Indirect visualization of endogenous nuclear actin by correlative light and electron microscopy (CLEM) using an actin-directed chromobody

Abdellatif, Mohamed E. A.; Hipp, Lisa; Plessner, Matthias; Walther, Paul; Knöll, Bernd

doi:10.1007/s00418-019-01795-3

Cited by 7 publications

(6 citation statements)

References 48 publications

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“…Blocking was done with 0.5% BSA containing PBS for 5 min, followed by incubation with biotinylated-phalloidin for 1 h at RT. Next, the grids were washed with blocking buffer 6 times with 2 min for each wash, followed by incubation with streptavidin colloidal gold conjugate for 40 min at RT ( 18 ). The grids were rewashed 4 times with 2 min for each wash using blocking buffer.…”

Section: Methodsmentioning

confidence: 99%

A Bumpy Ride of Mycobacterial Phagosome Maturation: Roleplay of Coronin1 Through Cofilin1 and cAMP

et al. 2021

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Phagosome-lysosome fusion in innate immune cells like macrophages and neutrophils marshal an essential role in eliminating intracellular microorganisms. In microbe-challenged macrophages, phagosome-lysosome fusion occurs 4 to 6 h after the phagocytic uptake of the microbe. However, live pathogenic mycobacteria hinder the transfer of phagosomes to lysosomes, up to 20 h post-phagocytic uptake. This period is required to evade pro-inflammatory response and upregulate the acid-stress tolerant proteins. The exact sequence of events through which mycobacteria retards phagolysosome formation remains an enigma. The macrophage coat protein Coronin1(Cor1) is recruited and retained by mycobacteria on the phagosome membrane to retard its maturation by hindering the access of phagosome maturation factors. Mycobacteria-infected macrophages exhibit an increased cAMP level, and based on receptor stimulus, Cor1 expressing cells show a higher level of cAMP than non-Cor1 expressing cells. Here we have shown that infection of bone marrow-derived macrophages with H37Rv causes a Cor1 dependent rise of intracellular cAMP levels at the vicinity of the phagosomes. This increased cAMP fuels cytoskeletal protein Cofilin1 to depolymerize F-actin around the mycobacteria-containing phagosome. Owing to reduced F-actin levels, the movement of the phagosome toward the lysosomes is hindered, thus contributing to the retarded phagosome maturation process. Additionally, Cor1 mediated upregulation of Cofilin1 also contributes to the prevention of phagosomal acidification, which further aids in the retardation of phagosome maturation. Overall, our study provides first-hand information on Cor1 mediated retardation of phagosome maturation, which can be utilized in developing novel peptidomimetics as part of host-directed therapeutics against tuberculosis.

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Section: Methodsmentioning

confidence: 99%

A Bumpy Ride of Mycobacterial Phagosome Maturation: Roleplay of Coronin1 Through Cofilin1 and cAMP

et al. 2021

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“…Since nanobodies consist of only one protein chain, they can also be fused to fluorescent proteins and expressed in cells, allowing live cell imaging. A commercially available Actin-Chromobody ® (Chromotek, Germany) have been used to track actin dynamics in plants, zebrafish, and nuclei of mammalian cells (Rocchetti et al, 2014; Panza et al, 2015; Plessner et al, 2015) as well as for super resolution live imaging of actin in neurons (Wegner et al, 2017) and for correlative light electron microscopy, where chromobodies were labeled with anti-GFP and gold-conjugated secondary antibodies (Abdellatif et al, 2019). A stable cell line expressing Actin-Chromobody has been generated, allowing tracking actin dynamics without the need of transfections (Keller et al, 2019).…”

Section: Methodsmentioning

confidence: 99%

Interrogating Synaptic Architecture: Approaches for Labeling Organelles and Cytoskeleton Components

Reshetniak

Rizzoli

2019

Front. Synaptic Neurosci.

