Part:BBa_K525730

DNA ligase from Escherichia coli (LigA) with PT7 and RBS

NAD⁺-dependent DNA ligase from E. coli with PT7-promoter, RBS, Freiburg Suffix

Usage and Biology

Bacterial DNA ligases are important enzymes for DNA repair and replication. They use NAD⁺ as a cofactor to bind hydrolysed AMP to the active site lysine under release of NMN. AMP is used to catalyse the formation of a phosphodiester bond in nicked DNA by transferring AMP to the 5'-phosphate group. This results in an attack of the nick 3'-OH on the 5'-phosphoanhydride linkage and release of free AMP:

During the reaction mechanism the DNA ligases functional domains undergo conformational changes promoting intra- and intermolecular interactions. The domains are highly conserved throughout the bacterial kingdom and categorized in the following way:

• Domain 1: Ia, Ib (NTase)
  
• Domain 2: Oligomer-binding (OB) beta-barrel
  
• Domain 3: Zinc (Zn)-finger, helix-hairpin-helix motif (HhH)
  
• Domain 4: BRCT domain
  

The NAD⁺-dependent DNA ligase from E. coli (LigA) can be applied to biochemical studies ranging from cloning procedures and enzymatic assays to biomedical investigations. For instance, the purified enzyme can contribute to in vitro experiments dealing with antibiotic drug design because bacterial DNA ligases are essential for fundamental life-sustaining processes and differentiate from eukaryotic DNA ligases due to their specifity for NAD⁺ as a cofactor.

Sequence and Features

Characterization

Detailed information about the characteristics can be found for the PT7 promoter, RBS and His-tag equipped form of LigA BBa_K525710.