RÉSUMÉ
Despite the introduction of novel sutureless posterior chamber intraocular lens (IOL) fixation techniques, some conditions still require suture-assisted scleral fixation. If the scleral fixation suture knot is left directly under the conjunctiva, it may become exposed, resulting in an increased risk of endophthalmitis. To avoid this problem, we offer a new alternative, simple, and safe way for burying the end of the suture using knots in this report.
Sujet(s)
Pose d'implant intraoculaire , Chambres de culture à diffusion , Matériels de fixation chirurgicaleRÉSUMÉ
Lithium chloride (LiCl) is an important mood-stabilizing therapeutic agent for bipolar disorders, which has also been shown to inhibit cancer cell metastasis. Investigations of LiCl-induced signaling have focused mainly on extracellular signal regulated kinase 1/2 (ERK1/2) and glycogen synthase kinase 3 (GSK-3). However, little is known about the differences in cellular activities resulting from specific signaling via each of these pathways. In this study, we investigated the difference in responses between the Wnt/ß-catenin and ERK pathways by LiCl or epidermal growth factor (EGF) treatment of osteosarcoma cells. In particular, we analyzed the mechanisms responsible for differences in cell mobility and cell proliferation when pERK or ß-catenin is activated. In osteosarcoma cells treated with LiCl or EGF, active ß-catenin and p-ERK protein levels were significantly increased compared to those in the control group. However, in wound healing and transwell invasion assays, U2OS and SaOS2 cell migration was significantly reduced by LiCl treatment but increased by EGF treatment. In addition, the proliferation of U2OS cells was reduced by LiCl treatment but increased by EGF treatment. Using immunofluorescence microscopy, we observed nuclear accumulation of phosphorylated ERK (pERK) with EGF treatment, but pERK was restricted to the perinuclear area with LiCl treatment. These results were confirmed using immunoblot assays after subcellular fractionation. Together, these data suggest that LiCl interferes with the translocation of pERK from the cytoplasm to the nucleus.
Sujet(s)
Facteur de croissance épidermique/pharmacologie , Chlorure de lithium/pharmacologie , Mitogen-Activated Protein Kinase 1/génétique , Mitogen-Activated Protein Kinase 3/génétique , Ostéoblastes/effets des médicaments et des substances chimiques , Cellules de la moelle osseuse/cytologie , Cellules de la moelle osseuse/effets des médicaments et des substances chimiques , Cellules de la moelle osseuse/métabolisme , Lignée cellulaire tumorale , Mouvement cellulaire/effets des médicaments et des substances chimiques , Mouvement cellulaire/génétique , Noyau de la cellule/effets des médicaments et des substances chimiques , Noyau de la cellule/métabolisme , Prolifération cellulaire/effets des médicaments et des substances chimiques , Prolifération cellulaire/génétique , Chambres de culture à diffusion , Régulation de l'expression des gènes tumoraux , Glycogen synthase kinase 3 beta/génétique , Glycogen synthase kinase 3 beta/métabolisme , Humains , Système de signalisation des MAP kinases/effets des médicaments et des substances chimiques , Mitogen-Activated Protein Kinase 1/antagonistes et inhibiteurs , Mitogen-Activated Protein Kinase 1/métabolisme , Mitogen-Activated Protein Kinase 3/antagonistes et inhibiteurs , Mitogen-Activated Protein Kinase 3/métabolisme , Ostéoblastes/métabolisme , Ostéoblastes/anatomopathologie , Phosphorylation/effets des médicaments et des substances chimiques , Culture de cellules primaires , Transport des protéines/effets des médicaments et des substances chimiques , Voie de signalisation Wnt/effets des médicaments et des substances chimiques , bêta-Caténine/génétique , bêta-Caténine/métabolismeRÉSUMÉ
Inflammatory changes are involved in tumor cell proliferation, migration, and invasion. Tumor necrosis factor-α (TNF-α) and lipopolysaccharide (LPS) play important roles in inflammatory regulation during tumor development. Oct4 acts as a transcription factor that modulates inflammatory changes in mesenchymal stem cells. In this study, we explored the role of Oct4 in the invasion and migration of oral squamous cell carcinoma (OSCC) cells. LPS and TNF-α were used to treat the OSCC cell lines HN4 and CAL27 to induce inflammation. The generation of inflammatory cytokines, including TNF-α, interleukin (IL)-1ß, and IL-6, was evaluated by enzyme-linked immunosorbent assay and real-time quantitative PCR. Western blot analysis was employed to detect the expression and phosphorylation of JNK1, p65, and STAT3, which are key modulators of inflammation. Wound scratch healing and transwell invasion assays were further used to determine the role of inflammation in the invasion and migration of OSCC cells. Robust inflammation was observed in HN4 and CAL27 cells treated with LPS and TNF-α. A marked increase in JNK1, p65, and STAT3 phosphorylation levels in OSCC cells was also detected after LPS and TNF-α treatment. The migration and invasion of HN4 and CAL27 cells were significantly boosted by stimulation with LPS and TNF-α. Furthermore, Oct4 mRNA and protein levels were significantly upregulated by stimulation with LPS and TNF-α. Silencing of Oct4 led to reduced inflammation and decreased levels of phosphorylated JNK1, p65, and STAT3 and impaired invasion and migration in LPS- and TNF-α-stimulated OSCC cells. Overall, LPS- and TNF-α-induced inflammation suppressed the migration and invasion of OSCC cells by upregulating Oct4 expression.
