Your search keyword '"Cell migration assays"' showing total 1,073 results

201. CT-1 induces angiogenesis by regulating the ADMA/DDAH Pathway

Author

Zhen Zhong Zheng, Xiao Tian Fu, Zhi Bing Guo, and Jin Liang

Subjects

Vascular Endothelial Growth Factor A, medicine.medical_specialty, Arginine, Nitric Oxide Synthase Type III, Angiogenesis, Neovascularization, Physiologic, lcsh:Medicine, Biology, Tetraspanin 24, Nitric Oxide, Transfection, General Biochemistry, Genetics and Molecular Biology, Amidohydrolases, chemistry.chemical_compound, angiogenesis, Cell Movement, Internal medicine, medicine, Citrulline, Human Umbilical Vein Endothelial Cells, enos, Humans, RNA, Messenger, Cells, Cultured, Cell Proliferation, Tube formation, Matrigel, Cell growth, lcsh:R, Molecular biology, Endothelial stem cell, ddah, Vascular endothelial growth factor A, Endocrinology, chemistry, Cytokines, Endothelium, Vascular, cardiotrophin-1 (ct-1), Cell Migration Assays, Signal Transduction, adma

Abstract

Background. Cardiotrophin-1 (CT-1), a member of the IL-6 superfamily, is elevated in the serum of patients with ischemic and valvular heart disease. In this study, we hypothesized that CT-1 induces endothelial cell angiogenesis and that the ADMA/DDAH pathway plays an important role in the process. Methods. pEGFP-N1-CTF1-GFP and pEGFP-N1 were constructed and used to transiently transfect to HUVECs, mediated by LipofectamineTM 2000. After transfection, the expression of CT-1 was examined by qRT-PCR and western blotting. Endothelial cell proliferation assay was evaluated using the 3-[4,5-dimethylthiazol-2-yl]-2,5 diphenyltetrazolium bromide (MTT) method. Migration assay was performed using transwell, tube formation test was examined on Matrigel, eNOSmRNA expression was assayed by qRT-PCR, DDAH I, DDAHII and VEGF expression were detected by western blotting, the level of ADMA and the activity of DDAH were measured by High Performance Liquid Chromatography, NOS activity and the concentration of NO were assayed by L-[3H] citrulline production from L-[3H]arginine. Results: Overexpression of CT-1, increased endothelial cell proliferation, migration and formation of blood vessels, upregulated the expression of eNOSmRNA, DDAHI, DDAHII and VEGF, elevated the activity of DDAH and NOS, decreased the level of ADMA and promoted NO synthesis. In contrast, ADMA partially inhibited the effects of CT-1 induction. Conclusions: Overexpression of CT-1 increases cell proliferation, migration and formation of blood vessels. This result also suggests that CT-1 may regulate angiogenesis through the ADMA/DDAH pathway.

Published

2015

202. Roles of store-operated Ca2+channels in regulating cell cycling and migration of human cardiac c-kit+progenitor cells

Author

Hui Che, Yan Wang, Guo-Sheng Xiao, Gang Li, Gui-Rong Li, and Hai-Ying Sun

Subjects

Cyclin E, ORAI1 Protein, Physiology, Biology, Cyclin D1, Cell Movement, Physiology (medical), Humans, Immunoprecipitation, Calcium Signaling, Stromal Interaction Molecule 1, Phosphorylation, RNA, Small Interfering, Progenitor cell, Cells, Cultured, Cell Proliferation, TRPC Cation Channels, Calcium signaling, Microscopy, Confocal, Voltage-dependent calcium channel, Reverse Transcriptase Polymerase Chain Reaction, Cell growth, Myocardium, Stem Cells, Cell Cycle, Membrane Proteins, Cell cycle, Neoplasm Proteins, Cell biology, Proto-Oncogene Proteins c-kit, Gene Knockdown Techniques, Cancer research, Calcium Channels, Stem cell, Cell Migration Assays, Cardiology and Cardiovascular Medicine, Proto-Oncogene Proteins c-akt

Abstract

Cardiac c-kit+progenitor cells are important for maintaining cardiac homeostasis and can potentially contribute to myocardial repair. However, cellular physiology of human cardiac c-kit+progenitor cells is not well understood. The present study investigates the functional store-operated Ca2+entry (SOCE) channels and the potential role in regulating cell cycling and migration using confocal microscopy, RT-PCR, Western blot, coimmunoprecipitation, cell proliferation, and migration assays. We found that SOCE channels mediated Ca2+influx, and TRPC1, STIM1, and Orai1 were involved in the formation of SOCE channels in human cardiac c-kit+progenitor cells. Silencing TRPC1, STIM1, or Orai1 with the corresponding siRNA significantly reduced the Ca2+signaling through SOCE channels, decreased cell proliferation and migration, and reduced expression of cyclin D1, cyclin E, and/or p-Akt. Our results demonstrate the novel information that Ca2+signaling through SOCE channels regulates cell cycling and migration via activating cyclin D1, cyclin E, and/or p-Akt in human cardiac c-kit+cells.

Published

2015

203. Periodontal healing with a preameloblast-conditioned medium in dogs

Author

Byung-Ock Kim, Sun-Kyoung Yu, Joo-Cheol Park, Seong-Ho Choi, and Dowon Lee

Subjects

Periodontium, 0301 basic medicine, Adolescent, Periodontal Ligament, Cementoblast, Dentistry, Real-Time Polymerase Chain Reaction, Andrology, Young Adult, 03 medical and health sciences, Calcification, Physiologic, Dogs, 0302 clinical medicine, stomatognathic system, Cell Movement, In vivo, medicine, Animals, Humans, Periodontal fiber, RNA, Messenger, Cementum, Cementogenesis, Tooth Root, Cells, Cultured, Dental Cementum, Wound Healing, business.industry, Chemistry, Cell Differentiation, 030206 dentistry, In vitro, Resorption, Mice, Inbred C57BL, RUNX2, 030104 developmental biology, medicine.anatomical_structure, Culture Media, Conditioned, Periodontics, Molar, Third, Cell Migration Assays, business, Ameloblast

Abstract

Background and Objective The predictability of conventional periodontal treatments for damaged periodontal tissue is limited, particularly on the regeneration of new cementum. As signaling molecules, a range of growth factors has been used to promote periodontal regeneration on periodontal ligament (PDL) and cementum defects. A preameloblast-conditioned medium (PA-CM) was prepared from cultured murine apical bud cells, which can differentiate into ameloblasts. We examined the effect of PA-CM on PDL cells and cementoblasts in vitro and evaluated histologically the effects of PA-CM on the regeneration of experimentally induced periodontal defects in vivo. Material and Methods In vitro, the effects of PA-CM on the migration of human PDL cells were examined using a scratch wound healing assay and a transwell assay. The differentiation and mineralization potential of PA-CM-treated human PDL cells and murine cementoblastic OCCM-30 cells was examined by real-time polymerase chain reaction and Alizarin red-S staining. In vivo, six mongrel dogs (12–16 kg; 6–8 mo old) were used. Twenty-four roots were replanted with either, (i) only periodontal defects (n = 12; control group), or (ii) periodontal defects and PA-CM treatment (n = 12; experimental group). In the experimental group, the PDL and cementum between notches was removed using a Gracey curette and soaked in 0.08 mL water containing 80 μg of a PA-CM for 2 min. The dogs were killed at 4 and 8 wk post-surgery. Results The in vitro results showed that PA-CM stimulated the migration of PDL cells and promoted the differentiation and mineralization of PDL cells and cementoblasts. Real-time polymerase chain reaction analysis revealed stronger expression of Runx2, Osx, OC, Bsp and Cap mRNAs in the PA-CM-treated PDL cells and cementoblasts than those in the control cells. In vivo, newly formed PDL-like tissue and cementum-like tissue were observed partially between the root surfaces and newly formed bone in the experimental group. The regenerated PDL-like tissue in the experimental group was significantly higher than that in the control group at 8 wk (p

Published

2015

204. Local Synthesis of Pepsin in Barrett’s Esophagus and the Role of Pepsin in Esophageal Adenocarcinoma

Author

Tina L. Samuels, Matthew J. Frelich, Nikki Johnston, Jon C. Gould, Craig R. Hoekzema, Matthew I. Goldblatt, Sang Hyuk Lee, and Matthew E. Bosler

Subjects

medicine.medical_specialty, Esophageal Neoplasms, Carcinogenesis, Interleukin-1beta, Adenocarcinoma, Gastroenterology, Article, Barrett Esophagus, Esophagus, Pepsin, Western blot, Internal medicine, Humans, Medicine, Cells, Cultured, Carcinogen, chemistry.chemical_classification, biology, medicine.diagnostic_test, business.industry, Reflux, Proton Pump Inhibitors, General Medicine, medicine.disease, Pepsin A, digestive system diseases, medicine.anatomical_structure, Enzyme, Otorhinolaryngology, chemistry, Barrett's esophagus, Disease Progression, Gastroesophageal Reflux, biology.protein, Cell Migration Assays, business

Abstract

Objective: Despite widespread use of proton pump inhibitors (PPIs), the incidence of esophageal adenocarcinoma (EAC) continues to rise. PPIs reduce reflux acidity, but only transiently inactivate gastric enzymes. Nonacid reflux, specifically nonacid pepsin, contributes to carcinogenesis in the larynx. Given the carcinogenic potential of pepsin and inefficacy of PPIs to prevent EAC, the presence and effect of pepsin in the esophagus should be investigated. Methods: Normal and Barrett’s biopsies from 8 Barrett’s esophagus patients were collected for pepsin analysis via Western blot and reverse transcriptase-polymerase chain reaction (RT-PCR). Human esophageal cells cultured from healthy patients were treated with pepsin (0.01-1 mg/mL; 1-20 hours), acid (pH 4) ± pepsin (5 minutes); real-time RT-PCR, ELISA, and cell migration were assayed. Results: Pepsin was detected in all 8 Barrett’s and 4 of 8 adjacent normal specimens. Pepsinogen mRNA was observed in 22 Barrett’s, but not in normal adjacent samples. Pepsin induced PTSG2 (COX-2) and IL-1β expression and cell migration in vitro. Conclusions: Pepsin is synthesized by metaplastic, Barrett’s esophageal mucosa. Nonacid pepsin increases metrics of tumorigenicity in esophageal epithelial cells in vitro. These findings implicate refluxed and locally synthesized pepsin in development and progression of EAC and, in part, explain the inefficacy of PPIs in the prevention of EAC.

Published

2015

205. Tanshinone IIA attenuates interleukin-17A-induced systemic sclerosis patient-derived dermal vascular smooth muscle cell activation via inhibition of the extracellular signal-regulated kinase signaling pathway

Author

Mengguo Liu, Ji Yang, and Ming Li

Subjects

Adult, Male, medicine.medical_specialty, Vascular smooth muscle, Time Factors, Myocytes, Smooth Muscle, Fluorescent Antibody Technique, Salvia miltiorrhiza, Tanshinone IIA, Pharmacology, Biology, Blotting, Far-Western, Collagen Type I, Muscle, Smooth, Vascular, Statistics, Nonparametric, Cell Movement, Internal medicine, medicine, Humans, Extracellular Signal-Regulated MAP Kinases, Cells, Cultured, Interleukin-17A, Cell Proliferation, lcsh:R5-920, Scleroderma, Systemic, Cell growth, Dermal vascular smooth muscle cells, Anti-Inflammatory Agents, Non-Steroidal, Interleukin-17, Reproducibility of Results, Cell migration, General Medicine, Clinical Science, Middle Aged, Enzyme Activation, Collagen, type I, alpha 1, Endocrinology, Collagen Type III, Abietanes, Systemic sclerosis, Female, Interleukin 17, Extracellular signal-regulated kinase, Signal transduction, lcsh:Medicine (General), Cell activation, Cell Migration Assays

Abstract

OBJECTIVE: Salvia miltiorrhiza has long been used to treat systemic sclerosis. Tanshinone IIA, one of the phytochemicals derived from the roots of Salvia miltiorrhiza, exhibits multiple biological activities. The present study aimed to investigate whether tanshinone IIA has an effect on the interleukin-17A-induced functional activation of systemic sclerosis patient-derived dermal vascular smooth muscle cells. METHODS: Systemic sclerosis patient-derived dermal vascular smooth muscle cells were incubated with various dosages of tanshinone IIA in the presence of interleukin-17A or the serum of systemic sclerosis patients. Cell proliferation was assessed using Cell Counting Kit-8. The expression of collagen 1 and 3 in cells was evaluated by immunofluorescence. Cell migration was measured using a transwell assay. The expression of phospho-extracellular signal-regulated kinase was detected by Western blotting. RESULTS: Our data demonstrate that tanshinone IIA exerts an inhibitory effect on interleukin-17A-induced systemic sclerosis patient-derived dermal vascular smooth muscle cell proliferation, collagen synthesis and migration. CONCLUSION: These findings suggest that tanshinone IIA might serve as a promising therapeutic agent for the treatment of systemic sclerosis.

