Team:HKUST-Hong Kong/notebook.html

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Notebook

Week 1 (4th-10th June)
Strain construction

Genomic DNA of E. coli DH10b extracted
Waiting for materials (bacterial strains, primers) to arrive

Week 2 (13th-17th June)
Strain construction

Genomic DNA of E. coli DH10b extracted. Genomic DNA of BL21 extracted
Cloned out split superfolder GFP construct
Finished design of PCR primers for nadE gene and λ RED

Culture Test

Wild type MIC test optimization (kanamycin gradient 0-25 µg/ml, serial dilutions)
Constructed standard curve for OD600 verses RR1 (wild type) CFU concentration

Week 3 (20th-24th June)
Strain construction

nadE: PCR out nadE gene from the genome of BL21
Split superfolder GFP system: The test of the intact (sfGFP 1-10 still ligated together with sfGFP11) superfolder GFP was successful. Confirmation tests and further experiments would be conducted soon.
2010 Slovenia’s method - CFP/YFP: BioBricks would be transformed into E. coli DH10b. Tests would be conducted soon.
λ RED and oriR101&repA101-ts: pKD46 has arrived and successfully extracted. RFP reporter system was ready. Primers of RepA101ts-OriR101 are ready.

Culture Test

Performed 2nd and 3rd MIC tests for wild type (kanamycin gradient 5-20 µg/ml, 2µg/ml intervals)
Minipreps of BBa_I763007 and BBa_E1010 were successful

Week 4 (27th June–1st July)
Strain construction

λ RED : protocol design finished; pKD46 arrived and digestion tests indicated that the plasmid was correct; PCR RFP with homologous sequence was successful
2010 Slovenia’s method - CFP/YFP: protocol design finished, successfully finished combined CFP and YFP
Split superfolder GFP system: protocol design finished; primer arrived
Pir gene and ori-γ: protocol under construction; primer for ori-γ arrived; BW25141 gDNA extraction successful

Culture Test

Ligation of pSB2K3 (from BBa_E1010) with RFP reporter device (BBa_I763007)
Transformation of the RFP/KanR plasmid to E. coli DH10b

Week 5 (8th-12th July)
Strain construction

ori-γ: Primers arrived, PCR was successful. Result: one of four samples was positive, but of low concentration
pir gene: gDNA of BW25141 successfully extracted
Split superfolder GFP system: GFP1-10 PCRed, GFP11 PCRed
2010 Slovenia’s method - CFP/YFP: Verified combined fluorescence protein
oriR101 & repA101-ts: Clone- out by PCR was successful

Culture Test

Successful construction of a RFP-labeled kanamycin-resistant strain
Information from literature search on mechanisms to raise the MIC for the proposed T4MO mutant slightly help it survive in kanamycin long enough to fulfill its function
MIC testing for RR-1

Week 6 (15th-19th July)
Strain construction

λ RED: PCR of RFP with homologous sequence successful
2010 Slovenia’s method - CFP/YFP: digestion and ligation of CFP, YFP with pBluescript KS+ promoter finished
Split superfolder GFP system: PCR of spilt superfolder GFP successful
2010 Slovenia’s method - CFP/YFP :Ligation with promoter is successful, but the green fluorescence could not be observed. Considering to redo construction
pToolkit construction: PCR of ori-γ successful; ligation with pKD46 backbone was done, confirmation still awaiting the results of colony PCR to check the existence of ori-γ; the sequencing PCR of the pir gene was done, now waiting to check the results
nadE gene: ligation nadE gene with double terminator not successful. Would repeat experiments next week

Culture Test

MIC test for wild type RR1 (kanamycin gradient 5-13 µg/ml, 1µg/ml intervals)
MIC test for mixed cultures of RFP/KanR and RR1(1:99)
Literature search – multidrug pump candidates

Bcr(~1.2kbp): overexpression increases kanamycin MIC ~2-4fold
NorM (~1.3kbp): overexpression reduces radical oxidative species (e.g. H₂O₂) inside the cell

Week 7 (22nd-26th July)
Strain construction

pir gene: Sequencing product did not meet sequencing requirement (a lot of 'N's) – sequencing rejected. To do: practice how to perform sequencing clean-up properly
Split superfolder GFP system: Construct to be ligated had very low recovery from gel purification; another trial would be done asap
2010 Slovenia’s method – CFP/YFP: combination of n-terminal and c-terminal CDS into same plasmid, driven by plac promoter of pBluescriptKS+ completed. Result: very weak fluorescence observed
nadE gene: successful ligation of nadE gene with terminator; correctness of construct confirmed by restriction digestion tests. Component was putatively finished as biobrick
oriR101&repA101-ts: basic protocol for site-directed-mutagenesis + fusion PCR tested to be successful. Repeating fusion PCR
λ RED: Previous experiment of gene swapping failed. Trouble-shooting in progress
pToolkit construction: results from colony PCR of ori-γ from transformed bacteria: successful completion of pToolkit. Further confirmation by restriction digestion to be done

Culture Test

Mixed culture MIC tests for RFP/KanR and RR1(99:1)
Multidrug Efflux Pump – Settled on Bcr as the candidate gene

2~4 folded increasing for Kan
Proton gradient (H⁺) driven
Pumps out other toxins
Unknown promoter

E. coli DH10a containing pUC18Not/T4MO arrived

Week 8 (1st-5th Aug)
Strain construction

pir gene: Sequencing result has just come out
Split superfolder GFP system: Finished ligation of lacI promotor and GFP 11 and verifying. GFP 1-10 PCRing
2010 Slovenia’s method - CFP/YFP: Finished construction but not verified
nadE gene: construction finished, but construct was still harbored in pSB1AK3. Consider relocation to pSB1C3 asap.
oriR101&repA101-ts: Been ligated to a backbone, verifying
λ RED: Waiting for the primers to construct the linear dsDNA sequence (for swapping)
pCarrier: Design of Multiple Cloning Site sequence had been completed, waiting for oligos to arrive.

