Resolving Cytosolic Diffusive States in Bacteria by Single-Molecule Tracking

Rocha, Julian; Corbitt, Jacqueline; Yan, Ting; Richardson, Charles J.; Gahlmann, Andreas

doi:10.1016/j.bpj.2019.03.039

Cited by 13 publications

(30 citation statements)

References 62 publications

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“…Thus, a single-state, confined (within the bacterial cell) Brownian diffusion model accurately describes the measured 3D motion trajectories of eYFP in living Y. enterocolitica cells. These results are consistent with previous work by our laboratory 22 and others 25 and confirm that eYFP has negligible (non)specific interactions with cellular contents or with itself and is thus a suitable probe for measuring the diffusion coefficients for eYFP-labeled proteins.…”

Section: Yesctq Shows Three Prominent Diffusive States In Living Cellssupporting

confidence: 92%

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Distinct cytosolic complexes containing the type III secretion system ATPase resolved by 3D single-molecule tracking in liveYersinia enterocolitica

Prindle

Rocha

Wang

et al. 2022

Preprint

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The membrane-embedded injectisome, the structural component of the virulence-associated type III secretion system (T3SS), is used by gram-negative bacterial pathogens to inject species-specific effector proteins into eukaryotic host cells. The cytosolic injectisome proteins are required for export of effectors and display both stationary, injectisome-bound populations as well as freely-diffusing cytosolic populations. How the cytosolic injectisome proteins interact with each other in the cytosol and associate with membrane-embedded injectisomes remains unclear. Here, we utilize 3D single-molecule tracking to resolve distinct cytosolic complexes of injectisome proteins in living Yersinia enterocolitica cells. Tracking of the eYFP-labeled ATPase, YeSctN, and its regulator, YeSctL, reveals that these proteins form a cytosolic complex with each other and then further with YeSctQ. YeSctNL and YeSctNLQ complexes can be observed in both in wild type cells and in ΔsctD mutants, which cannot assemble injectisomes. In ΔsctQ mutants, the relative abundance of the YeSctNL complex is considerably increased. These data indicate that distinct cytosolic complexes of injectisome proteins can form prior to injectisome binding - a feature that could contribute to injectisome functional regulation.

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Section: Yesctq Shows Three Prominent Diffusive States In Living Cellssupporting

confidence: 92%

“…We have previously reported the diffusive behaviors of free eYFP and eYFP-labeled Ye SctQ in Y. enterocolitica 19,22 . Here, we re-analyzed these data using a more complete library of apparent diffusion coefficient distributions (see Methods).…”

Section: Resultsmentioning

confidence: 99%

Distinct cytosolic complexes containing the type III secretion system ATPase resolved by 3D single-molecule tracking in liveYersinia enterocolitica

Prindle

Rocha

Wang

et al. 2022

Preprint

Self Cite

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“…3B). Under copper-depleted conditions, the fastest diffusion state has a diffusion constant D FD of 7.9 ± 0.6 μm 2 •s −1 , which we assigned as CusR mE freely diffusing (FD) in the cytoplasm (either as monomers or dimers), as these species are expected to exist and D FD is consistent with those for freely diffusing proteins in the bacterial cytoplasm (34,43,44). The slowest state has a diffusion constant D TB of 0.02 ± 0.01 μm 2 •s −1 , which we assigned as CusR mE tightly bound (TB) to the chromosome because CusR, when phosphorylated (i.e., activated), can bind tightly at cognate sites; D TB is also consistent with those for proteins that bind chromosome specifically (31,34,45,46), and its small magnitude mainly reflects chromosomal dynamics and experimental uncertainties in molecular localization.…”

Section: Copper Stress Leads To Cuss Concentration Increase and Mobilmentioning

confidence: 74%

Metal-induced sensor mobilization turns on affinity to activate regulator for metal detoxification in live bacteria

Sengupta

Genova

et al. 2020

Proc. Natl. Acad. Sci. U.S.A.

