a lysate with cell debris and released proteins from the cell. In order to see whether this
is achievable, we performed a colony-PCR like setting of RPA using a <i>E. Coli</i> culture in LB-medium with OD=1.0
+
is achievable, we performed a colony-PCR like setting of RPA using an <i>E. coli</i> culture in LB-medium with OD=1.0
and ran a normal RPA of purified plasmid as a control. We observed that the yield measured by on-gel concentration
+
and ran a regular RPA from purified plasmid as a control. As our first PCR produced a too long amplicon, we changed to a shorter PCR scheme, which should lead to an amplicon of 194 bp. The results are shown in <b>Figure 3</b>.
determination was approximately the same.  
+
A band at the expected length is visible in both the control condition and the <i>E. coli</i> environment. We observed that the yield measured by gel quantification was approximately the same. <br><br>
 +
Since the stability of RPA on paper for a long period of time would be crucial to our diagnostic device, we considered the possible reasons for the instability of our RPA mix. We could think of two main factors affecting the stability: humidity and temperature. As we want our platform to be distributable across the world, we needed to test those hypotheses. We found out, that the instability is mainly caused by exposure to air, presumably humidity. We could dramatically increase stability when covering the paperstrip in a plastic Petri dish and sealing it with Parafilm. The stability was increased when keeping the paperstrip at 4°C, but the RPA was also still active after 24 hours storage at room temperature, when protected in a sealed environment. The results are shown in <b>Figure 4</b>. We did not have time to conduct long-term storage tests, but we are hopeful that with the right sealing strategy, the RPA might still be active on paper after a year.  
  
 
</td>
 
</td>
 
<td colspan=2>
 
<td colspan=2>
 
<div class="captionPicture" align=center>
 
<div class="captionPicture" align=center>
<img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/8/85/T--Munich--RPAPagePicture_gel1.png" width="300">
+
<a href="#RPA_TEV_Popup""><img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/8/85/T--Munich--RPAPagePicture_gel1.png" width="300"></a>
 
<p>
 
<p>
<i>Figure 1: RPA reaction at 37 °C of Control by TwistDx and His<sub>6</sub>-TEV using VF2 and VR primers. </i>
+
<b>Figure 1:</b> RPA reaction at 37 °C of Control by TwistDx and His<sub>6</sub>-TEV using VF2 and VR primers.
 
</p>
 
</p>
 
 
<div class="captionPicture">
 
<div class="captionPicture">
<img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/0/07/T--Munich--RPAPagePicture_gel2.png" width="300">
+
<a href="#RPA_Lyophili_Popup"><img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/0/07/T--Munich--RPAPagePicture_gel2.png" width="300"></a>
 
<p>
 
<p>
<i>Figure 2: RPA reaction of lyophilised RPA mixture at 37 °C or 20 °C of His<sub>6</sub>-TEV using VF2 and VR primers.  
+
<b>Figure 2:</b> RPA reaction of lyophilised RPA mixture at 37 °C or 20 °C of His<sub>6</sub>-TEV using VF2 and VR primers.  
The control is a reaction mixture without the lyophilisation step.</i>
+
The control is a reaction mixture without the lyophilisation step.
 
</p>
 
</p>
</td>
+
<div class="captionPicture">
 +
<a href="#RPA_Benchmark_Popup"><img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/f/f2/T--Munich--RPAPagePicture_gel4.png" width="200"></a>
 +
<p>
 +
<b>Figure 3:</b> Colony-PCR of Cas13a Benchmark plasmid using RPA. Control is a standard RPA reaction of purified plasmid. The cells were lysed for 10 minutes at 95 °C prior to the RPA reaction.
 +
</p>
 +
 
 
</div>
 
</div>
  
</p>
 
</tr>
 
  
<tr class="lastRow">
 
<td colspan=2>
 
 
<div class="captionPicture">
 
<div class="captionPicture">
 
<img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/c/cb/T--Munich--RPAPagePicture_gel3.png" width="300">
 
<img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/c/cb/T--Munich--RPAPagePicture_gel3.png" width="300">
 
<p>
 
<p>
<i>Figure 3: RPA reaction after freeze-dried storage on paper at different conditions. Conditions that were taken  
+
<b>Figure 4:</b> RPA reaction after freeze-dried storage on paper at different conditions. Conditions that were taken  
 
into consideration are temperature and air accessibility. Air determines the samples that were accessible to air.
 
into consideration are temperature and air accessibility. Air determines the samples that were accessible to air.
The other samples were stored in a Petri dish sealed with parafilm.</i>
+
The other samples were stored in a Petri dish sealed with parafilm.
 