Culture Test

Completed the standard curve for OD600 versus RFP/KanR CFU concentration
Mixed culture MIC tests for RFP/KanR and RR1(1:99)
Successfully extracted T4MO from pUC18Not/T4MO, discovering the inclusion of a native constitutive promoter, and ligated to pBlueScript KS+ to create a SpeI site for biobrick assembly.
PCR amplified bcr gene from gDNA of E. coli stock

Week 9 (8th-12th Aug)
Strain construction

pir gene: Exact location of pir gene in BW25141 is mapped out
Split superfolder GFP system: Primers did not work: a lot of non- specific bindings, expected band size was not clearly present. New primers had been designed; waiting for new primers to come next week
2010 Slovenia’s method - CFP/YFP: CFP ligated with pET. YFP still on progress
oriR101&repA101-ts: Verifying oriR101&repA101-ts
λ RED: PCR with the new primers is successful. Modified protocol using KAN-resistance gene to swap out uidA gene
pCarrier: MCS had been hybridized. pSB1K3 is under digestion

Culture Test

Digestion of T4MO/pBS KS+ failed
Successfully ligated bcr gene with RBS (later confirmed to be false positive)

Week 10 (15th-19th Aug)
Strain construction

pir gene: Ligation done and being verified
Split superfolder GFP system: PCR with new primers. Split superfolder GFP11 digested and ligated with the promoter.
λ RED: The swapping seemed to be successful
oriR101&repA101-ts: Waiting for new primers
pCarrier: MCS and pSB1AK3 with nadE ligated, but not confirmed

Culture Test

Indole MIC test for wild type (1mM with kanamycin gradient):
Successfully ligated T4MO into pBS KS+

Week 11 (22nd-26th Aug)
Strain construction

pir gene: ligation of pir gene and pBluescriptK+, repeating dephosphorylation to prevent self-ligation of pBluescriptKS+ backbone
Split superfolder GFP system: Re-digestion and dephosphorylate R0010 in pSB1AK3, to reduce background self-ligation during transformation
2010 Slovenia’s method - CFP/YFP: digestion and ligation of pET_YFP; checking construct of pET_YFP; checking fluorescence
nadE gene: Complete.
oriR101&repA101-ts: ligation of oriR101, repA101 and the backbone pSA1K3 in process; transformation result available tomorrow; colony PCR of λ red done, failed.
pToolkit construction: Complete
pCarrier: Ligation of MCS to nadE in pSB1AK3 is complete; Digestion check showed negative result; Hybridization of MCS in progress

Culture Test

Indole MIC test (500µM with kanamycin gradient)
Ligation of the RBS+Bcr with pLac promoter failed

Week 12 (29th Aug-1st Sep)
Strain Construction

pir gene: Background self-ligation is under test, results will be available tomorrow
Split superfolder GFP system: Background self-ligation is under test, results will be available tomorrow; Ligating split GFP with lac promoter
2010 Slovenia’s method - CFP/YFP: pET_CFP and pET_YFP have been constructed and verified; transformation of each into BL21 has been done;
nadE gene: Completed; verified;
oriR101 + repA101ts: Construction is complete – verified by restriction digestion; BioBrick currently located on pSB1AK3;
λ RED:check whether swap is successful: screen 6 colonies for verification;
pToolkit construction: Complete
pCarrier: re-annealing of ssDNA of MCS; Re-planning of insertion position of MCS

Culture Test

Mixed culture MIC tests for RFP/KanR and RR1 (1:99)
Indole MIC test (300µM with kanamycin gradient)
Successfully ligated T4MO with GFP

Week 13 (5th-9th Sep)
Strain construction

λ RED : previous PCR verification (S2) not show very clear result, halted for this week; new verificationprimers (S2) arrived
oriR101&repA101-ts: Construction of oriR101+pSB1AK2 successful; oriR101+pSB1Cs (standard BioBrick format) ligation done, colony PCR checked, digestion test tmr
Spilt superfolder GFP system: 2010 Slovenia’s method; split superfolder GFP from Biobrick.
pir gene and ori-γ: ligationof pir gene and pBluescriptKS+done, but do not have clear verification result (colony PCR+, digestion test-); considering new verification test (2 new sets).
nadE gene: Completed; wait to do sequencing verification;
pCarrier: MCS reinsert, change the size and position of insertion;
pToolkit construction: accidentally disappear, redo the whole plasmid;
pCarrier: nadE part ready, working on MCS now.

Culutre Test

Mixed culture MIC tests for RFP/KanR and RR1 (1:99)
Indole MIC test (1mM indole concentration with kanamycin gradient)
Successfully ligated T4MO/GFP into kanamycin resistant backbone.

Week 14 (13th-17th Sep)
Strain Construction

λ RED:basically successful; new S2 primers arrived, first trial failed (negative control of pKD46+E. coli DH10B still have some bands); consider directly PCR out from pKD46
oriR101&repA101-ts: constructionof oriR101+pSB1AK3, oriR101+pSB1C3 (submitting format) finishedand successful; characterization of heat sensitivity in progress
Spilt superfolder GFP system: 2010 Slovenia’s method; split superfolder GFP from Biobrick;
pir gene and ori-γ: Pir ligation with pBS successful, ready for sequencing;
nadE gene: Completed; wait to do sequencing verification
pToolkit construction: accidentally lost, redo the whole thing
pCarrier : MCS insertion does not show good result halted for this year

Culture Test

Mixed culture MIC tests for RFP/KanR + RR1 (1:99) and T4MO/KanR + RR1 (1:1)
Indole MIC test (1mM and 2mM with kanamycin gradient) [2mM experiment failed]
Started to construct BioBrick of bcr gene for submission

