BBa_K648100

BBa_K648100 Version 1

Component

Source:
http://parts.igem.org/Part:BBa_K648100
Generated By: https://synbiohub.org/public/igem/igem2sbol/1
Created by: Elyse Merkel
Date created: 2011-09-27 11:00:00
Date modified: 2015-05-08 01:12:59

RecA1 DH10B



Types
DnaRegion

Roles
promoter

Regulatory

Sequences BBa_K648100_sequence (Version 1)

Description

RecA is a protein used by E. coli to repair and maintain DNA. Many normal laboratory strains of E. coli, for example DH10B, are mutants capable of an inactivated form of RecA known as RecA1. RecA 1 is deficient in all known function of the RecA gene specifically in ATPase activity, binding with DNA in the presence of ATP, and changing conformation in the presence of ATP and repressor cleavage. In order to restore RecA1 to RecA and to reduce its recombination ability while maintaining its repressor cleavage activity a series of mutations was made.

One such mutation occurs at amino acid 160, this adenine residue needed to be mutated to guanine to change RecA1 to RecA and restore its functions. In order to use the standard bio-bricking techniques we also had to remove naturally occurring enzymatic restriction sites. The Pst1 site CTGCAG needed to be converted to CTGCAA. Then the EcoR1 site GAATTC needed to be converted to GAATTT.

We also focused on how to mutate RecA so that it would detect damaged DNA without repairing the DNA. After literature research we identified two amino acids in the RecA sequence that were known to affect RecA???s ability to use recombination to repair the DNA. These sites were Arginine 243 and Lysine 286. Research suggested that changing Arginine 243 to Glutamine, and Lysine 286 to Asparagine would remove recombinase activity from RecA.

Notes

Trying to create RecA to be used with other Biobrick by removing Pst1 an EcoR1 sites

Source

RecA1

igem#experience
None
 
igem#sampleStatus
Not in stock
igem#status
Unavailable
 
synbiohub#ownedBy
user/james
 
synbiohub#ownedBy
user/myers
 
synbiohub#topLevel
BBa_K648100/1