</p>
 
</p>
 
</div>
 
</div>
 
</td>
 
</td>
  
 +
</p>
 +
</tr>
  
<td colspan=4 align="top" valign="text-top">
+
<tr class="lastRow">
<h3>RPA on paper time-stability optimisation</h3>
+
<td colspan=6>
<p> 
+
<h3>Coupling to Transcription</h3>
Since stability is an important question when developing a diagnostic test, we examined the bottleneck to the stability of
+
RPA reaction mix on paper. Basically, there is only two possible, though obvious, factors affecting the stability:
+
Exposure to humidity and temperature. So we tested both of these factors in an experiment and found out, that the bottleneck
+
is mainly presented by exposure to air, presumably humidity. We could dramatically increase stability when covering the
+
paperstrip in a plastic Petri dish and sealing it with Parafilm. The results are shown in Figure 3. <br><br>
+
 
+
 
+
<h3> Coupling RPA to In-Vitro Transcription </h3>
+
 
<br>
 
<br>
 
<p>
 
<p>
The fact that Cas13a is a RNA-guided RNAse made it necessary to not only amplify a DNA signal but also transcribe
+
The coupling of TX to RPA is in theory feasible because both reaction are conducted at 37°C, and still active at room temperature. We thus proceeded to try RPA-TX on the His<sub>6</sub>-TEV construct. However, we never succeeded to get the expected bands in the urea-PAGE following phenol-chloroform extraction. As our initial amplicon from the His-TEV construct was too long (1262 bp compared to 500 bp optimal amplification length from RPA), we believe that the enzyme did not manage to produce double-stranded DNA, and therefore transcription was not completed. At this point, we decided to create our benchmark plasmid described above, which has an amplicon of only 194 bp. We could characterize it for RPA, but unfortunately we did not have time to conduct RPA-TX experiments in bulk. Instead, we directly proceeded to attempting RPA-TX lyophilized on paper.
it into RNA. Thus, coupling the RPA reaction to <i>In-Vitro Transcription</i> was necessary. For this, we developed
+
a reaction mix in bulk that would perform both steps at a time. This is achievable since both reaction happen at 37 °C.
+
+
 
</p>
 
</p>
 
</td>
 
</td>
</tr>
 
  
  
  
 
<h3> Bringing RPA and In-Vitro Transcription on paper </h3>
 
<br>
 
<p>
 
The final step is bringing all the prior tested work on paper and stabilise it on their so it could be sealed into
 
the PDMS chip developed by the Hardware Team to automatise the amplification process and be able to subsequently
 
detect on a paperstrip using Cas13a from a simulated real-life sample. For this we ran tests and it did seem that
 
the RPA-Tx on paper could have worked judged by the 15%-Urea-PAGE. The gel showed two bands around the size of the
 
construct of 200 bp, one larger in size and less intense and one smaller in size and more intense. This could quite
 
possibly be the couple of DNA sample and derived RNA sample. Nevertheless, Cas13a-activity based on these samples
 
could not be shown.
 
 
</p>
 
 
</td>
 
 
</tr>
 
</tr>
  
  
<td colspan = 6 align="left">
+
<tr><td colspan=6>
<h3> Benchmark construct for Cas13a</h3>
+
<h3 id="transcriptionreadout">Bringing RPA and TX on Paper</h3>
 
