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Team:Gothenburg/Calendar
From 2014.igem.org
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<span class="hidden"> | <span class="hidden"> | ||
<p>On the first day of laboration, we prepared LB, YPD and SC-Ura/His/Trp-Leu and YPD media. | <p>On the first day of laboration, we prepared LB, YPD and SC-Ura/His/Trp-Leu and YPD media. | ||
| - | + | ||
| - | + | ||
</td> | </td> | ||
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<span class="hidden"> | <span class="hidden"> | ||
<p> Succesfully PCR amplified five out of the seven parts from yeast genome via a Phusion High-Fidelity DNA Polymerase. | <p> Succesfully PCR amplified five out of the seven parts from yeast genome via a Phusion High-Fidelity DNA Polymerase. | ||
| - | |||
<p>The PCR program used was: <br> | <p>The PCR program used was: <br> | ||
<ol> | <ol> | ||
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<li>10 min at 72ºC. </li> | <li>10 min at 72ºC. </li> | ||
</ol> | </ol> | ||
| - | <p>A diagnostic gel was performed and the | + | <p>A diagnostic gel was performed and the purification of the succesfully amplified parts was done using a PCR Purification Kit from GenJet following the instructions |
| - | + | ||
| - | + | ||
of the manufacture's manual but with no addition of isopropanol. <br> | of the manufacture's manual but with no addition of isopropanol. <br> | ||
</span> | </span> | ||
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<li>10 min at 72ºC. </li> | <li>10 min at 72ºC. </li> | ||
</ol> | </ol> | ||
| - | <p>A diagnostic gel was performed and the | + | <p>A diagnostic gel was performed and the purification of the succesfully amplified parts was done using a PCR Purification Kit from GenJet following the instructions |
| - | + | of the manufacture's manual but with no addition of isopropanol. <br> | |
</span> | </span> | ||
</td> | </td> | ||
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<ul class="titles"> | <ul class="titles"> | ||
<li>Dissolution of synthetic parts</li> | <li>Dissolution of synthetic parts</li> | ||
| - | <li>Amplification | + | <li>Amplification of synthetic parts</li> |
<li>PCR purification</li> | <li>PCR purification</li> | ||
<li>Concentration determination</li> | <li>Concentration determination</li> | ||
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<h2>Dissolution of synthetic parts</h2> | <h2>Dissolution of synthetic parts</h2> | ||
<p>The received synthetic part pCYC1 m2 was centrifuged at 3000g for 3min and then dissolved with 10UL of sterile water. The solution was transferred to 10UL of TE buffer, resulting in a final concentration of 10ng/UL.<br> | <p>The received synthetic part pCYC1 m2 was centrifuged at 3000g for 3min and then dissolved with 10UL of sterile water. The solution was transferred to 10UL of TE buffer, resulting in a final concentration of 10ng/UL.<br> | ||
| - | <h2>Amplification | + | <h2>Amplification of synthetic parts</h2> |
<p>Performed PCR amplification of the synthetic part pCYC1 m2.<br> | <p>Performed PCR amplification of the synthetic part pCYC1 m2.<br> | ||
<p>The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br> | <p>The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br> | ||
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<h1>5</h1> | <h1>5</h1> | ||
<ul class="titles"> | <ul class="titles"> | ||
| - | <li> | + | <li>Plasmid restriction</li> |
| - | <li> | + | <li>Gel extraction</li> |
| + | <li>Concentration determination</li> | ||
| + | <li>PCR amplification and merging</li> | ||
</ul> | </ul> | ||
| - | <span class="hidden">This | + | <span class="hidden"> |
| + | <h2>Plasmid restriction</h2> | ||
| + | <p>Repeated the cleavage of the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XhoI. <br> | ||
| + | <p>Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XhoI, 2UL of FastDigest buffer, 1UL of FastAP | ||
| + | (alkaline phosphatase) and up to 20 UL of deionized sterile water.<br> | ||
| + | <p>This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC.<br> | ||
| + | <p>A diagnostic gelGreen was performed and the expected band sizes were observed. <br> | ||
| + | <h2>Gel extraction</h2> | ||
| + | <p>Extracted the successfully cleaved plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. | ||
| + | <h2>Concentration determination</h2> | ||
| + | <p>Used a NanoDrop spectrometer to determinate the concentration of the previously extracted plasmids. The concentrations ranged from 5.95 to 7.75ng/UL.<br> | ||
| + | <h2>PCR amplification and merging</h2> | ||
| + | <p>Performed PCR to fuse the following fragments:<br> | ||
| + | <li>D-tag-CFP (previously merged) with pCYC1 </li> | ||
| + | <li>pHO and Sic1 (previously merged)with Cas9 </li> | ||
| + | <li>pDSE4-YFP-D-tag(previously merged) and Counter 1 (synthetic part)</li> | ||
| + | <p>The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br> | ||
| + | <ol> | ||
| + | <li>3 min at 98ºC </li> | ||
| + | <li>30s at 98ºC</li> | ||
| + | <li>Gradient from 43 to 60ºC for 30s</li> | ||
| + | <li>2min 30s at 72ºC</li> | ||
| + | <li>Go to step 2 (repeat 40 times)</li> | ||
