Difference between revisions of "Team:Dundee/Lab Book/Fingerprints"
(7 intermediate revisions by 2 users not shown) | |||
Line 9: | Line 9: | ||
− | <header id="header- | + | <header id="header-fingerprint"> |
<a class="anchor" id="top"></a> | <a class="anchor" id="top"></a> | ||
<center> | <center> | ||
Line 22: | Line 22: | ||
<div class="row"> | <div class="row"> | ||
<div class="col-lg-4"> | <div class="col-lg-4"> | ||
− | <a href="#section1" class="scroll"><span class="glyphicon glyphicon- | + | <a href="#section1" class="scroll"><span class="glyphicon glyphicon-tint" onclick="location.href='https://2015.igem.org/Team:Dundee/Lab_Book/FluID';" ></span></a> |
<h3>FluID</h3> | <h3>FluID</h3> | ||
<p class="about-content">FluID is a cell free, all in one spray which will be used to detect and dinstiguish between body fluids found at crime scenes.</p> | <p class="about-content">FluID is a cell free, all in one spray which will be used to detect and dinstiguish between body fluids found at crime scenes.</p> | ||
</div> | </div> | ||
<div class="col-lg-4"> | <div class="col-lg-4"> | ||
− | <a href="#section2"><span class="glyphicon glyphicon- | + | <a href="#section2"><span class="glyphicon glyphicon-pushpin" type="button" onclick="location.href='https://2015.igem.org/Team:Dundee/Lab_Book/Chromate_Detector';"></span></a> |
<h3>Chromate Biosensor</h3> | <h3>Chromate Biosensor</h3> | ||
<p class="about-content">Our chromate biosensor is a device that will be used to detect stainless steel residues left behind on bones in blunt or sharp force trauma cases.</p> | <p class="about-content">Our chromate biosensor is a device that will be used to detect stainless steel residues left behind on bones in blunt or sharp force trauma cases.</p> | ||
</div> | </div> | ||
<div class="col-lg-4"> | <div class="col-lg-4"> | ||
− | <a href="#section3"><span class="glyphicon glyphicon- | + | <a href="#section3"><span class="glyphicon glyphicon-hand-down" onclick="location.href='https://2015.igem.org/Team:Dundee/Lab_Book/Fingerprints';"></span></a> |
<h3>Fingerprint Ageing</h3> | <h3>Fingerprint Ageing</h3> | ||
<p class="about-content">This device will search for the presence of a specifc component found in fingerprint deposits whose presence/absence will indicate approximate fingerprint age.</p> | <p class="about-content">This device will search for the presence of a specifc component found in fingerprint deposits whose presence/absence will indicate approximate fingerprint age.</p> | ||
Line 38: | Line 38: | ||
</div> | </div> | ||
</section> | </section> | ||
+ | |||
+ | <div class="ribbon"> | ||
+ | <div class="rows"> | ||
<!-- WEEK 1 --> | <!-- WEEK 1 --> | ||
<div class="row"> | <div class="row"> | ||
+ | <div class="border-week"> | ||
<div class="box"> | <div class="box"> | ||
<div class="labtitle">Week Beginning 24/8/2015</div> | <div class="labtitle">Week Beginning 24/8/2015</div> | ||
Line 88: | Line 92: | ||
</div> | </div> | ||
</div> | </div> | ||
+ | </div> | ||
</div> | </div> | ||
Line 372: | Line 377: | ||
}); | }); | ||
− | + | $('.chevron_toggleable').on('click', function() { | |
+ | $(this).toggleClass('glyphicon-chevron-down glyphicon-chevron-up'); | ||
+ | }); | ||
+ | $('.plusminus-toggleable').on('click', function() { | ||
+ | $(this).toggleClass('glyphicon-plus-sign glyphicon-minus-sign'); | ||
+ | }); | ||
Line 379: | Line 389: | ||
</body> | </body> | ||
</html> | </html> | ||
− | |||
{{:Team:Dundee/footer}} | {{:Team:Dundee/footer}} |
Latest revision as of 23:40, 18 September 2015
Summary
Cloning of LS into the high expression vector pQE80-L was started this week.
