Team:Glasgow/Notebook/Protocols
From 2014.igem.org
(Difference between revisions)
RobbieEvans (Talk | contribs) |
|||
(17 intermediate revisions not shown) | |||
Line 12: | Line 12: | ||
- | < | + | <p id="ProtocolsLinks"> |
+ | This page shows our protocols for various lab procedures: | ||
+ | <ul> | ||
- | + | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#CreatingCompetentCells">Creating Chemically Competent Cells</a></li> | |
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#TransformationOfCompetentCells">Transformation of Competent Cells</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#DNACleanUp">DNA Clean-up</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#PCR">PCR</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#RestrictionDigests">Restriction Digests</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#GelExtraction">Gel Extraction</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#AnnealingOligos">Annealing Top and Bottom Strand Oligos</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#OligosPurification">Oligos Purification</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#MutagenicPCR">Site Directed Mutagenic PCR – Quikchange Protocol</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#IntegraseReaction">In vitro φC31 Integrase Reaction</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#Ligations">Ligations</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#DryingDNA">Drying DNA for Sequencing</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#DNAMiniPrep">DNA Mini-prep</a></li> | ||
+ | <li><a href="https://2014.igem.org/Team:Glasgow/Notebook/Protocols#Ecoli">E.coli Bacterial Strains Used</a></li> | ||
+ | </ul> | ||
+ | |||
+ | </p> | ||
<p id="CreatingCompetentCells"> | <p id="CreatingCompetentCells"> | ||
Line 24: | Line 42: | ||
<li>Pipette 400μl of culture into 20ml of fresh broth</li> | <li>Pipette 400μl of culture into 20ml of fresh broth</li> | ||
<li>Incubate the cultures in shaking 37⁰C water bath for 90 min</li> | <li>Incubate the cultures in shaking 37⁰C water bath for 90 min</li> | ||
- | <li>Calcium chloride and centrifuge tubes must be cooled on ice.</li> | + | <li>50 mM Calcium chloride and centrifuge tubes must be cooled on ice.</li> |
<li>Pour culture into centrifuge tubes, return to ice.</li> | <li>Pour culture into centrifuge tubes, return to ice.</li> | ||
<li>Centrifuge in a cold rotor for 2 min at 7000rpm (6000 G) </li> | <li>Centrifuge in a cold rotor for 2 min at 7000rpm (6000 G) </li> | ||
Line 36: | Line 54: | ||
</p> | </p> | ||
<p id="TransformationOfCompetentCells"> | <p id="TransformationOfCompetentCells"> | ||
+ | |||
+ | <h2>Transformation of Competent Cells</h2> | ||
<ol> | <ol> | ||
Line 44: | Line 64: | ||
<li>Place immediately on ice and leave for 5 min.</li> | <li>Place immediately on ice and leave for 5 min.</li> | ||
<li>Add 200μl of L-Broth and incubate at 37⁰C for 90 min. Expression step.</li> | <li>Add 200μl of L-Broth and incubate at 37⁰C for 90 min. Expression step.</li> | ||
- | <li>Spread 100-200μl on | + | <li>Spread 100-200μl on dried L-agar plates with required antibiotics. On half plates use 40μl.</li> |
