Biochemical and Biophysical Research Communications, Vol.334, No.4, 1233-1240, 2005
Protein fragment complementation in M.HhaI DNA methyltransferase
The 5mC DNA methyltransferase M.HhaI can be split into two individually inactive N- and C-terminal fragments that together can form an active enzyme in vivo capable of efficiently methylating DNA. This active fragment pair was identified by creating libraries of M.HhaI gene fragment pairs and then selecting for the pairs that code for an active 5mC methyltransferase. The site of bisection for successful protein fragment complementation in M.HhaI was in the variable region near the target recognition domain between motif VIII and TRD. This same region is the location of bifurcation in the naturally split 5mC methyltransferase M.AquI, the location for circular permutation in M.BssHII, and the location for previously engineered split versions of M.BspRI. (c) 2005 Elsevier Inc. All rights reserved.
Keywords:M.HhaI;DNA methyltransferase;protein fragment complementation;leucine zipper;incremental truncation;protein engineering;M.AquI;M.BssHII;M.BspRI;DNA methylation