Sujet(s)
Cellules épithéliales/effets des médicaments et des substances chimiques , Lipopolysaccharides/pharmacologie , Facteur de transcription Oct-3/génétique , Maturation post-traductionnelle des protéines , Facteur de nécrose tumorale alpha/pharmacologie , Lignée cellulaire tumorale , Mouvement cellulaire/effets des médicaments et des substances chimiques , Prolifération cellulaire/effets des médicaments et des substances chimiques , Chambres de culture à diffusion , Cellules épithéliales/métabolisme , Cellules épithéliales/anatomopathologie , Régulation de l'expression des gènes tumoraux , Humains , Inflammation , Interleukine-1 bêta/génétique , Interleukine-1 bêta/métabolisme , Interleukine-6/génétique , Interleukine-6/métabolisme , Mitogen-Activated Protein Kinase 8/génétique , Mitogen-Activated Protein Kinase 8/métabolisme , Modèles biologiques , Facteur de transcription Oct-3/antagonistes et inhibiteurs , Facteur de transcription Oct-3/métabolisme , Phosphorylation/effets des médicaments et des substances chimiques , Petit ARN interférent/génétique , Petit ARN interférent/métabolisme , Facteur de transcription STAT-3/génétique , Facteur de transcription STAT-3/métabolisme , Transduction du signal , Facteur de transcription RelA/génétique , Facteur de transcription RelA/métabolisme , Facteur de nécrose tumorale alpha/génétique , Facteur de nécrose tumorale alpha/métabolismeRÉSUMÉ
In vitro diffusion testing of topical formulations has long been examined using Franz diffusion chambers, however, Franz chambers are typically used with relatively large volumes, lack the air/membrane interface present in vivo, and do not account for changes in formula characteristics as solvent evaporates. Here we present our patented Munt-Dash diffusion chamber designed for direct spray application onto a model membrane. Diffusion characteristics from topical spray formulations utilizing both the Munt-Dash chamber and Franz diffusion chambers were evaluated and compared. Using diclofenac sodium and lidocaine hydrochloride as model drugs and shed snakeskin as a model for stratum corneum, test solutions were applied to Franz diffusion chambers using a pipette and to the Munt-Dash chamber using a high-speed syringe pump and sprayer. Both chambers presented permeability data consistent with previously reported in vitro and in vivo studies. Significant differences were observed in permeability by formulation and temperature. This suggests that although Franz chambers produce relevant data, the failure to account for small volumes and drying during application may produce misleading results. The Munt-Dash chamber may improve in vitro testing by providing these factors. This data suggests the Munt-Dash chamber is a suitable alternative to the Franz chamber for topical spray formulations.
Sujet(s)
Épiderme , Peau , Diffusion , Chambres de culture à diffusion , Techniques in vitro , PerméabilitéRÉSUMÉ
BACKGROUND: Anterior cervical discectomy and fusion (ACDF) with a rigid interbody spacer is commonly used in the treatment of cervical degenerative disc disease. Although ACDF relieves clinical symptoms, it is associated with several complications such as pseudoarthrosis and adjacent segment degeneration. The concept of dynamic fusion has been proposed to enhance fusion and reduce implant subsidence rate and post-fusion stiffness; this pilot preclinical animal study was conducted to begin to compare rigid and dynamic fusion in ACDF. QUESTIONS/PURPOSES: Using a pig model, we asked, is there (1) decreased subsidence, (2) reduced axial stiffness in compression, and (3) improved likelihood of bone growth with a dynamic interbody cage compared with a rigid interbody cage in ACDF? METHODS: ACDF was performed at two levels, C3/4 and C5/6, in 10 pigs weighing 48 to 55 kg at the age of 14 to 18 months (the pigs were skeletally mature). One level was implanted with a conventional rigid interbody cage, and the other level was implanted with a dynamic interbody cage. The conventional rigid interbody cage was implanted in the upper level in the first five pigs and in the lower level in the next five pigs. Both types of interbody cages were implanted with artificial hydroxyapatite and tricalcium phosphate bone grafts. To assess subsidence, we took radiographs at 0, 7, and 14 weeks postoperatively. Subsidence less than 10% of the disc height was considered as no radiologic abnormality. The animals were euthanized at 14 weeks, and each operated-on motion segment was harvested. Five specimens from each group were biomechanically tested under axial compression loading to determine stiffness. The other five specimens from each group were used for microCT evaluation of bone ingrowth and ongrowth and histologic investigation of bone formation. Sample size was determined based on 80% power and an α of 0.05 to detect a between-group difference of successful bone formation of 15%. RESULTS: With the numbers available, there was no difference in subsidence between the two groups. Seven of 10 operated-on levels with rigid cages had subsidence on a follow-up radiograph at 14 weeks, and subsidence occurred in two of 10 operated-on levels with dynamic cages (Fisher exact test; p = 0.07). The stiffness of the unimplanted rigid interbody cages was higher than the unimplanted dynamic interbody cages. After harvesting, the median (range) stiffness of the motion segments fused with dynamic interbody cages (531 N/mm [372 to 802]) was less than that of motion segments fused with rigid interbody cages (1042 N/mm [905 to 1249]; p = 0.002). Via microCT, we observed bone trabecular formation in both groups. The median (range) proportions of specimens showing bone ongrowth (88% [85% to 92%]) and bone volume fraction (87% [72% to 100%]) were higher in the dynamic interbody cage group than bone ongrowth (79% [71% to 81%]; p < 0.001) and bone volume fraction (66% [51% to 78%]; p < 0.001) in the rigid interbody cage group. The percentage of the cage with bone ingrowth was higher in the dynamic interbody cage group (74% [64% to 90%]) than in the rigid interbody cage group (56% [32% to 63%]; p < 0.001), and the residual bone graft percentage was lower (6% [5% to 8%] versus 13% [10% to 20%]; p < 0.001). In the dynamic interbody cage group, more bone formation was qualitatively observed inside the cages than in the rigid interbody cage group, with a smaller area of fibrotic tissue under histologic investigation. CONCLUSION: The dynamic interbody cage provided satisfactory stabilization and percentage of bone ongrowth in this in vivo model of ACDF in pigs, with lower stiffness after bone ongrowth and no difference in subsidence. CLINICAL RELEVANCE: The dynamic interbody cage appears to be worthy of further investigation. An animal study with larger numbers, with longer observation time, with multilevel surgery, and perhaps in the lumbar spine should be considered.