<li>Incubate plates</li> | <li>Incubate plates</li> | ||
</ol> | </ol> | ||
</p> | </p> | ||
- | <p id="DNACleanUp" | + | <p id="DNACleanUp"> |
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
+ | <h2>DNA Clean-up</h2> | ||
+ | <ol> | ||
+ | <li>Transfer supernatant to a mini-column</li> | ||
+ | <li>Spin for 1 min on full and pour out flowthrough</li> | ||
+ | <li>Add 500μl of PB, spin for 1 min and discard flowthrough</li> | ||
+ | <li>Add 800μl of PE, spin for 1 min and discard flowthrough</li> | ||
+ | <li>Spin again and discard flowthrough.</li> | ||
+ | <li>Add 50μl of EB to the centre of the white disc and stand for 1 min.</li> | ||
+ | <li>Move column to a 1.5ml Eppendorf (leaving behind the collection tube) and spin for 1 min.</li> | ||
+ | <li>Keep supernatant. DNA is in the liquid.</li> | ||
+ | </ol> | ||
+ | </p> | ||
+ | <p id="PCR"> | ||
+ | |||
+ | <h2>PCR</h2> | ||
+ | |||
+ | 50μl reaction volume – | ||
+ | |||
+ | |||
+ | <ul> | ||
+ | <li>10μl 5 x HF Buffer</li> | ||
+ | <li>5μl 5mM dNTPs</li> | ||
+ | <li>1μl 50mM MgCl2</li> | ||
+ | <li>1.5μl DMSO</li> | ||
+ | <li>5μl 5μM F primer</li> | ||
+ | <li>5μl 5μM R Primer</li> | ||
+ | <li>22μl ddH2O</li> | ||
+ | <li>1μl (1/100 dilution) template DNA</li> | ||
+ | <li>0.5μl polymerase</li> | ||
+ | </ul> | ||
+ | |||
+ | <br> | ||
+ | Programme Settings | ||
+ | |||
+ | <ol> | ||
+ | <li>98⁰C – 1 min</li> | ||
+ | <li>98⁰C – 20 sec</li> | ||
+ | <li>55⁰C – 30 sec</li> | ||
+ | <li>55⁰C – 30 sec (Back to step 2. x30)</li> | ||
+ | <li>72⁰C – 10 min</li> | ||
+ | <li>4⁰C – Hold</li> | ||
+ | </ol> | ||
+ | |||
+ | |||
+ | |||
+ | </p> | ||
+ | <p id="RestrictionDigests"> | ||
+ | |||
+ | <h2>Restriction Digests</h2> | ||
+ | |||
+ | <ol> | ||
+ | <li>Add | ||
+ | <br> | ||
+ | a. For a 20μl sample | ||
+ | <ol> | ||
+ | <li>2μl 10 x buffer</li> | ||
+ | <li>4μl DNA sample</li> | ||
+ | <li>14μl ddH20</li> | ||
+ | <li>0.5μl restriction enzyme</li> | ||
+ | </ol> | ||
+ | |||
+ | b. For a 30μl sample | ||
+ | <ol> | ||
+ | <li>3μl 10 x buffer</li> | ||
+ | <li>10μl DNA sample</li> | ||
+ | <li>17μl ddH20</li> | ||
+ | <li>0.75μl restriction enzyme</li> | ||
+ | </ol> | ||
+ | |||
+ | </li> | ||
+ | <li>Mix thoroughly</li> | ||
+ | <li>Incubate at 37⁰C for at least an hour</li> | ||
+ | |||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="GelExtraction"> | ||
+ | |||
+ | <h2>Gel Extraction</h2> | ||
+ | |||
+ | <ol> | ||
+ | <li>Place gel slice into a microfuge tube</li> | ||
+ | <li>Weigh microfuge tube, add 3 volumes of Buffer QG to volume of gel (100μg = ~100μl)</li> | ||
+ | <li>Incubate at 50⁰C for 10 min (until gel has dissolved) mix by vortex every 2-3 min in incubation</li> | ||
+ | <li>Add 1 gel volume of isopropanol to sample and mix.</li> | ||
+ | <li>Apply sample to spin column, centrifuge 1 min and discard flowthrough.</li> | ||
+ | <li>Add 500μl Buffer QG and centrifuge for 1 min.</li> | ||
+ | <li>Add 750μl Buffer PE, stand for 2-5 min and centrifuge for 1 min.</li> | ||
+ | <li>Discard flowthrough and centrifuge again for 1 min.</li> | ||