<br>
 
<br>
 
<p>
 
<p>
Since the T7 RNA Polymerase only binds double-stranded DNA, transcription would never work form the His<sub>6</sub>-TEV
+
Our final goal was to bring together RPA and TX lyophilized on paper and prove the possibility of amplifying target RNA from our benchmark plasmid. The paper should then be sealed inside the <a class="mylink" href="https://2017.igem.org/Team:Munich/Hardware/SampleProcessing">sample processing unit</a>. For this, we ran experiments and analyzed the RNA expression with urea-PAGE (<b>Figure 5</b>). The expected transcript length is 132 nucleotides. The reaction was ran for 30, 60 and 120 minutes on paper, and the control was a bulk overnight reaction, all at 37°C. We see a clear band at the right length, with increasing intensity as the reaction is ran for longer. As the intensity of the band seems to be linearly increasing, this suggests that the transcription by T7 polymerase is the rate limiting step.
construct we initially tested RPA on, because the amplicon was too long. An option would have been to order a different
+
<br>
primer. It comes with the risk of losing RPA activity due to the strict dependency on the primer mentioned above and would
+
need additional time for optimization. Thus, we decided against that option and constructed a benchmark target RNA plasmid for
+
Cas13a. This construct consists of target sequences we took for 16s rRNA of <i>E. Coli </i>, 16s rRNA of <i> B. subtilis</i>
+
and the 5'-UTR of the norovirus. It is flanked by VF2 and VR. Upstream of the target sequences is a T7 promoter that allows
+
<i>In-Vitro Transcription</i>. After cloning this into a plasmid, we had a system with which we could test our coupled RPA-Tx
+
and check whether it works on paper.
+
 
</p>
 
</p>
  
<h3> Bringing RPA and In-Vitro Transcription on paper </h3>
+
<div class="captionPicture" align=center>
<br>
+
<img alt="LightbringerReal" src="https://static.igem.org/mediawiki/2017/f/fc/T--Munich--RPAPagePicture_gel5.png" width="800">
 
<p>
 
<p>
The final step was bringing all the prior tested work on paper and stabilise it on there so it could be sealed
+
<b>Figure 5:</b> 15%-Urea-PAGE for concentration determination of the RPA-TX amplifications. The time gives incubation time at 37 °C before ending the reaction by phenol-chloroform extraction. Control is given by a RPA reaction where T7 RNA Polymerase was not added.
into the PDMS chip developed by the Hardware Team to automatise the amplification process and enable
+
<br>
subsequent detection on a paperstrip using Cas13a. For this we ran test experiment
+
and we showed that RPA-Tx on paper worked judged by the 15%-Urea-PAGE. The gel showed a band at the approximate size
+
of 130 bp of the Benchmark construct that increased in concentration during the RPA-Tx reaction.
+
This could quite possibly be the couple of DNA sample and derived RNA sample. Nevertheless,
+
Cas13a-activity based on these samples could not be shown.  
+
 
+
 
</p>
 
</p>
 +
</div>
  
<h3> Discussion </h3>
+
 
 +
<p>
 +
Finally, we proceeded to test the ability of our product from RPA-TX to trigger Cas13a collateral RNase activity. We conducted the RPA-TX from our benchmark plasmid on paper, then phenol-chloroform extracted the RNA, quantified the RNA concentration, and tested the amplified RNA with our Cas13a detection circuit (<b>Figure 6</b>). In this experiment and others, the positive control was lower than the higher concentrations of target RNA, which we attribute to low activity of the RNaseA used in the positive control. We found that the Cas13a response was as good as from normally <i>in vitro</i> or <i>in vivo</i> sourced target RNA, and we could similarly detect 10 nM of amplified RNA. Our control contained the result of an RPA amplification without TX, that was extracted similarly as the RPA-TX sample, and added in the same volume as the 10 nM amplified RNA sample.
 +
</p>
 +
<div class="captionPicture" align=center>
 +
<img alt="Graph" src="https://static.igem.org/mediawiki/2017/8/81/T--Munich--Amplification_rnase_alert.png" width="800">
 +
<p>
 +
<b>Figure 6:</b> Detection of the RPA-TX with varying sample concentration using Cas13a.
 
<br>
 
<br>
 +
</p>
 +
</div>
 +
<h3>Reproducibility</h3>
 
<p>
 
<p>
 +
The RPA amplification is a well standardized method, which is commercially available as a kit. We used our RPA-TX repeatedly on paper with different incubation times and stability conditions, and we found that the circuit worked well, even though the sequence length of the amplicon should be carefully designed. We however did not have time to try amplification from a variety of sequences or primers.</p>
  
