Abstract
Here we describe a non-radioactive assay that exploits the fluorescent dye SYBR Green to measure the helicase enzyme activity. SYBR Green I emits fluorescence upon intercalation with double-stranded DNA or RNA. The fluorescence is lost proportionally as the nucleic acid is converted to single strands by a helicase, and this decrease in fluorescence intensity can be used to measure the activity of the helicase enzyme. The reaction was prepared by mixing a double-stranded substrate with the helicase enzyme, buffer, ATP and SYBR Green I. After completion, the reaction was terminated by EDTA and fluorescence was measured. Using this technique, a linear increase in substrate release was observed with increasing time and helicase concentrations. The assay described here is speedy, efficient and economical; it holds promise for use in large-scale screening of drugs that target helicases.
| Original language | English (UK) |
|---|---|
| Pages (from-to) | 196-198 |
| Number of pages | 3 |
| Journal | Enzyme and Microbial Technology |
| Volume | 52 |
| Issue number | 3 |
| DOIs | |
| Publication status | Published - 5 Mar 2013 |
Keywords
- Helicase
- SYBR Green