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Originally published as Biophys J. BioFAST on November 19, 2004.
doi:10.1529/biophysj.104.039834
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Biophysical Journal 88:1191-1206 (2005)
© 2005 The Biophysical Society

Intrinsic Curvature in the VP1 Gene of SV40: Comparison of Solution and Gel Results

Yongjun Lu, Brock D. Weers and Nancy C. Stellwagen

Department of Biochemistry, University of Iowa, Iowa City, Iowa 52242

Correspondence: Address reprint requests to Nancy C. Stellwagen, Dept. of Biochemistry, University of Iowa, Iowa City, IA 52242. Tel.: 319-335-7896; Fax: 319-335-9570; E-mail: nancy-stellwagen{at}uiowa.edu.

DNA restriction fragments that are stably curved are usually identified by polyacrylamide gel electrophoresis because curved fragments migrate more slowly than normal fragments containing the same number of basepairs. In free solution, curved DNA molecules can be identified by transient electric birefringence (TEB) because they exhibit rotational relaxation times that are faster than those of normal fragments of the same size. In this article, the results observed in free solution and in polyacrylamide gels are compared for a highly curved 199-basepair (bp) restriction fragment taken from the VP1 gene in Simian Virus 40 (SV40) and various sequence mutants and insertion derivatives. The TEB method of overlapping fragments was used to show that the 199-bp fragment has an apparent bend angle of 46 ± 2° centered at sequence position 1922 ± 2 bp. Four unphased A- and T-tracts and a mixed A3T4-tract occur within a span of ~60 bp surrounding the apparent bend center; for brevity, this 60-bp sequence element is called a curvature module. Modifying any of the A- or T-tracts in the curvature module by site-directed mutagenesis decreases the curvature of the fragment; replacing all five A- and T-tracts by random-sequence DNA causes the 199-bp mutant to adopt a normal conformation, with normal electrophoretic mobilities and birefringence relaxation times. Hence, stable curvature in this region of the VP1 gene is due to the five unphased A- and T- tracts surrounding the apparent bend center. Discordant solution and gel results are observed when long inverted repeats are inserted within the curvature module. These insertion derivatives migrate anomalously slowly in polyacrylamide gels but have normal, highly flexible conformations in free solution. Discordant solution and gel results are not observed if the insert does not contain a long inverted repeat or if the long inverted repeat is added to the 199-bp fragment outside the curvature module. The results suggest that long inverted repeats can form hairpins or cruciforms when they are located within a region of the helix backbone that is intrinsically curved, leading to large mobility anomalies in polyacrylamide gels. Hairpin/cruciform formation is not observed in free solution, presumably because of rapid conformational exchange. Hence, DNA restriction fragments that migrate anomalously slowly in polyacrylamide gels are not necessarily stably curved in free solution.




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