RNA interference (RNAi) is a well-established
research tool and
is also maturing as a novel therapeutic approach. For the latter,
microRNA-like off-target activity of short interfering RNAs (siRNAs)
remains as one of the main problems limiting RNAi drug development.
In this communication, we report that replacement of a single internucleoside
phosphodiester in the seed region (nucleotides 2 to 7) of the guide
strand with an amide linkage suppressed the undesired microRNA-like
off-target activity by at least an order of magnitude. For the specific
siRNA targeting the PIK3CB gene, an amide modification between the
third and fourth nucleotides of the guide strand showed the strongest
enhancement of specificity (completely eliminated off-target silencing)
while maintaining high on-target activity. These results are important
because off-target activity is one of the main remaining roadblocks
for RNA based drug development.
The development of CRISPR-Cas9 mediated gene editing technology is revolutionizing molecular biology, biotechnology, and medicine. However, as with other nucleic acid technologies, CRISPR would greatly benefit from chemical modifications that optimize delivery, activity, and specificity of gene editing. Amide modifications at certain positions of short interfering RNAs have been previously shown to improve their RNAi activity and specificity, which motivated the current study on replacement of selected internucleoside phosphates of CRISPR RNAs with amide linkages. Herein, we show that amide modifications did not interfere with CRISPR-Cas9 activity when placed in the protospacer adjacent motif (PAM) distal region of CRISPR RNAs. In contrast, modification of the seed region led to a loss of DNA cleavage activity at most but not all positions. These results are encouraging for future studies on amides as backbone modifications in CRISPR RNAs.
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