Autophagy, tissue repair, and fibrosis: a delicate balance

Tissue repair and fibrosis, an abnormal form of repair, occur in most human organs in response to injury or inflammation. Fibroblasts play a major role in the normal repair process by differentiating into myofibroblasts that synthesize extracellular matrix (ECM) components and favor tissue remodeling to reestablish normal function and integrity. However, their persistent accumulation at the site of injury is a hallmark of fibrosis. Autophagy is a catabolic process that occurs in eukaryotic cells as a stress response to allow cell survival and maintenance of cellular homeostasis by degrading and recycling intracellular components. Recent advances identify autophagy as an important regulator of myofibroblast differentiation, tissue remodeling, and fibrogenesis. In this mini-review, we provide an overview of the interactions between autophagy, ECM, and fibrosis, and emphasize the molecular mechanisms involved in myofibroblast differentiation. We also describe the emerging concept of secretory autophagy as a new avenue for intercellular communication at the site of tissue injury and repair

Modulation de la stabilité de l'ARNm alphaENaC dans les cellules épithéliales alvéolaires : détermination du rôle des séquences 3' non traduites

Le transport actif de sodium par les cellules épithéliales alvéolaires est le principal mécanisme impliqué dans la régulation du niveau de liquide dans le poumon distal. Le canal épithélial sodique (ENaC) exprimé par les cellules épithéliales alvéolaires est essentiel à la résorption du liquide des poumons à la naissance ainsi que la résolution de l'œdème pulmonaire chez l'adulte. L'activité et l'expression du canal ENaC sont modulées par de nombreux stress pathophysiologiques. L'inflammation pulmonaire constitue un facteur important dans l'inhibition de l'expression du canal ENaC et pourrait favoriser la formation d'œdème pulmonaire. Nous avons précédemment démontré que différentes cytokines pro-inflammatoires, ainsi que les lipopolysaccharides (LPS) de Pseudomonas aeruginosa, inhibent l'expression de l'ARNm αENaC par des mécanismes de régulation transcriptionnelle et post-transcriptionnelle. Ces résultats suggèrent que les mécanismes qui modulent la stabilité des ARNm αENaC pourraient jouer un rôle important dans la régulation du niveau d’expression du transcrit en condition inflammatoire. Le principal objectif de mes travaux était de caractériser les mécanismes de modulation de l’ARNm αENaC dans les cellules épithéliales alvéolaires lors de différents stress pathophysiologiques et déterminer si cette modulation pouvait s’expliquer en partie par une régulation de la stabilité du transcrit. Mes travaux montrent que les LPS et la cycloheximide inhibent l’expression de l’ARNm αENaC de façon similaire via l’activation des voies de signalisation des MAPK ERK1/2 et p38. Cependant, les mécanismes de modulation de l’expression de l'ARNm αENaC sont différents puisque les LPS répriment la transcription du gène, alors que la cycloheximide diminuerait la stabilité du transcrit via des mécanismes post-transcriptionnels impliquant la région 3' non traduite (3'UTR) de l'ARNm αENaC. Pour mieux étudier le rôle du 3'UTR dans ce processus, nous avons développé un modèle Tet-Off nous permettant de mesurer la demi-vie de l’ARNm αENaC indépendamment de l’utilisation d’un inhibiteur de la transcription comme l'actinomycine D (Act. D). Nous avons montré que la demi-vie de l’ARNm αENaC était de 100min, un temps beaucoup plus court que celui rapporté dans la littérature. Nous avons démontré que l’Act. D a un effet stabilisateur important sur l’ARNm αENaC et qu’il ne peut être utilisé pour évaluer la stabilité du transcrit. À l’aide de différents mutants de délétion, nous avons entrepris de déterminer la nature des régions du 3’UTR impliquées dans la modulation de la stabilité du transcrit. Nous avons trouvé que le 3’UTR joue un rôle à la fois de stabilisation (région 3’UTR proximale) et de déstabilisation (région 3’UTR distale) du transcrit. Notre système nous a finalement permis de confirmer que la diminution de l’ARNm αENaC observée en présence de TNF-α s’expliquait en partie par une diminution importante de la stabilité du transcrit induite par cette cytokine. Enfin, nous avons identifié la nature des protéines pouvant se lier au 3’UTR de l’ARNm αENaC et déterminé lesquelles pouvaient moduler la stabilité du transcrit. Des trois protéines candidates trouvées, nous avons confirmé que la surexpression de DHX36 et TIAL1 diminue le niveau de transcrit par un mécanisme impliquant la stabilité du messager. Les travaux présentés ici montrent la complexité des voies de signalisation induites par différents stress sur les cellules épithéliales alvéolaires et montrent comment la stabilité de l’ARNm αENaC et en particulier, les séquences du 3’UTR jouent un rôle important dans la modulation du niveau de transcrit. Le modèle Tet-Off que nous avons développé permet d’estimer le temps de demi-vie réel de l’ARNm αENaC et montre que le 3’UTR du messager joue un rôle complexe dans la stabilisation du messager en condition de base ainsi qu’en condition pro-inflammatoire. Enfin, nous avons identifié deux protéines liant l’ARNm qui pourraient jouer un rôle important dans la modulation de la stabilité du transcrit.The epithelial sodium channel (ENaC) expressed in alveolar epithelial cells plays a major role for lung liquid clearance at birth and lung edema resorption in adulthood. The expression and activity of ENaC are inhibited by many pathophysiological stress that could have an impact in the clinical outcome of acute respiratory distress syndrome (ARDS). Pulmonary inflammation is an important factor in this inhibition that may promote or sustain pulmonary edema. We have previously shown that pro-inflammatory cytokines and lipopolysaccharide (LPS) from Pseudomonas aeruginosa inhibit αENaC mRNA expression by transcriptional and post-transcriptional mechanisms, suggesting that a modulation of αENaC mRNA stability could play a role in this process. The main objective of the present work was to characterize how different pathophysiological stress affect αENaC mRNA expression in alveolar epithelial cells and determine whether this modulation could be explained in part by regulating the stability of the transcript. Our study shows that LPS and cycloheximide decrease the level of αENaC mRNA with a similar time course and via the activation of the MAPK ERK1/2 and p38 signaling pathways. Despite similarities, there were important differences in the mechanisms involved in the modulation of αENaC mRNA expression. While LPS repress αENaC mRNA transcription, cycloheximide triggers post-transcriptional mechanisms involving the 3' untranslated region (3'UTR) of αENaC mRNA. To further study the role of αENaC 3'UTR in this process, we developed a Tet-Off model that allows us to measure the half-life of αENaC mRNA regardless of the use of a transcription inhibitor such as actinomycin D (Act. D). Using this system, we showed a 100 min half-life for αENaC mRNA, a much shorter time then the one reported for this mRNA using Act. D. We showed that Act. D has an important stabilizing effect on αENaC mRNA and cannot be used to assess the stability of the transcript. Using deletion mutants of the αENaC 3'UTR region, we determined how different portions of 3'UTR were important in modulating stability of the transcript. We found that the 3'UTR has dual functions, with portions important to promote stabilization (proximal 3'UTR) and others that strongly destabilize (distal 3'UTR) the transcript. Our system also allowed us to confirm that the decreased expression of αENaC mRNA induced by TNF-α results in part by a decreased stability of the mRNA. Finally, we identified several RNA-binding proteins that interact specifically with αENaC 3'UTR and determined if these proteins had an impact on transcript stability. Surexpression of two of these proteins in alveolar epithelial cells, DHX36 and TIAL1 was able to decrease the level of αENaC mRNA via a downregulation of mRNA stability. The work presented here shows the complexity of the signal transduction pathways elicited by different pathological stress conditions in alveolar epithelial cells and is the first to show that αENaC mRNA stability elicited by sequences in 3’UTR plays an important role in modulating the level of the transcript. The Tet-Off model that we developed allows to accurately estimate the half-life of αENaC mRNA and shows that the 3’UTR portion of the mRNA plays a complex role in the modulation of transcript stability in basal and pro-inflammatory conditions. Finally, we identified two putative RNA-binding proteins able to specifically recognize αENaC 3’UTR and modulate the transcript stability

