Background: In (␣42) 2 ␣4 nicotinic acetylcholine receptors, there is an agonist binding site at the ␣4/␣4 subunit interface. Results: ␣2, ␣3, and ␣6 accessory subunits can form an agonist site with ␣4. These promote activation upon agonist binding at ␣4/2 agonist sites. Conclusion: Accessory subunit agonist sites greatly influence receptor function. Significance: These sites are promising drug targets.
The highly infectious bacteria, Francisella tularensis, colonize a variety of organs and replicate within both phagocytic as well as non-phagocytic cells, to cause the disease tularemia. These microbes contain a conserved cluster of important virulence genes referred to as the Francisella Pathogenicity Island (FPI). Two of the most characterized FPI genes, iglC and pdpA, play a central role in bacterial survival and proliferation within phagocytes, but do not influence bacterial internalization. Yet, their involvement in non-phagocytic epithelial cell infections remains unexplored. To examine the functions of IglC and PdpA on bacterial invasion and replication during epithelial cell infections, we infected liver and lung epithelial cells with F. novicida and F. tularensis ‘Type B’ Live Vaccine Strain (LVS) deletion mutants (ΔiglC and ΔpdpA) as well as their respective gene complements. We found that deletion of either gene significantly reduced their ability to invade and replicate in epithelial cells. Gene complementation of iglC and pdpA partially rescued bacterial invasion and intracellular growth. Additionally, substantial LAMP1-association with both deletion mutants was observed up to 12 h suggesting that the absence of IglC and PdpA caused deficiencies in their ability to dissociate from LAMP1-positive Francisella Containing Vacuoles (FCVs). This work provides the first evidence that IglC and PdpA are important pathogenic factors for invasion and intracellular growth of Francisella in epithelial cells, and further highlights the discrete mechanisms involved in Francisella infections between phagocytic and non-phagocytic cells.
Sertoli cells of the mammalian seminiferous epithelium form unique subcellular actin‐related structures at intercellular junctions. The appearance of these so called “tubulobulbar complexes” (TBCs) precedes both sperm release at the apex of the epithelium and the movement of early spermatogenic cells out of the spermatogonial stem cell niche at the base of the epithelium. TBCs are considered to be part of the mechanism of junction endocytosis by Sertoli cells. The structures contain junction proteins and morphologically identifiable junctions, and are associated with markers of endocytosis. Here we review the current state of knowledge about the structure and function of TBCs. As the complexes form, they morphologically resemble and have the molecular signature of clathrin‐coated pits with extremely long necks. As they mature, the actin filament networks around the “necks” of the structures progressively disassemble and the membrane cores expand or swell into distinct “bulbs”. These bulbs acquire extensive membrane contact sites with associated cisternae of endoplasmic reticulum. Eventually the bulbs undergo scission and continue through endosomal compartments of the Sertoli cells. The morphology and composition of TBC indicates to us that the structures likely evolved from the basic clathrin‐mediated endocytosis mechanism common to cells generally, and along the way they incorporated unique features to accommodate the cyclic turnover of massive and “intact” intercellular junctions that occurs during spermatogenesis. Anat Rec, 301:2080–2085, 2018. © 2018 Wiley Periodicals, Inc.
Basal tubulobulbar complexes (TBCs) that occur at attachment sites between neighboring Sertoli cells are subcellular machines that internalize intercellular junctions during movement of spermatocytes from basal to adluminal compartments of the seminiferous epithelium. Each complex consists of an elongate tubular extension of two attached plasma membranes, and is capped at its distal end by a clathrin-coated pit. The tubular region is surrounded by a cuff of actin arranged in a dendritic network. Near the end of the complex, a bulbous region forms that lacks the actin cuff but is closely associated with cisternae of endoplasmic reticulum. The bulb eventually buds from the complex and enters endocytic compartments of the Sertoli cell. Previous research has shown that when the actin network is perturbed using the actin filament-disruptor, cytochalasin D, apical tubulobulbar complexes that are associated with spermatids were associated with lower levels of actin, patchy actin networks and swollen tubular regions. Here we explored the effects of actin network perturbation on the morphology of basal tubulobulbar complexes in stage V seminiferous tubules. Isolated rat testes were perfused ex vivo for one hour with oxygenated Krebs-Henseleit buffer (with BSA) containing either 40 μM cytochalasin D or control solution containing DMSO and perfusion-fixed for electron microscopy. Compared to control, actin cuffs in drug-treated TBCs appeared less uniform and patchy. In addition, the tubular regions of the complexes appeared swollen. Our results are consistent with the conclusion that intact networks of actin filaments are required for maintaining the structural integrity of basal TBCs. Anat Rec, 299:1449-1455, 2016. © 2016 Wiley Periodicals, Inc.
Francisella tularensis is a bacterium that can cause up to 60% mortality in humans. These microbes carry a cluster of conserved genes present in all F. tularensis subspecies called the Francisella pathogenicity island (FPI). Within the FPI, iglB, iglC, pdpA and vgrG genes are important for intracellular macrophage survival and virulence; yet, their role in epithelial cell infections, a major contributor to the progression of disease, is unclear. Given that F. tularensis uses dissimilar mechanisms to enter different cell types, we hypothesized that FPI genes play a crucial role in bacterial entry into epithelial cells. To test this hypothesis, BNL CL.2 hepatocytes were infected with F. novicida for up to 48 h. Detailed microscopic examination and gentamicin protection assay revealed that ΔiglB, ΔiglC, ΔvgrG, ΔpdpA Francisella mutants were invasion and replication deficient. We showed that gene complementation restored intracellular growth. Our data suggest that IglB, IglC, PdpA and VgrG are important for hepatocyte infections, as they are vital for efficient invasion and intracellular proliferation.Grant Funding Source: NSERC, CIHR
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