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FadD & FadL Module's Lablog

July - Week 4 (20/7~26/7)Open or Close

- PCR amplification of fadD, fadL inserts

- Purification of fadD, fadL PCR products

- LB plate preparation with chloramphenicol (34ug/ml) for selection of pSB1C3 clones

- DH5α competent cells are transformed with BBa_B0030 and BBa_R0040 separately by heat shock

- 1st Extraction of BBa_B0030, BBa_R0040 by miniprep
-> low product yield of BBa_R0040

- Extraction of BBa_R0040, by miniprep
-> low product yield

- New batch of BBa_R0040 transformants are prepared in LB broth
July - Week 5 (27/7~2/8)Open or Close

- Extraction of BBa_R0040 were performed with plasmid miniprep kit

- Restriction digestion were performed on:
fadL, fadD inserts with XbaI and PstI
BBa_R0040, BBa_B0030 with SpeI and PstI
Results: No band was observed for BBa_B0030 after digestion
-> Gel photo showed the extracted BBa_B0030 DNA was contaminated with RNA leading to overestimation of BBa_B0030 concentration for restriction digestion

- Purification was performed on the digested fadL and fadD inserts and BBa_R0040 products

- Ligation of digested fadD insert into BBa_B0030 vector was performed

- DH5α competent cell was transformed with pSB1C3_ R0040-fadL by heat shock protocol

- BBa_B0030 was performed again with plasmid DNA miniprep kit, the product was treated with additional RNase A

- Restriction digestion of BBa_B0030 was performed with SpeI and PstI

- Digested BBa_B0030 was purified with PCR purification kit

- fadL insert was ligated into BBa_R0040 vector

- LB plate with chloramphenicol (34 µg/mL) was prepared
Early AugustOpen or Close

Week 1 (3/8~9/8)

- DH5α competent cells were transformed with pSB1C3_ B0030-fadD by heat shock protocol

- pSB1C3_ R0040-fadL clones was screened with colony PCR method
-> non-specific bands were observed

- pSB1C3_ B0030-fadD clones were screened by colony PCR method
-> non-specific bands were observed

- Repeated colony PCR analysis on the pSB1C3_ R0040-fadL clones
-> Bands with expected size were observed in two clones and sent for DNA sequencing

- pSB1C3_ B0030-fadD clones were screening again with colony PCR method
-> DNA Bands with expected size were observed in 6 clones and sent for DNA sequencing

Week 2 (10/8~16/8)

- Sequencing results show that the transformants contained errors in DNA sequences
-> Missing one to two base pairs in the fadL gene in the pSB1C3_ R0040-fadL clones
-> Missing the ribosomal binding site in the pSB1C3_ B0030-fadD clones

- Repeat screening for pSB1C3_ R0040-fadL clones were performed with the colony PCR method
-> Bands with expected size were observed in 4 clones and sent for DNA sequencing

- PCR amplification of fadD, fadL genes with higher annealing temperature

- Purification of fadD, fadL PCR products

- Double restriction digestion on fadL, fadD PCR products with XbaI and PstI

- Extraction of BBa_B0034 (biobricks with the ribosomal binding site) plasmid by plasmid DNA miniprep kit

- Extraction of BBa_R0040 plasmid with plasmid DNA miniprep kit

- Double restriction digestion on BBa_R0040 plasmid with SpeI and PstI

- Purification of the digested BBa_R0040 plasmid
Late AugustOpen or Close

Week 3 (17/8~23/8)

- Sequencing results showed errors in DNA sequences in the clones prepared last week
-> Missing one to two base pairs in the fadL gene in the pSB1C3_ R0040-fadL plasmid

- Ligation was performed on the fadL insert and the BBa_R0040 vector

- DH5α competent cell was transformed with the pSB1C3_ R0040-fadL plasmid by the heat shock protocol

- Double restriction digestion on BBa_B0034 by SpeI and PstI

- Purification of the digested BBa_B0034 plasmid

- Ligation were performed on the fadD insert and the BBa_B0034 vector

- LB plate with ampicillin (100 µg/mL) were prepared for the selection of pSB1A2 clones

- DH5α competent cells were transformed with pSB1A2_ B0034-fadD by the heat shock protocol

- Screening for pSB1C3_ R0040-fadL clones were done by the colony PCR method
-> DNA bands with expected size were observed in only one clone and sent for DNA sequencing

Week 4 (24/8~30/8)

- Screening on the pSB1A2_ B0034-fadD clones were done by the colony PCR method
-> DNA bands with expected size were observed in 4 clones and sent for DNA sequencing

- PCR amplification of the fadD, fadL inserts were performed at higher annealing temperature

- LB plates with ampicillin (100 µg/mL) were prepared
September - Week 1 (31/8~6/9)Open or Close

- Sequencing results:
The identity of the DNA insert in pSB1C3_ R0040-fadL clone was confirmed by DNA sequencing.
Changes in DNA sequence were found in the fadD gene in pSB1A2_ B0034-fadD clones

Team:CityU HK/notebook/lablog

From 2014.igem.org

Latest revision as of 16:54, 17 October 2014

FadD & FadL Module's Lablog

Week 1 (3/8~9/8)

Week 2 (10/8~16/8)

Week 3 (17/8~23/8)

Week 4 (24/8~30/8)

Sponsors

Stay connected!