Sujet(s)
Transplantation osseuse/méthodes , Vertèbres cervicales/chirurgie , Chambres de culture à diffusion , Discectomie/méthodes , Ostéogenèse/physiologie , Animaux , Phénomènes biomécaniques , Phosphates de calcium , Vertèbres cervicales/physiopathologie , Durapatite , Dégénérescence de disque intervertébral/physiopathologie , Dégénérescence de disque intervertébral/chirurgie , Modèles animaux , Projets pilotes , Conception de prothèse , Arthrodèse vertébrale , SuidaeRÉSUMÉ
OBJECTIVE: To examine the effect of static versus expandable polyether ether ketone (PEEK) cages on both clinical and radiographic outcomes. METHODS: A retrospective cohort study was conducted on patients who underwent one-level transforaminal lumbar interbody fusion with either a static or expandable PEEK cage. Patient outcomes were obtained from chart review and radiographic outcomes were measured using standing, lateral radiographs. Recovery ratios and the proportion of patients achieving the minimally clinically important difference were calculated for Oswestry Disability Index (ODI), Physical Component Score-12, Mental Component Score-12, visual analogue scale for back, and visual analogue scale for leg at 1 year and compared between groups. Multivariate linear regression analysis was performed to determine the effect of cage type on the change in patient-reported outcome measures, controlling for demographic factors. RESULTS: A total of 240 patients (137 static, 103 expandable) were included in the final analysis. ΔPhysical Component Score-12 scores at 3 months were significantly greater for the static group (16.0 vs. 10.0, P = 0.043) compared with the expandable group. Multivariate regression demonstrated that use of an expandable cage was associated with greater improvements in ΔODI (ß: -7.82, P = 0.048) at 1 year. No differences were found in the perioperative change in sagittal spinal alignment within or between groups at 1 year. Subsidence rates failed to show any statistically significant difference between the 2 groups. CONCLUSIONS: Transforaminal lumbar interbody fusion with an expandable PEEK cage is an independent predictor of improved ODI scores at 1 year. Our study showed no significant differences in subsidence rates or changes in sagittal spinal alignment between static and expandable PEEK cages.
Sujet(s)
Benzophénones/composition chimique , Chambres de culture à diffusion , Vertèbres lombales/chirurgie , Polymères/composition chimique , Arthrodèse vertébrale/instrumentation , Adulte , Sujet âgé , Études de cohortes , Évaluation de l'invalidité , Femelle , Humains , Lombalgie/imagerie diagnostique , Lombalgie/chirurgie , Vertèbres lombales/imagerie diagnostique , Région lombosacrale/chirurgie , Mâle , Adulte d'âge moyen , Mesure de la douleur , Études rétrospectives , Rachis/imagerie diagnostique , Résultat thérapeutiqueRÉSUMÉ
BACKGROUND: Intervertebral fusions in cases of reduced bone density are a tough challenge. From a biomechanical point of view, most current studies have focused on the range of motion or have shown test setups for single-component tests. Definitive setups for biomechanical testing of the primary stability of a 360° fusion using a screw-rod system and cage on osteoporotic spine are missing. The aim of this study was to develop a test stand to provide information about the bone-implant interface under reproducible conditions. METHODS: After pretesting with artificial bone, functional spine units were tested with 360° fusion in the transforaminal lumbar interbody fusion technique. The movement sequences were conducted in flexion/extension, right and left lateral bending, and right and left axial rotation on a human model with osteopenia or osteoporosis under permanent maximum load with 7.5 N-m. RESULTS: During the testing of human cadavers, 4 vertebrae were fully tested and were inconspicuous even after radiological and macroscopic examination. One vertebra showed a subsidence of 2 mm, and 1 vertebra had a cage collapsed into the vertebra. CONCLUSIONS: This setup is suitable for biomechanical testing of cyclical continuous loads on the spine with reduced bone quality or osteoporosis. The embedding method is stable and ensures a purely single-level setup with different trajectories, especially when using the cortical bone trajectory. Optical monitoring provides a very accurate indication of cage movement, which correlates with the macroscopic and radiological results.
