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APOBEC3A and APOBEC3B Preferentially Deaminate the Lagging Strand Template during DNA Replication.

Cell Rep. 2016; 
HoopesJames I,CortezLuis M,MertzTony M,MalcEwa P,MieczkowskiPiotr A,RobertsStev
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DNA Sequencing CAN1 PCR products were Sanger sequenced (Eton Biosciences, San Diego, CA and GenScript, Piscataway, NJ) and mutations inactivating CAN1 (Table S1) identified using the Geneious software package (Biomatters Limited). Get A Quote

摘要

APOBEC family cytidine deaminases have recently been implicated as powerful mutators of cancer genomes. How APOBECs, which are ssDNA-specific enzymes, gain access to chromosomal DNA is unclear. To ascertain the chromosomal ssDNA substrates of the APOBECs, we expressed APOBEC3A and APOBEC3B, the two most probable APOBECs mediating cancer mutagenesis, in a yeast model system. We demonstrate, using mutation reporters and whole genome sequencing, that APOBEC3A- and APOBEC3B-induced mutagenesis primarily results from the deamination of the lagging strand template during DNA replication. Moreover, our results indicate that both genetic deficiencies in replication fork-stabilizing proteins and chemical... More

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