Published

2015

206. Piperine Inhibits Platelet-Derived Growth Factor-BB-Induced Proliferation and Migration in Vascular Smooth Muscle Cells

Author

Won-Hwan Park, Heeok Hong, Hyuck Kim, Kang Pa Lee, and Kwan Lee

Subjects

Male, MAPK/ERK pathway, Cyclin E, Vascular smooth muscle, MAP Kinase Signaling System, Polyunsaturated Alkamides, Cyclin D, medicine.medical_treatment, Blotting, Western, Myocytes, Smooth Muscle, Becaplermin, Medicine (miscellaneous), Cell Count, Real-Time Polymerase Chain Reaction, p38 Mitogen-Activated Protein Kinases, Muscle, Smooth, Vascular, Rats, Sprague-Dawley, chemistry.chemical_compound, Alkaloids, Piperidines, Cell Movement, Proliferating Cell Nuclear Antigen, medicine, Animals, Benzodioxoles, Cell Proliferation, Nutrition and Dietetics, biology, Gene Expression Profiling, Growth factor, Cell Cycle Checkpoints, Proto-Oncogene Proteins c-sis, Cell cycle, Rats, Cell biology, chemistry, Biochemistry, Piperine, biology.protein, Cell Migration Assays, Cyclin-Dependent Kinase Inhibitor p27, Platelet-derived growth factor receptor

Abstract

The proliferation and migration of vascular smooth muscle cells (VSMCs) in blood vessels are important in the pathogenesis of vascular disorders such as atherosclerosis and restenosis. Piperine, a major component of black pepper, has antioxidant, anticancer, and anti-inflammatory activity. However, the antiatherosclerotic effects of piperine have not been investigated. In this study, the effects of piperine on platelet-derived growth factor (PDGF)-BB-induced proliferation and migration of VSMCs were investigated. The antiproliferative effects of piperine were determined using MTT assays, cell counting, real-time polymerase chain reaction, and western blots. Our results showed that piperine significantly attenuated the proliferation of VSMCs by increasing the expression of p27(kip1), regulating the mRNA expression of cell cycle enzymes (cyclin D, cyclin E, and PCNA), and decreasing the phosphorylation of extracellular signal-regulated kinase (ERK)1/2 in a noncytotoxic concentration-dependent manner (30-100 μM). Moreover, we examined the effects of piperine on the migration of PDGF-BB-stimulated VSMCs, as determined by the Boyden chamber assay, H2DCFDA staining, and western blots. Our results showed that 100 μM piperine decreased cell migration, the production of reactive oxygen species (ROS), and phosphorylation of the p38 mitogen-activated protein kinase (MAPK). Taken together, our results suggest that piperine inhibits PDGF-BB-induced proliferation and the migration of VSMCs by inducing cell cycle arrest and suppressing MAPK phosphorylation and ROS. These findings suggest that piperine may be beneficial for the treatment of vascular-related disorders and diseases.

Published

2015

207. Proteomic and bioinformatic analyses of possible target-related proteins of gambogic acid in human breast carcinoma MDA-MB-231 cells

Author

Min Yang, Miao Liu, Xiao-Yi Song, Li-Xing Feng, De-An Guo, Baohong Jiang, Dong Li, Qing-Xi Yue, Yajun Cui, Xiao-Bo Qu, Xuan Liu, and Wan-Ying Wu

Subjects

Proteomics, Transcription, Genetic, Xanthones, Gene Expression, Antineoplastic Agents, Apoptosis, Breast Neoplasms, Vimentin, Keratin 18, chemistry.chemical_compound, Cell Line, Tumor, Drug Discovery, Humans, Medicine, Electrophoresis, Gel, Two-Dimensional, MTT assay, Cytoskeleton, Cell Proliferation, Keratin-18, biology, Traditional medicine, business.industry, Cell growth, Calcium-Binding Proteins, Computational Biology, General Medicine, Flow Cytometry, Cell biology, Transport protein, Blot, Protein Transport, Complementary and alternative medicine, chemistry, Protein Biosynthesis, Cell Migration Inhibition, Cancer cell, biology.protein, Gambogic acid, Ubiquitin-Specific Proteases, Cell Migration Assays, business, Oxidation-Reduction

Abstract

Gambogic acid (GA) is an anticancer agent in phase ‖b clinical trial in China but its mechanism of action has not been fully clarified. The present study was designed to search the possible target-related proteins of GA in cancer cells using proteomic method and establish possible network using bioinformatic analysis. Cytotoxicity and anti-migration effects of GA in MDA-MB-231 cells were checked using MTT assay, flow cytometry, wound migration assay, and chamber migration assay. Possible target-related proteins of GA at early (3 h) and late stage (24 h) of treatment were searched using a proteomic technology, two-dimensional electrophoresis (2-DE). The possible network of GA was established using bioinformatic analysis. The intracellular expression levels of vimentin, keratin 18, and calumenin were determined using Western blotting. GA inhibited cell proliferation and induced cell cycle arrest at G2/M phase and apoptosis in MDA-MB-231 cells. Additionally, GA exhibited anti-migration effects at non-toxic doses. In 2-DE analysis, totally 23 possible GA targeted proteins were found, including those with functions in cytoskeleton and transport, regulation of redox state, metabolism, ubiquitin-proteasome system, transcription and translation, protein transport and modification, and cytokine. Network analysis of these proteins suggested that cytoskeleton-related proteins might play important roles in the effects of GA. Results of Western blotting confirmed the cleavage of vimentin, increase in keratin 18, and decrease in calumenin levels in GA-treated cells. In summary, GA is a multi-target compound and its anti-cancer effects may be based on several target-related proteins such as cytoskeleton-related proteins.

Published

2015

208. Facile preparation of a photoactivatable surface on a 96-well plate: a versatile and multiplex cell migration assay platform

Author

Olivia Scheideler, Kazuo Yamaguchi, Masao Kamimura, Jun Nakanishi, Yoshihisa Shimizu, and Shota Yamamoto

Subjects

Surface Properties, Ultraviolet Rays, Cell, Drug Evaluation, Preclinical, General Physics and Astronomy, Nanotechnology, Madin Darby Canine Kidney Cells, Polyethylene Glycols, chemistry.chemical_compound, Dogs, Cell Movement, PEG ratio, medicine, Animals, Polylysine, Multiplex, Physical and Theoretical Chemistry, Cell adhesion, Cytochalasin D, Chemistry, Reproducibility of Results, Epithelial Cells, Cell migration, Equipment Design, medicine.anatomical_structure, Biophysics, Surface modification, Glass, Cell Migration Assays, Ethylene glycol

Abstract

Cell migration is an essential cellular activity in various physiological and pathological processes, such as wound healing and cancer metastasis. Therefore, in vitro cell migration assays are important not only for fundamental biological studies but also for evaluating potential drugs that control cell migration activity in medical applications. In this regard, robust control over cell migrating microenvironments is critical for reliable and quantitative analysis as cell migration is highly dependent upon the microenvironments. Here, we developed a facile method for making a commercial glass-bottom 96-well plate photoactivatable for cell adhesion, aiming to develop a versatile and multiplex cell migration assay platform. Cationic poly-d-lysine was adsorbed to the anionic glass surface via electrostatic interactions and, subsequently, functionalized with poly(ethylene glycol) (PEG) bearing a photocleavable reactive group. The initial PEGylated surface is non-cell-adhesive. However, upon near-ultraviolet (UV) irradiation, the photorelease of PEG switches the surface from non-biofouling to cell-adhesive. With this platform, we assayed cell migration in the following procedure: (1) create cell-attaching regions of precise geometries by controlled photoirradiation, (2) seed cells to allow them to attach selectively to the irradiated regions, (3) expose UV light to the remaining PEGylated regions to extend the cell-adhesive area, (4) analyse cell migration using microscopy. Surface modification of the glass surface was characterized by ζ-potential and contact angle measurements. The PEGylated surface showed cell-resistivity and became cell-adhesive upon releasing PEG by near-UV irradiation. The method was applied for parallelly evaluating the effect of model drugs on the migration of epithelial MDCK cells in the multiplexed platform. The dose-response relationship for cytochalasin D treatment on cell migration behavior was successfully evaluated with high reproducibility. Interestingly, the impact of blebbistatin on cell migration was dependent upon the widths of the migrating regions, resulting in both cases of migration acceleration and deceleration. These results clearly demonstrate that the cellular response to certain drugs is highly affected by their migrating geometries. Therefore, the obtained novel photoactivatable 96-well plate serves as a useful high-throughput platform for the identification of drug candidates that have an effect on cell migration behavior.

Published

2015

209. Arginine–glycine–aspartic acid functional branched semi-interpenetrating hydrogels

Author

John W. Haycock, Richard Plenderleith, Cornelia Rodenburg, Christopher J. Pateman, Stephen Rimmer, Frederik Claeyssens, and Chris Sammon

Subjects

Glycine, Biocompatible Materials, Peptide, macromolecular substances, Arginine, chemistry.chemical_compound, Cell Adhesion, Humans, Organic chemistry, Cell adhesion, Cells, Cultured, Cell Proliferation, chemistry.chemical_classification, Acrylamides, Aspartic Acid, technology, industry, and agriculture, Biomaterial, Hydrogels, General Chemistry, Polymer, Fibroblasts, Condensed Matter Physics, chemistry, Polymerization, Chemical engineering, Cell culture, Acrylamide, Self-healing hydrogels, Cell Migration Assays, Oligopeptides

Abstract

For the first time a series of functional hydrogels based on semi-interpenetrating networks with both\ud branched and crosslinked polymer components have been prepared and we show the successful use of\ud these materials as substrates for cell culture. The materials consist of highly branched poly(N-isopropyl\ud acrylamide)s with peptide functionalised end groups in a continuous phase of crosslinked poly(vinyl\ud pyrrolidone). Functionalisation of the end groups of the branched polymer component with the GRGDS\ud peptide produces a hydrogel that supports cell adhesion and proliferation. The materials provide a new\ud synthetic functional biomaterial that has many of the features of extracellular matrix, and as such can be\ud used to support tissue regeneration and cell culture. This class of high water content hydrogel material\ud has important advantages over other functional hydrogels in its synthesis and does not require postprocessing\ud modifications nor are functional-monomers, which change the polymerisation process,\ud required. Thus, the systems are amenable to large scale and bespoke manufacturing using conventional\ud moulding or additive manufacturing techniques. Processing using additive manufacturing is exemplified\ud by producing tubes using microstereolithography.

Published

2015

210. A ring barrier-based migration assay to assess cell migration in vitro

Author

Timo L.M. ten Hagen, Asha M. Das, Alexander M.M. Eggermont, and Surgery

Subjects

Migration Assay, Standard plate, Chemistry, food and beverages, Cell migration, Matrix (biology), Ring (chemistry), General Biochemistry, Genetics and Molecular Biology, In vitro, Cell biology, Cell polarity, In vitro study, Humans, Cell Migration Assays, Cells, Cultured

Abstract

Cell migration is a key feature of virtually every biological process, and it can be studied in a variety of ways. Here we outline a protocol for the in vitro study of cell migration using a ring barrier-based assay. A 'barrier' is inserted in the culture chamber, which prevents cells from entering a defined area. Cells of interest are seeded around this barrier, and after the formation of a peripheral monolayer the barrier is removed and migration into the cell-free area is monitored. This assay is highly reproducible and convenient to perform, and it allows the deduction of several parameters of migration, including total and effective migration, velocity and cell polarization. An advantage of this assay over the conventional scratch assay is that the cells move over an unaltered and virgin surface, and thus the effect of matrix components on cell migration can be studied. In addition, the cells are not harmed at the onset of the assay. Through computer automation, four individual barrier assays can be monitored at the same time. The procedure can be used in a 12-well standard plate allowing higher throughput, or it can be modified to perform invasion assays. The basic procedure takes 2-3 and to complete.