| + | <li>10 min at 72ºC.</li> | ||
| + | </ol> | ||
| + | <p> A diagnostic gelGreen was performed and the sizes of all the resulting fragments did not match the expected.<br> | ||
| + | |||
| + | </span> | ||
</td> | </td> | ||
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<h1>6</h1> | <h1>6</h1> | ||
<ul class="titles"> | <ul class="titles"> | ||
| - | <li> | + | <li>PCR amplification and merging</li> |
| - | <li> | + | <li>Gibson Assembly</li> |
</ul> | </ul> | ||
| - | <span class="hidden"> | + | <span class="hidden"> |
| + | <h2>PCR amplification and merging</h2> | ||
| + | <p>Repeated the PCR to fuse the following fragments:<br> | ||
| + | <li>D-tag-CFP (previously merged) with pCYC1 </li> | ||
| + | <li>pHO and Sic1 (previously merged)with Cas9 </li> | ||
| + | <li>pDSE4-YFP-D-tag(previously merged) and Counter 1 (synthetic part)</li> | ||
| + | <p>The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br> | ||
| + | <ol> | ||
| + | <li>3 min at 98ºC </li> | ||
| + | <li>10s at 98ºC</li> | ||
| + | <li>Gradient from 45 to 62ºC for 30s</li> | ||
| + | <li>2min 30s at 72ºC</li> | ||
| + | <li>Go to step 2 (repeat 40 times)</li> | ||
| + | <li>10 min at 72ºC.</li> | ||
| + | </ol> | ||
| + | <p> A diagnostic gelGreen was performed and the sizes of all the resulting fragments were smaller than expected and the bands were difuse.<br> | ||
| + | |||
| + | <h2>Gibson Assembly</h2> | ||
| + | <p> Attempted to transform the Daughter Resetter construct (pDSE4,YFP,D-tag and Counter 1) into E. coli following the Gibson Assembly protocol from New England Biolab. | ||
| + | <p> The cells were inoculated in LB-Amp medium and let to grow overnight. | ||
| + | </span> | ||
</td> | </td> | ||
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<h1>7</h1> | <h1>7</h1> | ||
<ul class="titles"> | <ul class="titles"> | ||
| - | <li> | + | <li>Plasmid Purification</li> |
| - | <li> | + | <li>Gel extraction</li> |
| + | <li>Gibson Assembly</li> | ||
</ul> | </ul> | ||
| - | <span class="hidden">This | + | <span class="hidden"> |
| + | <h2>Plasmid Purification</h2> | ||
| + | <p> Performed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416, p2055 and a plasmid containig our Cas9 sequence | ||
| + | (pTPG1-dCas9-UPGP)via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by | ||
| + | water on the last step. <br> | ||
| + | <h2>Plasmid restriction</h2> | ||
| + | <p>Cleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XhoI. <br> | ||
| + | <p>Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XhoI, 2UL of FastDigest buffer, 1UL of FastAP | ||
| + | (alkaline phosphatase) and up to 20 UL of deionized sterile water.<br> | ||
| + | <p>This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC.<br> | ||
| + | <p>A diagnostic gelGreen was performed and the expected band sizes were observed. <br> | ||
| + | <h2>Gel extraction</h2> | ||
| + | <p>Extracted the successfully cleaved plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. | ||
| + | <h2>Gibson Assembly</h2> | ||
| + | <p>Continued with the Gibson Assembly protocol (New England Biolab) and used p414 in the cells with the assembly poducts. A positive control with cells and the circular plasmid was also prepared.<br> | ||
| + | <p>All the inoculated cultures were placed at 37ºC. | ||
| + | </span> | ||
</td> | </td> | ||
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<h1>8</h1> | <h1>8</h1> | ||
<ul class="titles"> | <ul class="titles"> | ||
| - | <li> | + | <li>Observed results from the Gibson Assembly</li> |
| - | <li> | + | <li>Yeast Transformation</li> |
</ul> | </ul> | ||
| - | <span class="hidden"> | + | <span class="hidden"> |
| + | <h2>Observed results from the Gibson Assembly</h2> | ||
| + | <p>The positive control showed several monoclonal colonies.<br> | ||
| + | <p>However, the plate with the actual construct showed only one colony which is unlikely to contain the construct.<br> | ||
| + | <h2>Yeast Transformation</h2> | ||
| + | <p> Performed transformation on the competent cells previously prepared according to the protocol "Frozen-EZ Yeast Transformation II".<br> | ||
| + | <p> Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: | ||
| + | <li>Cas9 construct: pHO, Sic1 and Cas9 fragments into the plasmid p413</li> | ||
| + | <li>Daughter Resetter construct: D-tag, YFP, pDSE4 and Counter 1 synthetic part fragments into p414 plasmid</li> | ||
| + | <li>Counter 2 construct: D-tag, CFP, pCYC1 and Counter 2 synthetic part fragments into p416 plasmid</li> | ||
| + | </span> | ||
</td> | </td> | ||
Revision as of 01:09, 11 October 2014
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The team received mandatory safety training and general lab routine information.
A really cool video about Chalmers' chemical safety routine (recorded at our very own lab!) can be seen in http://www.chalmers.se/insidan/EN/about-chalmers/environmental-work/policies/chemical-safety-routine |
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As a part of the mandatory training required by the SysBio group, the team received instructions on how to operate the centrifuges
