Joining of nonhomologous DNA double strand breaks in vitro

doi:10.1093/nar/16.3.907

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Nucleic Acids Research, 1988, Vol. 16, No. 3 907-924
© 1988

Articles

Joining of nonhomologous DNA double strand breaks in vitro

Petra Pfeiffer and Walter Vielmetter

Institut für Genetik der Universität zu Köln Weyertal 121, D-5000 Köln 41, FRG

Received October 22, 1987. Accepted December 23, 1987.

Extracts of Xenopus laevis eggs can efficiently join ends ofduplex DNA that differ in structure and sequence. This was analysedby recircularisation of linear plasmid DNA molecules with dissimilartermini, generated by successive cuts with two different restrictionenzymes within the pSP65 polylinker. Use of various enzymesprovided blunt ended or 4 nucleotides long 3' and 5' protrudingsingle strand (PSS) termini which were successfully joined invitro in any tested combination. Sequence analysis of numerousjunctions from cloned reaction products of 7 terminus combinationsreveal: apart from very rare base exchanges and single nucleotideinsertions <10% deletions (1 to 18 nucleotides long) weredetected. Blunt/PSS or 3'PSS/5'PSS terminus pairs undergo simple"blunt end" joining which preserves PSS ends by fill-in. Incontrast, equally polar 3'PSS/3'PSS or 5'PSS/5'PSS terminuspairs are joined by a complex mode: PSS ends overlap by a definednumber of nucleotides, set by matching basepairs. Even one basematchsuffices to define the setting. This then determines the finalmismatch repair and fill-in pattern. We propose that yet unknownterminal DNA-binding proteins stabilize the energetically highlyunfavorable configuration of single matching basepairs and helpto support defined overlap structures.

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