Difference between revisions of "Team:UMaryland/Notebook"

Revision as of 02:33, 19 September 2015

Week 1

First week review

Prepared a bacterial culture containing constitutive GFP (K584001) to grow overnights (E. coli in LB with chloramphenicol)
Performed a transformation in order to replicate our DNA with the constitutive GFP, and plated half of them on the plates containing chloramphenicol and used the other half for another overnight batch
Performed a mini-prep on our overnights with the constitutive GFP in order to isolate plasmids and verify that they were present through spectrophotometry
Started two separate 3A assemblies in order to piece together the pBAD promoter with the miraculin gene and the constitutive GFP gene to the SRNBC gene (homolog to Hok/Sok)
Performed a transformation in order to clone our new plasmids, one containing the pBAD promoter and miraculin gene and the other containing SRNBC and the constitutive GFP

Transformed β-cyclase, AppY, and CRTBEY genes in bacteria to grow on plates overnight
Started a new 3A assembly for the SRNBC and constitutive GFP construct along with pBAD, constitutive colicinFy, and lysostaphin
Final products were SRNBC + constitutive GFP, SRNBC + constitutive colicinFy, and pBAD + lysostaphin
Prepared overnights for the pBAD + miraculin construct that grew on the plates and the β-cyclase, AppY, and CRTBEY genes
Performed minipreps on the overnights we had prepared the day before (for the β-cyclase, AppY, and CRTBEY genes) and shipped them off to be sequenced
Performed transformations on the SRNBC + constitutive GFP, SRNBC + constitutive colicinFy, and pBAD + lysostaphin digests and let them grow overnight

Week 2

Miraculin

- The pBAD +miraculin construct was moved back into psb1C3 backbone and sent for sequencing

Designing gBlocks

- Designed gblocks for epsilon-cyclase (from arabidopsis), pyocin and Hok/Sok

Week 3

Miraculin

- sequence confirmed through sequencing
- failed to extract using French press, FPLC and SDS-Page
- could be due to high arabinose induction (OD of 1)

PCR

- began work on Arduino code to cycle the machine
- purchased Peltier units and lm35 temperature sensors

@@ Line 261: / Line 261: @@
 <li>Prepared a bacterial culture containing constitutive GFP (K584001) to grow overnights (E. coli in LB with chloramphenicol)</li>
 <li>Performed a transformation in order to replicate our DNA with the constitutive GFP, and plated half of them on the plates containing chloramphenicol and used the other half for another overnight batch</li>
-<li>Miniprep<li>
+<li>Performed a mini-prep on our overnights with the constitutive GFP in order to isolate plasmids and verify that they were present through spectrophotometry<li>
-<li>analyzed sequences</li>
+<li>Started two separate 3A assemblies in order to piece together the pBAD promoter with the miraculin gene and the constitutive GFP gene to the SRNBC gene (homolog to Hok/Sok)</li>
-<li>prepared 3A assembly clone of pBAD-miraculin</li>
+<li>Performed a transformation in order to clone our new plasmids, one containing the pBAD promoter and miraculin gene and the other containing SRNBC and the constitutive GFP</li>
 </ul>
 <ul>
-<li>3A assembly</li>
+<li>Transformed β-cyclase, AppY, and CRTBEY genes in bacteria to grow on plates overnight</li>
-<li>two backbones</li>
+<li>Started a new 3A assembly for the SRNBC and constitutive GFP construct along with pBAD, constitutive colicinFy, and lysostaphin</li>
-<li>pSB1C3</li>
+<li>Final products were SRNBC + constitutive GFP, SRNBC + constitutive colicinFy, and pBAD + lysostaphin</li>
-<li>pBAD promoter + genes for miraculin</li>
+<li>Prepared overnights for the pBAD + miraculin construct that grew on the plates and the β-cyclase, AppY, and CRTBEY genes</li>
-<li>cut out pBAD with 2 enzymes (EcoRI and SpeI) and cut out miraculin (XbaI and PstI)</li>
+<li>Performed minipreps on the overnights we had prepared the day before (for the β-cyclase, AppY, and CRTBEY genes) and shipped them off to be sequenced</li>
-<li>want to put pBAD in front of miraculin</li>
+<li>Performed transformations on the SRNBC + constitutive GFP, SRNBC + constitutive colicinFy, and pBAD + lysostaphin digests and let them grow overnight</li>
-<li>put into backbone w/ different antibiotic resistance than original backbone: pSB1A3 (means of selection)</li>
-<li>plate had colonies<li>
-<li>Human Practices<li>
-Kevin got in contact w/ Bioacademy program @ Northwest High School
-Trying to set up a talk for this Wednesday
-Kevin + Adam + Dylan + Juhye going
-goal to target various age groups
-create game
-fundamentals of genetics via presentations, arts, etc.
-Conference scheduled for June 25th
-teams confirmed: UVA, UMBC, Stonybrook, Duke
-contact iGEM headquarters to inform them about meetup → Robert
-<p class=MsoNormal>Kevin got in contact w/ <span class=SpellE>Bioacademy</span>
-program @ Northwest High School <o:p></o:p></p>
-<p class=MsoNormal>Trying to set up a talk for this <span class=SpellE><span
-class=GramE>wednesday</span></span> <o:p></o:p></p>
-<p class=MsoNormal>Kevin + Adam + Dylan + <span class=SpellE>Juhye</span> going
-<o:p></o:p></p>
-<p class=MsoNormal><span class=GramE>goal</span> to target various age groups <o:p></o:p></p>
-<p class=MsoNormal><span class=GramE>create</span> game <o:p></o:p></p>
-<p class=MsoNormal><span class=GramE>fundamentals</span> of genetics via
-presentations, arts, etc. <o:p></o:p></p>
-<p class=MsoNormal>Conference scheduled for June 25th <o:p></o:p></p>
-<p class=MsoNormal>4 teams confirmed: UVA, UMBC, <span class=SpellE>Stonybrook</span>,
-<span class=GramE>Duke</span> <o:p></o:p></p>
-<p class=MsoNormal><span class=GramE>contact</span> <span class=SpellE>iGEM</span>
-headquarters to inform them about meetup &#8594; Robert</p>