We showed here the first steps of establishing an amplification circuit for our detection device.  
+
<h3>Discussion and Conclusion</h3>
Since we were able to screen for storage conditions and do colony PCR-like experiments with the RPA mixture on paper,
+
<p>
the reproducibility of the RPA reaction after dry-freezing it on paper is proven. Time-stability has
+
We successfully conducted RPA from DNA <i>in vitro</i> and in cell lysate context. We joined RPA and TX in a one batch reaction, and conducted it on paper, using purified DNA. We could detect RNA with gel quantification within 60 minutes. Finally, we were able to perform Cas13a detection from RPA-TX amplified target, both on paper and in bulk. The stability of RPA on paper needs to be improved, but we showed that protection from air provided a reasonable protection of the activity. One issue that still needs to be solved is that the coupled RPA-TX reaction was only tested for purified samples. All the parts we tested (RPA in cell lysate, RPA combined with TX, stability of the whole circuit on paper, detection from an amplified target) now need to be combined and associated with the <a class="mylink" href="https://2017.igem.org/Team:Munich/Hardware/SampleProcessing">sample processing unit</a> and our <a class="mylink" href="https://2017.igem.org/Team:Munich/Hardware/Detector">detector</a>. Our modular approach proved successful to develop parallel working units that have to be assembled into a fully functioning platform.  
also been shown for 24 hours, though this will need to be extended to longer time-scales to provide
+
it to the customer.  
+
 
+
<br>
+
One issue that can still occur is that so far, the coupled RPA-Tx reaction was only tested for purified samples.  
+
The fact of having lysate in the sample is likely have distorting effects on the efficiency on both reactions.
+
Since RPA worked in a colony PCR-like set up with prior lysis of the cells, that is already a good start but the
+
<i>In-Vitro Transcription</i> is usually more delicate, therefore bringing this on paper in a lysate environment
+
might prove to be more difficult.  
+
 
+
 
</p>
 
</p>
  
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<p>  
 
<p>  
 
     <ol style="text-align: left">
 
     <ol style="text-align: left">
      <li id="ref_1"></li>
+
    <li id="ref_1">Gao, Zhu and Huang. "Recombinase Polymerase Amplification: A New DNA/RNA Amplification Strategy." (2016)
       <li id="ref_2"></li>
+
    <i>Chinese journal of Biochemistry and Molecular Biology</i> 32(6): 627-634.</li>
       <li id="ref_3"></li>
+
       <li id="ref_2">Daher, Stewart, Boissinot and Bergeron. "Recombinase Polymerase Amplification for Diagnostic Applications"
       <li id="ref_4"></li>
+
       (2016) <i>Clinical Chemistry</i> 62(7): 947-958.</li>
      <li id="ref_5"></li>
+
       <li id="ref_3">Beckert and Masquida. "Synthesis of RNA by In Vitro Transcription." (2010) <i> Methods in Molecular Biology </i>
 +
        Volume 703</li>
 
    
 
    
 
     </ol>  
 
     </ol>  

Latest revision as of 03:59, 2 November 2017

Description

Design

Demonstrate

Measurement

Applied Design

Final Results

Achievements

Protocols

Notebook

Safety

Parts

Improved Part

Part Collection

InterLab

Model

Software

Collaboration

Detector

Quake Valve

Paperstrips

Sample Processing

Silver

Gold

Engagement

Collaborations

Team members

Sponsors

Attributions

Gallery

Results: Amplification

What worked:

What presented issues:

  • Amplifying long sequences with RPA.

Since real-world patient samples contain only traces of pathogens (attomolar at the lowest), any detection method relying on binding affinity (such as Cas13a with target RNA) needs prior amplification of the detected molecule to concentrations within the range of the Kd. After we confirmed that the detection limit of Cas13a is in the nanomolar region, we had to tackle the problem of low target concentrations in medical samples. We debated different amplification methods that would be simple and stable on our portable platform. Traditional PCR, using a proper thermocycler and well-defined cycling times, also requires a trained personnel to use them, which dioes not fit to our goal of a distributable diagnostic device. We therefore chose to explore isothermal amplification reactions, to facilitate hardware design, leading to decreased production and development costs. While Cas13a detects RNA, rather than DNA, we would eventually need to be able to detect both DNA and RNA samples. We therefore chose a combination of reverse-transcriptase-coupled isothermal recombinase polymerase amplification and subsequent in vitro transcription for amplification. We term this cascade of amplification reactions RT-RPA-TX. For detection of DNA samples, the RT step can be omitted. Finally, we lyophilize the reaction mixture on paper, to stabilize the sensitive enzymes for transport.

Cascade_1

Our amplification cascade consisting of RT-RPA-TX can be coupled to the Cas13a-based readout circuit to improve the sensitivity of CascAID.

