{"id":880,"date":"2014-01-14T06:00:00","date_gmt":"2014-01-14T06:00:00","guid":{"rendered":"https:\/\/www.idtdna.com\/page\/modification-highlight-modifications-that-block-nuclease-degradation"},"modified":"2025-08-22T16:09:31","modified_gmt":"2025-08-22T16:09:31","slug":"modification-highlight-modifications-that-block-nuclease-degradation","status":"publish","type":"post","link":"https:\/\/www.idtdna.com\/page\/support-and-education\/decoded-plus\/modification-highlight-modifications-that-block-nuclease-degradation\/","title":{"rendered":"Oligo modifications that block nuclease degradation"},"content":{"rendered":"<p>When oligonucleotides are used in cell culture experiments&mdash;such as in antisense and RNAi applications, and in ribozyme technology, degradation by nucleases is a concern. Oligonucleotide stability is typically crucial to these types of studies; yet unmodified DNA and RNA oligonucleotides are quickly digested <em>in vitro <\/em>by endogenous nucleases. Multiple endo- and exonucleases exist&nbsp;[<a href=\"#references\">1<\/a>]. In serum, the bulk of biologically relevant nucleolytic activity occurs as 3&prime; exonuclease activity [<a href=\"#references\">2<\/a>], while within the cell, nucleolytic activity is affected by both 5&prime; and 3&prime; exonucleases [<a href=\"#references\">3<\/a>].<\/p>\n<h2>Modifications<\/h2>\n<p>To limit nuclease degradation, investigators have substituted many different modifications into native phosphodiester oligodeoxyribonucleotide and ribonucleotide polymers. IDT offers several such modifications that are incorporated during oligonucleotide synthesis:<\/p>\n<h3>Phosphorothioate (PS) bonds<\/h3>\n<p>The <a href=\"\/site\/Catalog\/Modifications\/Category\/8\">phosphorothioate (PS) bond<\/a>&nbsp;substitutes a sulfur atom for a non-bridging oxygen in the phosphate backbone of an oligonucleotide. Approximately 50% of the time (due to the 2 resulting stereoisomers that can form), PS modification renders the internucleotide linkage more resistant to nuclease degradation. Therefore, IDT recommends including at least 3 PS bonds at the 5&prime; and 3&prime; oligonucleotide ends to inhibit exonuclease degradation. Including PS bonds throughout the entire oligonucleotide will help reduce attack by endonucleases as well but may also increase toxicity.<\/p>\n<h3>2'-O-Methyl (2'OMe)<\/h3>\n<p>A naturally occurring post-transcriptional modification of RNA, <a href=\"\/site\/catalog\/modifications\/category\/7\">2'OMe,&nbsp;<\/a>is found in tRNA and other small RNAs. Oligonucleotides can be directly synthesized to contain 2'OMe. This modification increases the melting temperature (T<sub><span>m<\/span><\/sub>) of RNA:RNA duplexes, but results in only small changes in RNA:DNA stability. It prevents attack by single-stranded endonucleases, but not exonuclease digestion. Therefore, it is important to end block these oligos as well. DNA oligonucleotides that include this modification are typically 5- to 10-fold less susceptible to DNases than unmodified DNA. The 2&prime;OMe modification is commonly used in antisense oligonucleotides to increase stability and binding affinity to target transcripts [<a href=\"#references\">4<\/a>].<\/p>\n<h3>2' Fluoro bases<\/h3>\n<p><a href=\"\/site\/catalog\/modifications\/product\/2309\">2'-fluoro bases<\/a> have a fluorine-modified ribose which increases binding affinity and also confers some relative nuclease resistance relative to native RNA. IDT recommends using this modification in conjunction with PS-modified bonds.<\/p>\n<h3>Inverted dT and ddT<\/h3>\n<p><a href=\"\/pages\/education\/decoded\/article\/inverted-bases\">Inverted dT <\/a>can be incorporated at the 3&prime; end of an oligonucleotide, leading to a 3'-3' linkage that will inhibit degradation by 3' exonucleases and extension by DNA polymerases. In addition, placing an inverted, 2&prime;,3&prime; dideoxy-dT base (5' Inverted ddT) at the 5&prime; end of an oligonucleotide prevents spurious ligations and may protect against some forms of enzymatic degradation.<\/p>\n<h3>Phosphorylation<\/h3>\n<p><a href=\"\/site\/Catalog\/Modifications\/Category\/1\">Phosphorylation<\/a> of the 3&prime; end of oligonucleotides will inhibit degradation by some 3&prime;-exonucleases.<\/p>\n<h3>C3 Spacer<\/h3>\n<p>The phosphoramidite <a href=\"\/site\/catalog\/modifications\/product\/1165\">C3 Spacer<\/a>&nbsp;can be incorporated internally, or at either end of an oligo to introduce a long hydrophilic spacer arm for the attachment of fluorophores or other pendent groups. The C3 spacer also can be used to inhibit degradation by 3' exonucleases.<\/p>\n<h2>Avoiding unanticipated effects<\/h2>\n<p>It is important to test any modified oligonucleotides to establish that they work in your specific experimental context. Other considerations include ensuring that the resulting modified oligos:<\/p>\n<ul>\n<li>Are not physiologically toxic<\/li>\n<li>Are not easily degraded<\/li>\n<li>Do not disrupt normal Watson&ndash;Crick base pairing<\/li>\n<li> Do not induce any unanticipated, sequence-independent biological effects; e.g., <a href=\"\/pages\/support\/faqs\/how-do-i-identify-crispr-editing-off-target-sites\">off-target effects<\/a>, or triggering an&nbsp;innate immune response. Residue modifications can also affect the ability of an oligo to trigger RNase H&ndash;mediated degradation of RNA following hybrid formation [<a href=\"#references\">4<\/a>].<\/li>\n<\/ul>\n<p>If you have any questions or want to discuss your experimental design, you can always <a href=\"\/pages\/support\/contact-us\">contact us<\/a>.<\/p>\n","protected":false},"excerpt":{"rendered":"<p>When oligonucleotides are used in cell culture experiments&mdash;such as in antisense and RNAi applications, and in ribozyme technology, degradation by nucleases is a concern. Oligonucleotide stability is typically crucial to these types of studies; yet unmodified DNA and RNA oligonucleotides are quickly digested in vitro by endogenous nucleases. Multiple endo- and exonucleases exist&nbsp;[1]. In serum, [&hellip;]<\/p>\n","protected":false},"author":1,"featured_media":0,"comment_status":"open","ping_status":"open","sticky":false,"template":"","format":"standard","meta":{"_acf_changed":false,"ct_builder_shortcodes":"","ct_template_type":"","ct_parent_template":0,"inline_featured_image":false,"footnotes":""},"class_list":["post-880","post","type-post","status-publish","format-standard","hentry"],"acf":[],"yoast_head":"<!-- This site is optimized with the Yoast SEO plugin v27.0 - https:\/\/yoast.com\/product\/yoast-seo-wordpress\/ -->\n<title>Oligo modifications that block nuclease degradation | IDT<\/title>\n<meta name=\"description\" content=\"Are you working with your oligos in cell culture? 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