Published

2015

211. The Functional Role of PMP22 Gene in the Proliferation and Invasion of Osteosarcoma

Author

Zhiping Chen and Shuyong Liu

Subjects

musculoskeletal diseases, Osteosarcoma, MAP Kinase Signaling System, Cell growth, Peroxiredoxins, General Medicine, Biology, medicine.disease, medicine.disease_cause, Metastasis, Primary bone, Lab/In Vitro Research, Cell culture, Cell Line, Tumor, Peripheral myelin protein 22, Cancer research, medicine, Humans, Neoplasm Invasiveness, Cell Migration Assays, Carcinogenesis, Gene, Myelin Proteins, Cell Proliferation

Abstract

Background As the most common primary bone tumor, osteosarcoma has an improved survival rates with advancement of treatment methods. A higher rate of metastasis, however, leads to the aggravation of the disease. Studies have shown that some genes, namely osteosarcoma metastasis-related genes, participate in the process of tumor metastasis. The peripheral myelin protein 22 (PMP22) gene has recently been found to be abundantly expressed in the oncogenesis of osteosarcoma. Its detailed role and function in the tumor metastasis, however, remains unknown. Material/Methods The recombinant retroviral plasmid pcDNA3.1-PMP22 was constructed and used to transfect osteosarcoma cells SOSP-M, whose cell proliferation was measured by MTT method. The formation of tumor cell colony, the cell migration and invasion were also measured. The signal transduction pathway MAPK was further analyzed by Western blotting. Results The pcDNA3.1-PMP22 plasmid was confirmed to have a 305bp PMP22 fragment by EcoRI-XhoI dual digestion. Compared to the control group, osteosarcoma cell invasion was significantly facilitated by the transfection of pcDNA3.1-PMP22 plasmid (p

Published

2015

212. Circ_0091581 Promotes the Progression of Hepatocellular Carcinoma Through Targeting miR-591/FOSL2 Axis.

Author

Ji C, Hong X, Lan B, Lin Y, He Y, Chen J, Liu X, Ye W, Mo Z, She Z, and Lin S

Subjects

Animals, Apoptosis, Carcinogens, Cell Line, Tumor, Cell Migration Assays, Cell Proliferation, Gene Expression Regulation, Neoplastic, Gene Transfer Techniques, Humans, Mice, Transcription Factor AP-1 metabolism, Xenograft Model Antitumor Assays methods, Carcinoma, Hepatocellular genetics, Carcinoma, Hepatocellular pathology, Fos-Related Antigen-2 metabolism, Liver Neoplasms genetics, Liver Neoplasms pathology, MicroRNAs antagonists & inhibitors, MicroRNAs genetics, RNA, Circular genetics, RNA, Circular metabolism

Abstract

Background: Circular RNAs (circRNAs) have shown crucial regulatory roles in cancer biology. We aimed to uncover the role and underlying mechanism of circ_0091581 in hepatocellular carcinoma (HCC) progression., Methods: The abundance of circ_0091581, microRNA-591 (miR-591) and FOS like 2, AP-1 transcription factor subunit (FOSL2) was measured by quantitative real-time polymerase chain reaction. Cell viability, colony formation ability, and invasion ability were assessed by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay, colony formation assay, and transwell invasion assay. The migration ability was analyzed by transwell migration assay and wound healing assay. Flow cytometry was used to evaluate the cell cycle and apoptosis of HCC cells. The interaction between miR-591 and circ_0091581 or FOSL2 was predicted by Circular RNA Interactome database or TargetScan database and confirmed by dual-luciferase reporter assay and RNA immune co-precipitation assay. FOSL2 protein expression was measured by Western blot assay. Xenograft tumor assay was conducted to analyze the role of circ_0091581 in HCC tumor growth in vivo., Results: Circ_0091581 was highly expressed in HCC tissue samples and cell lines in contrast to that in adjacent normal tissue samples and THLE-2 cell line. Circ_0091581 accelerated the viability, colony formation, metastasis, and cell cycle, while it impeded the apoptosis of HCC cells. MiR-591 bound to circ_0091581, and circ_0091581 knockdown-mediated effects in HCC cells were largely overturned by miR-591 silencing. FOSL2 was a target of miR-591, and FOSL2 overexpression largely reversed miR-591 accumulation-induced influences in HCC cells. FOSL2 protein expression was down-regulated by circ_0091581 silencing, and the addition of miR-591 inhibitor partly recovered the expression of FOSL2 in HCC cells. Circ_0091581 interference notably suppressed HCC tumor growth in vivo., Conclusion: Circ_0091581 acted as an oncogene to enhance the viability, colony formation, metastasis and cell cycle and inhibit the apoptosis of HCC cells through targeting miR-591/FOSL2 axis., (© 2020. Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2021

213. Rho/ROCK Pathway Regulates Migration and Invasion of Esophageal Squamous Cell Carcinoma by Regulating Caveolin-1

Author

Ruinuan Wu, Xiaoman Cai, Zhaohui Liu, Suzuan Chen, Guanghua Guo, Jing Yu, and Shengxin Tang

Subjects

0301 basic medicine, Adult, Male, Small interfering RNA, Esophageal Neoplasms, Caveolin 1, Metastasis, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Lab/In Vitro Research, Cell Line, Tumor, medicine, Humans, Neoplasm Invasiveness, Neoplasms, Squamous Cell, Neoplasm Metastasis, RNA, Small Interfering, Rho-associated protein kinase, Aged, Cell Proliferation, Neoplasm Staging, rho-Associated Kinases, biology, Cell growth, Cancer, General Medicine, Rho factor, Middle Aged, medicine.disease, Immunohistochemistry, Rho Factor, 030104 developmental biology, 030220 oncology & carcinogenesis, Lymphatic Metastasis, Cancer research, biology.protein, Carcinoma, Squamous Cell, Female, Esophageal Squamous Cell Carcinoma, Cell Migration Assays, Signal Transduction

Abstract

BACKGROUND Esophageal squamous cell carcinoma (ESCC) is a common cancer with poor prognosis. Caveolin-1 (Cav1) and Rho/ROCK pathway play important roles in tumor metastasis, separately. However, less research was focused on the relationship between Cav1 and Rho/ROCK in ECSS metastasis. Therefore, we investigated the relationship between Cav1 and Rho/ROCK pathway in ESCC metastasis. MATERIAL AND METHODS Cav1 and phosphorylated Cav1 (PY14Cav1) were examined in ESCC and in adjacent and non-tumorous tissues from ESCC patients by immunohistochemistry (IHC). Small interfering RNA (siRNA) targeting Cav1 or Rho/ROCK inhibitor was used to treat EC109, Eca109, TE1, and TE13 cells. Western blotting (WB) was used to detect Cav1 and PY14Cav1 expression. The wound healing scratch test and transwell assays were used to assess migration and invasion. RESULTS Cav1 and PY14Cav1 were gradually expressed at higher levels in ECSS than in adjacent and non-tumor tissues as ESCC stage and lymphatic metastasis increased, and this difference was significant (P

Published

2017

214. MicroRNA-379 inhibits cell proliferation and invasion in glioma via targeting metadherin and regulating PTEN/AKT pathway

Author

Hongqi Zhang and Li Li

Subjects

0301 basic medicine, Cancer Research, Biology, Biochemistry, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Genes, Reporter, Cell Line, Tumor, Glioma, microRNA, Genetics, medicine, Humans, Tensin, PTEN, RNA, Small Interfering, Luciferases, neoplasms, Molecular Biology, Protein kinase B, PI3K/AKT/mTOR pathway, Cell Proliferation, Binding Sites, Oligoribonucleotides, Base Sequence, Brain Neoplasms, Akt/PKB signaling pathway, PTEN Phosphohydrolase, Antagomirs, Membrane Proteins, RNA-Binding Proteins, MTDH, medicine.disease, Gene Expression Regulation, Neoplastic, MicroRNAs, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Cancer research, biology.protein, Molecular Medicine, Cell Migration Assays, Cell Adhesion Molecules, Proto-Oncogene Proteins c-akt, Signal Transduction

Abstract

Numerous microRNAs (miRNAs) are aberrantly expressed in glioma, and implicated in glioma occurrence and development. Therefore, the development of miRNAs as potential therapeutic targets for the treatment of patients with glioma has been proposed. miR‑379 has been shown to be aberrantly expressed in the progression of malignant tumours. However, the expression, biological functions and mechanism of miR‑379 in glioma are yet to be fully understood. Hence, the present study aimed to detect miR‑379 expression, investigate its functional relevance and explore its associated molecular mechanism in glioma. In this study, miR‑379 expression was significantly downregulated in glioma tissues and cell lines. Enforced miR‑379 expression markedly suppressed the cell proliferation and invasion of glioma. Metadherin (MTDH) was identified as a direct target of miR‑379 in glioma. The miR‑379 expression and MTDH mRNA levels exhibited an inverse association in glioma tissues. The restoration of the MTDH expression partially rescued the inhibitory effects of miR‑379 overexpression on glioma cell proliferation and invasion, and the upregulation of miR‑379 inhibited the activation of phosphatase and tensin homolog (PTEN)/AKT serine/threonine kinase (AKT) signaling pathway. Overall, these findings demonstrated that miR‑379 may play tumour‑suppressing roles in glioma through downregulation of MTDH and regulation of the PTEN/AKT signaling pathway, suggesting that miR‑379 might be a possible target for the treatment of patients with this malignancy.

Published

2017

215. Suppression of human breast cancer cells by tectorigenin through downregulation of matrix metalloproteinases and MAPK signaling in�vitro

Author

Xiangdong Kong, Jianliang Shen, Ming Wu, Liangming Pan, Linwen Zeng, and Shaofeng Yuan

Subjects

0301 basic medicine, Cancer Research, Apoptosis, Biochemistry, Cell Line, Metastasis, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Cell Line, Tumor, Genetics, medicine, Humans, Molecular Biology, Protein kinase B, Cell Proliferation, Matrigel, Dose-Response Relationship, Drug, Caspase 3, Chemistry, Cell growth, Cancer, Mesenchymal Stem Cells, Cell cycle, medicine.disease, Antineoplastic Agents, Phytogenic, G1 Phase Cell Cycle Checkpoints, Isoflavones, Gene Expression Regulation, Neoplastic, 030104 developmental biology, Matrix Metalloproteinase 9, Proto-Oncogene Proteins c-bcl-2, Oncology, 030220 oncology & carcinogenesis, Cancer cell, MCF-7 Cells, Cancer research, Matrix Metalloproteinase 2, Molecular Medicine, Female, Mitogen-Activated Protein Kinases, Poly(ADP-ribose) Polymerases, Cell Migration Assays, Proto-Oncogene Proteins c-akt, Signal Transduction

Abstract

Breast cancer is a major life‑threatening malignancy and is the second highest cause of mortality. The aim of the present study was to investigate the effects of tectorigenin (Tec), a Traditional Chinese Medicine, against human breast cancer cells in vitro. MDA‑MB‑231 and MCF‑7 human breast cancer cells were treated with various concentrations of Tec. Cell proliferation was evaluated using the Cell Counting kit‑8 assay, and apoptosis and the cell cycle were examined by flow cytometry. The migratory and invasive abilities of these cells were detected by Transwell and Matrigel assays, respectively. Metastasis‑, apoptosis‑ and survival‑related gene expression levels were measured by reverse transcription‑quantitative polymerase chain reaction and western blotting. The results indicated that Tec was able to inhibit the proliferation of MDA‑MB‑231 and MCF‑7 cells in a dose‑ and time‑dependent manner. Furthermore, Tec treatment induced apoptosis and G0/G1‑phase arrest, and inhibited cell migration and invasion. Tec treatment decreased the expression of matrix metalloproteinase (MMP)‑2, MMP9, BCL‑2, phosphorylated‑AKT and components of the mitogen‑activated protein kinase (MAPK) signaling pathway, and increased the expression of BCL‑2‑associated X, cleaved poly [ADP‑ribose] polymerase and cleaved caspase‑3. In conclusion, Tec treatment suppressed human breast cancer cells through the downregulation of AKT and MAPK signaling and the upregulated expression and/or activity of the caspase family in vitro. Therefore, Tec may be a potential therapeutic drug to treat human breast cancer.