K+ channels regulate ENaC expression via changes in promoter activity and control fluid clearance in alveolar epithelial cells

AbstractActive Na+ absorption by alveolar ENaC is the main driving force of liquid clearance at birth and lung edema resorption in adulthood. We have demonstrated previously that long-term modulation of KvLQT1 and KATP K+ channel activities exerts sustained control in Na+ transport through the regulation of ENaC expression in primary alveolar type II (ATII) cells. The goal of the present study was: 1) to investigate the role of the α-ENaC promoter, transfected in the A549 alveolar cell line, in the regulation of ENaC expression by K+ channels, and 2) to determine the physiological impact of K+ channels and ENaC modulation on fluid clearance in ATII cells. KvLQT1 and KATP channels were first identified in A549 cells by PCR and Western blotting. We showed, for the first time, that KvLQT1 activation by R-L3 (applied for 24h) increased α-ENaC expression, similarly to KATP activation by pinacidil. Conversely, pharmacological KvLQT1 and KATP inhibition or silencing with siRNAs down-regulated α-ENaC expression. Furthermore, K+ channel blockers significantly decreased α-ENaC promoter activity. Our results indicated that this decrease in promoter activity could be mediated, at least in part, by the repressor activity of ERK1/2. Conversely, KvLQT1 and KATP activation dose-dependently enhanced α-ENaC promoter activity. Finally, we noted a physiological impact of changes in K+ channel functions on ERK activity, α-, β-, γ-ENaC subunit expression and fluid absorption through polarized ATII cells. In summary, our results disclose that K+ channels regulate α-ENaC expression by controlling its promoter activity and thus affect the alveolar function of fluid clearance