Week 15 (20th-24th Sep)
Strain Construction

oriR101&repA101-ts: the progress is not ideal, cannot finishthe characterizationthis week
pir gene: sequence result: some key parts are missing. the target part developed an unexpected illegal cut (point mutation or star activity); insert the pir to pBS again (using different enzymes), sequenced again.
Split superfolder GFP system: the construction of split GFP+backbone finished; characterization in progress

Week 16 (27th-30th Sep)
Strain Construction

oriR101-ts: have already submitted and received by part registry; rough characterization successful; further characterization method confirmed;
Split superfolder GFP system: ligation GFP1-10 and GFP11 into one plasmid finished, but not have fluorescence; starting to insert GFP1-10 in pSB1C3, GFP11 in pSB1AK3; then use two antibiotics as selection markers, then check the fluorescence
pir gene: sequence failed (wrong gene…nadE actually)
pToolkit construction: construction in progress

Home

Our Project

Overview | Data Page

Experiments and Results

Strain Construction | Culture Test | Modeling

Miscellaneous

Notebook

iGEM Resources

Acknowledgements

The Team

iGEM Member List | Contributions

Achievements

Medal Requirements | BioSafety

BioBricks

Master List & Characterization Data

Human Practice

Workshop | Survey

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-<TH ROWSPAN=3 BGCOLOR="#A1C6B2">
-<a name=top></a><p>
-<h3>Notebook</h3>
-<font color=black>
-</p>
+<table style="border-collapse: collapse" width=963>
-<p >
+<TR bgcolor="#9CC3B1"><td>
-<h4 align=left><a name=constructing></a>1. Constructing EX – the bacterial strain that allows selection without use of antibiotics</h4>
-</p>
-<p align=justify style="margin: 20px 20px 20px 20px">
+<p align="center"><font face="Verdana, Arial, Helvetica, sans-serif" size="7" color="white">
+<br>Notebook</font></p>
-To study the population dynamics and behavior of a certain antibiotics sensitive strain of <i>E. coli</i> in a medium of antibiotic, our <i>E. Trojan</i> that is introduced into the culture medium must not process a wide spectrum of antibiotic resistance that impose a selective advantage. At the same time, <i>E. Trojan</i> needs to be transformed with the T4MO gene to carry out its job of signal disruption. <br><br>
-Summarizing the above criteria, a solution where the bacteria can be transform with the gene of interest while remaining sensitive to antibiotics is needed. Therefore the requisite is to construct a new bacterial strain that can perform plasmid selection without the use of antibiotics, and contains as little antibiotics resistance gene as possible.
-<a href=#top>[Top]</a>
-</p>
+<br>
+</td></tr></table>
+<br>
+<table style="border-collapse: collapse" width=963>
+<TR bgcolor="white"><td>
-<p>
+<p><strong>Week 1 (4th-10th June)</strong><br>
-<h4 align=left><a name=method></a>2. How to select against EX without the vector plasmid? Our alternative selection method</h4>
+  Strain  construction</p></font>
-</p>
+<ul>
-<p align=justify style="margin: 20px 20px 20px 20px">
+  <li>Genomic  DNA of <em>E. coli DH10b</em> extracted</li>
+  <li>Waiting  for materials (bacterial strains, primers) to arrive</li>
+</ul><br>
-Our EX will have one of its essential genes (genes that are required for viability) removed from its genome, and relocated onto an engineered plasmid pDummy. As illustrated, in order to survive, EX must rely on those extra-chromosomal copies of the essential gene; therefore, EX is addicted to pDummy. By having direct control over the replication of pDummy, we dictate the life and death of EX (and hence the name pDummy).
+<p><strong>Week </strong><strong>2</strong><strong> (13th-17th June)</strong><strong> </strong><br>
-<br><br>
+  Strain  construction</p>
+<ul>
-Here, we introduce a heat-sensitive origin of replication as the only origin of pDummy. When we intend to switch off the replication of pDummy, we can incubate EX at above 30°C. This origin would then cease to function, and pDummy cannot be maintained. Deprived of the essential gene and the corresponding vital product, EX cannot propagate, unless, it receives an alternative but heat insensitive analog of pDummy. <br><br>
+  <li>Genomic  DNA of <em>E. coli </em> DH10b extracted. Genomic DNA of BL21 extracted</li>
+  <li>Cloned out  split  superfolder GFP construct </li>
-This analog, named pCarrier, is the essentially our vector in cloning. Under an unfavorably high temperature, only those EX that are transformed with the insert-bearing pCarrier will be able to propagate and survive, while the others cannot undergo division and are virtually eliminated from the population. Eventually, the pDummy can be considered to be "shuffled out" by pCarrier. Our designed selection system, in short, bases itself on plasmid shuffling, and thus eliminates involvement of antibiotic resistance genes in any of the cloning steps.<a href=#top>[Top]</a><br>
+  <li>Finished  design of PCR primers for nadE gene and λ RED</li>
+</ul>
-<p>
+<p>Culture Test</p>
-<h4 align=left><a name=assembly></a>3. Stepping in the heart of construction - methods of assembly</h4>
+<ul>
-</p>
+   <li>Wild type MIC test optimization (kanamycin gradient 0-25 µg/ml, serial dilutions)</li>
-<p align=justify style="margin: 20px 20px 20px 20px">
+  <li>Constructed standard curve for  OD600 verses RR1 (wild type) CFU concentration </li>
+</ul>
-<b>3.1 Construction and maintenance of an antibiotic-resistance-gene-free plasmid through antibiotic selection – the unavoidable evil two plasmid system</b><br>
-Our ultimate goal is to construct our EX without conferring it any new antibiotic resistance. For this reason no resistance gene should be found in our dummy plasmid pDummy. <br><br>
