Quantifying Localizations and Dynamics in Single Bacterial Cells

Levels of macromolecules fluctuate both spatially and temporally in individual cells. Such heterogeneity could be exploited for bet hedging in uncertain environments, or be suppressed by negative feedback if perturbations are deleterious. For the master stress-response regulator in Escherichia coli,...

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Main Author: Landgraf, Dirk
Other Authors: Paulsson, Johan Martin
Language:en_US
Published: Harvard University 2012
Subjects:
Online Access:http://dissertations.umi.com/gsas.harvard:10612
http://nrs.harvard.edu/urn-3:HUL.InstRepos:9920184
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spelling ndltd-harvard.edu-oai-dash.harvard.edu-1-99201842015-08-14T15:41:42ZQuantifying Localizations and Dynamics in Single Bacterial CellsLandgraf, DirkClp proteasesRpoSsystematic biologybiophysicsmicrobiologyfluorescent proteinsmicroscopystress responseprotein degradationLevels of macromolecules fluctuate both spatially and temporally in individual cells. Such heterogeneity could be exploited for bet hedging in uncertain environments, or be suppressed by negative feedback if perturbations are deleterious. For the master stress-response regulator in Escherichia coli, RpoS, both of these scenarios have been suggested. RpoS levels are also exceedingly low and controlled by the ClpXP protease, which reportedly displays extreme spatial heterogeneity. However, little is known quantitatively about RpoS dynamics. This is partly because no functional protein fusions exist, but also because the quantitative tools for studying fluctuations and localizations are limited, particularly ones that can be independently validated. Here I develop such methods and begin applying them to RpoS. Protein localization measurements increasingly rely on fluorescent protein fusions and are difficult to verify independently. I designed a non-intrusive method for validating localization patterns in live bacterial cells by exploiting post-division heterogeneity in downstream processes. Applying this assay to the ClpXP protease, widely reported to form biologically relevant foci, revealed in fact that the protease molecules are not specifically localized inside cells, as confirmed by four independent methods. I further evaluated 20+ commonly used fluorescent reporters and found that many cause severe mislocalization when fused to homo-oligomers, likely due to avidity effects. Further reinvestigating other foci-forming proteins strongly suggests that the previously reported foci were all caused by the fluorescent proteins used. For mRNAs – which are often present in low numbers per cell and major sources of non-genetic heterogeneity – existing single-cell assays have unknown accuracy: the experimental counting errors could completely over-shadow the natural variation. I therefore optimized and cross-evaluated two single-molecule mRNA detection methods. Several problems were identified and solutions discussed. I succeeded in building a functional RpoS protein fusion, and used bulk methods to show that the RpoS feedback loop is effectively not operating during exponential- phase growth. Mathematical analyses and initial experiments in a microfluidic device further suggest that the RpoS system has several unusual properties contributing towards extremely fast stress response. A stochastic analysis further suggests that the RpoS feedback loop cannot suppress spontaneous fluctuations, and preliminary experiments indicate that large deviations might indeed play important roles.Paulsson, Johan Martin2012-11-19T15:33:18Z2012-11-1920122014-10-06T07:30:36ZThesis or DissertationLandgraf, Dirk. 2012. Quantifying Localizations and Dynamics in Single Bacterial Cells. Doctoral dissertation, Harvard University.http://dissertations.umi.com/gsas.harvard:10612http://nrs.harvard.edu/urn-3:HUL.InstRepos:9920184en_USopenhttp://nrs.harvard.edu/urn-3:HUL.InstRepos:dash.current.terms-of-use#LAAHarvard University
collection NDLTD
language en_US
sources NDLTD
topic Clp proteases
RpoS
systematic biology
biophysics
microbiology
fluorescent proteins
microscopy
stress response
protein degradation
spellingShingle Clp proteases
RpoS
systematic biology
biophysics
microbiology
fluorescent proteins
microscopy
stress response
protein degradation
Landgraf, Dirk
Quantifying Localizations and Dynamics in Single Bacterial Cells
description Levels of macromolecules fluctuate both spatially and temporally in individual cells. Such heterogeneity could be exploited for bet hedging in uncertain environments, or be suppressed by negative feedback if perturbations are deleterious. For the master stress-response regulator in Escherichia coli, RpoS, both of these scenarios have been suggested. RpoS levels are also exceedingly low and controlled by the ClpXP protease, which reportedly displays extreme spatial heterogeneity. However, little is known quantitatively about RpoS dynamics. This is partly because no functional protein fusions exist, but also because the quantitative tools for studying fluctuations and localizations are limited, particularly ones that can be independently validated. Here I develop such methods and begin applying them to RpoS. Protein localization measurements increasingly rely on fluorescent protein fusions and are difficult to verify independently. I designed a non-intrusive method for validating localization patterns in live bacterial cells by exploiting post-division heterogeneity in downstream processes. Applying this assay to the ClpXP protease, widely reported to form biologically relevant foci, revealed in fact that the protease molecules are not specifically localized inside cells, as confirmed by four independent methods. I further evaluated 20+ commonly used fluorescent reporters and found that many cause severe mislocalization when fused to homo-oligomers, likely due to avidity effects. Further reinvestigating other foci-forming proteins strongly suggests that the previously reported foci were all caused by the fluorescent proteins used. For mRNAs – which are often present in low numbers per cell and major sources of non-genetic heterogeneity – existing single-cell assays have unknown accuracy: the experimental counting errors could completely over-shadow the natural variation. I therefore optimized and cross-evaluated two single-molecule mRNA detection methods. Several problems were identified and solutions discussed. I succeeded in building a functional RpoS protein fusion, and used bulk methods to show that the RpoS feedback loop is effectively not operating during exponential- phase growth. Mathematical analyses and initial experiments in a microfluidic device further suggest that the RpoS system has several unusual properties contributing towards extremely fast stress response. A stochastic analysis further suggests that the RpoS feedback loop cannot suppress spontaneous fluctuations, and preliminary experiments indicate that large deviations might indeed play important roles.
author2 Paulsson, Johan Martin
author_facet Paulsson, Johan Martin
Landgraf, Dirk
author Landgraf, Dirk
author_sort Landgraf, Dirk
title Quantifying Localizations and Dynamics in Single Bacterial Cells
title_short Quantifying Localizations and Dynamics in Single Bacterial Cells
title_full Quantifying Localizations and Dynamics in Single Bacterial Cells
title_fullStr Quantifying Localizations and Dynamics in Single Bacterial Cells
title_full_unstemmed Quantifying Localizations and Dynamics in Single Bacterial Cells
title_sort quantifying localizations and dynamics in single bacterial cells
publisher Harvard University
publishDate 2012
url http://dissertations.umi.com/gsas.harvard:10612
http://nrs.harvard.edu/urn-3:HUL.InstRepos:9920184
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