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Metal detoxification is essential for bacteria’s survival in adverse environments and their pathogenesis in hosts. Understanding the underlying mechanisms is crucial for devising antibacterial treatments. In the Gram-negative bacteriumEscherichia coli, membrane-bound sensor CusS and its response regulator CusR together regulate the transcription of thecusoperon that plays important roles in cells’ resistance to copper/silver, and they belong to the two-component systems (TCSs) that are ubiquitous across various organisms and regulate diverse cellular functions. In vitro protein reconstitution and associated biochemical/physical studies have provided significant insights into the functions and mechanisms of CusS–CusR and related TCSs. Such studies are challenging regarding multidomain membrane proteins like CusS and also lack the physiological environment, particularly the native spatial context of proteins inside a cell. Here, we use stroboscopic single-molecule imaging and tracking to probe the dynamic behaviors of both CusS and CusR in live cells, in combination with protein- or residue-specific genetic manipulations. We find that copper stress leads to a cellular protein concentration increase and a concurrent mobilization of CusS out of clustered states in the membrane. We show that the mobilized CusS has significant interactions with CusR for signal transduction and that CusS’s affinity toward CusR switches on upon sensing copper at the interfacial metal-binding sites in CusS’s periplasmic sensor domains, prior to ATP binding and autophosphorylation at CusS’s cytoplasmic kinase domain(s). The observed CusS mobilization upon stimulation and its surprisingly early interaction with CusR likely ensure an efficient signal transduction by providing proper conformation and avoiding futile cross talks.

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“…Compared to other simulation-based frameworks for estimating transition rates [48][49][50] , anaDDA holds several advantages. First, the distributions of simulations are not exact as they are generated from a limited number of particles and therefore do not allow for using an MLE approach, which requires convergence based on exact probability even for small changes in the parameter space.…”

Section: Discussionmentioning

confidence: 99%

“…Using the estimated error for each individual localization can further improve the robustness of the analysis as has been demonstrated previously 53 . Another improvement which can be incorporated in our framework and has already been developed is to take the effect of particles moving out-of-focus, and the recovery of localizations depending on diffusion coefficients into account 38,50 .…”

Section: Discussionmentioning

confidence: 99%

Extracting transition rates in single-particle tracking using analytical diffusion distribution analysis

Vink

Brouns

Hohlbein

2020

Preprint

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Single-particle tracking is an important technique in the life sciences to understand the kinetics of biomolecules. Observed diffusion coefficients in vivo, for example, enable researchers to determine whether biomolecules are moving alone, as part of a larger complex or are bound to large cellular components such as the membrane or chromosomal DNA. A remaining challenge has been to retrieve quantitative kinetic models especially for molecules that rapidly interchange between different diffusional states. Here, we present analytic diffusion distribution analysis (anaDDA), a framework that allows extracting transition rates from distributions of observed diffusion coefficients. We show that theoretically predicted distributions accurately match simulated distributions and that anaDDA outperforms existing methods to retrieve kinetics especially in the fast regime of 0.1-10 transitions per imaging frame. AnaDDA does account for the effects of confinement and tracking window boundaries. Furthermore, we added the option to perform global fitting of data acquired at different frame times, to allow complex models with multiple states to be fitted confidently. Previously, we have started to develop anaDDA to investigate the target search of CRISPR-Cas complexes. In this work, we have optimized the algorithms and reanalysed experimental data of DNA polymerase I diffusing in live E. coli. We found that long-lived DNA interaction by DNA polymerase are more abundant upon DNA damage, suggesting roles in DNA repair. We further revealed and quantified fast DNA probing interactions that last shorter than 10 ms. AnaDDA pushes the boundaries of the timescale of interactions that can be probed with single-particle tracking and is a mathematically rigorous framework that can be further expanded to extract detailed information about the behaviour of biomolecules in living cells. the apparent diffusion coefficient D* is calculated from the mean squared displacement (MSD).The different mobilities of proteins switching between a DNA-bound state, in which proteins diffuse very slowly, and a DNA-free state, in which proteins diffuse through the cytoplasm, can provide kinetic information on the frequency and longevity of DNA-protein interactions.The ability to extract this information, however, is compromised by photo bleaching, which limits the length of each track to a few localisations in the case of fluorescent proteins 19 . Furthermore, the limited localization precision increases the apparent diffusion of immobile states. Therefore, measured displacements cannot be unambiguously assigned to either a bound or a diffusing state.As a consequence, histograms of D* values are often rather broad making a clear distinction between two diffusional states of a single species impossible. For the special case of noninterconverting D* distributions, the shape of distributions can be calculated for a fixed number of analysed steps 20,21 and, via fitting of the experimental data, used to extract the fractions of mobile and immobile proteins.Anothe...

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Resolving Cytosolic Diffusive States in Bacteria by Single-Molecule Tracking

Cited by 13 publications

References 62 publications

Distinct cytosolic complexes containing the type III secretion system ATPase resolved by 3D single-molecule tracking in liveYersinia enterocolitica

Distinct cytosolic complexes containing the type III secretion system ATPase resolved by 3D single-molecule tracking in liveYersinia enterocolitica

Metal-induced sensor mobilization turns on affinity to activate regulator for metal detoxification in live bacteria

Extracting transition rates in single-particle tracking using analytical diffusion distribution analysis

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