-Yet, such a plasmid would not be maintained by itself unless the host bacterium develops an addiction to it (i.e. losses the essential gene in its genome and depends on extra-chromosomal copies on pDummy), and inconveniently, the addiction can only be achieved after the introduction of the plasmid.<br><br>
-The solution is to develop a mutualistic relation between two plasmids and we planned to exploit positively regulated origin of replications. <br><br>
-Well studied examples are those in pSC101 and R6K origins of replication, where the origins of replication (OR) appear together with a constitutive gene (G). Initiation of replication happens if and only if the trans element of the gene is provided.<br></p>
-<p>
-Let’s consider the following scenario: <br>
-i.   G is placed on pDummy with no selection marker but with a normal replication origin<br>
-ii.  OR is the sole origin of replication of another plasmid (here we introduce a new plasmid pToolkit) with a selection marker<br>
-iii. pDummy and pToolkit are co-transformed to a bacterium which is under selection stress</p>
 <br>
-<p>
+<p><strong>Week </strong><strong>3</strong><strong> (20th-24th June)</strong><strong> </strong><br>
-We would obtain three possible outcomes:<br>
+  Strain  construction</p>
-<b>1. only pDummy is uptaken</b><br>
+<ul>
-- since pDummy has no selection marker, the host bacteria die under selection pressure and cannot propagate<br><br>
+  <li><i>nadE</i>:  PCR out <i>nadE</i> gene from the genome of BL21 </li>
-<b>2. only pToolkit is uptaken</b><br>
+  <li>Split superfolder GFP system: The test of the intact (sfGFP 1-10 still ligated together with sfGFP11) superfolder GFP was successful. Confirmation tests and further experiments would be conducted  soon.</li>
-- the host bacterium that uptakes pToolkit survives. Yet during propagation, pToolkit is not replicated because proteins of G are absent. Therefore daughter cells of the host bacterium will not receive copies of the pToolkit and die under selection pressure.<br><br>
+  <li>2010  Slovenia’s method - CFP/YFP: BioBricks  would be transformed into <em>E. coli</em> DH10b. Tests would be conducted soon.</li>
-<b>3. both pDummy and pToolkit are uptaken</b><br>
+  <li>λ RED  and oriR101&amp;repA101-ts: pKD46 has  arrived and successfully extracted. RFP reporter system was ready. Primers of  RepA101ts-OriR101 are ready. </li>
-- in presence of pDummy, pToolkit is maintained and confers the host bacterium with stress resistance. Daughters that receive copies of both plasmids will survive and eventually develop into a colony.<br><br></p>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Performed 2nd and 3rd MIC tests for  wild type (kanamycin  gradient 5-20 µg/ml, 2µg/ml intervals) </li>
+  <li>Minipreps of BBa_I763007 and BBa_E1010 were successful </li>
+</ul><br>
+<p><strong>Week </strong><strong>4</strong><strong> (2</strong><strong>7</strong><strong>th</strong><strong> June–1st</strong><strong> Ju</strong><strong>ly</strong><strong>)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>λ RED : protocol  design finished; pKD46 arrived and digestion tests indicated that the plasmid was correct; PCR RFP with  homologous sequence was successful</li>
+  <li>2010  Slovenia’s method - CFP/YFP: protocol design finished,  successfully finished combined CFP and YFP</li>
+  <li>Split superfolder GFP system: protocol design  finished; primer arrived</li>
+  <li>Pir gene and ori-γ: protocol  under construction; primer for ori-γ arrived; BW25141 gDNA extraction  successful</li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Ligation of pSB2K3 (from  BBa_E1010) with RFP reporter device (BBa_I763007) </li>
+  <li>Transformation  of the RFP/KanR plasmid to <em>E. coli </em>DH10b</li>
+</ul><br>
+<p><strong>Week </strong><strong>5</strong><strong> (</strong><strong>8th-12th </strong><strong>Ju</strong><strong>ly</strong><strong>)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>ori-γ:  Primers arrived, PCR was successful. Result: one of four samples was positive, but  of low concentration</li>
+  <li>pir  gene: gDNA of BW25141 successfully extracted</li>
+  <li>Split superfolder GFP system: GFP1-10 PCRed, GFP11 PCRed</li>
+  <li>2010 Slovenia’s method - CFP/YFP: Verified combined  fluorescence protein</li>
+  <li>oriR101 &amp; repA101-ts:  Clone- out by PCR was successful</li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Successful construction of a RFP-labeled kanamycin-resistant strain</li>
+  <li>Information from literature search on mechanisms  to raise the MIC for the proposed T4MO mutant slightly help it survive in  kanamycin long enough to fulfill its function</li>
+  <li>MIC testing  for RR-1 </li>
+</ul><br>
+<p><strong>Week </strong><strong>6</strong><strong> (</strong><strong>15th-19th </strong><strong>Ju</strong><strong>ly</strong><strong>)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>λ RED: PCR of RFP with homologous sequence successful</li>
+  <li>2010 Slovenia’s method - CFP/YFP: digestion and ligation of CFP, YFP with pBluescript KS+ promoter finished</li>
+  <li>Split superfolder GFP system: PCR of spilt superfolder GFP successful</li>
+  <li>2010 Slovenia’s method - CFP/YFP :Ligation with promoter is  successful, but the green fluorescence could not be observed. Considering to redo construction</li>
+  <li>pToolkit  construction: PCR of ori-γ successful; ligation with pKD46 backbone was done, confirmation still awaiting the results of colony PCR to check the existence of ori-γ; the sequencing PCR of  the pir gene was done, now waiting to check the results</li>
