N-Termini of EcoRI Restriction Endonuclease Dimer Are in Close Proximity on the Protein Surface

The N-terminal region of EcoRI endonuclease is essential for cleavage yet is invisible in the 2.5 Å crystal structure of endonuclease−DNA complex [Kim, Y., Grable, J. C., Love, R., Greene, P. J., Rosenberg, J. M. (1990) Science 249, 1307−1309]. We used site-directed fluorescence spectroscopy and che...

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Bibliographic Details
Published in:Biochemistry (Easton) 1998-11, Vol.37 (44), p.15457-15465
Main Authors: Liu, Wei, Chen, Yu, Watrob, Heather, Bartlett, Sue G, Jen-Jacobson, Linda, Barkley, Mary D
Format: Article
Language:English
Subjects:
Binding Sites - genetics
Cross-Linking Reagents
Cysteine - chemistry
Cysteine - genetics
Cysteine - metabolism
Deoxyribonuclease EcoRI - chemistry
Deoxyribonuclease EcoRI - genetics
Deoxyribonuclease EcoRI - metabolism
Dimerization
DNA, Bacterial - chemistry
DNA, Bacterial - genetics
DNA, Bacterial - metabolism
Fluorescence Polarization
Hydrolysis
Mutagenesis, Site-Directed
Peptide Fragments - chemistry
Peptide Fragments - genetics
Peptide Fragments - metabolism
Spectrometry, Fluorescence
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Summary:The N-terminal region of EcoRI endonuclease is essential for cleavage yet is invisible in the 2.5 Å crystal structure of endonuclease−DNA complex [Kim, Y., Grable, J. C., Love, R., Greene, P. J., Rosenberg, J. M. (1990) Science 249, 1307−1309]. We used site-directed fluorescence spectroscopy and chemical cross-linking to locate the N-terminal region and assess its flexibility in the absence and presence of DNA substrate. The second amino acid in each subunit of the homodimer was replaced with cysteine and labeled with pyrene or reacted with bifunctional cross-linkers. The broad absorption spectra and characteristic excimer emission bands of pyrene-labeled muteins indicated stacking of the two pyrene rings in the homodimer. Proximity of N-terminal cysteines was confirmed by disulfide bond formation and chemical cross-linking. The dynamics of the N-terminal region were determined from time-resolved emission anisotropy measurements. The anisotropy decay had two components:  a fast component with rotational correlation time of 0.3−3 ns representing probe internal motions and a slow component with 50−100 ns correlation time representing overall tumbling of the protein conjugate. We conclude that the N-termini are close together at the dimer interface with limited flexibility. Binding of Mg2+ cofactor or DNA substrate did not affect the location or flexibility of the N-terminal region as sensed by pyrene fluorescence and cross-linking, indicating that substrate binding is not accompanied by folding or unfolding of the N-terminus.
ISSN:0006-2960
1520-4995
DOI:10.1021/bi980557f