Title of article
Precise quantification of transcription factors in a surface-based single-molecule assay Original Research Article
Author/Authors
Kristin S. Gru?mayer، نويسنده , , Tanja Ehrhard، نويسنده , , Konstantinos Lymperopoulos، نويسنده , , Dirk-Peter Herten، نويسنده ,
Issue Information
روزنامه با شماره پیاپی سال 2013
Pages
7
From page
1
To page
7
Abstract
Biosensors have recognized a rapid development the last years in both industry and science. Recently, a single-molecule assay based on alternating laser excitation has been established for the quantitative detection of transcription factors. These proteins specifically recognize and bind DNA and play an important role in controlling gene expression. We implemented this assay format on a total internal reflection fluorescence microscope to detect transcription factors with immobilized single-molecule DNA biosensors. We quantify transcription factors via colocalization of the two halves of their binding site with immobilized single molecules of a two-color DNA biosensor. We could detect a model transcription factor, the bacterial lactose repressor, at different concentrations down to 150 pM. We found that robust modeling of stoichiometry derived TIRF data is achieved with Studentʹs t-distributions and nonlinear least-squares estimation with weights equal to the inverse of the expected number of bin entries. This significantly improved transcription factor concentration estimates with respect to distribution modeling with Gaussians without adding notable computational effort. The proposed model may enhance the precision of other single-molecule assays quantifying molecular distributions. Our measurements reliably confirm that the immobilized biosensor format is more sensitive than a previously published solution based approach.
Keywords
Biosensor , Quantitative detection , transcription factor , Single-molecule study , Surface immobilization
Journal title
Biophysical Chemistry
Serial Year
2013
Journal title
Biophysical Chemistry
Record number
1120682
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