+  <li><i>nadE</i>  gene: ligation <i>nadE</i> gene with double terminator not successful. Would repeat experiments next week</li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>MIC test for wild type RR1 (kanamycin gradient 5-13 µg/ml, 1µg/ml intervals) </li>
+  <li>MIC test for mixed cultures of  RFP/KanR and RR1(1:99)</li>
+  <li>Literature search – multidrug pump candidates </li>
+  <ul>
+    <li>Bcr(~1.2kbp):  overexpression increases kanamycin MIC ~2-4fold </li>
+    <li>NorM (~1.3kbp): overexpression reduces radical oxidative species  (e.g. H<sub>2</sub>O<sub>2</sub>) inside the cell</li>
+  </ul>
+</ul><br>
+<p><strong>Week </strong><strong>7 </strong><strong>(</strong><strong>22nd-26th </strong><strong>Ju</strong><strong>ly</strong><strong>)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>pir  gene: Sequencing product did not meet sequencing requirement (a lot of 'N's) – sequencing  rejected. To do: practice how to perform sequencing clean-up properly</li>
+  <li>Split superfolder GFP system: Construct to be ligated had very low recovery from gel purification; another trial would be done asap </li>
+  <li>2010 Slovenia’s method – CFP/YFP: combination of n-terminal and c-terminal CDS into same plasmid, driven  by plac promoter of pBluescriptKS+ completed. Result: very weak fluorescence observed</li>
+  <li><em>nadE</em> gene: successful ligation of nadE gene with terminator; correctness of construct confirmed by restriction digestion tests. Component was putatively finished as biobrick</li>
+  <li>oriR101&amp;repA101-ts: basic protocol for site-directed-mutagenesis + fusion PCR tested to be  successful. Repeating fusion PCR</li>
+  <li>λ RED: Previous experiment of gene swapping failed. Trouble-shooting in progress</li>
+  <li>pToolkit  construction:  results from colony PCR of ori-γ from transformed bacteria: successful  completion of pToolkit. Further confirmation by restriction digestion to be done</li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Mixed culture MIC tests for RFP/KanR and RR1(99:1)</li>
+  <li>Multidrug Efflux Pump – Settled  on Bcr as the candidate gene </li>
+  <ul>
+    <li>2~4 folded increasing for Kan</li>
+    <li>Proton gradient (H<sup>+</sup>) driven </li>
+    <li>Pumps out other toxins</li>
+    <li>Unknown promoter </li>
+  </ul>
+  <li><em>E. coli</em> DH10a containing pUC18Not/T4MO arrived</li>
+</ul><br>
+<p><strong>Week </strong><strong>8 </strong><strong>(</strong><strong>1st-5th  Aug</strong><strong>)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>pir  gene: Sequencing result has just come out</li>
+  <li>Split superfolder GFP system: Finished ligation of lacI promotor and  GFP 11 and verifying. GFP 1-10 PCRing</li>
+  <li>2010 Slovenia’s method - CFP/YFP: Finished construction but not verified</li>
+  <li><i>nadE</i>  gene: construction finished, but construct was still harbored in pSB1AK3. Consider relocation to pSB1C3 asap.</li>
+  <li>oriR101&amp;repA101-ts: Been ligated to a backbone, verifying</li>
+  <li>λ RED: Waiting for the primers to construct the linear dsDNA sequence (for swapping)</li>
+  <li>pCarrier: Design of Multiple Cloning Site sequence had been completed, waiting for oligos to arrive.
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Completed the standard curve for  OD600 versus RFP/KanR CFU concentration</li>
+  <li>Mixed culture MIC tests for RFP/KanR and RR1(1:99)</li>
+  <li>Successfully extracted T4MO  from pUC18Not/T4MO, discovering the inclusion of a native constitutive  promoter, and ligated to pBlueScript KS+ to create a SpeI site for biobrick  assembly. </li>
+  <li>PCR amplified <em>bcr </em>gene from gDNA of <em>E. coli </em>stock </li>
+</ul><br>
+<p><strong>Week </strong><strong>9 (</strong><strong>8th-12th  Aug)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>pir  gene: Exact location of pir gene in BW25141 is mapped out</li>
+  <li>Split  superfolder GFP system: Primers did not work: a lot of non- specific bindings, expected band size was not clearly present. New primers had been designed; waiting for new primers to come next week</li>
+  <li>2010 Slovenia’s method - CFP/YFP: CFP ligated with pET. YFP still on progress</li>
+  <li>oriR101&amp;repA101-ts:  Verifying oriR101&amp;repA101-ts </li>
+  <li>λ RED: PCR with the new primers is successful. Modified protocol using  KAN-resistance gene to swap out uidA gene</li>
+  <li>pCarrier:  MCS had been hybridized. pSB1K3 is under digestion</li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Digestion of T4MO/pBS KS+ failed</li>
+  <li>Successfully ligated <i>bcr</i> gene with RBS (later confirmed to be false positive) </li>
+</ul><br>
+<p><strong>Week 10 (15th-19th  Aug) </strong><br>
+  Strain construction<strong></strong></p>
+<ul>
+  <li>pir gene: Ligation done and being verified </li>
+  <li>Split superfolder GFP system: PCR with new primers. Split superfolder GFP11  digested and ligated with the promoter.</li>
+  <li>λ RED: The swapping seemed to be successful</li>
+  <li>oriR101&amp;repA101-ts: Waiting for new primers</li>
+  <li>pCarrier: MCS and pSB1AK3 with nadE ligated, but not confirmed </li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Indole MIC test for wild type (1mM with kanamycin gradient): </li>
+  <li>Successfully ligated T4MO into pBS KS+</li>
+</ul><br>
+<p><strong>Week </strong><strong>11 (</strong><strong>22nd-26th Aug)</strong><strong> </strong><br>
+  Strain  construction</p>
+<ul>
+  <li>pir gene: ligation of pir gene  and pBluescriptK+, repeating dephosphorylation to prevent self-ligation of  pBluescriptKS+ backbone<strong></strong></li>