and autoclaves of the labs.
We also worked on our risk declaration; a mandatory document containing our experiments descriptions and information about the chemicals we are going to use, their handling, storage and associated risk, as well as waste handling. |
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Our Risk Declaration was approved by the lab manager and our supervisors. We also sign a safety certificate stating that we are aware of the safety instructions and with that, completed the mandatory "check-in list for new incomers" of the lab. |
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On the first day of laboration, we prepared LB, YPD and SC-Ura/His/Trp-Leu and YPD media. |
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25
Succesfully PCR amplified five out of the seven parts from yeast genome via a Phusion High-Fidelity DNA Polymerase. The PCR program used was:
A diagnostic gel was performed and the purification of the succesfully amplified parts was done using a PCR Purification Kit from GenJet following the instructions
of the manufacture's manual but with no addition of isopropanol. |
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Plasmid Purification Performed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416, p2055 and a plasmid containig our Cas9 sequence
(pTPG1-dCas9-UPGP)via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by
water on the last step. Amplification and purification of partsPerformed a PCR amplification of the non-synthetic parts that failed on the day before and on the dCas9 sequence and the three fluorescent proteins
-Yellow, Cyano and Red (YFP, CFP and RFP, respectively). The PCR was done using the Phusion High-Fidelity DNA Polymerase (see protocol here) and the program used was:
A diagnostic gel was performed and the purification of the succesfully amplified parts was done using a PCR Purification Kit from GenJet following the instructions
of the manufacture's manual but with no addition of isopropanol. |
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Gel extractionExtracted the fluorecent proteins amplified on the day before with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. PCR amplification and mergingPerformed a PCR to fuse the pDSE4, pHO and dCas9 parts together. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed. The bands did not seem correct, so this PCR was repeated on the next day. |
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PCR amplification and mergingRepeated the PCR to fuse the pDSE4, pHO and dCas9 parts together. The PCR was done using the Phusion High-Fidelity DNA Polymerase (see protocol here) and the program used was:
A diagnostic gel was performed and this did not seemed to work either. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. |
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PCR amplification and mergingRepeated the PCR to fuse the pDSE4, pHO and dCas9 parts together.The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed, however the sizes of the resulting fragments did not match the expected. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. Samples were loaded into a gelGreen, that showed p413, p415 and p416 approximately in the 5000bp size band, while p414 presented two bands, one around 4000bp and another at 2000bp. this indicates that the 5000bp band corresponds to the uncut plasmid, while the 4000bp and 2000bp are probably contaminations. |
1
Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. PCR amplificationAmplified the parts pDSE4, cas9 and pHO. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed, however the sizes of the resulting fragments did not match the expected. |
2
PCR amplificationRepeated the amplification of the parts pDSE4, cas9 and pHO. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed and the sizes of the fragments matched for the pDSE4 and pHO, but not for the Cas9. Gel extractionExtracted the DNA fragments previously amplified with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Concentration determinationThe concentration of all the fragments obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 8.5 ng of DNA per UL to 42ng/UL. |
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Plasmid purificationPerformed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416 and p2055 via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Each plasmid was purified in duplicates. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and showed that the cleavage of plasmids p413, p415 and p416 was successful. Gel extractionExtracted the cleaved plasmids with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. |
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Concentration determinationThe concentration of the circular and linear plasmids obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 6.55 ng of DNA per UL to 543.4ng/UL. |
