Size Dependence of Protein Diffusion in the Cytoplasm of
            <i>Escherichia coli</i>

Nenninger, Anja; Mastroianni, Giulia; Mullineaux, Conrad W.

doi:10.1128/jb.00284-10

Cited by 121 publications

(148 citation statements)

References 32 publications

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“…For these reasons, we speak of RNAP diffusion and the RNAP spatial distribution even though we are actually measuring the fluorescence from ␤Ј-EGFP. In addition, because we are tagging the large RNAP by a single copy of the small EGFP, we expect the dynamics measured to be indicative of the true RNAP dynamics (24).…”

Section: Discussionmentioning

confidence: 99%

Spatial Distribution and Diffusive Motion of RNA Polymerase in Live Escherichia coli

2011

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By labeling the ␤ subunit of RNA polymerase (RNAP), we used fluorescence microscopy to study the spatial distribution and diffusive motion of RNAP in live Escherichia coli cells for the first time. With a 40-ms time resolution, the spatial distribution exhibits two or three narrow peaks of 300-to 600-nm full width at half-maximum that maintain their positions within 60 nm over 1 s. The intensity in these features is 20 to 30% of the total. Fluorescence recovery after photobleaching (FRAP) measures the diffusive motion of RNAP on the 1-m length scale. Averaged over many cells, 53% ؎ 19% of the RNAP molecules were mobile on the 3-s timescale, with a mean apparent diffusion constant ͳD RNAP ʹ of 0.22 ؎ 0.16 m 2 -s ؊1 . The remaining 47% were immobile even on the 30-s timescale. We interpret the immobile fraction as arising from RNAP specifically bound to DNA, either actively transcribing or not. The diffusive motion of the mobile fraction (f mobile ) probably involves both one-dimensional sliding during nonspecific binding to DNA and three-dimensional hopping between DNA strands. There is significant cell-to-cell heterogeneity in both D RNAP and f mobile .In prokaryotes such as Escherichia coli, several thousand copies of a single RNA polymerase (RNAP) are responsible for all transcription. Previous work has used fluorescence microscopy to study the spatial distribution of green fluorescent protein (GFP)-labeled RNAP in both E. coli (4) and Bacillus subtilis (15) cells that were chemically fixed following growth in rich medium. In both species, narrow regions of high local GFP-RNAP concentration are observed atop a broader background concentration. Such "RNAP foci" are thought to be transcription foci, i.e., localized regions of intensive transcription, including rRNA. Accordingly, the narrow features were not observed for growth in minimal medium or following treatments designed to mimic nutrient starvation (4). The underlying cause of such spatial organization in prokaryotes is not clear (17). Quantifying the number, intensity, and spatial extent of RNAP foci in live cells is difficult due to the small size of the E. coli nucleoid, the presence of a background RNAP distribution, the dependence of the features on growth conditions, and the dynamic nature of the spatial distributions.Here we present a detailed quantitative study of the spatial distribution and movement of RNAP in live bacterial cells, specifically a K-12 strain of E. coli. The spatially narrow, immobile RNAP features that we observe appear qualitatively similar to the foci in fixed cells reported earlier. To capture the underlying dynamics, we imaged RNAP with a 40-ms time resolution for 0.8-s intervals. Each cell exhibits two or three narrow RNAP foci with a full width at half-maximum intensity (FWHM) of about 500 nm, significantly broader than the diffraction limit. These narrow features account for 20 to 30% of the total intensity and maintain their positions to within 60 nm over 1 s, during which time the broader background RNAP distribution fl...

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Section: Discussionmentioning

confidence: 99%

Spatial Distribution and Diffusive Motion of RNA Polymerase in Live Escherichia coli

2011

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“…[1] With the growing awareness of this deficiency there is a drive towards studying proteins under physiologically relevant conditions, [3][4][5][6][7][8] including the application of spectroscopic techniques to proteins inside cells. [9][10][11] In-cell NMR spectroscopy provides the means to monitor protein conformation and dynamics at atomic resolution inside living cells. [11-24] 15 N-labelled "biologically inert" proteins overexpressed in the host E. coli, yield in-cell spectra closely similar to the spectrum of the purified protein.…”

Section: Introductionmentioning

confidence: 99%

Protein Interactions in the Escherichia coli Cytosol: An Impediment to In‐Cell NMR Spectroscopy

2011

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Protein science is shifting towards experiments performed under native or native-like conditions. In-cell NMR spectroscopy for instance has the potential to reveal protein structure and dynamics inside cells. However, not all proteins can be studied by this technique. (15)N-labelled cytochrome c (cyt c) over-expressed in Escherichia coli was undetectable by in-cell NMR spectroscopy. When whole-cell lysates were subjected to size-exclusion chromatography (SEC) cyt c was found to elute with an apparent molecular weight of >150 kDa. The presence of high molecular weight species is indicative of complex formation between cyt c and E. coli cytosolic proteins. These interactions were disrupted by charge-inverted mutants in cyt c and by elevated concentrations of NaCl. The physiologically relevant salt, KGlu, was less efficient at disrupting complex formation. Notably, a triple mutant of cyt c could be detected in cell lysates by NMR spectroscopy. The protein, GB1, yields high quality in-cell spectra and SEC analysis of lysates containing GB1 revealed a lack of interaction between GB1 and E. coli proteins. Together these data suggest that protein "stickiness" is a limiting factor in the application of in-cell NMR spectroscopy.

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“…They collected literature data [12,13,[65][66][67][68][69][70][71][72][73][74][75][76][77] of diffusion coefficients in the cytoplasm of E. coli and used Equation 5 to fit the data. From this fit they determined ξ of around 0.5 nm and R h ≈ 42 nm [15].…”

Section: Motion In the Cytoplasm Of Prokaryotesmentioning

confidence: 99%

The effect of macromolecular crowding on mobility of biomolecules, association kinetics, and gene expression in living cells

et al. 2014

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We discuss a quantitative influence of macromolecular crowding on biological processes: motion, bimolecular reactions, and gene expression in prokaryotic and eukaryotic cells. We present scaling laws relating diffusion coefficient of an object moving in a cytoplasm of cells to a size of this object and degree of crowding. Such description leads to the notion of the length scale dependent viscosity characteristic for all living cells. We present an application of the length-scale dependent viscosity model to the description of motion in the cytoplasm of both eukaryotic and prokaryotic living cells. We compare the model with all recent data on diffusion of nanoscopic objects in HeLa, and E. coli cells. Additionally a description of the mobility of molecules in cell nucleus is presented. Finally we discuss the influence of crowding on the bimolecular association rates and gene expression in living cells.

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Size Dependence of Protein Diffusion in the Cytoplasm of Escherichia coli

Cited by 121 publications

References 32 publications

Spatial Distribution and Diffusive Motion of RNA Polymerase in Live Escherichia coli

Spatial Distribution and Diffusive Motion of RNA Polymerase in Live Escherichia coli

Protein Interactions in the Escherichia coli Cytosol: An Impediment to In‐Cell NMR Spectroscopy

The effect of macromolecular crowding on mobility of biomolecules, association kinetics, and gene expression in living cells

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