+  <li>Split  superfolder GFP  system: Re-digestion  and dephosphorylate R0010 in pSB1AK3, to reduce background self-ligation during  transformation<strong> </strong></li>
+  <li>2010 Slovenia’s method - CFP/YFP: digestion  and ligation of pET_YFP; checking construct of pET_YFP; checking fluorescence<strong> </strong></li>
+  <li><em>nadE</em> gene: Complete.<strong> </strong></li>
+  <li>oriR101&amp;repA101-ts: ligation of oriR101, repA101 and the backbone  pSA1K3 in process; transformation  result available tomorrow; colony PCR of λ red done, failed.<strong> </strong></li>
+  <li>pToolkit construction: Complete<strong> </strong></li>
+  <li>pCarrier: Ligation  of MCS to <i>nadE</i> in pSB1AK3 is complete; Digestion check showed  negative result; Hybridization of MCS in progress<strong> </strong></li>
+</ul>
+<p>Culture Test<strong></strong></p>
+<ul>
+  <li>Indole MIC test (500µM with kanamycin gradient)</li>
+  <li>Ligation of the RBS+Bcr with  pLac promoter failed </li>
+</ul><br>
+<p><strong>Week </strong><strong>12 (</strong><strong>29th Aug-1st Sep)</strong><strong> </strong><br>
+  Strain Construction</p>
+<ul>
+  <li>pir gene: Background self-ligation is under test,  results will be available tomorrow </li>
+  <li>Split  superfolder GFP system: Background self-ligation is under test,  results will be available tomorrow; Ligating split GFP  with <em>lac</em> promoter </li>
+  <li>2010 Slovenia’s method - CFP/YFP: pET_CFP and pET_YFP  have been constructed and verified; transformation of  each into BL21 has been done; </li>
+  <li><em>nadE</em> gene: Completed; verified; </li>
+  <li>oriR101 + repA101ts: Construction is complete – verified by  restriction digestion; BioBrick currently  located on pSB1AK3; </li>
+  <li>λ RED:check whether swap is successful: screen 6  colonies for verification; </li>
+  <li>pToolkit construction: Complete </li>
+  <li>pCarrier: re-annealing of ssDNA of MCS; Re-planning of insertion position of MCS </li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Mixed culture MIC tests for RFP/KanR and RR1 (1:99) </li>
+  <li>Indole MIC test (300µM with kanamycin gradient)</li>
+  <li>Successfully  ligated T4MO with GFP</li>
+</ul><br>
+<p><strong>Week </strong><strong>13 (</strong><strong>5th-9th Sep)</strong><strong> </strong><br>
+  Strain construction</p>
+<ul>
+  <li>λ RED : previous PCR verification (S2) not show very clear  result, halted for this week; new verificationprimers (S2) arrived</li>
+  <li>oriR101&amp;repA101-ts: Construction of  oriR101+pSB1AK2 successful; oriR101+pSB1Cs (standard BioBrick format)  ligation done, colony PCR checked, digestion test tmr </li>
+  <li>Spilt superfolder GFP system: 2010 Slovenia’s  method; split superfolder GFP from Biobrick. </li>
+  <li>pir gene and ori-γ: ligationof pir gene  and pBluescriptKS+done, but do not have clear verification result (colony PCR+,  digestion test-); considering new verification test (2 new sets). </li>
+  <li><i>nadE</i> gene:  Completed; wait to do  sequencing verification; </li>
+  <li>pCarrier:  MCS reinsert, change the size  and position of insertion; </li>
+  <li>pToolkit  construction: accidentally disappear,  redo the whole plasmid; </li>
+  <li>pCarrier: <i>nadE</i> part ready, working on MCS now. </li>
+</ul>
+<p>Culutre Test</p>
-<p>
+<ul>
-Using this mutualistic relation, the desired pDummy can be maintained once the host bacterium develops an addiction it, and pToolkit can be lost in bacteria propagation if the expression of G can be shut off manually. Eventually, the bacteria not obtain any new antibiotic resistance genes but keep pDummy.
+  <li>Mixed culture MIC tests for RFP/KanR and RR1 (1:99) </li>
+  <li>Indole MIC test (1mM indole concentration with kanamycin gradient)</li>
-</p>
+  <li>Successfully  ligated T4MO/GFP into kanamycin resistant backbone. </li>
-<p align=justify style="margin: 20px 20px 20px 20px">
+</ul>
-<b>3.2 Development of addiction – use of the lambda RED recombination system</b><br>
-To develop the addiction in the host bacterium to pDummy, an essential gene for survival is to be deleted from the bacteria genome, provided that the bacteria can survive on extra-chromosomal copies after the deletion.<br><br>
-The deletion here is mediated through the lambda RED recombination system<br><br>
-[Nat is still writing...z.z]<br><br>
-The lambda RED recombination cassette is located on the pToolkit (and hence the name of the plasmid). Once the recombination is successful, it can be eliminated from the host bacterium together with the antibiotic resistance gene. <br><br>
-Therefore, once the co-transformation of pDummy and pToolkit is successful, linear dsDNAs having a reporter gene flanked by homologous sequences to the essential gene can be introduced into the bacteria. <br><br>
-When the recombination is kicked started, the essential gene will be swapped out and the reporter gene will be incorporated into the bacteria genome.<br><br>
-Since the linear dsDNAs do not have origin of replications, they are not inherited in daughters unless they are swapped into the genomes. Thus, any observable signals from the reporter would allow identification of successful recombination. Identified colonies can then be further treated to induce loss of pToolkit, which afterwards would be the completed strain of EX.<br><br>
-<b>3.3 Complementation between reporter genes – manifesting completion of EX engineering</b><br>
-To ensure that the final strain of EX has: 1. successfully had its essential gene deleted from genome, 2. maintained the pDummy, a complementation reporter system between the pDummy and swapped gene is preferred over a single reporter at the swapped site.<br><br>
-Different methods can achieve the above aim:<br>