+ | <li>Move spin column to microfuge tube</li> | ||
+ | <li>Add 30μl Buffer EB to centre of white disc stand for 1 min and centrifuge for 1 min.</li> | ||
+ | <li>Keep supernatant.</li> | ||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="AnnealingOligos"> | ||
+ | |||
+ | <h2>Annealing Top and Bottom Strand Oligos</h2> | ||
+ | |||
+ | Mix- | ||
+ | <ul> | ||
+ | <li>10μl top strand 100μM</li> | ||
+ | <li>10μl bottom strand 100μM</li> | ||
+ | <li>80μl ddH2O</li> | ||
+ | </ul> | ||
+ | To Anneal- | ||
+ | <ol> | ||
+ | <li>Heat in 85⁰C metal heating block for 5 min</li> | ||
+ | <li>Then turn off heat block leaving tube in block to cool down slowly (1-2 hours) to ~30⁰C</li> | ||
+ | <li>Dilute ‘annealed’ (cold) oligos - 1μl oligo and 99μl ddH2O</li> | ||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="OligosPurification"> | ||
+ | |||
+ | <h2>Oligos Purification</h2> | ||
+ | |||
+ | <ol> | ||
+ | |||
+ | <li>Prepare the polyacrylamide gel - | ||
+ | <br> | ||
+ | a. Prepare the following – | ||
+ | <ol> | ||
+ | <li>Urea – 18.2g</li> | ||
+ | <li>40% acrylamide – 8ml</li> | ||
+ | <li>Add ddH20 up to 40ml</li> | ||
+ | </ol> | ||
+ | b. Mix completely | ||
+ | <br> | ||
+ | c. Add 480μl of 10% Ammonium Peroxidisulphate | ||
+ | <br> | ||
+ | d. Add 24μl of TEMED | ||
+ | </li> | ||
+ | |||
+ | This creates a 1mm thick gel. | ||
+ | <li>Pre-run the gel at 400V and 30mmh to warm up</li> | ||
+ | <li>Prepare the samples by heating at 80⁰C on a heating block for 5 min and then add equal volume formamide loading buffer to sample volume.</li> | ||
+ | <li>Run the gel at 400v for 90 min</li> | ||
+ | <li>Stain the gel in the following for 5 min – | ||
+ | <br> | ||
+ | a. 70ml ddH20 | ||
+ | <br> | ||
+ | b. 20ml isopropanol | ||
+ | <br> | ||
+ | c. 10ml “stains all” | ||
+ | </li> | ||
+ | <li>Cut gel. Cut out the strongest full size oligo-bands and put in a labelled Eppendorf tube</li> | ||
+ | <li>Crush gel fragments</li> | ||
+ | <li>Add 500μl of TE</li> | ||
+ | <li>Put in a shaker at 37⁰C at 1150 overnight</li> | ||
+ | <li>Spin down at 10, 000 rpm for 1 min</li> | ||
+ | <li>Transfer the supernatant to a 0.22 coster filter</li> | ||
+ | <li>Resuspend the pellet with 100μl TE</li> | ||
+ | <li>Spin down supernatant for 1 min at 10, 000 rpm</li> | ||
+ | <li>Spin filter for 1 min at 3, 000 rpm</li> | ||
+ | <li>Transfer to Eppendorf tube</li> | ||
+ | <li>Dry vacuum for ~3 hours at 20⁰C to 200μl</li> | ||
+ | <li>Add 1/9 of the sample volume of Na acetate to the tube</li> | ||
+ | <li>Add 2.5 sample volumes of 100% ethanol to the tube</li> | ||
+ | <li>Mix well and store at -20⁰C overnight</li> | ||
+ | <li>Spin at full speed at -20⁰C for 30 min</li> | ||
+ | <li>Add 1ml of 80% ethanol after removing the supernatant without disturbing the pellet</li> | ||
+ | <li>Spin for 5 min at full speed</li> | ||
+ | <li>Remove the supernatant. If the pellet is disturbed, keep the removed supernatant in a separate Eppendorf.</li> | ||
+ | <li>Spin for 30 seconds at full speed then remove the final bit of supernatant.</li> | ||