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@@ Line 19: / Line 90: @@
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-<br> <br><br><hr><br><br>
+<div id='cssmenu'>
+<ul>
+   <li><a href='https://2014.igem.org/Team:CityU_HK/notebook/lablog'><span>FadD & FadL Module</span></a></li>
+   <li><a href='https://2014.igem.org/Team:CityU_HK/notebook/lablog_2'><span>'TesA Module</span></a></li>
+   <li class='last'><a href='https://2014.igem.org/Team:CityU_HK/notebook/lablog_3'><span>Desaturase Module</span></a></li>
+</ul>
+</div>
+<div><img src="https://static.igem.org/mediawiki/2014/e/ee/CityU_HK_lablog.png" width="100%"></div>
+<div class="container"><div class="row"><div class="col-md-12">
+<div class="arrow-down" id="arrow2"></div>
+</div></div></div>
+<h1 id="title">FadD & FadL Module's Lablog</h1>
+<!-- START -->
+     <div class="wrapper">
+                <div id="st-accordion" class="st-accordion">
+                    <ul>
+                        <li>
+                            <a href="#">July - Week 4 (20/7~26/7)<span class="st-arrow">Open or Close</span></a>
+                            <div class="st-content">
+                                <p><b>-</b> PCR amplification of fadD, fadL inserts</p>
+                                <p><b>-</b> Purification of fadD, fadL PCR products</p>
+                                <p><b>-</b> LB plate preparation with chloramphenicol (34ug/ml) for selection of pSB1C3 clones</p>
+                                <p><b>-</b> DH5α competent cells are transformed with BBa_B0030 and BBa_R0040 separately by heat shock</p>
+                                <p><b>-</b> 1st Extraction of BBa_B0030, BBa_R0040 by miniprep<br> -> low product yield of BBa_R0040</p>
+                                <p><b>-</b> Extraction of BBa_R0040, by miniprep<br> -> low product yield</p>
+                                <p><b>-</b> New batch of BBa_R0040 transformants are prepared in LB broth</p>
+                            </div>
+                        </li>
+<li>
+                            <a href="#">July - Week 5 (27/7~2/8)<span class="st-arrow">Open or Close</span></a>
+                            <div class="st-content">
+                                <p><b>-</b> Extraction of BBa_R0040 were performed with plasmid miniprep kit</p>
+                                <p><b>-</b> Restriction digestion were performed on:
+<br>   fadL, fadD inserts with XbaI and PstI
+<br>   BBa_R0040, BBa_B0030 with SpeI and PstI
+<br>Results: No band was observed for BBa_B0030 after digestion
+<br> -> Gel photo showed the extracted BBa_B0030 DNA was contaminated with RNA leading to overestimation of BBa_B0030 concentration for restriction digestion
+</p>
+                                <p><b>-</b> Purification was performed on the digested <i>fadL</i> and <i>fadD</i> inserts and BBa_R0040 products</p>
+                                <p><b>-</b> Ligation of digested <i>fadD</i> insert into BBa_B0030 vector was performed</p>
+                                <p><b>-</b> DH5α competent cell was transformed with pSB1C3_ R0040-fadL by heat shock protocol</p>
+                                <p><b>-</b> BBa_B0030 was performed again with plasmid DNA miniprep kit, the product was treated with additional RNase A</p>
+                                <p><b>-</b> Restriction digestion of BBa_B0030 was performed with SpeI and PstI</p>
+                                <p><b>-</b> Digested BBa_B0030 was purified with PCR purification kit</p>
+                                <p><b>-</b> <i>fadL</i> insert was ligated into BBa_R0040 vector</p>
+                                <p><b>-</b> LB plate with chloramphenicol (34 µg/mL) was prepared</p>
+                            </div>
+                        </li>
+<li>
+                            <a href="#">Early August<span class="st-arrow">Open or Close</span></a>
+                            <div class="st-content">
+                                <h2 class="title"><b>Week 1 (3/8~9/8)</b></h2>
+                                <p><b>-</b> DH5α competent cells were transformed with pSB1C3_ B0030-fadD by heat shock protocol</p>
+                                <p><b>-</b> pSB1C3_ R0040-<i>fadL</i> clones was screened with colony PCR method                  <br> -> non-specific bands were observed</p>
+                                <p><b>-</b> pSB1C3_ B0030-<i>fadD</i> clones were screened by colony PCR method                    <br> -> non-specific bands were observed</p>
+                                <p><b>-</b> Repeated colony PCR analysis on the pSB1C3_ R0040-fadL clones                    <br> -> Bands with expected size were observed in two clones and sent for DNA sequencing</p>
+                                <p><b>-</b> pSB1C3_ B0030-<i>fadD</i> clones were screening again with colony PCR method                    <br> -> DNA Bands with expected size were observed in 6 clones and sent for DNA sequencing</p>
+                                <h2 class="title"><b>Week 2 (10/8~16/8)</b></h2>
