Abstract

The Human Genome Project has facilitated the sequencing of many species, yet the current Sanger method is too expensive, labor intensive and time consuming to accomplish medical resequencing of human genomes en masse. Of the 'next-generation' technologies, cyclic reversible termination (CRT) is a promising method with the goal of producing accurate sequence information at a fraction of the cost and effort. The foundation of this approach is the reversible terminator (RT), its chemical and biological properties of which directly impact the performance of the sequencing technology. Here, we have discovered a novel paradigm in RT chemistry, the attachment of a photocleavable, 2-nitrobenzyl group to the N(6)-position of 2'-deoxyadenosine triphosphate (dATP), which, upon incorporation, terminates DNA synthesis. The 3'-OH group of the N(6)-(2-nitrobenzyl)-dATP remains unblocked, providing favorable incorporation and termination properties for several commercially available DNA polymerases while maintaining good discrimination against mismatch incorporations. Upon removal of the 2-nitrobenzyl group with UV light, the natural nucleotide is restored without molecular scarring. A five-base experiment, illustrating the exquisite, stepwise addition through a homopolymer repeat, demonstrates the applicability of the N(6)-(2-nitrobenzyl)-dATP as an ideal RT for CRT sequencing.

Keywords

AlkylationBiologyDeoxyadenosineDNABiochemistryCatalysis

MeSH Terms

AlkylationBase Pair MismatchDNADNA-Directed DNA PolymeraseDeoxyadenine NucleotidesDeoxyadenosinesPhotochemistrySequence AnalysisDNAUltraviolet Rays

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Publication Info

Year
2007
Type
article
Volume
35
Issue
19
Pages
6339-6349
Citations
43
Access
Closed

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43
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Cite This

Weidong Wu, Brian P. Stupi, Vladislav A. Litosh et al. (2007). Termination of DNA synthesis by N6 -alkylated, not 3′- O -alkylated, photocleavable 2′-deoxyadenosine triphosphates. Nucleic Acids Research , 35 (19) , 6339-6349. https://doi.org/10.1093/nar/gkm689

Identifiers

DOI
10.1093/nar/gkm689
PMID
17881370
PMCID
PMC2095803

Data Quality

Data completeness: 86%