+ | <li>Leave open at room temperature to dry for 5-10 min.</li> | ||
+ | <li>Add 20μl of 0.1 x TE and leave to dissolve for ~30 min.</li> | ||
+ | <li>Calculate the oligo concentration through the use of a spectrophotometer.</li> | ||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="MutagenicPCR"> | ||
+ | |||
+ | <h2>Site Directed Mutagenic PCR – Quikchange Protocol</h2> | ||
+ | |||
+ | <ol> | ||
+ | <li>Prepare the 25μl reaction as below – | ||
+ | |||
+ | <ol type="a"> | ||
+ | <li>2.5μl of 10 x Pfu buffer</li> | ||
+ | <li>1μl (of a 1/10 dilution) plasmid template</li> | ||
+ | <li>~62.5ng or 6pmol top primer (1/10 dilution)</li> | ||
+ | <li>~62.5ng or 6pmol bottom primer (1/10 dilution)</li> | ||
+ | <li>2.5μl 2mM dNTP mix</li> | ||
+ | <li>15-17μl ddH20</li> | ||
+ | </ol> | ||
+ | |||
+ | </li> | ||
+ | <li>Add 0.5μl of Pfu-turbo polymerase</li> | ||
+ | <li>Run with the following PCR programme – | ||
+ | <ol type="a"> | ||
+ | <li>95⁰C for 1 min</li> | ||
+ | <li>95⁰C for 40 sec</li> | ||
+ | <li>53⁰C for 40 sec</li> | ||
+ | <li>68⁰C for 14 min</li> | ||
+ | <li>Go back to step b and repeat 15 times</li> | ||
+ | <li>4⁰C hold</li> | ||
+ | |||
+ | </ol> | ||
+ | </li> | ||
+ | <li>Set up the following restriction digest – | ||
+ | |||
+ | <ol type="a"> | ||
+ | <li>10μl of Quikchange reaction</li> | ||
+ | <li>1μl of Buffer A</li> | ||
+ | <li>9μl of ddH20</li> | ||
+ | <li>1μl of DpnI</li> | ||
+ | </ol> | ||
+ | |||
+ | </li> | ||
+ | <li>Vortex and then incubate at 37⁰C for 2 hours</li> | ||
+ | <li>Transform 1μl of reaction</li> | ||
+ | |||
+ | |||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="IntegraseReaction"> | ||
+ | |||
+ | <h2>In vitro φC31 Integrase Reaction</h2> | ||
+ | |||
+ | 20µl sample | ||
+ | |||
+ | <ol> | ||
+ | <li>Add | ||
+ | |||
+ | |||
+ | <ul> | ||
+ | <li>5µl 4 x IRB5 buffer</li> | ||
+ | <li>4 µl plasmid DNA</li> | ||
+ | <li>2 µl integrase</li> | ||
+ | <li>11 µl ddH2O</li> | ||
+ | </ul> | ||
+ | |||
+ | or | ||
+ | |||
+ | <ul> | ||
+ | <li>14 µl 1.43 x IRB3</li> | ||
+ | <li>4 µl plasmid DNA</li> | ||
+ | <li>2 µl integrase</li> | ||
+ | |||
+ | </ul> | ||
+ | |||
+ | </li> | ||
+ | <li>Incubate at 30°C for 1hr 15min – 2hrs</li> | ||
+ | <li>Heat at 78 – 80 °C for 10mins (to kill enzyme)</li> | ||
+ | <li>Spin down</li> | ||
+ | |||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="Ligations"> | ||
+ | |||
+ | <h2>Ligations</h2> | ||
+ | |||
+ | 10 µl sample | ||
+ | |||
+ | <ol> | ||
+ | <li>Add: | ||
+ | |||
+ | <ul> | ||
+ | <li>1 µl 10x ligation buffer</li> | ||
+ | <li>4 µl Insert</li> | ||
+ | <li>5 µl Vector</li> | ||
+ | <li>0.5 µl ligase</li> | ||
+ | </ul> | ||
+ | |||
+ | or | ||
+ | |||
+ | <ul> | ||
+ | <li>5μl of gel purified vector</li> | ||
+ | <li>1μl (of 1/100 dilution) of annealed oligos (or ddH2O control) to make a 10mM oligo solution</li> | ||
+ | <li>1μl of 10 x ligation buffer</li> | ||
+ | <li>3μl of ddH20</li> | ||
+ | <li>0.5μl ligase</li> | ||
+ | </ul> | ||
+ | |||
+ | </li> | ||
+ | |||
+ | <li>Vortex</li> | ||
