Team:Yale/Our Project/Notebook/Week 8

From 2010.igem.org

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<li id="nb"><a href="https://2010.igem.org/Team:Yale/Our Project/Notebook/Week 7">week 7</a></li>
<li id="nb"><a href="https://2010.igem.org/Team:Yale/Our Project/Notebook/Week 7">week 7</a></li>
<li id="nb"><b><a href="https://2010.igem.org/Team:Yale/Our Project/Notebook/Week 8">week 8</a></b></li>
<li id="nb"><b><a href="https://2010.igem.org/Team:Yale/Our Project/Notebook/Week 8">week 8</a></b></li>
 +
<li id="nb"><a href="https://2010.igem.org/Team:Yale/Our Project/Notebook/Week 9">week 9</a></li>
<li><a href="https://2010.igem.org/Team:Yale/Our Project/Protocols">protocols</a></li>
<li><a href="https://2010.igem.org/Team:Yale/Our Project/Protocols">protocols</a></li>
<li><a href="https://2010.igem.org/Team:Yale/Our Project/Safety">safety</a></li>
<li><a href="https://2010.igem.org/Team:Yale/Our Project/Safety">safety</a></li>
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<!------------- atgc ------------->
<!------------- atgc ------------->
-
>sequence of desired phsABC/B0015 construct (in
+
>sequence of desired phsABC/B0015 construct (minus background) <br/>
 +
gaggaggtttattactagatgagcattagtcgtcgttcttttttgcagggggtaggcatcggctgctctgcctgcgcgctgggcgcttttccgcccgggg
 +
cgctggcgcgcaacccgattgccggcattaacggtaaaaccacgctaacgccaagcttgtgcgaaatgtgttcctttcgttgccctattcaggcgcaggt
 +
agtcaataacaagaccgtttttatccagggcaatccttctgcgccgcagcaggggacgcgcatatgcgccaggggcgggagcggcgtcagcctggtcaat
 +
gacccgcaacggattgtaaaacctatgaaacgcaccgggccacgcggcgacggtgaatggcaggtgattagctggcaacaggcttaccaggaaatcgcgg
 +
cgaaaatgaatgccatcaaagcgcagcatggccccgagagcgtggctttctcttccaaatcgggctcgctctccagccatcttttccatctggctacggc
 +
ctttggttcgcctaatacctttacgcacgcctcaacatgccctgccgggaaagccattgcggcaaaagtgatgatgggcggcgatctggcgatggatatc
 +
gctaacacgcgctatctggtttcgtttggccacaatttgtatgaagggattgaagttgccgatacccatgagttaatgaccgcgcaggagaagggggcca
 +
aaatggtgagcttcgatccgcgtttgtcgatattttccagcaaggcggatgagtggcacgctattcgtcccgggggggatttagcggttctgctggcgat
 +
gtgccacgtcatgattgatgaacagctctacgatgcgtcttttgttgagcgttataccagcggatttgaacagttagcacaggcggtaaaagagacgacg
 +
ccggaatgggccgccgcgcaggccgatgtcccagccgacgttattgtccgggtgacacgcgaactggctgcctgcgcgcctcacgctattgtcagtcctg
 +
gtcatcgcgcgacgttctcgcaggaagagatcgatatgcggcgtatgatttttacgcttaatgtgctgctcggtaatattgagcgcgaaggcgggctata
 +
tcagaaaaaaaacgcgtctgtttacaataaactggccggagaaaaggtcgcgccaacgctggcgaaactcaacattaaaaatatgccgaaaccgacggcg
 +
caacgcatcgatttggtcgcaccgcagtttaaatatatcgccgctggcggcggcgtggtgcaaagcattattgactcggcgttaacccagaagccttacc
 +
cgataaaggcgtggattatgtcgcggcataatcctttccagaccgtcacctgtcgttcggacctggtaaaaaccgttgagcaactggatctggtggtcag
 +
ctgcgatgtctatttgagcgagagcgcggcatatgccgactatctgctgccggaatgcacctatctcgaacgggacgaagaggtatccgatatgtcggga
 +
ctgcacccggcttacgctctgcgccaacaggtcgtagagccgattggcgaggcgcgtccgagttggcaaatctggaaagaacttggcgagcagttgggat
 +
tagggcagtactatccgtggcaggatatgcagacgcgccaactctatcagttgaacggcgaccatgccttagcgaaggaactgcgacagaaagggtatct
 +
cgaatggggcgttccgctgctattacgcgaaccagaatccgttcgtcagtttacggcgcgttaccccggcgctatcgcgacggacagtgacaacacctat
 +
ggcgaacagcttcgcttcaaatcgccctccggcaaaatcgaactttattccgcaaccctggaggaattgctccctggctacggcgttccgcgcgttcgtg
 +
actttgcgctgaaaaaagagaatgagctttacttcattcagggcaaggtggccgtgcataccaatggcgcgacgcagtacgtacctttactcagcgagct
 +
aatgtgggataacgcggtctgggttcatccgcaaacggcgcaagaaaaaggcattaagaccggcgatgagatctggctggaaaatgccacgggtaaagag
 +
aaaggtaaggcgctggtgacgcccggtatccgcccggacacgctttttgtctatatgggatttggcgctaaagctggggccaaaacggcggcgacgacac
 +
acggtatccactgcggaaatttactgccgcacgtgacgagtccggtatccggtacggtagtgcataccgcaggcgtgacgctgagccgggcatgaatgaa