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PCR amplification and mergingRepeated the PCR to fuse the pDSE4, pHO and dCas9 parts together.The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed, however the sizes of the resulting fragments did not match the expected. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. Samples were loaded into a gelGreen, that showed p413, p415 and p416 approximately in the 5000bp size band, while p414 presented two bands, one around 4000bp and another at 2000bp. this indicates that the 5000bp band corresponds to the uncut plasmid, while the 4000bp and 2000bp are probably contaminations. |
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Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. PCR amplificationAmplified the parts pDSE4, cas9 and pHO. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed, however the sizes of the resulting fragments did not match the expected. |
2
PCR amplificationRepeated the amplification of the parts pDSE4, cas9 and pHO. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed and the sizes of the fragments matched for the pDSE4 and pHO, but not for the Cas9. Gel extractionExtracted the DNA fragments previously amplified with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Concentration determinationThe concentration of all the fragments obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 8.5 ng of DNA per UL to 42ng/UL. |
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Plasmid purificationPerformed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416 and p2055 via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Each plasmid was purified in duplicates. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and showed that the cleavage of plasmids p413, p415 and p416 was successful. Gel extractionExtracted the cleaved plasmids with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. |
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Concentration determinationThe concentration of the circular and linear plasmids obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 6.55 ng of DNA per UL to 543.4ng/UL. |
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Plasmid restrictionCleaved the plasmids p414TEF with the enzymes SacI and XbaI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and showed multiple size bands for the samples treated with XbaI. Consultation to the literature showed that this enzyme has not an unique restriction site for p414. Therefore the restriction was repeated with the enzyme SpeI, that has an unique cleavage site in p414 located 6bp away from the XbaI's desirable cleavage site. The same procedure described above was used, substituting XbaI for SpeI. The disgnostic gel performed on this second cleavage showed correct band sizes, but with too low lines. This indicates low concentration of the plasmid, therefore it was not extracted. |
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Plasmid restrictionCleaved the plasmids p414TEF with the enzymes SacI and SpeI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of SpeI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and showed again too light bands or no bands at all. |
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Plasmid restrictionRepeated the cleavage the plasmids p414TEF with the enzymes SacI and SpeI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of SpeI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and SacI seemed to be leaving an excessive amount of uncut plasmid while SpeI apparently degrades the sample. |
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Plasmid restrictionRepeated the cleavage the plasmids p414TEF with the enzymes SacI with SpeI or BamHI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of SpeI or BamHI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each and without phosphatase were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 20 minutes and then enzymatic inactivation was performed for 5min in a heating block at 75ºC for samples containing BamHI and at 65ºC for samples containing SpeI. A diagnostic gelGreen was performed and SacI again seemed to be leaving an excessive amount of uncut plasmid. However, samples treated with SacI and SpeI with and without phosphatase and one of the samples treated with SacI, BamHI and phosphatase seemed to work and were extracted. Gel extractionExtracted the succesfully cleaved plasmids with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. |
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PCR amplification and mergingPerformed a PCR to fuse the following fragments: The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gelRed was performed and revealed the expected band sizes for the merging of D-tag with CFP and pHO with Sic1. Gel extractionExtracted the successfully merged fragments with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. |
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PCR amplification and mergingPerformed a PCR to fuse the following fragments: The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gelRed was performed and revealed the expected band sizes for the merging of D-tag with YFP. Gel extractionExtracted the successfully merged fragments with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Dissolution of synthetic partsThe received synthetic parts (g-blocks) were centrifuged at 3000g for 3min and then dissolved with 10UL of sterile water. The solution was transferred to 10UL of TE buffer, resulting in a final concentration of 10ng/UL. |
