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dc.contributor.authorKaye, Bryan
dc.contributor.authorYoo, Tae Yeon
dc.contributor.authorFoster, Peter
dc.contributor.authorYu, Che-Hang
dc.contributor.authorNeedleman, Daniel
dc.date.accessioned2019-10-03T14:39:03Z
dc.date.issued2017
dc.identifier.citationKaye, Bryan, Tae Yeon Yoo, Peter J. Foster, Che-Hang Yu, and Daniel J. Needleman. 2017. “Bridging Length Scales to Measure Polymer Assembly.” Edited by Manuel Théry. Molecular Biology of the Cell 28 (10): 1379–88. https://doi.org/10.1091/mbc.e16-05-0344.
dc.identifier.issn1059-1524
dc.identifier.issn1939-4586
dc.identifier.urihttp://nrs.harvard.edu/urn-3:HUL.InstRepos:41461244*
dc.description.abstractTime-resolvable quantitative measurements of polymer concentration are very useful to elucidate protein polymerization pathways. There are numerous techniques to measure polymer concentrations in purified protein solutions, but few are applicable in vivo. Here we develop a methodology combining microscopy and spectroscopy to overcome the limitations of both approaches for measuring polymer concentration in cells and cell extracts. This technique is based on quantifying the relationship between microscopy and spectroscopy measurements at many locations. We apply this methodology to measure microtubule assembly in tissue culture cells and Xenopus egg extracts using two-photon microscopy with FLIM measurements of FRET. We find that the relationship between FRET and two-photon intensity quantitatively agrees with predictions. Furthermore, FRET and intensity measurements change as expected with changes in acquisition time, labeling ratios, and polymer concentration. Taken together, these results demonstrate that this approach can quantitatively measure microtubule assembly in complex environments. This methodology should be broadly useful for studying microtubule nucleation and assembly pathways of other polymers.
dc.language.isoen_US
dc.publisherAmerican Society for Cell Biology
dash.licenseLAA
dc.titleBridging length scales to measure polymer assembly
dc.typeJournal Article
dc.description.versionVersion of Record
dc.relation.journalMolecular Biology of the Cell
dash.depositing.authorNeedleman, Daniel Joseph::d96a02ce893259d40dd77efe8101c37d::600
dc.date.available2019-10-03T14:39:03Z
dash.workflow.comments1Science Serial ID 65407
dc.identifier.doi10.1091/mbc.E16-05-0344
dash.source.volume28;10
dash.source.page1379


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