+ | <li>Leave at room temperature overnight</li> | ||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="DryingDNA"> | ||
+ | |||
+ | <h2>Drying DNA for Sequencing</h2> | ||
+ | |||
+ | <ol> | ||
+ | <li>Add 8 µl of DNA sample to 1.5 µl Eppendorf</li> | ||
+ | <li>Dry DNA in Vacuum Dryer Centrifuge for 30min to 1 hour (with lid open)</li> | ||
+ | <li>In separate tubes, add 1.5 µl of primer for 1st sequencing sample and 5 µl of primer for each reaction after (5 µl x n + 10 µl) n=No. of sequencing reactions</li> | ||
+ | |||
+ | </ol> | ||
+ | |||
+ | <table> | ||
+ | <th>Concentration needed for primers</th> | ||
+ | <tr> | ||
+ | <td>VF</td> | ||
+ | <td>10pmol/µl</td> | ||
+ | </tr> | ||
+ | <tr> | ||
+ | <td>VR</td> | ||
+ | <td>10pmol/µl</td> | ||
+ | </tr> | ||
+ | |||
+ | </table> | ||
+ | |||
+ | </p> | ||
+ | <p id="DNAMiniPrep"> | ||
+ | |||
+ | <h2>DNA Mini-prep</h2> | ||
+ | |||
+ | <ol> | ||
+ | <li>Add 1.4ml of cell culture to 1.5ml Eppendorf, spin at full speed for 2min.</li> | ||
+ | <li>Pour out supernatant. Repeat this with another 1.4ml of culture.</li> | ||
+ | <li>Remove any remaining broth.</li> | ||
+ | <li>Add 250 µl of P1 and resuspend.</li> | ||
+ | <li>Add 250 µl of P2, invert 6 times to mix and leave for 2 min.</li> | ||
+ | <li>Add 350 µl of N3 and invert 6-8 times.</li> | ||
+ | <li>Spin on full for 10 min.</li> | ||
+ | <li>Keep supernatant. DNA is in the liquid.</li> | ||
+ | <li>Carry out DNA Clean-up as above using Qiagen miniprep columns.</li> | ||
+ | </ol> | ||
+ | |||
+ | </p> | ||
+ | <p id="Ecoli"> | ||
+ | |||
+ | <h2>E.coli Bacterial Strains Used</h2> | ||
+ | |||
+ | <ul> | ||
+ | <li>DS941 is AB1157 recF, lacIq lacZ Delta M15</li> | ||
+ | <li>DS941-Z1 as DS941 but with tet repressor and extra copies of lacI</li> | ||
+ | <li>Top10</li> | ||
+ | <li>DH5 α</li> | ||
+ | <li>DH5 α</li> | ||
+ | </ul> | ||
+ | |||
+ | </p> | ||
+ | |||
+ | |||
+ | |||
+ | <a class="editlink" href="https://2014.igem.org/wiki/index.php?title=Team:Glasgow/Notebook/Protocols&action=edit">Edit</a> | ||
</div> | </div> |
Latest revision as of 01:53, 18 October 2014
Protocols
This page shows our protocols for various lab procedures:
- Creating Chemically Competent Cells
- Transformation of Competent Cells
- DNA Clean-up
- PCR
- Restriction Digests
- Gel Extraction
- Annealing Top and Bottom Strand Oligos
- Oligos Purification
- Site Directed Mutagenic PCR – Quikchange Protocol
- In vitro φC31 Integrase Reaction
- Ligations
- Drying DNA for Sequencing
- DNA Mini-prep
- E.coli Bacterial Strains Used
Creating Chemically Competent Cells
- Pipette 400μl of culture into 20ml of fresh broth
- Incubate the cultures in shaking 37⁰C water bath for 90 min
- 50 mM Calcium chloride and centrifuge tubes must be cooled on ice.
- Pour culture into centrifuge tubes, return to ice.
- Centrifuge in a cold rotor for 2 min at 7000rpm (6000 G)
- Pour out the supernatant, being careful about the pellet
- Add 10μl of calcium chloride, immediately return to ice and leave for 1 hour (or longer)
- Repeat the centrifuge step, pour out supernatant
- Store on ice, add 1ml of calcium chloride. Resuspend and return to ice.