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Amplification and purification of synthetic partsPerformed a PCR amplification of the synthetic parts previously diluted. Namely The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed and showed the expected band sizes for all the fragments except pCYC1. Gel extractionExtracted the successfully merged parts with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Preparation of competent cellsFollowing the instructions of the protocol "Frozen-EZ Yeast Transformation II" by ZymoResearch, Saccaromyces cerevisiae competent cells were prepared and stored at -80ºC. |
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Amplification and purification of synthetic partsRepeated the PCR amplification of the synthetic part pCYC1 m1. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed and showed the expected band sizes. Gel extractionExtracted the successfully merged part with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Yeast Transformation Performed transformation on the competent cells previously prepared according to the protocol "Yeast Transformation". Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: |
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Plasmid restrictionCleaved the plasmids p413TEF and p416TEF with the enzymes SacI and XbaI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 30 minutes and then enzymatic inactivation was performed for 5min in a heating block at 65ºC. A diagnostic gelGreen was performed and showed fragments with the correct sizes. Gel extractionExtracted the successfully restricted plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. |
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Dissolution of synthetic partsThe received synthetic part pCYC1 m2 was centrifuged at 3000g for 3min and then dissolved with 10UL of sterile water. The solution was transferred to 10UL of TE buffer, resulting in a final concentration of 10ng/UL. Amplification of synthetic partsPerformed PCR amplification of the synthetic part pCYC1 m2. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gel was performed and showed the expected band sizes. PCR purificationThe purification of the succesfully amplified part was done using a PCR Purification Kit from GenJet following the instructions
of the manufacture's manual but with no addition of isopropanol and elution was done with 30UL of sterile water. Concentration determinationThe concentration of the pCYC1 m2 samples obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 15.1 ng of DNA per UL to 34.2ng/UL. |
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Yeast Transformation Performed transformation on the competent cells previously prepared according to the protocol "Yeast Transformation". Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: |
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Observation of the previously transformed cellsOne of the plates with cells transformed on the 28th showed growth, but with contamination by filamentous fungi, while the other presented no growth at all. A single yeast colony from the contaminated plate was replated on a YPD-agar plate. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF and p416TEF with the enzymes SacI and XbaI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 30 minutes and then enzymatic inactivation was performed for 5min in a heating block at 65ºC. A diagnostic gelGreen was performed and showed fragments with the correct sizes. Gel extractionExtracted the successfully restricted plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Preparation of Competent cellsCompetent E.coli cells were prepared according to the protocol described by Hanahan(1983) and stored at -80ºC. |
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Inoculation of cellsThe single colony replated on the day before was inoculated in 4mL YPD medium as an overnight culture for transformation. |
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Yeast Transformation Performed transformation on the competent cells previously prepared according to the protocol "Yeast Transformation". Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: Inoculation of cellsCells transformed on the 28th that showed growth after 3 days were plated on new adequate selective media. |
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Yeast Transformation Performed transformation on the competent cells previously prepared according to the protocol "Yeast Transformation". Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: |