+                                <p><b>-</b> Sequencing results show that the transformants contained errors in DNA sequences<br> -> Missing one to two base pairs in the <i>fadL</i> gene in the pSB1C3_ R0040-fadL clones<br> -> Missing the ribosomal binding site in the pSB1C3_ B0030-<i>fadD</i> clones</p>
+                                <p><b>-</b> Repeat screening for pSB1C3_ R0040-<i>fadL</i> clones were performed with the colony PCR method<br> -> Bands with expected size were observed in 4 clones and sent for DNA sequencing</p>
+                                <p><b>-</b> PCR amplification of <i>fadD</i>, <i>fadL</i> genes with higher annealing temperature</p>
+                                <p><b>-</b> Purification of <i>fadD</i>, <i>fadL</i> PCR products</p>
+                                <p><b>-</b> Double restriction digestion on <i>fadL</i>, <i>fadD</i> PCR products with XbaI and PstI</p>
+                                <p><b>-</b> Extraction of BBa_B0034 (biobricks with the ribosomal binding site) plasmid by plasmid DNA miniprep kit</p>
+                                <p><b>-</b> Extraction of BBa_R0040 plasmid with plasmid DNA miniprep kit</p>
+                                <p><b>-</b> Double restriction digestion on BBa_R0040 plasmid with SpeI and PstI</p>
+                                <p><b>-</b> Purification of the digested BBa_R0040 plasmid</p>
+                            </div>
+                        </li>
+<li>
+                            <a href="#">Late August<span class="st-arrow">Open or Close</span></a>
+                            <div class="st-content">
+                                <h2 class="title"><b>Week 3 (17/8~23/8)</b></h2>
+                                <p><b>-</b> Sequencing results showed errors in DNA sequences in the clones prepared last week<br> -> Missing one to two base pairs in the <i>fadL</i> gene in the pSB1C3_ R0040-fadL plasmid</p>
+                                <p><b>-</b> Ligation was performed on the <i>fadL</i> insert and the BBa_R0040 vector</p>
+                                <p><b>-</b> DH5α competent cell was transformed with the pSB1C3_ R0040-fadL plasmid by the heat shock protocol</p>
+                                <p><b>-</b> Double restriction digestion on BBa_B0034 by SpeI and PstI </p>
+                                <p><b>-</b> Purification of the digested BBa_B0034 plasmid</p>
+                                <p><b>-</b> Ligation were performed on the <i>fadD</i> insert and the BBa_B0034 vector</p>
+                                <p><b>-</b> LB plate with ampicillin (100 µg/mL) were prepared for the selection of pSB1A2 clones</p>
+                                <p><b>-</b> DH5α competent cells were transformed with pSB1A2_ B0034-<i>fadD</i> by the heat shock protocol</p>
+                                <p><b>-</b> Screening for pSB1C3_ R0040-<i>fadL</i> clones were done by the colony PCR method                <br> -> DNA bands with expected size were observed in only one clone and sent for DNA sequencing</p>
+                                <h2 class="title"><b>Week 4 (24/8~30/8)</b></h2>
+                                <p><b>-</b> Screening on the pSB1A2_ B0034-fadD clones were done by the colony PCR method <br> -> DNA bands with expected size were observed in 4 clones and sent for DNA sequencing</p>
+                                <p><b>-</b> PCR amplification of the <i>fadD</i>, <i>fadL</i> inserts were performed at higher annealing temperature</p>
+                                <p><b>-</b> LB plates with ampicillin (100 µg/mL) were prepared</p>
+                            </div>
+                        </li>
+<li>
+                            <a href="#">September - Week 1 (31/8~6/9)<span class="st-arrow">Open or Close</span></a>
+                            <div class="st-content">
+                                <p><b>-</b> Sequencing results:
+<br>  The identity of the DNA insert in pSB1C3_ R0040-fadL clone was confirmed by DNA sequencing.
+<br>  Changes in DNA sequence were found in the fadD gene in pSB1A2_ B0034-fadD clones
+</p>
+                            </div>
+                        </li>
+                    </ul>
+                </div>   <!-- end of .st-accordion-->
+</div>  <!--end of wrapper-->
-<center> <font size = "6" > <b> Lab Log </b> </font> </center>
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+<!--==================== footer ===========================-->
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+      <h3>Sponsors</h3>
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+     <a href="http://www6.cityu.edu.hk/bhdbapp/deptweb/index.html" target="_blank"><img src="https://static.igem.org/mediawiki/2014/9/98/CityU_HK_bchlogo.png" width="80"></a>
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+      <h3>Stay connected!</h3>
+      <p>email: <a href="mailto:cityuhk.igem@gmail.com">cityuhk.igem@gmail.com</a></p>
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