Autophagy drives fibroblast senescence through MTORC2 regulation

Sustained macroautophagy/autophagy favors the differentiation of fibroblasts into myofibroblasts. Cellular senescence, another means of responding to long-term cellular stress, has also been linked to myofibroblast differentiation and fibrosis. Here, we evaluate the relationship between senescence and myofibroblast differentiation in the context of sustained autophagy. We analyzed markers of cell cycle arrest/senescence in fibroblasts in vitro, where autophagy was triggered by serum starvation (SS). Autophagic fibroblasts expressed the senescence biomarkers CDKN1A/p21 and CDKN2A/p16 and exhibited increased senescenceassociated GLB1/beta-galactosidase activity. Inhibition of autophagy in serum-starved fibroblasts with 3-methyladenine, LY294002, or ATG7 (autophagy related 7) silencing prevented the expression of senescence-associated markers. Similarly, suppressing MTORC2 activation using rapamycin or by silencing RICTOR also prevented senescence hallmarks. Immunofluorescence microscopy showed that senescence and myofibroblast differentiation were induced in different cells, suggesting mutually exclusive activation of senescence and myofibroblast differentiation. Reactive oxygen species (ROS) are known inducers of senescence and exposing fibroblasts to ROS scavengers decreased ROS production during SS, inhibited autophagy, and significantly reduced the expression of senescence and myofibroblast differentiation markers. ROS scavengers also curbed the AKT1 phosphorylation at Ser473, an MTORC2 target, establishing the importance of ROS in fuelling MTORC2 activation. Inhibition of senescence by shRNA to TP53/p53 and shRNA CDKN2A/p16 increased myofibroblast differentiation, suggesting a negative feedback loop of senescence on autophagy-induced myofibroblast differentiation. Collectively, our results identify ROS as central inducers of MTORC2 activation during chronic autophagy, which in turn fuels senescence activation and myofibroblast differentiation in distinct cellular subpopulations

The LUX-ZEPLIN (LZ) Experiment

We describe the design and assembly of the LUX-ZEPLIN experiment, a direct detection search for cosmic WIMP dark matter particles. The centerpiece of the experiment is a large liquid xenon time projection chamber sensitive to low energy nuclear recoils. Rejection of backgrounds is enhanced by a Xe skin veto detector and by a liquid scintillator Outer Detector loaded with gadolinium for efficient neutron capture and tagging. LZ is located in the Davis Cavern at the 4850' level of the Sanford Underground Research Facility in Lead, South Dakota, USA. We describe the major subsystems of the experiment and its key design features and requirements

First Dark Matter Search Results from the LUX-ZEPLIN (LZ) Experiment

The LUX-ZEPLIN (LZ) experiment is a dark matter detector centered on a dual-phase xenon time projection chamber operating at the Sanford Underground Research Facility in Lead, South Dakota, USA. This Letter reports results from LZ's first search for Weakly Interacting Massive Particles (WIMPs) with an exposure of 60 live days using a fiducial mass of 5.5 t. A profile-likelihood ratio analysis shows the data to be consistent with a background-only hypothesis, setting new limits on spin-independent WIMP-nucleon, spin-dependent WIMP-neutron, and spin-dependent WIMP-proton cross-sections for WIMP masses above 9 GeV/c$^2$. The most stringent limit is set at 30 GeV/c$^2$, excluding cross sections above 5.9$\times 10^{-48}$ cm$^2$ at the 90\% confidence level.Comment: 9 pages, 6 figures. See https://tinyurl.com/LZDataReleaseRun1 for a data release related to this pape

The LUX-ZEPLIN (LZ) radioactivity and cleanliness control programs

LUX-ZEPLIN (LZ) is a second-generation direct dark matter experiment with spin-independent WIMP-nucleon scattering sensitivity above 1.4×10−48cm2 for a WIMP mass of 40GeV/c2 and a 1000days exposure. LZ achieves this sensitivity through a combination of a large 5.6t fiducial volume, active inner and outer veto systems, and radio-pure construction using materials with inherently low radioactivity content. The LZ collaboration performed an extensive radioassay campaign over a period of six years to inform material selection for construction and provide an input to the experimental background model against which any possible signal excess may be evaluated. The campaign and its results are described in this paper. We present assays of dust and radon daughters depositing on the surface of components as well as cleanliness controls necessary to maintain background expectations through detector construction and assembly. Finally, examples from the campaign to highlight fixed contaminant radioassays for the LZ photomultiplier tubes, quality control and quality assurance procedures through fabrication, radon emanation measurements of major sub-systems, and bespoke detector systems to assay scintillator are presented

The LUX-ZEPLIN (LZ) experiment

We describe the design and assembly of the LUX-ZEPLIN experiment, a direct detection search for cosmic WIMP dark matter particles. The centerpiece of the experiment is a large liquid xenon time projection chamber sensitive to low energy nuclear recoils. Rejection of backgrounds is enhanced by a Xe skin veto detector and by a liquid scintillator Outer Detector loaded with gadolinium for efficient neutron capture and tagging. LZ is located in the Davis Cavern at the 4850’ level of the Sanford Underground Research Facility in Lead, South Dakota, USA. We describe the major subsystems of the experiment and its key design features and requirements