Published

2017

216. MicroRNA-28 promotes cell proliferation and invasion in gastric cancer via the PTEN/PI3K/AKT signalling pathway

Author

Xiaozhen Cheng, Tao Shou, Lihua Li, Lian Deng, Libo Yang, Xiongjie Zhu, Yanfang Zheng, and Jinting Wang

Subjects

0301 basic medicine, Cancer Research, Biochemistry, Phosphatidylinositol 3-Kinases, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Genes, Reporter, Stomach Neoplasms, Cell Line, Tumor, microRNA, Genetics, medicine, Humans, PTEN, Tensin, RNA, Small Interfering, Luciferases, Molecular Biology, PI3K/AKT/mTOR pathway, Cell Proliferation, Binding Sites, Oligoribonucleotides, Base Sequence, Oncogene, biology, PTEN Phosphohydrolase, Antagomirs, Cancer, medicine.disease, Gene Expression Regulation, Neoplastic, MicroRNAs, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Protein kinase B signaling, Cancer cell, biology.protein, Cancer research, Molecular Medicine, Cell Migration Assays, Proto-Oncogene Proteins c-akt, Signal Transduction

Abstract

Gastric cancer is the fourth most common malignant disease and second leading cause of cancer‑associated mortalities worldwide. Previous studies revealed aberrantly expressed microRNAs (miRNAs) in various types of human cancer; these miRNAs play important roles in tumourigenesis and tumour development. miRNAs present a considerable potential for novel therapeutic approaches for treating human cancer. Therefore, the investigation of novel miRNAs involved in gastric cancer progression provides an opportunity to improve the prognosis of patients with gastric cancer. miRNA‑28 (miR‑28) has been investigated with regards to its expression and biological functions in many types of human cancer. However, previous studies have not discussed the expression patterns, roles and associated molecular mechanisms of miR‑28 in gastric cancer. In the present study, miR‑28 expression was identified to be upregulated in gastric cancer tissues and cell lines. miR‑28 inhibition functionally inhibited cell proliferation and invasion in gastric cancer in vitro. Using bioinformatics analysis, luciferase reporter assay, reverse transcription‑quantitative polymerase chain reaction and western blot analysis, phosphatase and tensin homolog (PTEN) was mechanically identified as a direct target of miR‑28 in gastric cancer. PTEN was downregulated in gastric cancer and negatively correlated with miR‑28 levels. Inhibition of PTEN restored the biological effects of miR‑28 downregulation on the proliferation and invasion of gastric cancer cells. Notably, the downregulation of miR‑28 results in the regulation of the phosphatidylinositol 3‑kinase/protein kinase B signaling pathway in gastric cancer. These results suggested that miR‑28 may be targeted for the development of novel treatments for gastric cancer in the future.

Published

2017

217. miR-373 suppresses gastric cancer metastasis by downregulating vimentin

Author

Xinye Han, Yongmin Yan, Hui Shi, Wenrong Xu, Hui Qian, Wenqian Jiang, Yinghong Shi, and Bin Zhang

Subjects

Male, 0301 basic medicine, Cancer Research, Cell, Apoptosis, Vimentin, Biology, Biochemistry, Metastasis, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Genes, Reporter, Stomach Neoplasms, Cell Line, Tumor, Genetics, medicine, Humans, Luciferases, Molecular Biology, Aged, Cell Proliferation, Binding Sites, Oligoribonucleotides, Base Sequence, Oncogene, digestive, oral, and skin physiology, Antagomirs, Cancer, Middle Aged, Cell cycle, medicine.disease, Molecular medicine, Gene Expression Regulation, Neoplastic, MicroRNAs, 030104 developmental biology, medicine.anatomical_structure, Oncology, Lymphatic Metastasis, 030220 oncology & carcinogenesis, Cancer cell, biology.protein, Cancer research, Molecular Medicine, Female, Neoplasm Grading, Cell Migration Assays, Signal Transduction

Abstract

MicroRNA-373 (miR-373) has been reported to be an oncogene in a number of solid human tumors. However, the role of miR‑373 in gastric cancer has not been completely elucidated and the mechanisms remain unclear. In the present study, we compared miR‑373 expression between clinical gastric cancer tissues and paired non‑tumorous tissues by reverse transcription‑quantitative polymerase chain reaction. The impact of miR‑373 on proliferation, migration and invasion in gastric cancer cells was additionally investigated. Hsa‑miR‑373 mimics were applied to mimic the function of endogenous miR‑373. A colony formation assay and flow cytometry were performed to analyze the proliferation of gastric cancer cells. Wound healing and Transwell invasion assays were employed to detect the migratory and invasive abilities of gastric cancer cells. Western blotting was used to test the expression of epithelial‑mesenchymal transition‑associated proteins. The results demonstrated that the level of miR‑373 in gastric cancer was upregulated compared with paired non‑tumorous tissues. It was confirmed that miR‑373 inhibited the migration and invasion of the gastric cancer cell lines SGC‑7901 and HGC‑27 by downregulating vimentin expression. The results of the present study demonstrated an oncogenic role of miR‑373 in the metastasis of human gastric cancer, and may provide a novel therapeutic strategy for gastric cancer.

Published

2017

218. MicroRNA-381 inhibits cell proliferation and invasion in endometrial carcinoma by targeting the IGF-1R

Author

Chunhua Tu, Fen Wang, and Junhui Wan

Subjects

0301 basic medicine, Cancer Research, Biology, medicine.disease_cause, Biochemistry, Receptor, IGF Type 1, 03 medical and health sciences, 0302 clinical medicine, Growth factor receptor, Cell Movement, Genes, Reporter, Cell Line, Tumor, microRNA, Genetics, medicine, Humans, Neoplasm Invasiveness, Luciferases, Molecular Biology, Protein kinase B, Cell Proliferation, Mitogen-Activated Protein Kinase 1, Binding Sites, Mitogen-Activated Protein Kinase 3, Oligoribonucleotides, Base Sequence, Oncogene, Antagomirs, Receptors, Somatomedin, Cell cycle, Endometrial Neoplasms, Gene Expression Regulation, Neoplastic, MicroRNAs, 030104 developmental biology, Oncology, Lymphatic Metastasis, 030220 oncology & carcinogenesis, Cancer research, Molecular Medicine, Female, Ectopic expression, Signal transduction, Cell Migration Assays, Carcinogenesis, Proto-Oncogene Proteins c-akt, Plasmids, Signal Transduction

Abstract

Endometrial carcinoma (EC) is the sixth most common type of malignant tumor occurring in females. MicroRNAs (miRNAs) serve as oncogenes or tumor suppressors in human cancer and play important roles in tumorigenesis, and tumor development by regulating various processes. Thus, further investigation into miRNAs involved in EC formation and progression may aid in developing effective therapeutic strategies for patients with this disease. miRNA‑381 (miR‑381) is aberrantly expressed in multiple types of human cancer. However, the expression pattern, biological roles and underlying mechanisms of miR‑381 in EC are poorly understood. In the present study, the results showed that miR‑381 was downregulated in EC tissues and cell lines. Decreased miR‑381 expression correlated with the International Federation of Gynecology and Obstetrics stage, lymph nodes metastasis and myometrial invasion of EC. The ectopic expression of miR‑381 significantly inhibited the proliferation and invasion of EC cells. Through a series of experiments, the insulin‑like growth factor receptor 1 (IGF‑1R) was identified as a novel direct target of miR‑381 in EC. Furthermore, IGF‑1R was highly expressed in EC tissues and inversely correlated with miR‑381 levels. IGF‑1R overexpression partially abrogated the tumor‑suppressive effects of miR‑381 on the proliferation and invasion of EC cells. miR‑381 targeted IGF‑1R to inactivate the protein kinase B (AKT) and extracellular signal‑regulated kinase (ERK) signaling pathways in EC. These results suggest that miR‑381 acts as a tumor suppressor in EC by directly targeting IGF‑1R, and indirectly regulating the AKT and ERK signaling pathways. Thus, miR‑381 should be investigated as a prognostic biomarker and novel therapeutic target for the treatment of patients with EC.

Published

2017

219. Using the Dot Assay to Analyze Migration of Cell Sheets

Author

Christina H. Stuelten

Subjects

0301 basic medicine, Cancer Research, General Chemical Engineering, Immunoblotting, Breast Neoplasms, Biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Mice, Breast cancer, Epidermal growth factor, Cell Line, Tumor, medicine, Animals, Humans, Cell sheet, Migration Assay, General Immunology and Microbiology, General Neuroscience, Cell migration, medicine.disease, Phenotype, Epithelium, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Cell culture, Female, Cell Migration Assays

Abstract

Although complex organisms appear static, their tissues are under a continuous turnover. As cells age, die, and are replaced by new cells, cells move within tissues in a tightly orchestrated manner. During tumor development, this equilibrium is disturbed, and tumor cells leave the epithelium of origin to invade the local microenvironment, to travel to distant sites, and to ultimately form metastatic tumors at distant sites. The dot assay is a simple, two-dimensional unconstrained migration assay, to assess the net movement of cell sheets into a cell-free area, and to analyze parameters of cell migration using time-lapse imaging. Here, the dot assay is demonstrated using a human invasive, lung colony forming breast cancer cell line, MCF10CA1a, to analyze the cells' migratory response to epidermal growth factor (EGF), which is known to increase malignant potential of breast cancer cells and to alter the migratory phenotype of cells.

Published

2017

220. Long non-coding RNA LINC00261 sensitizes human colon cancer cells to cisplatin therapy

Author

Z.K. Wang, P.F. Zhang, L. Yang, H. Mao, G.H. Dai, L.L. Wu, and Ying Zhou

Subjects

0301 basic medicine, Physiology, Colorectal cancer, Tetrazolium Salts, Apoptosis, Biochemistry, 0302 clinical medicine, General Pharmacology, Toxicology and Pharmaceutics, lcsh:QH301-705.5, Research Articles, beta Catenin, lcsh:R5-920, Reverse Transcriptase Polymerase Chain Reaction, General Neuroscience, Wnt signaling pathway, General Medicine, Colon cancer, Gene Expression Regulation, Neoplastic, 030220 oncology & carcinogenesis, Colonic Neoplasms, RNA, Long Noncoding, Mechanism, Cell Migration Assays, lcsh:Medicine (General), HT29 Cells, medicine.drug, Signal Transduction, Immunology, Blotting, Western, Biophysics, Down-Regulation, Ocean Engineering, Antineoplastic Agents, Biology, 03 medical and health sciences, Downregulation and upregulation, medicine, Humans, Viability assay, Cisplatin resistance, Cell Proliferation, Cisplatin, Analysis of Variance, Cancer, Reproducibility of Results, Cell Biology, β-catenin, medicine.disease, HCT116 Cells, Thiazoles, 030104 developmental biology, lcsh:Biology (General), Cell culture, Cancer research, Apoptosis Regulatory Proteins, LINC00261

Abstract

Colon cancer is one of the most common digestive tumors. The present study aimed to explore the functional role, as well as the underlying mechanism of long non-coding RNA LINC00261 in colon cancer. Expression of LINC00261 was analyzed in colon cancer cell lines and human normal cell lines. Acquired resistance cell lines were then built and the acquired resistance efficiency was detected by evaluating cell viability. Thereafter, the effects of LINC00261 overexpression on cisplatin-resistant colon cancer cells were measured, as well as cell apoptosis, viability, migration, and invasion. Subsequently, we investigated the interaction of LINC00261 and β-catenin. The results showed that the LINC00261 gene was down-regulated in colon cancer cell lines and tissues, and in cisplatin-resistant cells. LINC00261 overexpression might relieve cisplatin resistance of colon cancer cells via promoting cell apoptosis, and inhibiting cell viability, migration, and invasion. Moreover, LINC00261 might down-regulate nuclear β-catenin through restraining β-catenin from cytoplasm into nuclei or it could also promote β-catenin degradation and inhibit activation of Wnt pathway. Finally, LINC00261 reduced cisplatin resistance of colon cancer in vivo and enhanced the anti-colon cancer effect of cisplatin through reducing tumor volume and weight.