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Synaptic transmission has been studied for decades, as a fundamental step in brain function. The structure of the synapse, and its changes during activity, turned out to be key aspects not only in the transfer of information between neurons, but also in cognitive processes such as learning and memory. The overall synaptic morphology has traditionally been studied by electron microscopy, which enables the visualization of synaptic structure in great detail. The changes in the organization of easily identified structures, such as the presynaptic active zone, or the postsynaptic density, are optimally studied via electron microscopy. However, few reliable methods are available for labeling individual organelles or protein complexes in electron microscopy. For such targets one typically relies either on combination of electron and fluorescence microscopy, or on super-resolution fluorescence microscopy. This review focuses on approaches and techniques used to specifically reveal synaptic organelles and protein complexes, such as cytoskeletal assemblies. We place the strongest emphasis on methods detecting the targets of interest by affinity binding, and we discuss the advantages and limitations of each method.

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“…Interactions between endogenous proteins and ectopically expressed chromobodies can potentially influence the localization and function of the protein of interest. Binding of nanobodies to their target during Rocchetti et al, 2014;Panza et al, 2015;Plessner et al, 2015;Moutel et al, 2016;Periz et al, 2017;Wegner et al, 2017;Abdellatif et al, 2019;Tosetti et al, 2019 Active Rothbauer et al, 2006Rothbauer et al, , 2008Bazl et al, 2007;Schornack et al, 2009;Kirchhofer et al, 2010;Caussinus et al, 2011;Casas-Delucchi et al, 2012;Han et al, 2012;Li et al, 2012;Pellis et al, 2012;Ries et al, 2012;Herce et al, 2013Herce et al, , 2017Szymborska et al, 2013;Truan et al, 2013;Bleck et al, 2014;Wang et al, 2014;Ariotti et al, 2015Ariotti et al, , 2017Ariotti et al, , 2018Finnigan et al, 2015;Harmansa et al, 2015Harmansa et al, , 2017Kamiyama et al, 2015;Kaplan and Ewers, 2015;Katoh et al, 2015;Klamecka et al, 2015;Nieuwenhuizen et al, 2015;Platonova et al, 2015a,b;Roebroek et al, 2015;Shin et al, 2015;Wedeking et al, 2015;…”

Section: Delocalization Of Targeted Proteinsmentioning

confidence: 99%

Nanobody-Based Probes for Subcellular Protein Identification and Visualization

Beer

Giepmans

2020

Front. Cell. Neurosci.

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Understanding how building blocks of life contribute to physiology is greatly aided by protein identification and cellular localization. The two main labeling approaches developed over the past decades are labeling with antibodies such as immunoglobulin G (IgGs) or use of genetically encoded tags such as fluorescent proteins. However, IgGs are large proteins (150 kDa), which limits penetration depth and uncertainty of target position caused by up to ∼25 nm distance of the label created by the chosen targeting approach. Additionally, IgGs cannot be easily recombinantly modulated and engineered as part of fusion proteins because they consist of multiple independent translated chains. In the last decade single domain antigen binding proteins are being explored in bioscience as a tool in revealing molecular identity and localization to overcome limitations by IgGs. These nanobodies have several potential benefits over routine applications. Because of their small size (15 kDa), nanobodies better penetrate during labeling procedures and improve resolution. Moreover, nanobodies cDNA can easily be fused with other cDNA. Multidomain proteins can thus be easily engineered consisting of domains for targeting (nanobodies) and visualization by fluorescence microscopy (fluorescent proteins) or electron microscopy (based on certain enzymes). Additional modules for e.g., purification are also easily added. These nanobody-based probes can be applied in cells for live-cell endogenous protein detection or may be purified prior to use on molecules, cells or tissues. Here, we present the current state of nanobodybased probes and their implementation in microscopy, including pitfalls and potential future opportunities.

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Indirect visualization of endogenous nuclear actin by correlative light and electron microscopy (CLEM) using an actin-directed chromobody

Cited by 7 publications

References 48 publications

A Bumpy Ride of Mycobacterial Phagosome Maturation: Roleplay of Coronin1 Through Cofilin1 and cAMP

A Bumpy Ride of Mycobacterial Phagosome Maturation: Roleplay of Coronin1 Through Cofilin1 and cAMP

Interrogating Synaptic Architecture: Approaches for Labeling Organelles and Cytoskeleton Components

Nanobody-Based Probes for Subcellular Protein Identification and Visualization

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