-i. Alpha complementation can be used in <i>E. coli</i> strains where the lacZ gene is completely removed. The larger fragment ω can be swapped for the essential gene while the smaller α fragment can stay on pDummy. In a X-gal rich medium, blue colonies suggest the desired engineered strains.<br><br>
-ii. Complementation between split fluorescent proteins (sFP). 2010 iGEM Slovenia team has demonstrated the principle that N-terminal and C-terminal fragments of sFPS are able to complement in vivo and two sets of sfFPS are able to undergo Forster resonance energy transfer (FRET). This idea is adopted but an alternative set of candidate, split superfolder GFPs (sfGFP), was developed.</p>
-<p align=justify style="margin: 20px 20px 20px 20px">
-<b>3.4 Summary of construction flow:</b><br>
-. Assembly pDummy and pToolkit<br>
-. Co-transform both plasmid into <i>E. coli</i> and maintain stable strains<br>
-. Introduce linear dsDNAs and induce recombination<br>
-. Isolate recombinants<br>
-. Induce loss of pToolkit
-<a href=#top>[Top]</a>
-</p>
 <br>
-<p >
+<p><strong>Week </strong><strong>14 (</strong><strong>13th-17th Sep)</strong> <br>
-<h4 align=left><a name=component></a>4. Details of the components – a closer look to the molecular basis of assembly</h4>
+  Strain Construction</p>
-</p>
+<ul>
-<p align=justify style="margin: 20px 20px 20px 20px">
+  <li>λ RED:basically successful; new S2 primers arrived,  first trial failed (negative control of pKD46+<i>E. coli</i> DH10B still have some  bands); consider directly PCR out from pKD46 </li>
-<b>4.1 Temperature-sensitive origin of replication_oriR101 & repA101-ts (BBa_K524000)</b><br>
+  <li>oriR101&amp;repA101-ts: constructionof  oriR101+pSB1AK3, oriR101+pSB1C3 (submitting format) finishedand successful; characterization of  heat sensitivity in progress </li>
+  <li>Spilt superfolder GFP system: 2010 Slovenia’s  method; split  superfolder GFP from Biobrick; </li>
+  <li>pir gene  and ori-γ: Pir ligation with pBS successful, ready for sequencing; </li>
+  <li><i>nadE</i> gene: Completed; wait to do sequencing  verification </li>
+  <li>pToolkit  construction: accidentally  lost, redo the whole thing </li>
+  <li>pCarrier : MCS insertion does not  show good result halted for this year </li>
+</ul>
+<p>Culture Test</p>
+<ul>
+  <li>Mixed culture MIC tests for RFP/KanR + RR1 (1:99) and T4MO/KanR + RR1 (1:1)</li>
+  <li>Indole MIC test (1mM and 2mM with kanamycin gradient) [2mM experiment failed] </li>
+  <li>Started to construct BioBrick of  bcr gene for submission</li>
+</ul><br>
+<p><strong>Week 15 </strong> <strong>(</strong><strong>20th-24th</strong><strong> Sep)</strong> <br>
+  Strain Construction</p>
+<ul>
+  <li>oriR101&amp;repA101-ts: the progress is not ideal, cannot finishthe characterizationthis week </li>
+  <li>pir gene: sequence result: some key parts are missing. the target part developed an unexpected illegal cut (point mutation or star activity); insert the pir to pBS again (using different enzymes), sequenced again. </li>
+  <li>Split superfolder GFP system: the construction of split GFP+backbone finished; characterization in  progress </li>
+</ul><br>
+<p><strong>Week 16 (27th-30th Sep)</strong><br>
+  Strain Construction</p>
+<ul>
+  <li>oriR101-ts: have already submitted and  received by part registry; rough characterization successful; further  characterization method confirmed; </li>
+  <li>Split superfolder GFP system: ligation GFP1-10 and GFP11 into  one plasmid finished, but not have fluorescence; starting to insert GFP1-10 in  pSB1C3, GFP11 in pSB1AK3; then use two antibiotics as selection markers, then  check the fluorescence </li>
+  <li>pir  gene: sequence failed (wrong gene…<i>nadE</i> actually) </li>
-oriR101 & repA101-ts is a set of low copy origin of replication derived from the pSC101 origin of replication. The repA101-ts gene codes for a heat-labile protein that is required in trans for the initiation of replication at oriR101. In our construct, our characterization has shown that plasmids with this origin of replication can only be maintained below than 300°C, and partial maintenance of plasmid was observed within temperature range from 290°C to 330°C. This part was cloned out from pKD46 plasmid (courtesy of The Coli Genetic Stock Center), and standardized by a nucleotide mutation.<br>
+<li>pToolkit construction: construction  in progress</li>
+</ul>
+<br />
-</p>
-<p align=justify style="margin: 20px 20px 20px 20px">
-<b>4.2 split superfolder green fluroscent protein_split sfGFP<br>
-sfGFP1-10 (BBa_K524001) [Twins: BBa_K524006]<br>
-sfGFP11 (BBa_K524002) [Twins: BBa_K524007]</b><br>
-The sfGFPs are mutated variants of GFPs that has improved folding kinetics and resistance to chemical denaturants. Split sfGFPs at amino acid residues 214 and 215 have been reported to undergo spontaneous complementation to give green fluorescence. The two split constructs were produced from an existing BioBrick – pBAD driven sfGFP BBa_I746908. CDS of sfGFP amino acid residues 1-214 were copied out for sfGFP1-10 using PCR and stop codon was added to the end. The sfGFP11 was produced in a similar fashion, with a start codon added to the front of the CDS of amino acid residues 215 to 238.
 </p>
-<p align=justify style="margin: 20px 20px 20px 20px">
-<b>4.3 Essential gene <i>nadE</i> (BBa_K524003)</b><br>
-<i>nadE</i> is a vital gene in <i>E. coli</i>. It codes for NAD+ synthetase. In principle, removal of such gene from the genome would cause addiction of bacteria to a plasmid that has a copy of the gene. CyaR (a sRNA) regulates the expression of <i>nadE</i> post-transcriptionally. This feature is retained in our construct. Transcription of <i>nadE</i> operon requires the sigma-70 factor and is terminated by downstream extragenic sites. The <i>nadE</i> gene was cloned out from the genome of strain BL21(DE3), and was completed the <i>nadE</i> by having B0015 terminator assembled to its end.