Transformation of Competent Cells
- Add 100μl of competent cells to cooled Eppendorfs
- Add 1μl of DNA
- Incubate on ice for 20 min
- Heat shock at 37⁰C for 5 min
- Place immediately on ice and leave for 5 min.
- Add 200μl of L-Broth and incubate at 37⁰C for 90 min. Expression step.
- Spread 100-200μl on dried L-agar plates with required antibiotics. On half plates use 40μl.
- Incubate plates
DNA Clean-up
- Transfer supernatant to a mini-column
- Spin for 1 min on full and pour out flowthrough
- Add 500μl of PB, spin for 1 min and discard flowthrough
- Add 800μl of PE, spin for 1 min and discard flowthrough
- Spin again and discard flowthrough.
- Add 50μl of EB to the centre of the white disc and stand for 1 min.
- Move column to a 1.5ml Eppendorf (leaving behind the collection tube) and spin for 1 min.
- Keep supernatant. DNA is in the liquid.
PCR
50μl reaction volume –- 10μl 5 x HF Buffer
- 5μl 5mM dNTPs
- 1μl 50mM MgCl2
- 1.5μl DMSO
- 5μl 5μM F primer
- 5μl 5μM R Primer
- 22μl ddH2O
- 1μl (1/100 dilution) template DNA
- 0.5μl polymerase
Programme Settings
- 98⁰C – 1 min
- 98⁰C – 20 sec
- 55⁰C – 30 sec
- 55⁰C – 30 sec (Back to step 2. x30)
- 72⁰C – 10 min
- 4⁰C – Hold
Restriction Digests
- Add
a. For a 20μl sample- 2μl 10 x buffer
- 4μl DNA sample
- 14μl ddH20
- 0.5μl restriction enzyme
- 3μl 10 x buffer
- 10μl DNA sample
- 17μl ddH20
- 0.75μl restriction enzyme
- Mix thoroughly
- Incubate at 37⁰C for at least an hour
Gel Extraction
- Place gel slice into a microfuge tube
- Weigh microfuge tube, add 3 volumes of Buffer QG to volume of gel (100μg = ~100μl)
- Incubate at 50⁰C for 10 min (until gel has dissolved) mix by vortex every 2-3 min in incubation
- Add 1 gel volume of isopropanol to sample and mix.
- Apply sample to spin column, centrifuge 1 min and discard flowthrough.
- Add 500μl Buffer QG and centrifuge for 1 min.
- Add 750μl Buffer PE, stand for 2-5 min and centrifuge for 1 min.
- Discard flowthrough and centrifuge again for 1 min.
- Move spin column to microfuge tube
- Add 30μl Buffer EB to centre of white disc stand for 1 min and centrifuge for 1 min.
- Keep supernatant.
Annealing Top and Bottom Strand Oligos
Mix-- 10μl top strand 100μM
- 10μl bottom strand 100μM
- 80μl ddH2O
- Heat in 85⁰C metal heating block for 5 min
- Then turn off heat block leaving tube in block to cool down slowly (1-2 hours) to ~30⁰C
- Dilute ‘annealed’ (cold) oligos - 1μl oligo and 99μl ddH2O
Oligos Purification
- Prepare the polyacrylamide gel -
a. Prepare the following –- Urea – 18.2g
- 40% acrylamide – 8ml
- Add ddH20 up to 40ml
c. Add 480μl of 10% Ammonium Peroxidisulphate
d. Add 24μl of TEMED
This creates a 1mm thick gel.
- Pre-run the gel at 400V and 30mmh to warm up
- Prepare the samples by heating at 80⁰C on a heating block for 5 min and then add equal volume formamide loading buffer to sample volume.