 +
tcatttaacgaatcagtacgtcatgctgcatgatgaaaaacgttgtatcggctgccaggcgtgtaccgttgcctgcaaagtgcttaatgacgtaccggag
 +
ggatttagccgcgtacaggtacaaattcgcgcccctgaacaggcatccaacgcactaacccattttcaatttgtccgcgtctcctgtcagcactgtgaaa
 +
atgcgccatgtgtcagcgtttgtcctaccggagcgtcatatcgtgatgaaaacgggatcgtgcaggtggataaatcgcgctgtattggctgcgattattg
 +
tgttgccgcgtgtcctttccatgtgcgctatttgaatccgcaaaccggtgtcgccgacaagtgtaacttctgcgccgacacgcggttggcggctggccag
 +
tctccggcgtgcgtatccgtttgcccaacggacgcgctgaaattcggcagactggatgagagcgagatccagcgctgggtcggtcagaaagaggtctatc
 +
gccagcaggaggcgcgtagcggcgcggtcagtctgtaccgtcgtaaagaagtccatcaggagggtaaagcatgaatgaatactatctggggagcggaact
 +
acattatgcgccagattattggccgctgtggttaatttacgcaggcgtcgtggtgctgctcatgcttgttgggctggttatccatgcgttattgcgccgg
 +
atgctggcgccaaaaacggcgggcggtgaagaacatcgtgactatctctactcgctggcgattcgccgctggcattggggaaatgcgttactgtttgttt
 +
tattactgttaagcggtttatttggtcatttttctctcggccctgtagcgctaatggtacaagtgcatacctggtgtggttttgccttactggctttctg
 +
ggtcgggtttgtgctgatcaacctcaccacaggtaacgggcgtcactatcgggtaaatttttccggactggtaacgcgctgcatacgccagacgcgtttt
 +
tacctttttggcattatgaaaggggaagcgcatccgttcgtggcaacagagcagaataagttcaatccactgcaacaactggcatatctggcgattatgt
 +
acgcgctggtaccgctgttaatcatcaccggtttgctgtgtctctatccgcaggttgcgggtctgggccctgtgatgctggtgctgcatatggcgcttgc
 +
tatcatcggcttactgtttatttgcgcgcatctctatctgtgtactcttggcgacacgccgggacaaattttccgtagcatggttgacggctatcatcgt
 +
catcgtaccgcgccgcgcggggataagtccgccgtctgatactagagccaggcatcaaataaaacgaaaggctcagtcgaaagactgggcctttcgtttt
 +
atctgttgtttgtcggtgaacgctctctactagagtcacactggctcaccttcgggtgggcctttctgcgtttata <br/><br/>
 +
>Forward sequence of ligation sample <br/>
 +
nnnnnngnnttnnnnnnnnnnntaggcgtatcacgaggcagaatttcagataaaaaaaatccttagctttcgctaaggatgatttctggaattcgcggcc
 +
gcttctagagaggaggtttatatgagcattagtcgtcgttcttttttgcagggggtaggcatcggctgctctgcctgcgcgctgggcgcttttccgcccg
 +
gggcgctggcgcgcaacccgattgccggcattaacggtaaaaccacgctaacgccaagcttgtgcgaaatgtgttcctttcgttgccctattcaggcgca
 +
ggtagtcaataacaagaccgtttttatccagggcaatccttctgcgccgcagcaggggacgcgcatatgcgccaggggcgggagcggcgtcagcctggtc
 +
aatgacccgcaacggattgtaaaacctatgaaacgcaccgggccacgcggcgacggtgaatggcaggtgattagctggcaacaggcttaccaggaaatcg
 +
cggcgaaaatgaatgccatcaaagcgcagcatggccccgagagcgtggctttctcttccaaatcgggctcgctctccagccatcttttccatctggctac
 +
ggcctttggttcgcctaatacctttacgcacgcctcaacatgccctgccgggaaagccattgcggcaaaagtgatgatgggcggcgatctggcgatggat
 +
atcgctaacacgcgctatctggtttcgtttggccacaatttgtatgaagggattgaagttgccgatacccatgagttaatgaccgcgcaggagaaggggg
 +
ccaaaatggtgagcttcgatccgcgtttgtcgatattttccagcaaggcggatgagtggcacgctattcgtcccgggggggatttagcggttctgctggc
 +
gatgtgccacgtcatgattgatgaacagctctacgatgcgtcttttgttgagcgttataccagcggatttgaacagttagcacaggcggtaaaagagacg
 +
acgccggaatgggccnngcgcaggccgatgtn
 +
<br/> <br/>
 +
>Reverse sequence of ligation sample <br/>
 +
actatctggggangcggaactacattatgcgccagattattggccgctgnggttaatttacgcaggcgtcgtggtgctgctcatgcttgttgggctggtt
 +
atccatgcgttattgcgccggatgctggcgccaaaaacggcgggcggtgaagaacatcgtgactatctctactcgctggcgattcgccgctggcattggg
 +
gaaatgcgttactgtttgttttattactgttaagcggtttatttggtcatttttctctcggccctgtagcgctaatggtacaagtgcatacctggtgtgg
 +
ttttgccttactggctttctgggtcgggtttgtgctgatcaacctcaccacaggtaacgggcgtcactatcgggtaaatttttccggactggtaacgcgc
 +
tgcatacgccagacgcgtttttacctttttggcattatgaaaggggaagcgcatccgttcgtggcaacagagcagaataagttcaatccactgcaacaac
 +
tggcatatctggcgattatgtacgcgctggtaccgctgttaatcatcaccggtttgctgtgtctctatccgcaggttgcgggtctgggccctgtgatgct
 +
ggtgctgcatatggcgcttgctatcatcggcttactgtttatttgcgcgcatctctatctgtgtactcttggcgacacgccgggacaaattttccgtagc
 +
atggttgacggctatcatcgtcatcgtaccgcgccgcgcggggataagtccgccgtctgatactagagccaggcatcaaataaaacgaaaggctcagtcg
 +