Aim of experiment: To set digest LS with BamHI and KpnI and set up ligations with the high expression vector pQE80-L.
Protocols Used: Restriction Digests Ligations
Results: N/A
Next Steps: Ligations will be left in the cold room over the weekend and transformed into M15pREP4 E.coli on Monday.
Summary
Cloning of LS into pQE80-L was completed this week and cloning of LS into pSB1C3 was begun.
Aim of experiment: To set up transformations of pQE80-L-LS into M15pREP4 E.coli
Protocols Used: Transformations
Results: N/A
Next Steps: If the transformations are successful, colonies will be selected for overnight cultures tomorrow.
Aim of experiment: To set up overnight cultures of M15pREP4 E.coli containing pQE80-L-LS.
Protocols Used: Overnight Cultures
Results: N/A
Next Steps: The overnight cultures will be miniprepped tomorrow.
Aim of experiment: To miniprep the M15pREP4 E.coli Overnight Cultures containing pQE80-L-LS.
Protocols Used: Plasmid Purification
Results: N/A
Next Steps: The miniprep with highest concentration will be sent for sequencing.
Aim of experiment: To digest the LS PCR product with EcoRI and PstI and then set up ligations with pSB1C3.
Protocols Used: Restriction Digests Ligations
Results: N/A
Next Steps: Ligations will be left over the weekend and transformed into JM110 E.coli on Monday.
Summary
Cloning of LS into pSB1C3 was completed this week and sequencing confirmed it was successfully inserted into pQE80-L so overexpression assays were performed where LS was characterised via Western Blotting.
Aim of experiment: To transform pSB1C3-LS into JM110 E.coli.
Protocols Used: Transformations
Results:N/A
Next Steps:If transformations are successful, overnight cultures will be set up tomorrow.
Aim of experiment: To set up overnight cultures of JM110 E.coli containing pSB1C3-LS from the transformations carried out yesterday.
Protocols Used: Overnight Cultures
Results: N/A
Next Steps: The overnight cultures will be miniprepped and sent for sequencing tomorrow.
Aim of experiment: To miniprep the JM110 E.coli Overnight Cultures containing pSB1C3-LS.
Protocols Used:
Plasmid Purification (QIAprep® Spin Miniprep Kit)Results: N/A
Next Steps: The miniprep with the highest concentration will be sent for sequencing to confirm presence of insert. Sequencing for pQE80-L-LS came back correct so overexpression assays will be started tomorrow.
Aim of experiment: To set up overexpression assays of LS using different concentrations of IPTG.
Protocols Used: Overexpression Assays Note: Cultures were induced with 0 mM, 0.5 mM, 1 mM and 2 mM IPTG. The membrane for the blot was left blocking overnight.
Results: Figure 3
Next Steps: The gel shows a band corresponding to the expected size of LS. However, Western Blotting will confirm if it is indeed LS.
Aim of experiment: To complete characterisation of LS via Western Blotting.
Protocols Used: Westen Blotting
Results: Figure 4
Next Steps: The blot shows that LS has been successfully detected at the expected size of 80 kDa. There is also partial degradation of the protein. Nevertheless, purification of LS will be started next week.
Summary
Purification of lanosterol synthase was started this week.
Aim of Experiment: To set up overnight cultures of M15pREP4 E.coli containing pQE80-L-LS.
Protocols Used: Overnight Cultures Note: 150 ml cultures were set up.
Results: N/A
Next Steps: The overnight cultures will be used to innoculate a 3 L day culture tomorrow.
Aim of experiment: To set up 3 L day cultures of M15pREP4 E.coli containing pQE80-L-LS.
Protocols Used: Protein Purification Note: The protocol was stopped at Step 6- protein purification will be continued tomorrow.
Results: N/A
Next Steps: Affinity chromatography will be carried out tomorrow.
Aim of experiment: To continue purification of LS.
Protocols Used: Protein Purification Note: Protocol was stopped at Step 13.
Next Steps: The SDS gel suggests that the peak observed in the affinity chromatography step may due to a smaller sized protein which has shown up strongly on the gel. However, there is still a band observable around the 75 kDa marker which may be LS. The samples will be pooled together and concentrated. A small sample will be blotted and then size exclusion chromaography can be performed.