Sujet(s)
Implant résorbable , Maladies osseuses métaboliques/thérapie , Chambres de culture à diffusion , Modèles anatomiques , Ostéoporose/thérapie , Rachis/chirurgie , Sujet âgé , Sujet âgé de 80 ans ou plus , Phénomènes biomécaniques , Maladies osseuses métaboliques/imagerie diagnostique , Maladies osseuses métaboliques/chirurgie , Vis orthopédiques , Cadavre , Conception d'appareillage , Femelle , Humains , Mâle , Test de matériaux , Ostéoporose/imagerie diagnostique , Ostéoporose/chirurgie , Conception de prothèse , Amplitude articulaire , Arthrodèse vertébrale , Rachis/imagerie diagnostiqueRÉSUMÉ
Tripartite motif-containing 21 (TRIM21) has been confirmed to mediate the production of inflammatory mediators via NF-κB signaling. However, the function of TRIM21 in microglia-mediated neuroinflammation remains unclear. This study aimed to explore the effect of TRIM21 on LPS-activated BV2 microglia and its underlying mechanism. BV2 cells exposed to lipopolysaccharide (LPS) were used to simulated neuroinflammation in vitro. Loss-of-function and gain-of-function of TRIM21 in BV2 cells were used to assess the effect of TRIM21 on LPS-induced neuroinflammation. BV2 microglia and HT22 cells co-culture system were used to investigate whether TRIM21 regulated neuronal inflammation-mediated neuronal death. TRIM21 knockdown triggered the polarization of BV2 cells from M1 to M2 phenotype. Knockdown of TRIM21 reduced the secretion of TNF-α, IL-6, and IL-1ß, while increased the content of IL-4 in LPS-treated cells. Knockdown of TRIM21 inhibited the expression of p65 and the binding activity of NF-κB-DNA. Additionally, TRIM21 siRNA eliminated the increase in NLRP3 and cleaved caspase-1 proteins expression and caspase-1 activity induced by LPS. TRIM21 knockdown could resist cytotoxicity induced by activated microglia, including increasing the viability of co-cultured HT22 cells and reducing the emancipation of LDH. Moreover, the increased apoptosis and caspase-3 activity of HT22 neurons induced by activated BV2 cells were blocked by TRIM21 siRNA. Blocking of NF-κB abolished the effect of TRIM21 in promoting the expression of M1 phenotype marker genes. Similarly, the blockade of NF-κB pathway eliminated the promotion of TRIM21 on neurotoxicity induced by neuroinflammation. TRIM21 knockdown suppressed the M1 phenotype polarization of microglia and neuroinflammation-mediated neuronal damage via NF-κB/NLRP3 inflammasome pathway, which suggested that TRIM21 might be a potential therapeutic target for the therapy of central nervous system diseases.
Sujet(s)
Inflammasomes/effets des médicaments et des substances chimiques , Lipopolysaccharides/toxicité , Microglie/effets des médicaments et des substances chimiques , Protéine-3 de la famille des NLR contenant un domaine pyrine/génétique , Neurones/effets des médicaments et des substances chimiques , Ribonucléoprotéines/génétique , Facteur de transcription RelA/génétique , Animaux , Caspase-1/génétique , Caspase-1/métabolisme , Différenciation cellulaire , Lignée cellulaire , Techniques de coculture , Chambres de culture à diffusion , Régulation de l'expression des gènes , Hippocampe/cytologie , Hippocampe/métabolisme , Inflammasomes/génétique , Inflammasomes/métabolisme , Interleukine-1 bêta/génétique , Interleukine-1 bêta/métabolisme , Interleukine-4/génétique , Interleukine-4/métabolisme , Interleukine-6/génétique , Interleukine-6/métabolisme , Souris , Microglie/cytologie , Microglie/métabolisme , Protéine-3 de la famille des NLR contenant un domaine pyrine/métabolisme , Neurones/cytologie , Neurones/métabolisme , Petit ARN interférent/génétique , Petit ARN interférent/métabolisme , Ribonucléoprotéines/antagonistes et inhibiteurs , Ribonucléoprotéines/métabolisme , Transduction du signal , Facteur de transcription RelA/métabolisme , Facteur de nécrose tumorale alpha/génétique , Facteur de nécrose tumorale alpha/métabolismeRÉSUMÉ
Chronic alcohol alters the immune system enhancing the susceptibility to inflammation, bacterial, and viral infections in alcohol users. We have shown that alcohol causes increased permeability of mesenteric lymphatic vessels in alcohol-fed rats. The mechanisms of alcohol-induced lymphatic leakage are unknown. Endothelial cell monolayer permeability is controlled by junctional proteins complexes called tight junctions (TJ) and adherens junctions (AJ), and each can be regulated by MAPK activation. We hypothesize that ethanol induces lymphatic endothelial cell (LEC) permeability via disruption of LEC TJ through MAPK activation. An in vitro model of rat LECs was used. Ethanol-supplemented medium was added at concentrations of 0, 25, and 50 mM to confluent cells. Resistance-based barrier function, transwell permeability, cell viability, TJ, AJ, and MAPK protein activity, TJ and AJ gene expressions, and the role of p38 MAPK in barrier function regulation were measured. Ethanol increased the permeability of LECs compared to controls that was not associated with decreased cell viability. LECs treated with 50 mM ethanol showed an increase in phosphorylated levels of p38. No significant changes in TJ and AJ gene or protein expressions were observed after ethanol treatment. p38 inhibition prevented ethanol-induced increases in permeability. These findings suggest that p38 may play a role in the regulation of ethanol-induced LEC permeability, but altered permeability may not be associated with decreased TJ or AJ protein expression. Further investigation into junctional protein localization is needed to better understand the effects of ethanol on lymphatic endothelial cell-to-cell contacts and hyperpermeability.