aaagactgggcctttcgttttatctgttgtttgtcggtgaacgctctctactagagtcacactggctcaccttcgggtgggcctttctgcgtttatatac
 +
tagtagcggccgctgcagtccggcaaaaaagggcaaggtgtcaccaccctgccctttttctttaaaaccgaaaagattacttcgcgttatgcaggcttcc
 +
tcgctcactgactcgctgcgctcggtcgtngnnnnnnnnnn
<!------------- atgc ------------->
<!------------- atgc ------------->
 +
</div>
</ul>
</ul>
<h4>Beginning of second ligation efforts </h4>
<h4>Beginning of second ligation efforts </h4>
<ul>  
<ul>  
-
<li>With the phsABC insert finally in B0015, the next step is to insert the Q04121 promoter in front of phsABC. Begin with sequential double digests of Q04121 and the phsABC/B0015 construct</li>
+
<li>With the phsABC insert finally in B0015, the next step is to insert the Q04121 promoter in front of phsABC. Begin with double digests of Q04121 and the phsABC/B0015 construct double digest</li>
 +
<li>Q04121 double digest: 6 uL of Q04121, 5 uL of EcoRI buffer, 1.8 uL of EcoRI, 1.8 uL of SpeI, 0.5 uL of 100x BSA, and 34.9 uL of water.  </li>
 +
<li>phsABC/B0015 construct sequential digest: 5 uL of DNA, 5 uL of NEB buffer 4, 0.5 uL of BSA, 1.8 uL of XbaI, and 37.7 uL of water.</li>
 +
<li> Run both of the digests for six hours at 37˚C before heat-killing with 20 minutes at 80˚C, then add 0.5 uL 5 M NaCl and 1.8 uL of EcoRI to the vector and let it have a five hour digestion period at 37˚C followed by another heat-kill at 80˚C. </li>
</ul>
</ul>
<i> This day's work is also recorded on page 83 & 84 of the lab notebook hard copy. </i>
<i> This day's work is also recorded on page 83 & 84 of the lab notebook hard copy. </i>
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<li>
<li>
-
Thursday 7/29--
+
Thursday 7/29--First attempt at Q04121 ligation
</li>
</li>
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<!------------- Thursday ------------->
<!------------- Thursday ------------->
-
Extra content
+
<h4>Ligation of Q04121 and phsABC/B0015 construct </h4>
 +
<ul>
 +
<li>Given that the DNA concentration of the 5.8 kb Q04121 insert is 20 ng/uL and that of the 7.8 kb vector is 19.3 ng/uL, calculate that 2.15 uL of insert is stoichiometric equivalent of 3 uL of vector.  Based on this set-up the following ligation reactions and let them run for 8 hours at 16˚C before a 20 minute heat-kill. </li>
 +
<b> Control ligation </b> 2 uL of ligase buffer, 1 uL T4 ligase, 3 uL of vector, and 14 uL of water. <br/>
 +
<b> 2:1 Insert:vector ligation </b> 2 uL of ligase buffer, 1 uL T4 ligase, 3 uL of vector, 4.3 uL insert, and 9.7 uL of water. <br/>
 +
<b> 5:1 Insert:vector ligation </b> 2 uL of ligase buffer, 1 uL T4 ligase, 3 uL of vector, 10.8 uL of insert, and 3.2 uL of water. <br/>
 +
<li> After the ligations were heat-killed, transformed them into Top10 supercompetent cells using the <a href="https://2010.igem.org/Team:Yale/Our_Project/Protocols/transformation"> standard transformation protocol </a> and a pUC19 control.  Plated on kanamycin plates and left in incubator overnight. </li>
 +
</ul>
<i> This day's work is also recorded on page 84 of the lab notebook hard copy. </i>
<i> This day's work is also recorded on page 84 of the lab notebook hard copy. </i>
<!------------- Thursday ------------->
<!------------- Thursday ------------->
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<li>
<li>
-
Friday 7/30--
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Friday 7/30--No colonies visible from 7/29 transformation, so returned plates to incubator.
</li>
</li>
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<a id="link" href="javascript:ReverseDisplay('friday')">See more/less</a>
 
