Difference between revisions of "Part:BBa K592009:Experience"

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'''Paris_Saclay 2013 :'''
  
 
Our team improved the biobrick BBa_K592009 by assembly of biobricks B0034, BBa_K592009 and B0015 to construct a composite part including a ribosome binding site, full length of amilCP gene and double terminator. We used it as one of our reporter gene in Escherichia coli to controlled activator or repressor activity of our promotor under aerobic or anaerobic conditions (Pndh*, PnirB, PnarG, PnarK, PbphR1, PbphR2).
 
Our team improved the biobrick BBa_K592009 by assembly of biobricks B0034, BBa_K592009 and B0015 to construct a composite part including a ribosome binding site, full length of amilCP gene and double terminator. We used it as one of our reporter gene in Escherichia coli to controlled activator or repressor activity of our promotor under aerobic or anaerobic conditions (Pndh*, PnirB, PnarG, PnarK, PbphR1, PbphR2).

Revision as of 02:29, 5 October 2013

This experience page is provided so that any user may enter their experience using this part.
Please enter how you used this part and how it worked out.

Applications of BBa_K592009

User Reviews

UNIQb5558f383ff99555-partinfo-00000000-QINU UNIQb5558f383ff99555-partinfo-00000001-QINU

Paris_Saclay 2013 :

Our team improved the biobrick BBa_K592009 by assembly of biobricks B0034, BBa_K592009 and B0015 to construct a composite part including a ribosome binding site, full length of amilCP gene and double terminator. We used it as one of our reporter gene in Escherichia coli to controlled activator or repressor activity of our promotor under aerobic or anaerobic conditions (Pndh*, PnirB, PnarG, PnarK, PbphR1, PbphR2).

Construction : Pndh* (repressor) + BBa_K1155003 :

  • In anaerobic conditions : Pndh* is repressed --> BBa_K1155003 isn't expessed --> no color
  • In aerobic conditions : Pndh* isn't repressed --> BBa_K1155003 is expressed --> violet color

PsPfnr3008.jpg


UNIQb5558f383ff99555-partinfo-00000002-QINU UNIQb5558f383ff99555-partinfo-00000003-QINU

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iGEM Michigan 2013

The 2013 Michigan igem team successfully used this part to produce amilCP.

Michiganigempartmainfig2.jpg

Fig 2. - An inducible fim transcriptor system changes states and produces protein output

NEB 10-beta E. coli, which lack the native fim switch (fimS) and known fim recombinases, were co-transformed with K1077007(amilCP j23100 fim switch) or K1077003(GFP j23100 fim switch), and K1077002 (aTc inducible fimE, HSL inducible hbiF) and plated on to LB plates with or without inducer. A) Close up of 3 colonies on a plate containing K1077007 and K1077002 co transformants. Three distinct phenotypes were observed: Solid Blue colonies(bottom left), Mixed colonies that had distinct white and blue regions(bottom middle), and Solid White colonies(top right). Therefore, the uninduced fim transcriptor in the context of K1077002 is subject to leaky fimE and/or hbiF activity. B) Quantification of the phenotypes observed on the plate in A. C) When induced with 4.32µM aTc and grown overnight (left) , no GFP is produced as expected due to induced fimE turning the switch OFF. When induced with 1µM HSL and grown overnight (right), GFP is produced as expected due to induced hbiF turning the switch ON.

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Immudzen

As part of the 2013 CU Boulder project we worked on separating RFP from AmilCP and we measured the spectrum of AmilCP from 400 nm to 600 nm.

Cu Amilcp.png

We also found that when running on an agarose gel RFP will run down on the gel while AmilCP runs up on the gel.

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iGEM 2013 Hong_Kong_HKUST Trevor Y.H. HO

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This part was employed in testing our Gibson Assembly protocol. In the experiment design, the mRFP coding DNA sequence in J04450 was replaced with that of amilCP. The resulting plate from transformation of the post-reaction mixture is shown. The color of the blue chromoprotein was clearly distinguished from that of mRFP, which aided in my evaluation of the performance of Gibson Assembly.
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An image showing a streaked plate of DH10b carrying pSB1C3-R0010-B0034-K592009-B0015.
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BBa_K592009 iGEM Groningen 2012

Our team has managed to couple this biobrick part with our promoters: alsT, fnr, and sboA. The cloning was done in BBa_K818000 (plasmid backbone for B. subtilis, engineered by team Groningen 2012), to allow color expression in B. subtilis. We utilized a strong RBS BBa_B0034 for pigment expression in E. coli and B. subtilis.

The purple/blue colour was strongly visible in E.coli without any induction, while the expression in B. subtilis was more subtle (B. subtilis colony looks slightly blue on the plate agar).

After induction of the promoter before AmilCP, B. subtilis also turned clearly purple/blue. Please have a look at the page of BBa_K818400 for more information.



No review score entered. User:agynna

iGEM Team Uppsala University 2012

We have observed that expression of amilCP confers a noticeable fitness cost in E coli. This is surprising, given that such behaviour is not seen in other homologous chromoproteins and fluorescent proteins. We thus recommend using the new aeBlue (BBa_K864401) chromoprotein for blue color expression, which also has a more clear blue color.


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