Sujet(s)
Perméabilité des membranes cellulaires/effets des médicaments et des substances chimiques , Cellules endothéliales/effets des médicaments et des substances chimiques , Éthanol/pharmacologie , p38 Mitogen-Activated Protein Kinases/génétique , Jonctions adhérentes/effets des médicaments et des substances chimiques , Jonctions adhérentes/métabolisme , Animaux , Animaux nouveau-nés , Antigènes CD/génétique , Antigènes CD/métabolisme , Transport biologique , Cadhérines/génétique , Cadhérines/métabolisme , Claudine-5/génétique , Claudine-5/métabolisme , Derme/cytologie , Derme/métabolisme , Chambres de culture à diffusion , Impédance électrique , Cellules endothéliales/cytologie , Cellules endothéliales/métabolisme , Régulation de l'expression des gènes , Occludine/génétique , Occludine/métabolisme , Phosphorylation/effets des médicaments et des substances chimiques , Culture de cellules primaires , Rats , Jonctions serrées/effets des médicaments et des substances chimiques , Jonctions serrées/métabolisme , Protéine-1 de la zonula occludens/génétique , Protéine-1 de la zonula occludens/métabolisme , p38 Mitogen-Activated Protein Kinases/métabolismeRÉSUMÉ
Tissue Cage (TC) model was used to evaluate the pharmacokinetics and ex vivo pharmacodynamics of Minocycline (MINO) after intramuscular (IM) administration to donkeys at 4 mg/kg body-weight. The Cmax of MINO with 1.79 and 2.63 µg mL-1 was obtained at 2.96 and 1.41 h in TCF (tissue cage fluid) and plasma respectively. The absorption half-lives (t1/2ka) of MINO were calculated to be 0.71 h in TCF and 0.32 h in plasma, whereas the elimination half-lives (t1/2ke) were 10.46 h in TCF and 5.95 h in plasma. The distribution volume (Vd/F) of MINO was estimated to be 1.84 L kg-1 in TCF and 1.28 L kg-1 in plasma. The total clearance (CLb/F) of MINO was computed as 0.12 and 0.15 L/ (h·kg) in TCF and plasma respectively. The area under the concentration-time curve (AUC) of MINO was 32.77 µg mL-1h in TCF and 25.27 µg mL-1h in plasma, respectively.The ex vivo time-kill curves were established for plasma and TCF samples using Salmonella abortus equi. The MIC and MBC of MINO against salmonella were 0.08 and 0.16 µg mL-1 for plasma, 0.04 and 0.08 µg mL-1 for TCF. The plasma Cmax/MIC and AUC/MIC values after IM administration were 32.88 ± 9.87 and 315.88 ± 42.65 h, respectively. The TCF Cmax/MIC and AUC/MIC values after IM administration were 44.75 ± 9.32 and 819.25 ± 65.23 h, respectively. The values of T > MIC were approximately >36 h in plasma and > 65 h in TCF. These findings from this study suggest that MINO may be therapeutically effective in diseases of donkeys caused by salmonella when used at a dose of 4 mg/kg IM administration.
Sujet(s)
Antibactériens/pharmacologie , Antibactériens/pharmacocinétique , Equidae/métabolisme , Minocycline/pharmacologie , Minocycline/pharmacocinétique , Salmonella/effets des médicaments et des substances chimiques , Animaux , Aire sous la courbe , Chambres de culture à diffusion , Femelle , Injections musculaires/médecine vétérinaire , Mâle , Tests de sensibilité microbienne/médecine vétérinaireRÉSUMÉ
In endothelial cells (ECs), the onset of apicobasal polarity is primarily regulated by the interaction of integrins with the surrounding extracellular matrix (ECM). ECs secrete and polymerize fibronectin (FN), a unique, permissive substrate that allows for vascular morphogenesis and lumen formation. We previously identified a signaling pathway that, under the control of the adhesion site adaptor protein PPFIA1, integrates the polarized secretion of freshly synthesized FN with the recycling of conformationally active α5ß1 integrin, the main FN receptor in ECs. To characterize the functional role of PPFIA1-dependent signaling in ECs, we set up a Transwell-based assay to quantify the polarized secretion of ECM proteins. To this aim, we allowed ECs to form a confluent monolayer on the Transwell membrane and checked its integrity by measuring transendothelial electric resistance and controlling the stability of tight junctions over time by fluorescent confocal microscope analysis. Finally, we quantified apical and basolateral FN secretion in control and PPFIA1-silenced EC culture medium by western blot analysis coupled to spike-in normalization.
Sujet(s)
Protéines adaptatrices de la transduction du signal/génétique , Cellules endothéliales/métabolisme , Matrice extracellulaire/métabolisme , Fibronectines/génétique , Intégrine alpha5bêta1/génétique , Jonctions serrées/métabolisme , Protéines adaptatrices de la transduction du signal/antagonistes et inhibiteurs , Protéines adaptatrices de la transduction du signal/métabolisme , Transport biologique , Polarité de la cellule , Chambres de culture à diffusion , Cellules endothéliales/ultrastructure , Matrice extracellulaire/ultrastructure , Fibronectines/métabolisme , Régulation de l'expression des gènes , Appareil de Golgi/métabolisme , Appareil de Golgi/ultrastructure , Humains , Intégrine alpha5bêta1/métabolisme , Microscopie de fluorescence/méthodes , Culture de cellules primaires , Petit ARN interférent/génétique , Petit ARN interférent/métabolisme , Transduction du signal , Jonctions serrées/ultrastructureRÉSUMÉ
While metastasis - the spread of cancer from the primary location to distant sites in the body - remains the principle cause of cancer death, it is incompletely understood. It is a complex process, requiring the metastatically successful cancer cell to negotiate a formidable series of interconnected steps, which are described in this paper. For each step, we review the range of in vitro assays that may be used to study them. We also provide a range of detailed, step-by-step protocols that can be undertaken in most modestly-equipped laboratories, including methods for converting qualitative observations into quantitative data for analysis. Assays include: (1) a gelatin degradation assay to study the ability of endothelial cells to degrade extracellular matrix during tumour angiogenesis; (2) the morphological characterisation of cells undergoing epithelial-mesenchymal transition (EMT) as they acquire motility; (3) a 'scratch' or 'wound-healing' assay to study cancer cell migration; (4) a transwell assay to study cancer cell invasion through extracellular matrix; and (5) a static adhesion assay to examine cancer cell interactions with, and adhesion to, endothelial monolayers. This toolkit of protocols will enable researchers who are interested in metastasis to begin to focus on defined aspects of the process. It is only by further understanding this complex, fascinating and clinically relevant series of events that we may ultimately devise ways of better treating, or even preventing, cancer metastasis. The assays may also be of more broad interest to researchers interested in studying aspects of cellular behaviour in relation to other developmental and disease processes.
