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A Structural Model For Sequence-Specific Proflavin-DNA Interactions During In Vitro Frameshift Mutagenesis
Authors:Helen M Berman  Joel L Sussman  Leemor Joshua-Tor  Galena G Revich  Lynn S Ripley
Institution:1. Department of Chemistry , Rutgers University , P.O. Box 939, Piscataway , NJ , 08855-0939;2. Department of Structural Chemistry , The Weizmann Institute of Science , Rehovot , 76100 , ISRAEL;3. Division of Chemistry , California Institute of Technology , Pasedena , CA , 91125 , USA;4. Dept. of Microbiology and Molecular Genetics , University of Medicine and Dentistry of New Jersey , 185 South Orange Avenue, Newark , NJ , 07103
Abstract:Abstract

Molecular models describing intermediates that may lead to proflavin-induced 1 bp deletions during in vitro polymerization by E. coli DNA polymerase I Klenow fragment are proposed. The models provide structural explanations for the fact that the induced frameshifts always occur opposite template bases that are adjacent to 5′ pyrimidines and are based on the underlying hypothesis that the deletions arise because the polymerase passes by a template base without copying it. Because the most frequent mutations are opposite Pu in the template sequence 5′ Py Pu 3′, a single-strand loop-out model was constructed for this sequence and proflavin was added, using structures found in crystalline oligonucleotides and their complexes with proflavin. The model seeks to rationalize the roles of the 5′ pyrimidine and proflavin in facilitating the bypass. Four potential roles for proflavin in mutagenesis are described: 1) stacking on the looped-out base; 2) stacking on the base pair immediately preceding the site of mutation; 3) hydrogen bonding with the 5′ pyrimidine; 4) hydrogen bonding with the phosphate backbone. These models point to the possibility that a number of proflavin-DNA interactions may be involved. In contrast, modeling does not suggest a role for classically intercalated proflavin in frameshift mutagenesis arising during in vitro DNA polymerization.
Keywords:
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