-</p>
-<p align=justify style="margin: 20px 20px 20px 20px">
-<b>4.4 Replication initiator pi protein encoded by pir gene (BBa_K524004) and ori-gamma from R6K plasmid</b><br>
-ori-gamma is one of three replication origins (the other two being alpha and beta) of the R6K origin. Initiation of replication at ori-gamma requires the pi protein in trans, which is encoded by the pir gene. Yet doubling the concentration of pi protein would effectively shut down the replication as well. Expression of pi protein is autogenously regulated. The pir construct was cloned out from the genome of strain BW25141 (courtesy of The Coli Genetic Stock Center) and standardized. The ori-gamma was adopted from the R6K origin of replication BBa_J61001.
-</p>
-<p align=justify style="margin: 20px 20px 20px 20px">
-<b>4.5 iGEM 2010 Slovenia Split/FRET constructs</b><br>
-The split CFP and YFP from the BioBricks of Slovenia team last year were used as alternative reporters. The idea is to put one of the terminal fragments of a split fluorescence protein into the pDummy, and swap out the essential <i>nadE</i> gene from the genome with the other terminal fragment. Driven by pLac R0010, both fragments should express simultaneously when induced by IPTG and fluorescence signal would be observed as an indicator of successful recombination. <a href=#top>[Top]</a>
-</p>
 </font>
 </TH>
-    <TD bgcolor="white" width=160 height=150>
-<p>
-<h2>Notebook</h2>
-</font>
-</p>
-<br><br><br>
-<img src="https://static.igem.org/mediawiki/2011/3/3a/Ust_27.jpg" width=100 height=100><BR>
-<a href=#constructing>1. Constructing EX</a> <br>
-<a href=#method>2. How to Select? </a><br>
-<a href=#assembly>3. Methods of Assembly </a><br>
-<a href=#component>4. Component Details</a><br><br>
 </TD>
+   </TR>
+</table>
-    </TR>
-<TR>
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-</TD>
-    </TR>
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-<font color=#CDD2C2>
-</font>
+<table border="0" cellspacing="0" cellpadding="10" width=963>
+<tr>
+<td width="100px" height="150px"; bgcolor="#980000" >
+<p name=1 align="center">
-</TD>
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong" target=_top>
-    </TR>
+<b><font color="#FFE1E1" size=3>Home</font></b>
+</p>
+</td>
+<td width="382px" bgcolor="#CCFF99" valign="baseline">
+<p align="center" valign="baseline">
+<b><font color="green">Our Project</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/overview.html" target=_top>Overview</a><font color="green"> | </font>
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/data.html" target=_top>Data Page</a><br></p>
-</table>
+<p align="center" valign="baseline">
+<b><font color="green">Experiments and Results</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/asm.html"  target=_top>Strain Construction</a><font color="green"> | </font>
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/mic.html"  target=_top>Culture Test</a><font color="green"> | </font>
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/modeling.html"  target=_top>Modeling</a><br></p>
-<br>
+<p align="center" valign="baseline">
+<b><font color="green">Miscellaneous</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/notebook.html" target=_top>Notebook</a></p>
+</td>
+<td width="302px" bgcolor="#D09C00" valign="baseline">
+<p align="center" valign="baseline">
+<b><font color="#FFF4D0">iGEM Resources</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/acknowledgement.html" target=_top>Acknowledgements</a></p>
+<p align="center" valign="baseline">
+<b><font color="#FFF4D0">The Team</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/team.html" target=_top>iGEM Member List</a><font color="#FFF4D0"> | </font>
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/contribution.html" target=_top>Contributions</a><br></p>
+<p align="center" valign="baseline">
+<b><font color="#FFF4D0">Achievements</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/medal.html" target=_top>Medal Requirements</a><font color="#FFF4D0"> | </font>
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+<p align="center" valign="baseline">
+<b><font color="#FFF4D0">BioBricks</font></b></p>
+<p align="center" valign="baseline">
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/characterization.html" target=_top>Master List & Characterization Data</a><br></p>
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-<a href="mic.html"  target=_top>Culture Tests</a> |
-<a href="modeling.html"  target=_top>Modeling</a><br>
-<span style="line-height:1; font-weight:600">Miscellaneous</span><br>
+<td width="180px"bgcolor="#980000"valign="baseline">
-<a href="notebook.html" target=_top>Notebook</a>
+<p align="center" valign="baseline">
-</font></a><br></font></p>
+<b><font color="#FFE0E0">Human Practice</font></b></p>
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+<p align="center" valign="baseline">
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+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/workshop.html" target=_top>Workshop</a><font color="white"> | </font>
+<a href="https://2011.igem.org/Team:HKUST-Hong_Kong/survey.html" target=_top>Survey</a><br></p>
-iGEM Resources</font></b></p>
-<p align="left"><font face="Verdana, Arial, Helvetica, sans-serif" size="1" color="#FFFFFF">
-<a href="acknowledgement.html" target=_top>Acknowledgements</a><br>
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