Difference between revisions of "Part:BBa K801100"

Revision as of 21:00, 26 October 2012

RFP Coding Device - RFC10 and RFC25 compatible

This is an improved version of the RFP generating device BBa_J04450 designed by [http://openwetware.org/wiki/Davidson:Davidson_2005 Team Davidson 2005] that is now RFC10 and RFC25 compatible.

In 2012 the Registry of Standard Biological Parts defined BBa_J04450 as the standard shipping part that is required for submission of backbones, creating the need for a RFC25 compatible standard shipping part.

Sequence and Features

Composite part of the following BioBricks:

LacI R0010	B0034	mRFP1 E1010	B0015

• BBa_R0010: Promoter (lacI regulated)
  
• BBa_B0034: RBS (Elowitz 1999)
  
• BBa_E1010: Red Fluorescent Protein from Discosoma striata
  
• BBa_B0015: Double Terminator
  

Functional parameters

The colonies are clearly red in color under natural light after about 18 hours. Smaller colonies are visibly red under UV. The RFP part does not contain a degradation tag and the RBS is strong.

• LacI sensitive
• CAP sensitive

This part is commonly used, but can fail if the system contains LacI or CAP protein.
(--Meagan 15:39, 23 July 2009 (UTC))

• 

  Petri dish with BBa_J04450 visualized under non-UV lightbox

• 

  Petri dish with BBa_J04450 visualized under 254 nm wavelength UV lightbox

• 

  Colonies with and without BBa_J04450 on petri dish.

Usage as a cloning tool

[http://2010.igem.org/Team:Groningen Team Groningen 2010] reports the usage of this part as a cloning tool. When ligating any part, or part assembly, into any standard backbone that contains this part, the non-restricted and single-restricted backbones that self-circularize will produce red colonies on rich media plates (we use TY). These undesired transformants can than be avoided in the screening for the correct construct. With this method, the backbone desired for a new construct does not need to be purified from agarose gel to decrease the amount of undesired tranformants caused by ligation of the original part present in the backbone. The amount of incorrect transformants depends, of course, on the ratio of backbone (mixed with BBa_J04450) vs. BioBrick insert, the size of the BioBrick insert, and whether the insert is an assembly of two BioBricks. The images below show two ligations with different efficiencies.

• 

  An inefficient assembly ligation of two BioBricks into the pSB1C3 backbone producing many red colonies.

• 

  A more efficient, single BioBrick ligation into the pSB1C3 backbone.

Extension of the standard compability to RFC10 and RFC25

[http://2012.igem.org/Team:TU_Munich Team TU_Munich 2012] extended the standard compability of the RFP coding device (BBa_J04450) to RFC10 and [http://hdl.handle.net/1721.1/45140 RFC25] by adding the NgoMIV and AgeI restriction sites into the prefix and suffix of this part. Additionally two AgeI restriction sites that were present in the generator itself were deleted.

This part may be used as a standard insert for RFC10 as well as [http://hdl.handle.net/1721.1/45140 RFC25] backbones. This improvement became necessary because insertion of BBa_J04450 into a RFC25 compatible backbone leads to the deletion of the desired [http://hdl.handle.net/1721.1/45140 RFC25] restriction sites that are needed for protein fusions.

Absorption spectrum from RFP1 produced by BBa_K801100

Absorption spectrum of BBa_K801100

Picture of fluorescence of BBa_K801100

The BioBrick BBa_K801100 was characterized by expression of RFP1 BBa_E1010 in E. coli XL1 blue. Afterward the cells were desintegrated using ultrasonic sound and cell debris was pelleted using centrifugation. The cell extract was measured in a photometer. The spectrum measured is shown in the figure on the right.
(by [http://2012.igem.org/Team:TU_Munich Team TU_Munich 2012])