- Run the gel at 400v for 90 min
- Stain the gel in the following for 5 min –
a. 70ml ddH20
b. 20ml isopropanol
c. 10ml “stains all” - Cut gel. Cut out the strongest full size oligo-bands and put in a labelled Eppendorf tube
- Crush gel fragments
- Add 500μl of TE
- Put in a shaker at 37⁰C at 1150 overnight
- Spin down at 10, 000 rpm for 1 min
- Transfer the supernatant to a 0.22 coster filter
- Resuspend the pellet with 100μl TE
- Spin down supernatant for 1 min at 10, 000 rpm
- Spin filter for 1 min at 3, 000 rpm
- Transfer to Eppendorf tube
- Dry vacuum for ~3 hours at 20⁰C to 200μl
- Add 1/9 of the sample volume of Na acetate to the tube
- Add 2.5 sample volumes of 100% ethanol to the tube
- Mix well and store at -20⁰C overnight
- Spin at full speed at -20⁰C for 30 min
- Add 1ml of 80% ethanol after removing the supernatant without disturbing the pellet
- Spin for 5 min at full speed
- Remove the supernatant. If the pellet is disturbed, keep the removed supernatant in a separate Eppendorf.
- Spin for 30 seconds at full speed then remove the final bit of supernatant.
- Leave open at room temperature to dry for 5-10 min.
- Add 20μl of 0.1 x TE and leave to dissolve for ~30 min.
- Calculate the oligo concentration through the use of a spectrophotometer.
Site Directed Mutagenic PCR – Quikchange Protocol
- Prepare the 25μl reaction as below –
- 2.5μl of 10 x Pfu buffer
- 1μl (of a 1/10 dilution) plasmid template
- ~62.5ng or 6pmol top primer (1/10 dilution)
- ~62.5ng or 6pmol bottom primer (1/10 dilution)
- 2.5μl 2mM dNTP mix
- 15-17μl ddH20
- Add 0.5μl of Pfu-turbo polymerase
- Run with the following PCR programme –
- 95⁰C for 1 min
- 95⁰C for 40 sec
- 53⁰C for 40 sec
- 68⁰C for 14 min
- Go back to step b and repeat 15 times
- 4⁰C hold
- Set up the following restriction digest –
- 10μl of Quikchange reaction
- 1μl of Buffer A
- 9μl of ddH20
- 1μl of DpnI
- Vortex and then incubate at 37⁰C for 2 hours
- Transform 1μl of reaction
In vitro φC31 Integrase Reaction
20µl sample- Add
- 5µl 4 x IRB5 buffer
- 4 µl plasmid DNA
- 2 µl integrase
- 11 µl ddH2O
- 14 µl 1.43 x IRB3
- 4 µl plasmid DNA
- 2 µl integrase
- Incubate at 30°C for 1hr 15min – 2hrs
- Heat at 78 – 80 °C for 10mins (to kill enzyme)
- Spin down
Ligations
10 µl sample- Add:
- 1 µl 10x ligation buffer
- 4 µl Insert
- 5 µl Vector
- 0.5 µl ligase
- 5μl of gel purified vector
- 1μl (of 1/100 dilution) of annealed oligos (or ddH2O control) to make a 10mM oligo solution
- 1μl of 10 x ligation buffer
- 3μl of ddH20
- 0.5μl ligase
- Vortex
- Leave at room temperature overnight
Drying DNA for Sequencing
- Add 8 µl of DNA sample to 1.5 µl Eppendorf
- Dry DNA in Vacuum Dryer Centrifuge for 30min to 1 hour (with lid open)
- In separate tubes, add 1.5 µl of primer for 1st sequencing sample and 5 µl of primer for each reaction after (5 µl x n + 10 µl) n=No. of sequencing reactions
Concentration needed for primers | |
---|---|
VF | 10pmol/µl |
VR | 10pmol/µl |
DNA Mini-prep
- Add 1.4ml of cell culture to 1.5ml Eppendorf, spin at full speed for 2min.
- Pour out supernatant. Repeat this with another 1.4ml of culture.
- Remove any remaining broth.
- Add 250 µl of P1 and resuspend.
- Add 250 µl of P2, invert 6 times to mix and leave for 2 min.
- Add 350 µl of N3 and invert 6-8 times.
- Spin on full for 10 min.
- Keep supernatant. DNA is in the liquid.
- Carry out DNA Clean-up as above using Qiagen miniprep columns.
E.coli Bacterial Strains Used
- DS941 is AB1157 recF, lacIq lacZ Delta M15
- DS941-Z1 as DS941 but with tet repressor and extra copies of lacI
- Top10
- DH5 α
- DH5 α