Mix and measure fluorescence screening for selective quadruplex binders | Zendy

Sattanathan Paramasivan | Zendy; Philip H. Bolton | Zendy

AI Assistant Blog Pricing

Home ZAIA Blog

Open Access

Mix and measure fluorescence screening for selective quadruplex binders

Author(s) -

Sattanathan Paramasivan,

Philip H. Bolton

Publication year - 2008

Publication title -

nucleic acids research

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 9.008

H-Index - 537

eISSN - 1362-4954

pISSN - 0305-1048

DOI - 10.1093/nar/gkn487

Subject(s) - g quadruplex , biology , computational biology , dna , fluorescence , telomere , genome , folding (dsp implementation) , reporter gene , biophysics , genetics , gene , gene expression , physics , quantum mechanics , electrical engineering , engineering

The human genome contains thousands of regions, including that of the telomere, that have the potential to form quadruplex structures. Many of these regions are potential targets for therapeutic intervention. There are many different folding patterns for quadruplex DNAs and the loops exhibit much more variation than do the quartets. The successful targeting of a particular quadruplex structure requires distinguishing that structure from all of the other quadruplex structures that may be present. A mix and measure fluorescent screening method has been developed, that utilizes multiple reporter molecules that bind to different features of quadruplex DNA. The reporter molecules are used in combination with DNAs that have a variety of quadruplex structures. The screening is based on observing the increase or decrease in the fluorescence of the reporter molecules. The selectivity of a set of test molecules has been determined by this approach.

The content you want is available to Zendy users.

Already have an account? Click here to sign in.

Having issues? You can contact us here

Accelerating Research