Sujet(s)
Dosage biologique , Transition épithélio-mésenchymateuse/génétique , Matrice extracellulaire/composition chimique , Modèles biologiques , Néovascularisation pathologique/anatomopathologie , Lignée cellulaire tumorale , Mouvement cellulaire , Chambres de culture à diffusion , Cellules endothéliales/métabolisme , Cellules endothéliales/anatomopathologie , Matrice extracellulaire/anatomopathologie , Matrice extracellulaire/ultrastructure , Colorants fluorescents/composition chimique , Gélatine/composition chimique , Gélatine/métabolisme , Or colloïdal/composition chimique , Humains , Invasion tumorale , Métastase tumorale , Tumeurs/vascularisation , Tumeurs/génétique , Tumeurs/métabolisme , Tumeurs/anatomopathologie , Néovascularisation pathologique/génétique , Néovascularisation pathologique/métabolisme , ProtéolyseRÉSUMÉ
We studied the effect of non-selective agonist of VIP receptors of vasoactive intestinal polypeptide in different concentrations on the frequency, force, and duration of isometric contraction of myocardial strips of the right atrium under conditions of spontaneous activity, as well as the force and duration of contractions of the right ventricle in rats. It was found that the agonist produced a positive inotropic and chronotropic effect that depended on its concentration. The maximum effect was observed at vasoactive intestinal peptide concentration of 10-11 M.
Sujet(s)
Contraction isométrique/effets des médicaments et des substances chimiques , Contraction myocardique/effets des médicaments et des substances chimiques , Récepteur peptide intestinal vasoactif/génétique , Peptide vasoactif intestinal/pharmacologie , Animaux , Chambres de culture à diffusion , Relation dose-effet des médicaments , Expression des gènes , Atrium du coeur/effets des médicaments et des substances chimiques , Ventricules cardiaques/effets des médicaments et des substances chimiques , Contraction isométrique/physiologie , Contraction myocardique/physiologie , Myocarde/métabolisme , Rats , Récepteur peptide intestinal vasoactif/métabolisme , Techniques de culture de tissusRÉSUMÉ
In vitro cultures of primary human airway epithelial cells (hAECs) grown at air-liquid interface have become a valuable tool to study airway biology under normal and pathologic conditions, and for drug discovery in lung diseases such as cystic fibrosis (CF). An increasing number of different differentiation media, are now available, making comparison of data between studies difficult. Here, we investigated the impact of two common differentiation media on phenotypic, transcriptomic, and physiological features of CF and non-CF epithelia. Cellular architecture and density were strongly impacted by the choice of medium. RNA-sequencing revealed a shift in airway cell lineage; one medium promoting differentiation into club and goblet cells whilst the other enriched the growth of ionocytes and multiciliated cells. Pathway analysis identified differential expression of genes involved in ion and fluid transport. Physiological assays (intracellular/extracellular pH, Ussing chamber) specifically showed that ATP12A and CFTR function were altered, impacting pH and transepithelial ion transport in CF hAECs. Importantly, the two media differentially affected functional responses to CFTR modulators. We argue that the effect of growth conditions should be appropriately determined depending on the scientific question and that our study can act as a guide for choosing the optimal growth medium for specific applications.
Sujet(s)
Lignage cellulaire/effets des médicaments et des substances chimiques , Milieux de culture/pharmacologie , Protéine CFTR/génétique , Cellules épithéliales/effets des médicaments et des substances chimiques , H(+)-K(+)-Exchanging ATPase/génétique , Transcriptome , Aminopyridines/pharmacologie , Benzodioxoles/pharmacologie , Différenciation cellulaire/effets des médicaments et des substances chimiques , Lignage cellulaire/génétique , Milieux de culture/composition chimique , Mucoviscidose/génétique , Mucoviscidose/métabolisme , Mucoviscidose/anatomopathologie , Protéine CFTR/métabolisme , Chambres de culture à diffusion , Cellules épithéliales/métabolisme , Cellules épithéliales/anatomopathologie , Régulation de l'expression des gènes , Cellules caliciformes/cytologie , Cellules caliciformes/effets des médicaments et des substances chimiques , Cellules caliciformes/métabolisme , H(+)-K(+)-Exchanging ATPase/métabolisme , Humains , Concentration en ions d'hydrogène , Culture de cellules primaires , Muqueuse respiratoire/effets des médicaments et des substances chimiques , Muqueuse respiratoire/métabolisme , Muqueuse respiratoire/anatomopathologie , Analyse de séquence d'ARNRÉSUMÉ
Agar have long been used as a growth media for plants. Here, we made agar media with embedded fluidic channels to study the effect of exposure to nutrient solution on root growth and pull-out force. Black Eye bean (Vigna Unguiculata) and Mung bean (Vigna Radiata) were used in this study due to their rapid root development. Agar media were fabricated using casting process with removable cores to form channels which were subsequently filled with nutrient solution. Upon germination, beans were transplanted onto the agar media and allowed to grow. Pull-out force was determined at 96, 120 and 144 h after germination by applying a force on the hypocotyl above the gel surface. The effect of nutrients was investigated by comparing corresponding data obtained from control plants which have not been exposed to nutrient solution. Pull-out force of Black Eye bean plantlets grown in agar with nutrient solution in channels was greater than those grown in gel without nutrients and was 110% greater after 144 h of germination. Pull-out force of Mung bean plantlets grown in agar with and without nutrient solution was similar. Tap root lengths of Black Eye bean and Mung Bean plantlets grown in agar with nutrient solution are shorter than those grown without nutrient.