Recombinase Polymerase Amplification

The Recombinase Polymerase Amplification (RPA) developed by TwistDx is an isothermal amplification method for DNA. Rather than melting the double strand and annealing the primers through temperature cycles, it uses a recombinase that binds the primers and assists in the annealing process. Another protein, single-strand DNA binding protein (SSB), promotes the binding of the primers to the recombinase in this process. Hence, the first step in the development of an isothermal amplification method of an RNA signal via RT-RPA-TX was testing the RPA itself in bulk. For this, we took our previously cloned His-tagged TEV Protease (BBa_K2323002 improved from BBa_K1319008) and ran dummy PCR reactions using the TwistDx RPA kit and the universal biobrick primers VF2 (BBa_G00100) and VR (BBa_G00101). We ran the provided test reaction of the TwistDx RPA kit as a positive control (TwistAmp exo). The results are shown in Figure 1. The first point to note is that PCR primers and RPA primers have different requirements. Due to the need for affinity of the recombinase to the primers, RPA primers tend to be shorter with a higher GC content. Therefore VF2 and VR might not be ideal primers for RPA. The second point is that RPA's optimum amplification length is 500 bp. For longer amplifications, it is possible that the polymerase falls off the strand. This could explain why we see at maximum a band of 500 bp, and shorter bands, although our amplicon should be 1262 bp. We could therefore see that amplification using RPA was possible in bulk, but that primer design would need to be optimized for our final product.

To better assess the RPA reaction, we therefore constructed a benchmark pSB1C3 plasmid coding for 3 of our target sequences (E. coli, B. subtilis and Norovirus) under the control of a T7 promoter. It is flanked by VF2 and VR primer binding sequences, so that it can be amplified similarly to our first His-TEV construct, but the amplicon is only 194 bp. This was a great benchmarking sequence, as the plasmid could be used for amplification from lysed cells, as would be the case with a real sample. The sequence was short enough, could be coupled with transcription and consisted of relevant targets for our readout.

RPA on Paper

The next step was to bring the RPA reaction on paper. For this, we lyophilized the reaction mixture provided by TwistDx on paper and tried to run RPA reactions directly from it by inserting the blotting paper into the PCR tube. Activity could be shown on an agarose gel, but time-stability experiments showed that the activity of the RPA kit decreases quickly. In the user's manual, it is stated that after breaking the seal, one should use the reaction mix within one hour. We can confirm this statement since activity declined rapidly after as little as two hours and was non-existent after 24 hours, as is visible in Figure 2. Furthermore, temperature seems to be a very important factor during amplification using RPA. The samples incubated at 20°C, though still active, showed dramatically decreased activity compared to the same samples at 37°C.

For usage of RPA on a detection device that does not require purification of the sample, the reaction needs to take place in the environment of a lysate with cell debris and released proteins from the cell. In order to see whether this is achievable, we performed a colony-PCR like setting of RPA using an E. coli culture in LB-medium with OD=1.0 and ran a regular RPA from purified plasmid as a control. As our first PCR produced a too long amplicon, we changed to a shorter PCR scheme, which should lead to an amplicon of 194 bp. The results are shown in Figure 3. A band at the expected length is visible in both the control condition and the E. coli environment. We observed that the yield measured by gel quantification was approximately the same.

Since the stability of RPA on paper for a long period of time would be crucial to our diagnostic device, we considered the possible reasons for the instability of our RPA mix. We could think of two main factors affecting the stability: humidity and temperature. As we want our platform to be distributable across the world, we needed to test those hypotheses. We found out, that the instability is mainly caused by exposure to air, presumably humidity. We could dramatically increase stability when covering the paperstrip in a plastic Petri dish and sealing it with Parafilm. The stability was increased when keeping the paperstrip at 4°C, but the RPA was also still active after 24 hours storage at room temperature, when protected in a sealed environment. The results are shown in Figure 4. We did not have time to conduct long-term storage tests, but we are hopeful that with the right sealing strategy, the RPA might still be active on paper after a year.

LightbringerReal

Figure 1: RPA reaction at 37 °C of Control by TwistDx and His6-TEV using VF2 and VR primers.

LightbringerReal

Figure 2: RPA reaction of lyophilised RPA mixture at 37 °C or 20 °C of His6-TEV using VF2 and VR primers. The control is a reaction mixture without the lyophilisation step.

LightbringerReal

Figure 3: Colony-PCR of Cas13a Benchmark plasmid using RPA. Control is a standard RPA reaction of purified plasmid. The cells were lysed for 10 minutes at 95 °C prior to the RPA reaction.