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<div style="display:none;" id="friday">
 
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<!------------- Friday ------------->
 
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Extra content
 
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<i> This day's work is also recorded on page 85 of the lab notebook hard copy. </i>
 
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<!------------- Friday ------------->
 
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</div>
 
<li>
<li>
-
Saturday short content
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Saturday 7/31--Plates from ligation transformation showed growth.
</li>
</li>
-
<a id="link" href="#" onclick="toggle_visibility('saturday'); return false;">See more</a>
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<a id="link" href="javascript:ReverseDisplay('saturday')">See more/less</a>
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<div style="display:none" id="saturday">
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<div style="display:none;" id="saturday">
<!------------- Saturday ------------->
<!------------- Saturday ------------->
-
Extra content
+
<h4>Second ligation transformants </h4>
 +
<ul>
 +
<li>The pUC19 and control ligation plates both showed many colonies, but the 2:1 ligation showed even more, while the 5:1 ligation showed 18 large colonies. </li>
 +
<i> This day's work is also recorded on page 85 of the lab notebook hard copy. </i>
<!------------- Saturday ------------->
<!------------- Saturday ------------->
</div>
</div>
-
<li>
 
-
Sunday short content
 
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</li>
 
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<a id="link" href="#" onclick="toggle_visibility('sunday'); return false;">See more</a>
 
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<div style="display:none" id="sunday">
 
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<!------------- Sunday ------------->
 
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Extra content
 
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<!------------- Sunday ------------->
 
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</div>
 
<!------------- LAB NOTEBOOK ------------->
<!------------- LAB NOTEBOOK ------------->

Latest revision as of 03:50, 28 October 2010

iGEM Yale

lab notebook: week 8 (7/26-8/1)

  • Monday 7/26--Efforts to confirm that ligation of phsABC and B0015 actually occurred.
  • See more/less
  • Tuesday 7/27--Diagnostic double digest of likely ligations
  • See more/less
  • Wednesday 7/28--Sequencing confirms ligation success!
  • See more/less
  • Thursday 7/29--First attempt at Q04121 ligation
  • See more/less
  • Friday 7/30--No colonies visible from 7/29 transformation, so returned plates to incubator.
  • Saturday 7/31--Plates from ligation transformation showed growth.
  • See more/less