Sujet(s)
Systèmes de délivrance de médicaments/méthodes , Nutriments/pharmacologie , Racines de plante/croissance et développement , Agar-agar/pharmacologie , Chambres de culture à diffusion , Germination/effets des médicaments et des substances chimiques , Phénomènes mécaniques , Nutriments/métabolisme , Vigna/croissance et développementRÉSUMÉ
INTRODUCTION: Patients suffering from degenerative scoliosis curves often present with radicular symptoms mainly on the concave side of their curves. Standard treatment includes posterior decompressions, followed by fusions. These procedures carry large morbidity rates. We have observed resolution of radicular and stenotic symptoms with Direct Lateral Interbody Fusions (DLIF). AIM: In this study we radiographically assess indirect decompression effect of DLIF procedure. METHODS: We conducted a case series of four patients with 2-stage procedures. All patients presented with back pain and leg symptoms. Stage one included the insertion of the DLIF polyetheretherketone cages and rh-BMP2. This was followed by a second stage posterior fixation utilizing percutaneous pedicle screws and rods. Plain radiographs were utilized to determine the concave and convex sides of the scoliosis. Pre- and post-DLIF measurements were made from axial and sagittal MRIs. Measurements included central, subarticular, and foraminal areas. Statistical significance was estimated via paired sample t-test. RESULTS: All patients had complete resolution of leg symptoms with remarkable improvement in all areas measured. When both concave and convex sides of the curve are considered, an increase of 49% in the central canal, 82% in the subarticular area, and 71% in the foraminal area was measured. When only the concave levels were measured, there was a 90% increase (0.22 cm2 vs. 0.41 cm2) in the subarticular area and 77% (0.46 cm2 vs. 0.81 cm2) increase in the foraminal area (p < .001). CONCLUSION: The DLIF procedure provides an indirect decompression of the neural elements along with its role in spinal fusion. This negates the need for posterior decompression surgery in degenerative scoliosis associated with spinal stenosis, which might lead to less blood loss and surgical time in these complex surgeries.
Sujet(s)
Décompression chirurgicale/méthodes , Chambres de culture à diffusion , Vis pédiculaires , Radiculopathie/chirurgie , Scoliose/chirurgie , Arthrodèse vertébrale/méthodes , Sujet âgé , Protéine morphogénétique osseuse de type 2/usage thérapeutique , Femelle , Humains , Imagerie par résonance magnétique , Mâle , Adulte d'âge moyen , Radiculopathie/étiologie , Protéines recombinantes/usage thérapeutique , Études rétrospectives , Scoliose/complicationsRÉSUMÉ
The characterization of degradation of biodegradable materials for tissue regeneration is classically carried out in three steps: in vitro degradation analysis, in vitro cell culture, and in vivo animal experiments. Each step involves an increasing complexity and should serve a more sophisticated material selection, which serves as an orientation to clinical studies and the final application in patients. Recently, the usefulness of degradation analyses is being discussed. In this context, the aim of this work is to increase the importance of in vitro degradation analysis by using flowing media to move closer to the in vivo situation. In the long term, this should lead to a more sensitive biomaterial characterization as well as to a replacement of time-consuming static or quasi-dynamic incubation experiments. The practicability of the novel chamber is demonstrated in context of a degradation study of silica/collagen/calcium phosphate composites in flowing media with physiological (2.4 mM) and lowered (0.5 mM) calcium ion concentrations. This is done by comparison with static and quasi-dynamic incubation experiments. In order to keep all media regimes comparable to each other, for the dynamic experiment, a flow rate was chosen equivalent to the medium exchange in quasi-dynamic incubation. Under flow-through conditions, there is a clearly decreased tendency to lower the calcium concentration, so that a concentration close to the physiological initial situation can be continuously maintained.
Sujet(s)
Implant résorbable , Chambres de culture à diffusion , Test de matériaux/instrumentation , Calcium/composition chimique , Phosphates de calcium/composition chimique , Techniques de culture cellulaire , Collagène/composition chimique , Milieux de culture , Conception d'appareillage , SiliceRÉSUMÉ
CGA1-78 (Vasostatin-1, VS-1) a N-terminal Chromogranin A (CGA)-derived peptide, has been shown to have a protective effect against TNF-α-induced impairment of endothelial cell integrity. However, the mechanisms of this effect have not yet been clarified. CGA47-66 (Chromofungin, CHR) is an important bioactive fragment of CGA1-78. The present study aims to explore the protective effects of CHR on the vascular endothelial cell barrier response to TNF-α and its related Ca2+ signaling mechanisms. EA.hy926 cells were used as a vascular endothelial culture model. The synthetic peptides CHR and CGA4-16 were assessed for their ability to suppress TNF-α-induced EA.hy926 cells hyper-permeability through Transwell® and TEER assays. Changes in [Ca2+]i were measured through confocal laser scanning microscopy. SOC channel currents (Isoc) were measured via patch-clamp analysis. RT-PCR and western blot were used to analyze mRNA and protein expression of the transient receptor potential channels TRPC1 and TRPC4, respectively. FITC and rhodamine-phalloidin fluorescence were used to assess cell morphology and the distribution of MyPT-1 and F-actin. Compared to untreated cells, TNF-α increased the permeability of EA.hy926 cells that was inhibited by pre-treatment with CHR (10-1000 nM) in concentration-dependent manner, and the effect was most obvious at 100 nM, but CGA4-16 (100 nM) had no effect. TNF-α treatment increased the phosphorylation of MyPT-1 and stress fiber formation. CHR (10-1000 nM) pretreatment inhibited the cytoskeletal rearrangements and increased [Ca2+]i in response to TNF-α treatment. CHR also reduced TRPC1 expression following TNF-α induction. Similar to SOC inhibitor 2-APB, CHR suppressed IP3 mediated SOC activation. These findings suggest that CHR inhibits TNF-α-induced Ca2+ influx and protects the barrier function of vascular endothelial cells, and that these effects are related to the inhibition of SOC and Ca2+ signaling by CHR.
