Time-resolved fluorescence of 2-aminopurine in DNA duplexes in the presence of the EcoP15I Type III restriction-modification enzyme

Anita C. Jones; Bonnist; Bonnist; Butterer; Crampton; Crampton; David T.F. Dryden; Dryden; Dryden; Dryden; Finger; Gasteiger; Geoffrey G. Wilson; Guest; Hochstrasser; Janscak; Lenz; Loenen; Long Ma; Matje; Möncke-Buchner; Mücke; Neely; Neely; Nordlund; Owczarzy; Rachofsky; Rao; Reddy; Richardson; Rist; Schwarz; Somsen; Su; Su; Ward; Wyszomirski; Xiaohua Wu; Youngblood; Zang

Time-resolved fluorescence of 2-aminopurine in DNA duplexes in the presence of the EcoP15I Type III restriction-modification enzyme

Authors: Anita C. Jones
Bonnist
Bonnist
Butterer
Crampton
Crampton
David T.F. Dryden
Dryden
Dryden
Dryden
Finger
Gasteiger
Geoffrey G. Wilson
Guest
Hochstrasser
Janscak
Lenz
Loenen
Long Ma
Matje
Möncke-Buchner
Mücke
Neely
Neely
Nordlund
Owczarzy
Rachofsky
Rao
Reddy
Richardson
Rist
Schwarz
Somsen
Su
Su
Ward
Wyszomirski
Xiaohua Wu
Youngblood
Zang
Publication date: 1 June 2014
Publisher: 'Elsevier BV'
Doi

Abstract

AbstractEcoP15I is a Type III DNA restriction and modification enzyme of Escherichia coli. We show that it contains two modification (Mod) subunits for sequence-specific methylation of DNA and one copy of a restriction endonuclease (Res) subunit for cleavage of DNA containing unmethylated target sequences. Previously the Mod2 dimer in the presence of cofactors was shown to use nucleotide flipping to gain access to the adenine base targeted for methylation (Reddy and Rao, J. Mol. Biol. 298 (2000) 597–610.). Surprisingly the Mod2 enzyme also appeared to flip a second adenine in the target sequence, one which was not subject to methylation. We show using fluorescence lifetime measurements of the adenine analogue, 2-aminopurine, that only the methylatable adenine undergoes flipping by the complete Res1Mod2 enzyme and that this occurs even in the absence of cofactors. We suggest that this is due to activation of the Mod2 core by the Res subunit