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Observation of the previously transformed cellsOne of the plates with cells transformed on the 28th showed growth, but with contamination by filamentous fungi, while the other presented no growth at all. A single yeast colony from the contaminated plate was replated on a YPD-agar plate. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF and p416TEF with the enzymes SacI and XbaI. Approximately 500ng of the plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared. This reaction mixture was incubated at in a water bath at 37ºC for 30 minutes and then enzymatic inactivation was performed for 5min in a heating block at 65ºC. A diagnostic gelGreen was performed and showed fragments with the correct sizes. Gel extractionExtracted the successfully restricted plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Preparation of Competent cellsCompetent E.coli cells were prepared according to the protocol described by Hanahan(1983) and stored at -80ºC. |
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Inoculation of cellsThe single colony replated on the day before was inoculated in 4mL YPD medium as an overnight culture for transformation. |
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Yeast Transformation Performed transformation on the competent cells previously prepared according to the protocol "Yeast Transformation". Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: Inoculation of cellsCells transformed on the 28th that showed growth after 3 days were plated on new adequate selective media. |
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PCR amplification and mergingPerformed PCR to fuse the following fragments: The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gelGreen was performed and the sizes of all the resulting fragments match the expected. Gel extractionExtracted the successfully merged parts with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Plasmid restrictionWhile reviewing primer design documents, the team realized we were using the wrong enzyme to cleave the plasmids: it should be SacI with XhoI instead of XbaI. Therefore, our plasmids did not have the correct overlap with the constructs. Cleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XhoI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XhoI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and the cleavage showed to be unsuccessful. |
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Plasmid restrictionRepeated the cleavage of the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XhoI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XhoI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and the expected band sizes were observed. Gel extractionExtracted the successfully cleaved plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Concentration determinationUsed a NanoDrop spectrometer to determinate the concentration of the previously extracted plasmids. The concentrations ranged from 5.95 to 7.75ng/UL. PCR amplification and mergingPerformed PCR to fuse the following fragments: The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gelGreen was performed and the sizes of all the resulting fragments did not match the expected. |
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PCR amplification and mergingRepeated the PCR to fuse the following fragments: The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was:
A diagnostic gelGreen was performed and the sizes of all the resulting fragments were smaller than expected and the bands were difuse. Gibson AssemblyAttempted to transform the Daughter Resetter construct (pDSE4,YFP,D-tag and Counter 1) into E. coli following the Gibson Assembly protocol from New England Biolab. The cells were inoculated in LB-Amp medium and let to grow overnight. |
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Plasmid Purification Performed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416, p2055 and a plasmid containig our Cas9 sequence
(pTPG1-dCas9-UPGP)via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by
water on the last step. Plasmid restrictionCleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XhoI. Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XhoI, 2UL of FastDigest buffer, 1UL of FastAP
(alkaline phosphatase) and up to 20 UL of deionized sterile water. This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC. A diagnostic gelGreen was performed and the expected band sizes were observed. Gel extractionExtracted the successfully cleaved plasmids with a GeneJet gel extraction kit. The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step. Gibson AssemblyContinued with the Gibson Assembly protocol (New England Biolab) and used p414 in the cells with the assembly poducts. A positive control with cells and the circular plasmid was also prepared. All the inoculated cultures were placed at 37ºC. |
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Observed results from the Gibson AssemblyThe positive control showed several monoclonal colonies. However, the plate with the actual construct showed only one colony which is unlikely to contain the construct. Yeast Transformation Performed transformation on the competent cells previously prepared according to the protocol "Frozen-EZ Yeast Transformation II". Equimollar quantities of the fragments were added to plasmids with different markers. More specifically: |
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