Sujet(s)
Signalisation calcique/effets des médicaments et des substances chimiques , Chromogranine A/pharmacologie , Cellules endothéliales/effets des médicaments et des substances chimiques , Fragments peptidiques/pharmacologie , Canaux cationiques TRPC/métabolisme , Facteur de nécrose tumorale alpha/antagonistes et inhibiteurs , Cytosquelette d'actine/effets des médicaments et des substances chimiques , Cytosquelette d'actine/métabolisme , Cytosquelette d'actine/ultrastructure , Actines/génétique , Actines/métabolisme , Calcium/métabolisme , Lignée de cellules transformées , Perméabilité des membranes cellulaires/effets des médicaments et des substances chimiques , Chambres de culture à diffusion , Relation dose-effet des médicaments , Cellules endothéliales/cytologie , Cellules endothéliales/métabolisme , Régulation de l'expression des gènes , Humains , Inositol 1,4,5-trisphosphate/métabolisme , Myosin-light-chain phosphatase/génétique , Myosin-light-chain phosphatase/métabolisme , Techniques de patch-clamp , Phosphorylation , Canaux cationiques TRPC/antagonistes et inhibiteurs , Canaux cationiques TRPC/génétique , Facteur de nécrose tumorale alpha/pharmacologieRÉSUMÉ
Pancreatic cancer has a high mortality rate due to poor rates of early diagnosis. One tumor suppressor gene in particular, p53, is frequently mutated in pancreatic cancer, and mutations in p53 can inactivate normal wild type p53 activity and increase expression of transcription factor forkhead box M1 (FoxM1). Overexpression of FoxM1 accelerates cellular proliferation and cancer progression. Therefore, inhibition of FoxM1 represents a therapeutic strategy for treating pancreatic cancer. Broussoflavonol B (BF-B), isolated from the stem bark of Broussonetia kazinoki Siebold has previously been shown to inhibit the growth of breast cancer cells. This study aimed to investigate whether BF-B exhibits anti-pancreatic cancer activity and if so, identify the underlying mechanism. BF-B reduced cell proliferation, induced cell cycle arrest, and inhibited cell migration and invasion of human pancreatic cancer PANC-1 cells (p53 mutated). Interestingly, BF-B down-regulated FoxM1 expression at both the mRNA and protein level. It also suppressed the expression of FoxM1 downstream target genes, such as cyclin D1, cyclin B1, and survivin. Cell cycle analysis showed that BF-B induced the arrest of G0/G1 phase. BF-B reduced the phosphorylation of extracellular signal-regulated kinase ½ (ERK½) and expression of ERK½ downstream effector c-Myc, which regulates cell proliferation. Furthermore, BF-B inhibited cell migration and invasion, which are downstream functional properties of FoxM1. These results suggested that BF-B could repress pancreatic cancer cell proliferation by inactivation of the ERK/c-Myc/FoxM1 signaling pathway. Broussoflavonol B from Broussonetia kazinoki Siebold may represent a novel chemo-therapeutic agent for pancreatic cancer.
Sujet(s)
Antinéoplasiques d'origine végétale/pharmacologie , Broussonetia/composition chimique , Flavonols/pharmacologie , Protéine M1 à motif en tête de fourche/génétique , Points de contrôle de la phase G1 du cycle cellulaire/effets des médicaments et des substances chimiques , Régulation de l'expression des gènes tumoraux , Antinéoplasiques d'origine végétale/isolement et purification , Apoptose/effets des médicaments et des substances chimiques , Apoptose/génétique , Lignée cellulaire tumorale , Mouvement cellulaire/effets des médicaments et des substances chimiques , Prolifération cellulaire/effets des médicaments et des substances chimiques , Cycline B1/génétique , Cycline B1/métabolisme , Cycline D1/génétique , Cycline D1/métabolisme , Chambres de culture à diffusion , Flavonols/isolement et purification , Protéine M1 à motif en tête de fourche/antagonistes et inhibiteurs , Protéine M1 à motif en tête de fourche/métabolisme , Points de contrôle de la phase G1 du cycle cellulaire/génétique , Humains , Mitogen-Activated Protein Kinase 1/génétique , Mitogen-Activated Protein Kinase 1/métabolisme , Mitogen-Activated Protein Kinase 3/génétique , Mitogen-Activated Protein Kinase 3/métabolisme , Pancréas/métabolisme , Pancréas/anatomopathologie , Écorce/composition chimique , Extraits de plantes/composition chimique , Protéines proto-oncogènes c-myc/génétique , Protéines proto-oncogènes c-myc/métabolisme , Transduction du signal , Survivine/génétique , Survivine/métabolisme , Protéine p53 suppresseur de tumeur/génétique , Protéine p53 suppresseur de tumeur/métabolismeRÉSUMÉ
This study sought to investigate the biological effects of specific MIF inhibitor, ISO-1, on the proliferation, migration and invasion of PANC-1 human pancreatic cells in vitro, and on tumour growth in a xenograft tumour model in vivo. The effect of ISO-1 on PANC-1 cell proliferation was examined using CCK-8 cell proliferation assay. The effect of ISO-1 on collective cell migration and recolonization of PANC-1 cells was evaluated using the cell-wound closure migration assay. The effect of ISO-1 on the migration and invasion of individual PANC-1 cells in a 3-dimensional environment in response to a chemo-attractant was investigated through the use of Transwell migration/invasion assays. Quantitative real time PCR and western blot analyses were employed to investigate the effects of ISO-1 on MIF, NF-κB p65 and TNF-α mRNA and protein expression respectively. Finally, a xenograft tumor model in BALB/c nude mice were used to assess the in vivo effects of ISO-1 on PANC-1-induced tumor growth. We found high expression of MIF in pancreatic cancer tissues. We demonstrated that ISO-1 exerts anti-cancer effects on PANC-1 cell proliferation, migration and invasion in vitro, and inhibited PANC-1 cell-induced tumour growth in xenograft mice in vivo. Our data suggests that ISO-1 and its derivative may have potential therapeutic applications in pancreatic cancer.