Topic
Intercellular connection
About: Intercellular connection is a research topic. Over the lifetime, 98 publications have been published within this topic receiving 2187 citations.
Papers published on a yearly basis
Papers
TL;DR: Plasmodesmata are now thought of as fluid, dynamic structures that can be modified both structurally and functionally to cope with the requirements of specific cells and tissues.
Abstract: In 1879 Eduard Tangle discovered cytoplasmic connections between cells in the cotyledons of Strychnos nuxvomica , which he interpreted to be protoplasmic contacts. This led him to hypothesize that ‘the protoplasmic bodies . . . are united by thin strands passing through connecting ducts in the walls, which put the cells into connection with each other and so unite them to an entity of higher order’ (Carr 1976). This challenged the then current view that cells functioned as autonomous units. It was after much research in many other species and cell types that Strasburger, in 1901, named these structures plasmodesmata (Carr 1976). During the division and differentiation of meristematic cells, plasmodesmata are formed across each developing cell plate, allowing cytoplasmic and endomembrane continuity to occur between all daughter cells, and ultimately, between all cells in a developing tissue (Mezitt & Lucas 1996). Those plasmodesmata that form during cell division are termed primary plasmodesmata (Jones 1976). Those that form de novo across existing cell walls are called secondary plasmodesmata (Ehlers & Kollmann 2001). The formation of secondary plasmodesmata allows cells to increase their potential for molecular trafficking and allows connections to be created between cells that are not related cytokinetically. As cells expand and differentiate, their fate determines the extent to which their cytoplasmic connectivity to other cells is maintained (Mezitt & Lucas 1996). Some cell types, such as those of the leaf mesophyll, remain closely connected to their neighbours, and may even lay down additional plasmodesmata to increase the continuity (Ding et al . 1992a). In other areas of the plant, for instance in vascular tissue, certain cells greatly reduce the number of plasmodesmata in their adjoining walls (Gamalei 1989). In this way, the cytoplasmic continuity can be altered depending on the tissue type (Botha & Evert 1988; Brown et al . 1995). However, although reductions in the number of plasmodesmata are common, only guard cells surrounding stomata (Erwee, Goodwin & van Bel 1985; Palevitz & Hepler 1985) and differentiating xylem elements (Lachaud & Maurousset 1996) lose all symplastic connections at maturity. In all other cells, some degree of intercellular connection is maintained. This plasmodesmal continuum that potentially exists throughout the whole plant is termed the symplast (Munch 1930). However, the symplast is not the open continuum that Munch originally hypothesized, but is divided into functional domains, each tightly regulated by different forms of plasmodesmata (Erwee & Goodwin 1985; Ehlers & Kollmann 2001). Plasmodesmata are now thought of as fluid, dynamic structures that can be modified both structurally and functionally to cope with the requirements of specific cells and tissues.
399 citations
TL;DR: This Review recounts how perception of the slit diaphragm has changed over time as a result of intense research, from its first anatomical description as a thin intercellular connection, to an appreciation of its role as a dynamic signalling hub.
Abstract: The architectural design of our kidneys is amazingly complex, and culminates in the 3D structure of the glomerular filter. During filtration, plasma passes through a sieve consisting of a fenestrated endothelium and a broad basement membrane before it reaches the most unique part, the slit diaphragm, a specialized type of intercellular junction that connects neighbouring podocyte foot processes. When podocytes become stressed, irrespective of the causative stimulus, they undergo foot process effacement and loss of slit diaphragms--two key steps leading to proteinuria. Thus, proteinuria is the unifying denominator of a broad spectrum of podocytopathies. With the rising prevalence of chronic kidney disease and the fact that glomerular diseases account for the majority of patients with end-stage renal disease, further investigation and elucidation of this unique structure is of paramount importance. This Review recounts how perception of the slit diaphragm has changed over time as a result of intense research, from its first anatomical description as a thin intercellular connection, to an appreciation of its role as a dynamic signalling hub. These observations led to the introduction of novel concepts in podocyte biology, which could pave the way to development of highly desired, specific therapeutic strategies for glomerular diseases.
253 citations
TL;DR: A new type of intercellular connection, the tunneling nanotube (TNT), is observed in many cell types in vitro and recently also in developing embryos of different species in vivo, with a particular focus on the TNT-dependent electrical coupling between developing embryonic cells.
210 citations
TL;DR: A new method by which influenza A virus (IAV) spreads from cell to cell: IAV uses intracellular connections, which requires actin dynamics and is enhanced by viral infection and the absence of microtubules.
Abstract: In the extracellular environment, cell-free virions seek out naive host cells over long distances and between organisms. This is the primary mechanism of spread for most viruses. Here we provide evidence for an alternative pathway previously undescribed for orthomyxoviruses, whereby the spread of influenza A virus (IAV) infectious cores to neighboring cells can occur within intercellular connections. The formation of these connections requires actin dynamics and is enhanced by viral infection. Connected cells have contiguous membranes, and the core infectious viral machinery (RNP and polymerase) was present inside the intercellular connections. A live-cell movie of green fluorescent protein (GFP)-tagged NS1 of IAV shows viral protein moving from one cell to another through an intercellular connection. The movement of tagged protein was saltatory but overall traveled only in one direction. Infectious virus cores can move from one cell to another without budding and release of cell-free virions, as evidenced by the finding that whereas a neuraminidase inhibitor alone did not inhibit the development of IAV microplaques, the presence of a neuraminidase inhibitor together with drugs inhibiting actin dynamics or the microtubule stabilizer paclitaxel (originally named taxol) precluded microplaque formation. Similar results were also observed with parainfluenza virus 5 (PIV5), a paramyxovirus, when neutralizing antibody was used to block spread by cell-free virions. Intercellular spread of infectious core particles was unaffected or enhanced in the presence of nocodazole for IAV but inhibited for PIV5. The intercellular connections have a core of filamentous actin, which hints toward transport of virus particles through the use of a myosin motor.
IMPORTANCE Here we describe a new method by which influenza A virus (IAV) spreads from cell to cell: IAV uses intracellular connections. The formation of these connections requires actin dynamics and is enhanced by viral infection and the absence of microtubules. Connected cells appeared to have contiguous membranes, and the core infectious viral machinery (RNP and polymerase) was present inside the intercellular connections. Infectious virus cores can move from one cell to another without budding and release of cell-free virions. Similar results were also observed with parainfluenza virus 5 (PIV5).
130 citations
TL;DR: A new scalable method using Faraday waves to enable rapid aggregation of human induced pluripotent stem cell-derived cardiomyocytes into predefined 3D constructs that resembles the cellular architecture of a native heart tissue for diverse basic research and clinical applications is reported.
116 citations
Related Topics (5)
Performance Metrics
| Year | Papers |
|---|---|
| 2022 | 1 |
| 2021 | 4 |
| 2020 | 4 |
| 2019 | 2 |
| 2018 | 6 |
| 2017 | 5 |