Published

2017

221. Epithelial-to-Mesenchymal Transition and Migration of Human Peritoneal Mesothelial Cells Undergoing Senescence

Author

Janusz Witowski, Edyta Kawka, Andras Rudolf, Manuel López Cabrera, Pilar Sandoval, Angela Rynne Vidal, and Achim Jörres

Subjects

0301 basic medicine, Senescence, Epithelial-Mesenchymal Transition, medicine.medical_treatment, Cell Culture Techniques, Real-Time Polymerase Chain Reaction, Peritoneal dialysis, 03 medical and health sciences, 0302 clinical medicine, Peritoneum, Transforming Growth Factor beta, Medicine, Humans, In patient, Epithelial–mesenchymal transition, Cellular Senescence, biology, business.industry, Mesothelial cell senescence, transforming growth factor-beta, Epithelial Cells, General Medicine, Transforming growth factor beta, Immunohistochemistry, body regions, 030104 developmental biology, medicine.anatomical_structure, Nephrology, 030220 oncology & carcinogenesis, biology.protein, Cancer research, Thickening, business, Cell Migration Assays, Mesothelial Cell, Signal Transduction

Abstract

Background Epithelial-to-mesenchymal transition (EMT) of human peritoneal mesothelial cells (HPMCs) contributes to fibrotic thickening of the peritoneum that develops in patients on peritoneal dialysis (PD). The process is thought to be largely mediated by transforming growth factor-beta (TGF-β). As TGF-β has also been implicated in senescence of HPMCs, we have performed an exploratory study to examine if senescent HPMCs can undergo EMT. Methods Omentum-derived HPMCs were rendered senescent by repeated passages in culture. Features of EMT were assessed by immunostaining and quantitative polymerase chain reaction (qPCR) at various stages of the HPMC lifespan and after treatment with or without TGF-β. The motility of HPMCs was assessed in a scratch wound migration assay. Results Replicative senescence of HPMCs was associated with a gradual increase in the constitutive expression of EMT markers, including increased production of extracellular matrix proteins. However, senescent HPMCs also retained epithelial cell features such as cytokeratin, calretinin, and E-cadherin and showed decreased, rather than increased, motility. In contrast, exposure to TGF-β resulted in an up-regulation of mesenchymal markers and down-regulation of epithelial markers. Such effects of TGF-β occurred both in young and senescent cells, although they were less pronounced in senescence. Conclusions Senescence of HPMCs is associated with spontaneous development of several EMT features. At the same time, senescent HPMCs preserve epithelial cell-like characteristics and are less prone to develop a full EMT phenotype in response to TGF-β. These observations may support the concept of cellular senescence being antagonistically pleiotropic with regard to EMT.

Published

2017

222. Effect of metformin combined with chemotherapeutic agents on gastric cancer cell line AGS

Author

Xiaochang, Wu

Subjects

Time Factors, Dose-Response Relationship, Drug, Paclitaxel, Apoptosis, Drug Synergism, Metformin, Doxorubicin, Stomach Neoplasms, Cell Line, Tumor, Humans, Neoplasm Invasiveness, Cisplatin, Cell Migration Assays, Cell Proliferation

Abstract

To explore the effect of metformin combined with chemotherapeutic agents on gastric cancer cell line AGS, 24 patients with gastric cancer were tracked for treatment. CCK-8, Transwell model and flow cytometry were used to detect the cell proliferation, migration ability and other indexes. The metformin inhibited the AGS cell proliferation in a dose- and time-dependent manner (P0.05). The application of metformin, cisplatin, adriamycin or paclitaxel alone could effectively lower the migration and invasion ability of AGS cells. The metformin in combination with the three chemotherapeutic agents could effectively promote the apoptosis of AGS cells. The metformin in combination with chemotherapeutic agents can effectively and apparently treat the patients with gastric cancer, more significantly in clinic compared to the traditional administration mode. It can effectively promote the apoptosis of AGS cells, thus, it's worth adopting in clinic.

Published

2017

223. Wnt/β-catenin and ERK pathway activation: A possible mechanism of photobiomodulation therapy with light-emitting diodes that regulate the proliferation of human outer root sheath cells

Author

Jung E, Kim, Young J, Woo, Ki M, Sohn, Kwan H, Jeong, and Hoon, Kang

Subjects

Cell Survival, MAP Kinase Signaling System, Blotting, Western, Apoptosis, Real-Time Polymerase Chain Reaction, Cell Movement, Cytokines, Humans, Intercellular Signaling Peptides and Proteins, Low-Level Light Therapy, Cell Migration Assays, Hair Follicle, Wnt Signaling Pathway, Biomarkers, Cells, Cultured, Cell Proliferation

Abstract

Outer root sheath cells (ORSCs) play important roles in maintaining hair follicle structure and provide support for the bulge area. The hair growth promoting effects of photobiomodulation therapy (PBMT) have been reported, but the mechanisms for this in human ORCs (hORSCs) have rarely been studied.The aim of this study was to investigate the effect of various wavelengths of light-emitting diode (LED) irradiation on human ORSCs (hORSCs).LED irradiation effects on hORSC proliferation and migration were examined with MTT assay, BrdU incorporation assay and migration assays. hORSCs were irradiated using four LED wavelengths (415, 525, 660, and 830 nm) with different low energy levels. LED irradiation effects on the expression of molecules associated with the Wnt/β-catenin signaling and ERK pathway, hair stem cell markers, and various growth factors and cytokines in hORSCs were examined with real-time PCR and Western blot assay. The effect of the LED-irradiated hORSCs on cell proliferation of human dermal papilla cells (hDPCs) was examined with co-culture and MTT assay.PBMT with LED light variably promoted hORSC proliferation and suppressed cell apoptosis depending on energy level. LED irradiation induced Wnt5a, Axin2, and Lef1 mRNA expression and β-catenin protein expression in hORSCs. Phosphorylation of ERK, c-Jun, and p38 in hORSCs was observed after LED light irradiation, and ERK inhibitor treatment before irradiation reduced ERK and c-Jun phosphorylation. Red light-treated hORSCs showed substantial increase in IL-6, IL-8, TNF-a, IGF-1, TGF-β1, and VEGF mRNA. Light irradiation at 660 and 830 nm projected onto hORSCs accelerated in vitro migration. LED-irradiated hORSCs increased hDPCs proliferation when they were co-cultured. The conditioned medium from LED-irradiated hORSCs was sufficient to stimulate hDPCs proliferation.These results demonstrate that LED light irradiation induced hORSC proliferation and migration and inhibited apoptosis in vitro. The growth-promoting effects of LEDs on hORSCs appear to be associated with direct stimulation of the Wnt5a/β-catenin and ERK signaling pathway. Lasers Surg. Med. 49:940-947, 2017. © 2017 Wiley Periodicals, Inc.

Published

2017

224. Up-regulation of long non-coding RNA PCAT-1 correlates with tumor progression and poor prognosis in gastric cancer

Author

W-C, Cui, Y-F, Wu, and H-M, Qu

Subjects

Male, Apoptosis, Kaplan-Meier Estimate, Middle Aged, Prognosis, Up-Regulation, Stomach Neoplasms, Cell Line, Tumor, Lymphatic Metastasis, Biomarkers, Tumor, Disease Progression, Humans, Female, Neoplasm Invasiveness, RNA, Long Noncoding, Cell Migration Assays, Aged, Cell Proliferation

Abstract

Long non-coding RNAs (lncRNAs), emerging non-coding RNAs, have been proved to serve as a critical role in the proliferation, metastasis apoptosis of gastric cancer. However, the potential biological role PCAT-1 in gastric cancer (GC) remains undefined. The present study aimed to investigate the expression and clinical significance of PCAT-1 in GC.The expression of PCAT-1 was detected with a quantitative Real-time PCR assay. The association between PCAT-1 expression and clinicopathological factors, as well as survival rates, was analyzed. Cox proportional-hazards regression analysis was applied in order to estimate univariate and multivariate hazard ratios for overall survival. Then, effects of PCAT-1 on the biological behavior of GC cells were investigated.We found that PCAT-1 expression was elevated in GC tissues and cell lines, and PCAT-1 levels were highly positively correlated with invasion depth (p0.001), TNM stages (p0.001) and lymphatic metastasis (p = 0.003). The biological function of PCAT-1 was explored and the results showed silencing of PCAT-1 could suppress cell proliferation, migration and invasion in vitro. Kaplan-Meier analysis demonstrated that increased PCAT-1 expression contributed to poor overall survival (OS) (p0.01). Furthermore, in a multivariate Cox model, our results showed that PCAT-1 expression was an independent poor prognostic factor for OS in GC.Our finding suggested that PCAT-1 may have potential roles as a biomarker and/or a therapeutic target in gastric cancer.

Published

2017

225. MicroRNA-124a inhibits cell proliferation and migration in liver cancer by regulating interleukin-11

Author

Shuo Wang, Pengcheng Gu, Liedao Yu, Yang Lu, and Xiangjin Lin

Subjects

0301 basic medicine, STAT3 Transcription Factor, Cancer Research, MMP2, Apoptosis, Biochemistry, Metastasis, 03 medical and health sciences, Prostate cancer, 0302 clinical medicine, Cell Movement, Genes, Reporter, microRNA, Genetics, medicine, Humans, Phosphorylation, Luciferases, Molecular Biology, Cell Proliferation, Tissue Inhibitor of Metalloproteinase-2, Binding Sites, Oligoribonucleotides, Oncogene, Base Sequence, business.industry, Caspase 3, Cancer, Bone metastasis, Antagomirs, Hep G2 Cells, medicine.disease, Interleukin-11, Gene Expression Regulation, Neoplastic, MicroRNAs, 030104 developmental biology, Oncology, Matrix Metalloproteinase 9, Proto-Oncogene Proteins c-bcl-2, 030220 oncology & carcinogenesis, Cancer research, Molecular Medicine, Matrix Metalloproteinase 2, Liver cancer, business, Cell Migration Assays, Signal Transduction

Abstract

Liver cancer is the sixth most common malignant tumour and ranks in the top three cancers with regard to mortality due to metastasis and postsurgical recurrence. It is significant to understand the mechanisms underlying liver cancer for diagnosis and treatment. Cumulative evidence suggests that the abnormal regulation of microRNAs (miRNAs/miRs) may contribute to the development and metastasis of cancer. miR‑124a acts as a tumour suppressor in osteosarcoma, endometrial carcinoma, prostate cancer, and glioblastoma. However, the effects of miR‑124a in liver cancer and its biological mechanism are not fully understood. It has been demonstrated that miR‑124a is downregulated and interleukin (IL)‑11 is upregulated in the liver cancer tissues. In the present study, miR‑124a upregulation inhibited cell proliferation, migration and promoted cell apoptosis. Through a dual‑luciferase reporter assay, it was verified that IL‑11 is a direct target of miR‑124a. Furthermore, the overexpression of miR‑124a repressed the secretion of IL‑11 from hepatoma cells. Finally, it was identified that mimics of miR‑124a increased the expression of tissue inhibitor of matrix metalloproteinase‑2 (TIMP‑2) and Caspase‑3 and decreased the expression levels of matrix metalloproteinase 2 (MMP2), MMP9, B‑cell lymphoma 2, signal transducer and activator of transcription 3 (STAT3), and phosphorylated‑STAT3. In conclusion, the results indicated that miR‑124a has an important role as a tumour suppressor gene by targeting IL‑11. These findings may provide novel insights for clinical treatments to prevent the development of liver cancer.

