A Novel 2′-Deoxy-2′-Fluoro (2′F-ANA) Ribose Modification Significantly Enhances the Duration, and Efficiency, of Nucleic Acid Mediated Gene Silencing.

The field of nucleic acid mediated gene silencing has been reinvigorated with the widespread adoption of RNA interference using siRNA. Since issues of delivery, stability, and duration of effect remain relevant to siRNA, and all other types of gene silencing nucleic acids, we are studying chemical modifications that may enhance the efficiency of molecules employed for this purpose. To this end, we synthesized 2′-deoxy-2′-fluoro-d-arabinonucleic acid (2′F-ANA) modifications of DNA as our prior work suggested that they would simultaneously raise the Tm of mRNA:DNA hybrids, increase resistance to nucleases, and very importantly, still permit RNaseH binding and catalysis of the target mRNA because the 2′F-ANA of the arabinose sugar ring projects, like DNA, into the major groove of the helix. Accordingly, we compared the gene silencing efficacy of 2′F-ANA modified oligonucleotides (ON) with traditional phosphorothioate (PS) antisense oligodeoxynucleotides (AS ODN) with respect to cellular delivery, intracellular stability, dose response, and duration of gene silencing in living myeloid leukemia cells. 2′F-ANA modification were made to form either “altimers” where triplets of nucleotides with F-ANA modified sugars alternated with triplets of nucleotides with deoxyribose sugars, or “gapmers” where 7, 2′fluorinated oligonucleotides flank 7 central unmodified nucleotides. The mRNA target for these comparative studies was a region within the c-myb mRNA that was previously shown by us to be accessible for hybridization in vivo (