COGNET, Laurent; TARDIN, Catherine; NÉGRIER, Marie-Laure Martin; BREILLAT, Christelle; COUSSEN, Françoise; CHOQUET, Daniel; LOUNIS, Brahim

doi:10.1117/1.2940600

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COGNET, Laurent
Centre de physique moléculaire optique et hertzienne [CPMOH]

TARDIN, Catherine
Centre de physique moléculaire optique et hertzienne [CPMOH]

NÉGRIER, Marie-Laure Martin
Centre de physique moléculaire optique et hertzienne [CPMOH]

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Journal of Biomedical Optics. 2008-06-23, vol. 13, n° 3, p. 031216

Society of Photo-optical Instrumentation Engineers

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Using single-molecule microscopy, we present a method to quantify the number of single autofluorescent proteins when they cannot be optically resolved. This method relies on the measurement of the total intensity emitted by each aggregate until it photobleaches. This strategy overcomes the inherent problem of blinking of green fluorescent proteins. In the case of small protein aggregates, our method permits us to describe the mean composition with a precision of one protein. For aggregates containing a large number of proteins, it gives access to the average number of proteins gathered and a signature of the inhomogeneity of the aggregates' population. We applied this methodology to the quantification of small purified citrine multimers.< Leer menos

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aggregation

bioluminescence

fluorescence

molecular biophysics

optical saturable absorption

proteins

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Robust single-molecule approach for counting autofluorescent proteins.

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