4.8 Article

Sequence specific fluorescence detection of double strand DNA

Journal

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
Volume 125, Issue 5, Pages 1195-1202

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/ja021011q

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Funding

  1. NIGMS NIH HHS [GM19789-02, GM 27681] Funding Source: Medline

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Methods for the fluorescent detection of specific sequences of double strand DNA in homogeneous solution may be useful in the field of human genetics. A series of hairpin polyamides with tetramethyl rhodamine (TMR) attached to an internal pyrrole ring were synthesized, and the fluorescence properties of the polyamide-fluorophore conjugates in the presence and absence of duplex DNA were examined. We observe weak TMR fluorescence in the absence of DNA. Addition of greater than or equal to 1:1 match DNA affords a significant fluorescence increase over equimolar mismatch DNA for each polyamide-TMR conjugate. Polyamide-fluorophore conjugates offer a new class of sensors for the detection of specific DNA sequences without the need for denaturation. The polyamide-dye fluorescence-based method can be used to screen in parallel the interactions between aromatic ring pairs and the minor groove of DNA even when the binding site contains a non-Watson-Crick DNA base pair. A ranking of the specificity of three polyamide ring pairs-Py/Py, lm/Py, and lm/lm-was established for all 16 possible base pairs of A, T, G, and C in the minor groove. We find that Im/Im is an energetically favorable ring-pair for minor groove recognition of the T.G base pair.

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