Difference between revisions of "Team:UiOslo Norway/Lab"
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<ol> | <ol> | ||
| − | <li> Gibson </li> | + | <li><h3> Gibson </h3></li> |
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V<sub>vector</sub> = y <br> | V<sub>vector</sub> = y <br> | ||
V<sub>gibson</sub> = x+y <br> | V<sub>gibson</sub> = x+y <br> | ||
| − | V<sub>water</sub> = 0µl<br> | + | V<sub>water</sub> = 0µl<br> <br> |
(ii) Incubation for 1h, not 15 min | (ii) Incubation for 1h, not 15 min | ||
(iii) Before transformation: One transformation with x ul concentrated Gibson solution and one transformation with | (iii) Before transformation: One transformation with x ul concentrated Gibson solution and one transformation with | ||
| − | Gibson solution diluted 1:3 and transformation with 3*x ul diluted Gibson solution. <br> | + | Gibson solution diluted 1:3 and transformation with 3*x ul diluted Gibson solution. <br> <br><br> |
| − | <li> Transformation <h3> </li> | + | <li> <h3>Transformation </h3> </li> |
<b> E.coli TOP10: </b> | <b> E.coli TOP10: </b> | ||
| Line 46: | Line 46: | ||
plasmids.<br> | plasmids.<br> | ||
<a class="bodyURLcolor" href="https://www.thermofisher.com/us/en/home/references/protocols/cloning/competent-cells-protocol/routine-cloning-using-top10-competent-cells.html">Chemical Transformation Procedure </a></h3> <br> | <a class="bodyURLcolor" href="https://www.thermofisher.com/us/en/home/references/protocols/cloning/competent-cells-protocol/routine-cloning-using-top10-competent-cells.html">Chemical Transformation Procedure </a></h3> <br> | ||
| − | <b>Modifications </b> <br> | + | <b>Modifications </b> <br><br> |
In Step 5, Incubate for exactly 30-45 seconds in the 42°C water bath. Do not mix or shake. | In Step 5, Incubate for exactly 30-45 seconds in the 42°C water bath. Do not mix or shake. | ||
In Step 7, Add 200-250 µl of rom temperatured S.O.C medium to each vial. S.O.C is a rich medium; sterile | In Step 7, Add 200-250 µl of rom temperatured S.O.C medium to each vial. S.O.C is a rich medium; sterile | ||
technique must be practiced to avoid contamination <br><br> | technique must be practiced to avoid contamination <br><br> | ||
| − | <b> E.coli DH5Alpha: </b> | + | <b> E.coli DH5Alpha: </b> <br> |
| − | Modifications: | + | Modifications: <br> |
| − | Step 15 and Step 16 not done <br> | + | Step 15 and Step 16 not done <br><br><br> |
| − | <li> PCR </li> | + | <li><h3> PCR</h3> </li> |
The goal of PCR is to amplify a section of DNA of interest for DNA analysis (e.g. gene insertion, sequencing, etc). The amplification rate is exponential. | The goal of PCR is to amplify a section of DNA of interest for DNA analysis (e.g. gene insertion, sequencing, etc). The amplification rate is exponential. | ||
| Line 70: | Line 70: | ||
| − | <li> Gel </li> | + | <li> <h3>Gel</h3> </li> |
For making a small 1% gel: | For making a small 1% gel: | ||
| Line 82: | Line 82: | ||
| − | <li> Miniprep </li> <br> | + | <li<h3>> Miniprep <h3></li> <br> |
<a class="bodyURLcolor" href="https://static.igem.org/mediawiki/2017/8/85/T--UiOslo_Norway--miniPrep.pdf"> Protocol </a> | <a class="bodyURLcolor" href="https://static.igem.org/mediawiki/2017/8/85/T--UiOslo_Norway--miniPrep.pdf"> Protocol </a> | ||
<b> Modifications: </b> | <b> Modifications: </b> | ||
| Line 90: | Line 90: | ||
</ul> | </ul> | ||
| − | <li>INTERLAB </li> | + | <li><h3>INTERLAB<h3> </li> |
96-Well Transformation Protocol: <br> | 96-Well Transformation Protocol: <br> | ||
<a class="bodyURLcolor" href="http://parts.igem.org/Help:Protocols/Transformation#96-Well_Transformation_Protocol | <a class="bodyURLcolor" href="http://parts.igem.org/Help:Protocols/Transformation#96-Well_Transformation_Protocol | ||
Revision as of 12:07, 30 October 2017
Protocols
Gibson
Gibson Assembly allows for successful assembly of multiple DNA fragments, regardless of fragment length or end compatibility. (1). The method
was invented in 2009 by Daniel G. Gibson, of the J. Craig Venter Institute. The assembly reaction is carried out in
one single reaction-tube, all at once, at 50° Celsius for 15-60 minutes. The process involves three different
enzymatic actions. A 5’ exonuclease creates overhangs, enabling matched fragments to anneal. Then a DNA polymerase
fills gap between the annealed strands and the 5´ end. Finally, a DNA ligase seals the gaps between the filled in
gap and the annealed strands. -
Transformation
E.coli TOP10:
One Shot® TOP10 E. coli are provided at a transformation efficiency of 1 x 109 cfu/µg supercoiled DNA and are
ideal for high-efficiency cloning and plasmid propagation. They allow stable replication of high-copy number
plasmids. PCR
The goal of PCR is to amplify a section of DNA of interest for DNA analysis (e.g. gene insertion, sequencing, etc). The amplification rate is exponential.
- Tag polimerase (25µl reaction) Protocol Here
- Phusion polymerase (20µl reaction?): Protocol Here
-
Gel
For making a small 1% gel:
INTERLAB
96-Well Transformation Protocol:
Protocol used for Gibson
(i) ModificationsVinsert = x
Vvector = y
Vgibson = x+y
Vwater = 0µl
(ii) Incubation for 1h, not 15 min (iii) Before transformation: One transformation with x ul concentrated Gibson solution and one transformation with Gibson solution diluted 1:3 and transformation with 3*x ul diluted Gibson solution.
Chemical Transformation Procedure
Modifications
In Step 5, Incubate for exactly 30-45 seconds in the 42°C water bath. Do not mix or shake. In Step 7, Add 200-250 µl of rom temperatured S.O.C medium to each vial. S.O.C is a rich medium; sterile technique must be practiced to avoid contamination
E.coli DH5Alpha:
Modifications:
Step 15 and Step 16 not done
- Weigh out 0.5 g of agarose and mix it with 50 ml of 1x TAE buffer in a 100 ml Erlenmeyer flask.
- Dissolve the agarose by bringing the mixture to the boiling point in a microwave oven, followed by mixing (by swirling the flask). Repeat the heating and mixing until all the agarose has dissolved.
- Cool the agarose solution to ~50 o C by leaving it on the bench for ~20 min (or you may accelerate the cooling by applying cold water from the tap to the outside of the flask).
- Using gloves, add 5 l GelRed (10 000x). Swirl the flask gently to mix, try to avoid bubbles.
- Pour the gel carefully into the mold. Bubbles may be removed/punctured by using a pipette tip.
Protocol
Modifications:
During the first attempt ethanol was not added to the PE buffer, which resulted in an unsuccessful miniprepl
In the second attempt 72/4% ethanol was added, as opposed to the recommended 96-100%, resulting in a successful miniprep
Protocol
Plate reader protocol: Protocol