LightbringerReal

Figure 4: RPA reaction after freeze-dried storage on paper at different conditions. Conditions that were taken into consideration are temperature and air accessibility. Air determines the samples that were accessible to air. The other samples were stored in a Petri dish sealed with parafilm.

Coupling to Transcription


The coupling of TX to RPA is in theory feasible because both reaction are conducted at 37°C, and still active at room temperature. We thus proceeded to try RPA-TX on the His6-TEV construct. However, we never succeeded to get the expected bands in the urea-PAGE following phenol-chloroform extraction. As our initial amplicon from the His-TEV construct was too long (1262 bp compared to 500 bp optimal amplification length from RPA), we believe that the enzyme did not manage to produce double-stranded DNA, and therefore transcription was not completed. At this point, we decided to create our benchmark plasmid described above, which has an amplicon of only 194 bp. We could characterize it for RPA, but unfortunately we did not have time to conduct RPA-TX experiments in bulk. Instead, we directly proceeded to attempting RPA-TX lyophilized on paper.

Bringing RPA and TX on Paper


Our final goal was to bring together RPA and TX lyophilized on paper and prove the possibility of amplifying target RNA from our benchmark plasmid. The paper should then be sealed inside the sample processing unit. For this, we ran experiments and analyzed the RNA expression with urea-PAGE (Figure 5). The expected transcript length is 132 nucleotides. The reaction was ran for 30, 60 and 120 minutes on paper, and the control was a bulk overnight reaction, all at 37°C. We see a clear band at the right length, with increasing intensity as the reaction is ran for longer. As the intensity of the band seems to be linearly increasing, this suggests that the transcription by T7 polymerase is the rate limiting step.

LightbringerReal

Figure 5: 15%-Urea-PAGE for concentration determination of the RPA-TX amplifications. The time gives incubation time at 37 °C before ending the reaction by phenol-chloroform extraction. Control is given by a RPA reaction where T7 RNA Polymerase was not added.

Finally, we proceeded to test the ability of our product from RPA-TX to trigger Cas13a collateral RNase activity. We conducted the RPA-TX from our benchmark plasmid on paper, then phenol-chloroform extracted the RNA, quantified the RNA concentration, and tested the amplified RNA with our Cas13a detection circuit (Figure 6). In this experiment and others, the positive control was lower than the higher concentrations of target RNA, which we attribute to low activity of the RNaseA used in the positive control. We found that the Cas13a response was as good as from normally in vitro or in vivo sourced target RNA, and we could similarly detect 10 nM of amplified RNA. Our control contained the result of an RPA amplification without TX, that was extracted similarly as the RPA-TX sample, and added in the same volume as the 10 nM amplified RNA sample.

Graph

Figure 6: Detection of the RPA-TX with varying sample concentration using Cas13a.

Reproducibility

The RPA amplification is a well standardized method, which is commercially available as a kit. We used our RPA-TX repeatedly on paper with different incubation times and stability conditions, and we found that the circuit worked well, even though the sequence length of the amplicon should be carefully designed. We however did not have time to try amplification from a variety of sequences or primers.

Discussion and Conclusion

We successfully conducted RPA from DNA in vitro and in cell lysate context. We joined RPA and TX in a one batch reaction, and conducted it on paper, using purified DNA. We could detect RNA with gel quantification within 60 minutes. Finally, we were able to perform Cas13a detection from RPA-TX amplified target, both on paper and in bulk. The stability of RPA on paper needs to be improved, but we showed that protection from air provided a reasonable protection of the activity. One issue that still needs to be solved is that the coupled RPA-TX reaction was only tested for purified samples. All the parts we tested (RPA in cell lysate, RPA combined with TX, stability of the whole circuit on paper, detection from an amplified target) now need to be combined and associated with the sample processing unit and our detector. Our modular approach proved successful to develop parallel working units that have to be assembled into a fully functioning platform.

References

  1. Gao, Zhu and Huang. "Recombinase Polymerase Amplification: A New DNA/RNA Amplification Strategy." (2016) Chinese journal of Biochemistry and Molecular Biology 32(6): 627-634.
  2. Daher, Stewart, Boissinot and Bergeron. "Recombinase Polymerase Amplification for Diagnostic Applications" (2016) Clinical Chemistry 62(7): 947-958.
  3. Beckert and Masquida. "Synthesis of RNA by In Vitro Transcription." (2010) Methods in Molecular Biology Volume 703