Published

2017

226. High-Efficiency Transfection of Glioblastoma Cells and a Simple Spheroid Migration Assay

Author

Carsten, Hagemann, Diana, Amend, Almuth F, Kessler, Thomas, Linsenmann, Ralf-Ingo, Ernestus, and Mario, Löhr

Subjects

Gene Knockout Techniques, Cell Movement, Cell Survival, Cell Line, Tumor, Spheroids, Cellular, Gene Expression, Humans, Cell Migration Assays, Glioblastoma, Transfection

Abstract

Despite international research efforts, patients with glioblastoma multiforme (GBM)-the most common malignant brain tumors in adults-exhibit a very unfavorable prognosis. Their aggressive local growth pattern and increased invasiveness, due to a high motility of the tumor cells, hamper treatment. However, the molecular mechanisms regulating glioblastoma cell migration are still elusive. Here, we describe the combination of a highly efficient cell transfection by Nucleofection

Published

2017

227. Arginine kinase from Haemonchus contortus decreased the proliferation and increased the apoptosis of goat PBMCs in vitro

Author

Javaid Ali Gadahi, Xiaokai Song, Mingmin Lu, XinChao Liu, Ruofeng Yan, Muhammad Ehsan, Wenxiang Gao, Yujian Wang, Lixin Xu, and Xiangrui Li

Subjects

Male, 0301 basic medicine, medicine.medical_treatment, Proliferation, Gene Expression, Apoptosis, Rats, Sprague-Dawley, 0302 clinical medicine, Haemonchus contortus, Gene expression, Cloning, Molecular, Phylogeny, biology, medicine.diagnostic_test, Reverse Transcriptase Polymerase Chain Reaction, Goats, Arginine Kinase, Immunohistochemistry, Recombinant Proteins, Specific Pathogen-Free Organisms, Infectious Diseases, Cytokine, Cytokines, Female, Haemonchus, Cell Migration Assays, Sequence Analysis, Blotting, Western, 030231 tropical medicine, Antibodies, Helminth, Nitric Oxide, Peripheral blood mononuclear cell, lcsh:Infectious and parasitic diseases, 03 medical and health sciences, Immune system, Western blot, medicine, Animals, lcsh:RC109-216, Cell Proliferation, Cell growth, Research, PBMC, Computational Biology, Arginine kinase, Molecular biology, Rats, 030104 developmental biology, Immunology, Leukocytes, Mononuclear, biology.protein, Parasitology

Abstract

Background Arginine kinase (AK), an important member of phosphagen kinase family has been extensively studied in various vertebrates and invertebrates. Immunologically, AKs are important constituents of different body parts, involved in various biological and cellular functions, and considered as immune-modulator and effector for pro-inflammatory cytokines. However, immunoregulatory changes of host cells triggered by AK protein of Haemonchus contortus, a parasitic nematode of ruminants, are still unknown. The current study was focused on cloning and characterisation of Hc-AK, and its regulatory effects on cytokines level, cell migration, cell proliferation, nitric oxide production and apoptosis of goat peripheral blood mononuclear cells (PBMCs) were observed. Methods The full-length sequence of the Hc-AK gene was amplified by reverse transcription-polymerase chain reaction (RT-PCR) and sub-cloned into the prokaryotic expression vector pET-32a. The biochemical characteristics of recombinant protein Hc-AK, which was purified by affinity chromatography, were performed based on the enzymatic assay. Binding of rHc-AK with PBMCs was confirmed by immunofluorescence assay (IFA). Immunohistochemical analysis was used to detect localisation of Hc-AK within adult worms sections. The immunoregulatory effects of rHc-AK on cytokine secretions, cell proliferation, cell migration, nitric oxide production and apoptosis were determined by co-incubation of rHc-AK with goat PBMCs. Results The full-length ORF (1080 bp) of the Hc-AK gene was successfully cloned, and His-tagged AK protein was expressed in the Escherichia coli strain BL21. The recombinant protein of Hc-AK (rHc-AK) was about 58.5 kDa together with the fused vector protein of 18 kDa. The biochemical assay showed that the protein encoded by the Hc-ak exhibited enzymatic activity. Western blot analysis confirmed that the rHc-AK was recognised by the sera from rat (rat-antiHc-AK). The IFA results showed that rHc-AK could bind on the surface of goat PBMCs. Immunohistochemically, Hc-AK was localised at the inner and outer membrane as well as in the gut region of adult worms. The binding of rHc-AK to host cells increased the levels of IL-4, IL-10, IL-17, IFN-γ, nitric oxide (NO) production and cell apoptosis of goat PBMCs, whereas, TGF-β1 levels, cell proliferation and PBMCs migration were significantly decreased in a dose dependent manner. Conclusions Our findings suggested that rHc-AK is an important excretory and secretory (ES) protein involved in host immune responses and exhibit distinct immunomodulatory properties during interaction with goat PBMCs. Electronic supplementary material The online version of this article (doi:10.1186/s13071-017-2244-z) contains supplementary material, which is available to authorized users.

Published

2017

228. Use of Patterned Collagen Coated Slides to Study Normal and Scleroderma Lung Fibroblast Migration

Author

Ahmed Abdi, Bahja, Lopez, Henry, Karrar, Sarah, Renzoni, Elisabetta, Wells, Athol, Tam, Angela, Etomi, Oseme, Hsuan, J. Justin, Martin, George R., Shiwen, Xu, Denton, Christopher P., Abraham, David, Stratton, Richard, Arthritis Research UK, British Lung Foundation, and Raynaud's and Scleroderma Association

Subjects

GROWTH-FACTOR, Science, IMATINIB MESYLATE, PLACEBO-CONTROLLED TRIAL, Article, DOUBLE-BLIND, Cell Movement, Humans, STEM-CELL FACTOR, Lung, Cells, Cultured, DISEASE-MECHANISMS, Platelet-Derived Growth Factor, Extracellular Matrix Proteins, Science & Technology, Scleroderma, Systemic, integumentary system, SYSTEMIC-SCLEROSIS, Fibroblasts, Extracellular Matrix, Multidisciplinary Sciences, Science & Technology - Other Topics, MAST-CELLS, Medicine, IDIOPATHIC PULMONARY-FIBROSIS, Collagen, Cell Migration Assays, SKIN

Abstract

Systemic sclerosis (SSc) is a spreading fibrotic disease affecting the skin and internal organs. We aimed to model pathogenic fibroblast migration in SSc in order to identify enhancing factors, measure the effect of migrating cells on underlying extracellular matrix (ECM) and test possible therapeutic inhibitors. Novel patterned collagen substrates were used to investigate alignment and migration of skin and lung fibroblasts from SSc patients and healthy controls. Normal lung but not skin fibroblasts consistently elongated and aligned with underlying collagen and migrated dependent on PDGF or serum. SSc lung fibroblasts remained growth factor dependent, did not migrate more rapidly and were less restricted to alignment of the collagen. Multiple collagen proline and lysine-modifying enzymes were identified in SSc but not control fibroblast extracellular matrix preparations, indicating differential levels of ECM modification by the diseased cells. Profiling of migrating cells revealed a possible SCF/c-Kit paracrine mechanism contributing to migration via a subpopulation of cells. Heparin, which binds ligands including PDGF and SCF, and imatininib which blocks downstream tyrosine kinase receptors, both inhibited lung fibroblast migration individually but showed synergy in SSc cells. Pathologic lung fibroblasts from SSc patients modify ECM during migration but remain growth factor dependent and sensitive to inhibitors.

Published

2017

229. Characterization of a group I Nme protein of Capsaspora owczarzaki-a close unicellular relative of animals

Author

Martina Deželjin, Helena Ćetković, Iñaki Ruiz-Trillo, Maja Herak Bosnar, Robert Belužić, Matija Harcet, Helena Bilandžija, Andreja Mikoč, and Dragutin Perina

Subjects

0301 basic medicine, Capsaspora, Biology, Pathology and Forensic Medicine, Metastasis Suppression, Evolution, Molecular, NATURAL SCIENCES, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Humans, Metastasis suppressor, Amino Acid Sequence, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Transition (genetics), Kinase, Biochemistry and Molecular Biology, Eukaryota, metastasis suppressor, Nme1, Nm23, Capsaspora owczarzaki, evolution, Cell Biology, NM23 Nucleoside Diphosphate Kinases, biology.organism_classification, Multicellular organism, 030104 developmental biology, Enzyme, chemistry, Biochemistry, Cell Migration Assays, 030217 neurology & neurosurgery, HeLa Cells

Abstract

Nucleoside diphosphate kinases are enzymes present in all domains of life. In animals, they are called Nme or Nm23 proteins, and are divided into group I and II. Human Nme1 was the first protein identified as a metastasis suppressor. Because of its medical importance, it has been extensively studied. In spite of the large research effort, the exact mechanism of metastasis suppression remains unclear. It is unknown which of the biochemical properties or biological functions are responsible for the antimetastatic role of the mammalian Nme1. Furthermore, it is not clear at which point in the evolution of life group I Nme proteins acquired the potential to suppress metastasis, a process that is usually associated with complex animals. In this study we performed a series of tests and assays on a group I Nme protein from filasterean Capsaspora owczarzaki, a close unicellular relative of animals. The aim was to compare the protein to the well-known human Nme1 and Nme2 homologs, as well as with the homolog from a simple animal - sponge (Porifera), in order to see how the proteins changed with the transition to multicellularity, and subsequently in the evolution of complex animals. We found that premetazoan-type protein is highly similar to the homologs from sponge and human, in terms of biochemical characteristics and potential biological functions. Like the human Nme1 and Nme2, it is able to diminish the migratory potential of human cancer cells in culture.

Published

2017

230. Partition-Defective 3 (PARD3) Regulates Proliferation, Apoptosis, Migration, and Invasion in Esophageal Squamous Cell Carcinoma Cells

Author

Zhichao Hou, Ablajan Abdurahmam, Haiping Zhang, Abuduaini Tuerhong, Lei Wang, Ilyar Sheyhidin, and Ayshamgul Hasim

Subjects

0301 basic medicine, Esophageal Neoplasms, Apoptosis, Cell Cycle Proteins, Biology, medicine.disease_cause, 03 medical and health sciences, Cell Movement, Lab/In Vitro Research, Cell Line, Tumor, medicine, Gene silencing, Humans, Neoplasm Invasiveness, Gene Silencing, RNA, Messenger, RNA, Small Interfering, Adaptor Proteins, Signal Transducing, Cell Proliferation, Regulation of gene expression, Cell growth, Cell Cycle, Membrane Proteins, Cell migration, General Medicine, Cell cycle, digestive system diseases, Gene Expression Regulation, Neoplastic, 030104 developmental biology, Phenotype, Cell culture, Cancer research, Carcinoma, Squamous Cell, Esophageal Squamous Cell Carcinoma, Carcinogenesis, Cell Migration Assays

Abstract

BACKGROUND Altered expression of partition-defective 3 (PARD3), a polarity-related gene associated with oncogenesis, has been identified in some cancers, but the role of PARD3 in esophageal squamous cell carcinoma (ESCC) remains unclear. MATERIAL AND METHODS PARD3 expression in Eca109 cells was silenced using siRNA and overexpressed using an expression vector. We investigated the role of PARD3 in ESCC growth and motility to evaluate its potential role in ESCC. Transwell assay was used to evaluated cell migration and invasion. PARD3 protein expression was assessed by Western blot. RESULTS PARD3 overexpression promoted apoptosis, impaired proliferation, and inhibited cell migration and invasion in Eca109 cells, while PARD3 silencing promoted proliferation and increased migration and invasion. Overexpression of PARD3 exerted its antitumor activity in vitro by impairing cell proliferation, inducing apoptosis, and inhibiting migration and invasion of Eca109 cells, suggesting that PARD3 might play a tumor suppressor role in ESCC. CONCLUSIONS Overexpression of PARD3 could be a promising new therapeutic intervention against ESCC.

