Abstract
dUTP is a close structural congener of dTTP and can be readily incorporated into DNA opposite to adenine during DNA replication leading to non-mutagenic dU/A base pairs (‘uracilation’). We find that dU/A pairs located within DNA transcriptional templates optimized for either T7 RNA polymerase (T7 RNAP) or human RNA polymerase II (pol II) have inhibitory and mutagenic effects on transcription. The data for T7 RNAP establishes that even a single dU/A pair can inhibit promoter binding and transcription initiation up to 30-fold, and that inhibitory effects on transcription elongation are also possible. Sequencing of the mRNA transcribed from uniformly uracilated DNA templates by T7 RNAP indicated an increased frequency of transversion and insertion mutations compared to all T/A templates. Strong effects of dU/A pairs on cellular transcription activity and fidelity were also observed with RNA pol II using uracil base excision repair (UBER)-deficient human cells. At the highest levels of template uracilation, transcription by RNA pol II was completely blocked. We propose that these effects arise from the decreased thermodynamic stability and increased dynamics of dU/A pairs in DNA. The potential implications of these findings on gene regulation and disease are discussed.
Highlights
ASubstrates (321 bp) were prepared containing just T/A (T321) or 50 and 100% dU/A base pairs (U50321 and U321). bkcat/Kmrel is the relative catalytic efficiency calculated using the ratioU promoter/(kcat/Km)T promoter
The numbering -1, -3, -6 refers to position of the T→U substitution relative to the transcription start site (+1). bThe number 23 refers to the length of the substrate. ckcat/Kmrel is the relative catalytic efficiency calculated using the ratiouracilated promoter/(kcat/Km)T promoter The concentration of DNA in each reaction used as 5-120 nM and that of T7 RNAP was 10 nM
Kcat/Km kcat/Kmrel b aThe superscripts I, IE and PIE refer to the region containing initiation, initiation and elongation, promoter, initiation and elongation, respectively
Summary
ASubstrates (321 bp) were prepared containing just T/A (T321) or 50 and 100% dU/A base pairs (U50321 and U321). bkcat/Kmrel is the relative catalytic efficiency calculated using the ratio (kcat/Km)U promoter/(kcat/Km)T promoter. Kcat/Km kcat/Kmrel b aSubstrates (321 bp) were prepared containing just T/A (T321) or 50 and 100% dU/A base pairs (U50321 and U321). Bkcat/Kmrel is the relative catalytic efficiency calculated using the ratio (kcat/Km)U promoter/(kcat/Km)T promoter. The concentrations of DNA in each reaction were 1-60 nM for T321 and U50321, and 5-120 nM for U321.
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