Accurate in vitro, translesion synthesis by Escherichia coli DNA polymerase I (large fragment) on a site-specific, aminofluorenemodified oligonucleotide

We have measured the accuracy of in vitro synthesis by DNA polymerase I (large fragment) during translesion synthesis past an aminofluorene (AF) adduct. These studies were carried out using a site-specifically modified template which contained a single AF adduct. The template was prepared by first m...

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Veröffentlicht in:Carcinogenesis (New York) 1991-09, Vol.12 (9), p.1641-1646
Hauptverfasser: Michales, Mark Leo, Reid, Thomas M., King, Charles M., Romano, Louis J.
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Sprache:eng
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Zusammenfassung:We have measured the accuracy of in vitro synthesis by DNA polymerase I (large fragment) during translesion synthesis past an aminofluorene (AF) adduct. These studies were carried out using a site-specifically modified template which contained a single AF adduct. The template was prepared by first modifying the lone guanine in a 17 base long oligonucleotide and extensively purifying and characterizing this product. The modified 17mer was then ligated to a synthetic duplex to produce a 31 nucleotide long template strand containing the AF adduct annealed to a 14mer, such that the 3′-hydroxyl primer terminus was four nucleotides before the modified guanine. Synthesis on this template by DNA polymerase I efficiently bypassed the AF adduct and produced full-length duplex 3lmers. T7 DNA plymerase, on the other hand, was unable to utilize the AF-modified template though it was active on an identical unmodified one. The strand synthesized by DNA polymerase I was then separated from the modified strand, annealed to a complementary oligonucleotide, and the resulting heteroduplex cloned into M13. Each of the 49 clones isolated had sequences which indicated that cytidine had been incorporated opposite the AF-modlfled guanine.
ISSN:0143-3334
1460-2180
DOI:10.1093/carcin/12.9.1641