Published

2017

231. Methods for Studying the Role of RAAS in the Modulation of Vascular Repair-Relevant Functions of Stem/Progenitor Cells

Author

Yagna P R, Jarajapu

Subjects

Colony-Forming Units Assay, Mice, Inbred C57BL, Renin-Angiotensin System, Mice, Immunomagnetic Separation, Stem Cells, Animals, Humans, Bone Marrow Cells, Cell Migration Assays, Flow Cytometry, Cells, Cultured, Cell Proliferation

Abstract

In recent years, previously unknown functions have been conferred to the RAAS and have been explored in mechanistic studies and disease models. Implication of bone marrow stem/progenitor cells in the cardiovascular protective or detrimental effects of RAAS is a prominent advancement because of the translational significance. Selected members of RAAS are now known to modulate migration, proliferation, and mobilization of bone marrow cells in response to ischemic insult, which are sensitive indicators of vascular repair-relevant functions. In this Chapter, protocols for most frequently used, in vitro, ex vivo, and in vivo assays to explore the potential of RAAS members to stimulate vascular repair-relevant functions of bone marrow stem/progenitor cells of human and murine origin.

Published

2017

232. Glucose-regulated protein 78 demonstrates antiviral effects but is more suitable for hepatocellular carcinoma prevention in hepatitis B

Author

Nai Q. Zheng, Xiao M. Peng, Zi H. Zheng, Hai X. Xu, and Ming X. Huang

Subjects

0301 basic medicine, Hepatitis B virus, Small interfering RNA, Hepatocellular carcinoma, Cell, Gene Expression, Antiviral therapy, Biology, Virus Replication, medicine.disease_cause, Chronic hepatitis B, lcsh:Infectious and parasitic diseases, 03 medical and health sciences, Cell Movement, Virology, medicine, Humans, Glucose-regulated protein 78, lcsh:RC109-216, Secretion, Hepatitis B e Antigens, Endoplasmic Reticulum Chaperone BiP, Heat-Shock Proteins, Research, Liver Neoplasms, virus diseases, Hep G2 Cells, Entecavir, Hepatitis B, medicine.disease, digestive system diseases, 030104 developmental biology, Infectious Diseases, medicine.anatomical_structure, HBeAg, Gene Knockdown Techniques, Hepatocytes, Cell Migration Assays, medicine.drug

Abstract

Background Hepatitis B virus (HBV) is the leading cause of liver cirrhosis and hepatocellular carcinoma in Asia and Africa. Existing antivirals cannot cure HBV or eliminate risk of hepatocellular carcinoma. Glucose-regulated protein 78 (GRP78) can inhibit HBV replication, but promote virion secretion and hepatocellular cancer cell invasion. For these reasons, the overall effect of GRP78 on HBV production and whether to utilize the HBV replication-inhibitory effect of GRP78 up-regulation or the hepatocellular cancer cell invasion-inhibitory effect of its down-regulation were further investigated in order to improve the efficacy of current antiviral therapy. Methods GRP78 regulations in HepG2.2.15 cells were conducted by transfections of expressing vector and small interfering RNA, respectively. The changes in HBV replication, hepatitis B e antigen (HBeAg) synthesis and hepatoma cell motility were monitored. Results GRP78 overall decreased HBV production due to its HBV replication-inhibitory effect time-dependently overwhelming virion secretion-promoting effect in HepG2.2.15 cells. Unlike the parental cells (HepG2), HepG2.2.15 cells demonstrated decreased expressions of the major genes in the interferon-β1-dependent pathway. Moreover, the expressions of these genes were not affected by GRP78 regulations. However, GRP78 was found to inhibit HBeAg secretion and to increase the retro-transportation of capsid assembly-interfering HBeAg precursor from the endoplasmic reticulum into the cytosol where new viral nucleocapsids formed. Furthermore, GRP78 overexpression promoted wound healing process (the motility) of HepG2.2.15 cells. In contrast, GRP78 knockdown enhanced HBV replication and HBeAg secretion, but they were abolished by entecavir and furin inhibitor, respectively. Conclusions GRP78 mainly demonstrates anti-HBV effects, reducing HBV production and HBeAg secretion. With due regard to the hepatocellular cancer invasion risk of the overexpression and the rectifiability of the unpleasant effects of the knockdown, GRP78 down-regulation may be more suitable to serve as an additive strategy to cover the hepatocellular cancer prevention shortage of current antiviral therapy in the future.

Published

2017

233. A dual-docking microfluidic cell migration assay (D

Author

Ke, Yang, Jiandong, Wu, Guoqing, Xu, Dongxue, Xie, Hagit, Peretz-Soroka, Susy, Santos, Murray, Alexander, Ling, Zhu, Michael, Zhang, Yong, Liu, and Francis, Lin

Subjects

Chemotactic Factors, Cell Movement, Neutrophils, Chemotaxis, Immune System, Humans, Computer Simulation, Microfluidic Analytical Techniques, Cell Migration Assays, Immunologic Memory, Article

Abstract

Chemotaxis is a classic mechanism for guiding cell migration and an important topic in both fundamental cell biology and health science. Neutrophil is a widely used model to study eukaryotic cell migration and neutrophil chemotaxis itself can lead to protective or harmful immune actions to the body. While much has been learnt from past research about how neutrophils effectively navigate through a chemoattractant gradient, many interesting questions remain unclear. For example, while it is tempting to model neutrophil chemotaxis using the well-established biased random walk theory, the experimental proof was challenged by the cell’s highly persistent migration nature. Special experimental design is required to test the key predictions from the random walk model. Another question that interests the cell migration community for decades concerns the existence of chemotactic memory and its underlying mechanism. Although chemotactic memory has been suggested in various studies, a clear quantitative experimental demonstration will improve our understanding of the migratory memory effect. Motivated by these questions, we developed a microfluidic cell migration assay (so-called dual-docking chip or D2-Chip) that can test both the biased random walk model and the memory effect for neutrophil chemotaxis on a single chip enabled by multi-region gradient generation and dual-region cell alignment. Our results provide experimental support for the biased random walk model and chemotactic memory for neutrophil chemotaxis. Quantitative data analyses generate new insights into neutrophil chemotaxis and memory by making connections to entropic disorder, cell morphology and oscillating migratory response.

Published

2017

234. Galectin-1 from conditioned medium of three-dimensional culture of adipose-derived stem cells accelerates migration and proliferation of human keratinocytes and fibroblasts

Author

Min Ho, Kim, Wen Hao, Wu, Jee Hyun, Choi, Jihyun, Kim, Jin Hyun, Jun, Yong, Ko, and Jong Hun, Lee

Subjects

Keratinocytes, Proteomics, Wound Healing, Galectin 1, Stem Cells, Fibroblasts, In Vitro Techniques, Adipose Tissue, Re-Epithelialization, Culture Media, Conditioned, Humans, Cell Migration Assays, Cells, Cultured, Cell Proliferation, Skin

Abstract

Keratinocytes and fibroblasts cells play important roles in the skin-wound healing process and are the cell types activated by trauma. Activated cells participate in epithelialization, granulation, scar tissue formation, wound remodeling, and angiogenesis via a series of cellular activities including migration and proliferation. Previous studies reported that the conditioned medium (CM) of adipose-derived stem cells (ADSCs) stimulated the migration and proliferation of cell types involved in the skin wound healing process; however, these studies only show ADSC-CM effects that were obtained using 2-dimensional (2D) culture. Recently, 3-dimensional (3D) culture has been considered as a more physiologically appropriate system than 2D culture for ADSC cultures; therefore, ADSC-CM was collected from 3D culture (ADSC-CM-3D) and compared with ADSC-CM from 2D culture (ADSC-CM-2D) to investigate the effects on the migration and proliferation of human keratinocytes (HaCaTs) and fibroblasts. The migrations of the HaCaT cells and fibroblasts were significantly higher with ADSC-CM-3D compared with the 2D culture; similarly, the proliferation of HaCaT cells was also highly stimulated by ADSC-CM-3D. Proteomic analyses of the ADSC-CM revealed that collagens and actins were highly expressed in the 3D-culture system. Chitinase 3-like 1 (CHI3L1), tissue inhibitor of metalloproteinases (TIMP), and galectin-1 were specifically expressed only in ADSC-CM-3D. Especially, through antibody neutralization, galectin-1 in ADSC-CM-3D was found to be an important factor for the migration of human keratinocytes. Therefore, these results suggest that ADSC-CM-3D was more effective in the wound healing than ADSC-CM-2D, and galectin-1 in ADSC-CM-3D was could be a promising option for skin-wound healing. Furthermore, the differential expressions of several ADSC-CM proteins between the 2D- and 3D-culture systems may be used as basic information for the development of efficient wound-healing strategies.

Published

2017

235. MicroRNA-103 suppresses glioma cell proliferation and invasion by targeting the brain-derived neurotrophic factor

Author

Ying Liu, Jianwei Song, and Ling Wang

Subjects

0301 basic medicine, Adult, Male, Cancer Research, Cell, Biology, Biochemistry, 03 medical and health sciences, Neurotrophic factors, Cell Movement, Genes, Reporter, Glioma, Cell Line, Tumor, microRNA, Brain Injuries, Traumatic, Genetics, medicine, Humans, Luciferases, neoplasms, Molecular Biology, Aged, Cell Proliferation, Brain-derived neurotrophic factor, Binding Sites, Oligoribonucleotides, 030102 biochemistry & molecular biology, Oncogene, Base Sequence, Brain Neoplasms, Brain-Derived Neurotrophic Factor, Antagomirs, Cell cycle, Middle Aged, medicine.disease, Molecular medicine, nervous system diseases, Gene Expression Regulation, Neoplastic, MicroRNAs, medicine.anatomical_structure, Oncology, Cancer research, Molecular Medicine, Female, Cell Migration Assays, Plasmids, Signal Transduction

Abstract

Glioma is the most common and aggressive of malignant brain tumours. MicroRNAs (miRNAs/miRs) are involved in tumour development of various human cancers, including glioma. Therefore, miRNAs may have potential tumour diagnostic, prognostic and therapeutic values in human glioma. miR‑103 is abnormally expressed in various human cancer types. However, the detailed expression pattern, biological functions and underlying molecular mechanism of miR‑103 in glioma remain unclear. Therefore, the present study aimed to investigate the expression, biological roles and underlying mechanisms of miR‑103 in glioma. Results of the present study demonstrated that miR‑103 was significantly down‑regulated in glioma tissues and cell lines. Functional experiments demonstrated that miR‑103 overexpression inhibited the proliferation and invasion of glioma cells in vitro. Additionally, brain‑derived neurotrophic factor (BDNF) was identified as a direct functional target of miR‑103 in glioma. Furthermore, mRNA and protein expression levels of BDNF were highly upregulated in glioma tissues compared with normal brain tissues. Spearman's correlation analysis indicated a negative association between miR‑103 and BDNF mRNA expression levels in glioma tissues. Furthermore, rescue experiments demonstrated that BDNF up‑regulation reversed the suppressive effects of miR‑103 on glioma cell proliferation and invasion. Therefore, the authors of the present study hypothesized that the interaction between miR‑103 and BDNF serves a role in glioma progression and, in the future, may serve as a therapeutic target for glioma treatment.

Published

2017

236. Unforeseen swimming and gliding mode of an insect gut symbiont, Burkholderia sp. RPE64, with wrapping of the flagella around its cell body

Author

Daisuke Nakane, Yoshitomo Kikuchi, Nagisa Mikami, Takayuki Nishizaka, and Yoshiaki Kinosita

Subjects

0301 basic medicine, Burkholderia, media_common.quotation_subject, 030106 microbiology, Cell, Motility, Insect, Flagellum, Microbiology, Article, 03 medical and health sciences, Cell Movement, medicine, Animals, Aliivibrio fischeri, Ecology, Evolution, Behavior and Systematics, Cells, Cultured, media_common, Total internal reflection fluorescence microscope, biology, biology.organism_classification, Bobtail squid, 030104 developmental biology, medicine.anatomical_structure, Flagella, Cell Body, Biophysics, Cell Migration Assays

Abstract

A bean bug symbiont, Burkholderia sp. RPE64, selectively colonizes the gut crypts by flagella-mediated motility: however, the mechanism for this colonization remains unclear. Here, to obtain clues to this mechanism, we characterized the swimming motility of the Burkholderia symbiont under an advanced optical microscope. High-speed imaging of cells enabled the detection of turn events with up to 5-ms temporal resolution, indicating that cells showed reversal motions (θ ~ 180°) with rapid changes in speed by a factor of 3.6. Remarkably, staining of the flagellar filaments with a fluorescent dye Cy3 revealed that the flagellar filaments wrap around the cell body with a motion like that of a ribbon streamer in rhythmic gymnastics. A motility assay with total internal reflection fluorescence microscopy revealed that the left-handed flagellum wound around the cell body and propelled it forward by its clockwise rotation. We also detected periodic-fluorescent signals of flagella on the glass surface, suggesting that flagella possibly contacted the solid surface directly and produced a gliding-like motion driven by flagellar rotation. Finally, the wrapping motion was also observed in a symbiotic bacterium of the bobtail squid, Aliivibrio fischeri, suggesting that this motility mode may contribute to migration on the mucus-filled narrow passage connecting to the symbiotic organ.

Published

2017

237. A Device for Performing Cell Migration/Wound Healing in a 96-Well Plate

Author

Ricky N S Wong, Patrick Y K Yue, and Po Ying Poon

Subjects

0301 basic medicine, medicine.medical_specialty, Materials science, General Chemical Engineering, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Cell Movement, medicine, Humans, 96 well plate, Cells, Cultured, Wound Healing, General Immunology and Microbiology, General Neuroscience, Pipette, food and beverages, Cell migration, Surgery, 030104 developmental biology, Cell Migration Assay, Cell culture, Wound healing assay, Cell Migration Assays, Wound healing, Confluent monolayer, Developmental Biology, Biomedical engineering

Abstract

The cell migration/wounding assay is a commonly used method to study cell migration and other biological processes, such as angiogenesis and tumor metastasis. In this assay, cells are grown to form a confluent monolayer and a mechanical wound is created by scratching with a device. Then the migration rate of the cells towards the denuded area can be monitored by imaging. Our 8-channel mechanical wounder is designed to tackle most of the problems associated with the cell migration assay. Firstly, our wounder can be easily sterilized by autoclaving or with common disinfectants. Secondly, the individual adjustable pins allow even contact with the cell culture plate so that sharp and reproducible wounds can be created. Thirdly, the guiding bars on both sides of the wounder ensure consistent wounding position in each well. The use of disposable plastic pipette tips for wounding can further provide better handling of the wounder as well as to minimize cross-contamination. In conclusion, our cell wounder can provide researchers with a user friendly and reproducible device for performing the cell migration assay using the standard 96-well culture plate.

Published

2017

238. Quantifying the roles of random motility and directed motility using advection-diffusion theory for a 3T3 fibroblast cell migration assay stimulated with an electric field

Author

Yung-Shin Sun, Matthew J. Simpson, and Kai-Yin Lo

Subjects

0301 basic medicine, Drift velocity, Random motility, Motility, Biology, 01 natural sciences, Models, Biological, Haptotaxis, 010305 fluids & plasmas, Quantitative Biology::Cell Behavior, Diffusion, 03 medical and health sciences, Mice, Electricity, Structural Biology, Cell Movement, Modelling and Simulation, Electric field, 0103 physical sciences, Keller-Segal model, Animals, Cell migration, Diffusion (business), Electrotaxis, Molecular Biology, Simulation, Advection, Applied Mathematics, Partial differential equation, 3T3 Cells, Computer Science Applications, 030104 developmental biology, Directed motility, Modeling and Simulation, Electric potential, Biological system, Saturation (chemistry), Cell Migration Assays, Research Article

Abstract

Background Directed cell migration can be driven by a range of external stimuli, such as spatial gradients of: chemical signals (chemotaxis); adhesion sites (haptotaxis); or temperature (thermotaxis). Continuum models of cell migration typically include a diffusion term to capture the undirected component of cell motility and an advection term to capture the directed component of cell motility. However, there is no consensus in the literature about the form that the advection term takes. Some theoretical studies suggest that the advection term ought to include receptor saturation effects. However, others adopt a much simpler constant coefficient. One of the limitations of including receptor saturation effects is that it introduces several additional unknown parameters into the model. Therefore, a relevant research question is to investigate whether directed cell migration is best described by a simple constant tactic coefficient or a more complicated model incorporating saturation effects. Results We study directed cell migration using an experimental device in which the directed component of the cell motility is driven by a spatial gradient of electric potential, which is known as electrotaxis. The electric field (EF) is proportional to the spatial gradient of the electric potential. The spatial variation of electric potential across the experimental device varies in such a way that there are several subregions on the device in which the EF takes on different values that are approximately constant within those subregions. We use cell trajectory data to quantify the motion of 3T3 fibroblast cells at different locations on the device to examine how different values of the EF influences cell motility. The undirected (random) motility of the cells is quantified in terms of the cell diffusivity, D, and the directed motility is quantified in terms of a cell drift velocity, v. Estimates D and v are obtained under a range of four different EF conditions, which correspond to normal physiological conditions. Our results suggest that there is no anisotropy in D, and that D appears to be approximately independent of the EF and the electric potential. The drift velocity increases approximately linearly with the EF, suggesting that the simplest linear advection term, with no additional saturation parameters, provides a good explanation of these physiologically relevant data. Conclusions We find that the simplest linear advection term in a continuum model of directed cell motility is sufficient to describe a range of different electrotaxis experiments for 3T3 fibroblast cells subject to normal physiological values of the electric field. This is useful information because alternative models that include saturation effects involve additional parameters that need to be estimated before a partial differential equation model can be applied to interpret or predict a cell migration experiment. Electronic supplementary material The online version of this article (doi:10.1186/s12918-017-0413-5) contains supplementary material, which is available to authorized users.

Published

2017

239. Polydimethylsiloxane-polycarbonate Microfluidic Devices for Cell Migration Studies Under Perpendicular Chemical and Oxygen Gradients

Author

Chien-Chung Peng, Sih Ling Yeh, Hung-Ju Chiang, Wei-Hao Liao, and Yi-Chung Tung

Subjects

Materials science, General Chemical Engineering, Microfluidics, Cell Culture Techniques, Bioengineering, Oxygen Gradient, Cell Migration, 02 engineering and technology, 01 natural sciences, Chemical reaction, General Biochemistry, Genetics and Molecular Biology, Issue 120, chemistry.chemical_compound, Cell Movement, Lab-On-A-Chip Devices, Humans, Gaseous diffusion, Dimethylpolysiloxanes, Thin film, Polycarbonate, Electrochemical gradient, Polydimethylsiloxane, General Immunology and Microbiology, Cell Culture, General Neuroscience, 010401 analytical chemistry, Cell migration, Equipment Design, Microfluidic Analytical Techniques, 021001 nanoscience & nanotechnology, Chemical Gradient, 0104 chemical sciences, Oxygen, chemistry, visual_art, Biophysics, visual_art.visual_art_medium, Cell Migration Assays, 0210 nano-technology

Abstract

This paper reports a microfluidic device made of polydimethylsiloxane (PDMS) with an embedded polycarbonate (PC) thin film to study cell migration under combinations of chemical and oxygen gradients. Both chemical and oxygen gradients can greatly affect cell migration in vivo; however, due to technical limitations, very little research has been performed to investigate their effects in vitro. The device developed in this research takes advantage of a series of serpentine-shaped channels to generate the desired chemical gradients and exploits a spatially confined chemical reaction method for oxygen gradient generation. The directions of the chemical and oxygen gradients are perpendicular to each other to enable straightforward migration result interpretation. In order to efficiently generate the oxygen gradients with minimal chemical consumption, the embedded PC thin film is utilized as a gas diffusion barrier. The developed microfluidic device can be actuated by syringe pumps and placed into a conventional cell incubator during cell migration experiments to allow for setup simplification and optimized cell culture conditions. In cell experiments, we used the device to study migrations of adenocarcinomic human alveolar basal epithelial cells, A549, under combinations of chemokine (stromal cell-derived factor, SDF-1α) and oxygen gradients. The experimental results show that the device can stably generate perpendicular chemokine and oxygen gradients and is compatible with cells. The migration study results indicate that oxygen gradients may play an essential role in guiding cell migration, and cellular behavior under combinations of gradients cannot be predicted from those under single gradients. The device provides a powerful and practical tool for researchers to study interactions between chemical and oxygen gradients in cell culture, which can promote better cell migration studies in more in vivo-like microenvironments.

Published

2017

240. M

Author

Ke, Yang, Jiandong, Wu, Hagit, Peretz-Soroka, Ling, Zhu, Zhigang, Li, Yaoshuo, Sang, Jolly, Hipolito, Michael, Zhang, Susy, Santos, Craig, Hillier, Ricardo Lobato, de Faria, Yong, Liu, and Francis, Lin

Subjects

Cell Movement, Neutrophils, Chemotaxis, Neoplasms, Humans, Biosensing Techniques, Smartphone, Microfluidic Analytical Techniques, Cell Migration Assays, Article

Abstract

Mobile sensing based on the integration of microfluidic device and smartphone, so-called MS2 technology, has enabled many applications over recent years, and continues to stimulate growing interest in both research communities and industries. In particular, it has been envisioned that MS2 technology can be developed for various cell functional assays to enable basic research and clinical applications. Toward this direction, in this paper, we describe the development of a MS2-based cell functional assay for testing cell migration (the Mkit). The system is constructed as an integrated test kit, which includes microfluidic chips, a smartphone-based imaging platform, the phone apps for image capturing and data analysis, and a set of reagent and accessories for performing the cell migration assay. We demonstrated that the Mkit can effectively measure purified neutrophil and cancer cell chemotaxis. Furthermore, neutrophil chemotaxis can be tested from a drop of whole blood using the Mkit with red blood cell (RBC) lysis. The effects of chemoattractant dose and gradient profile on neutrophil chemotaxis were also tested using the Mkit. In addition to research applications, we demonstrated the effective use of the Mkit for on-site test at the hospital and for testing clinical samples from chronic obstructive pulmonary disease patient. Thus, this developed Mkit provides an easy and integrated experimental platform for cell migration related research and potential medical diagnostic applications.

Published

2017

241. [Effect of polyunsaturated fatty acids ω-3 and ω-6 on angiogenesis formation in human gastric cancer]

Author

Jiachi, Ma, Yuntao, Ma, Tiankang, Guo, Quan, Chen, Yiping, Li, He, Su, Xiaochang, Chen, Xiaodan, Zhao, Qinjin, Guo, and Jianbo, Qi

Subjects

Neovascularization, Pathologic, Angiogenesis Inhibitors, Cell Count, Coculture Techniques, Dinoprostone, Lactones, Cell Movement, Cyclooxygenase 2, Stomach Neoplasms, Cell Line, Tumor, Fatty Acids, Omega-6, Fatty Acids, Omega-3, Fatty Acids, Unsaturated, Human Umbilical Vein Endothelial Cells, Humans, Angiogenesis Inducing Agents, Sulfones, Alprostadil, Cell Migration Assays, Cell Proliferation

Abstract

To investigate the effects of polyunsaturated fatty acids (PUFA) ω-3 and ω-6, and their middle metabolites PGE2 and PGE3 on angiogenesis formation of gastric cancer, and to explore associated mechanism.The effects of ω-3, ω-6, PGE2, PGE3 on the proliferation and migration of human umbilical vein endothelial cell (HUVEC) were measured by proliferation and migration assay respectively. The angiogenesis assay in vivo was used to measure the effects of ω-3, ω-6, PGE2 and PGE3 on neovascularization. In all the assays, groups without ω-3, ω-6, PGE2 and PGE3 were designed as the control.With the increased concentration of ω-6 from 1 μmol/L to 10 μmol/L, the proliferation ability of HUVECs enhanced, and the number of migration cells also increased from 28.2±3.0 to 32.8±2.1, which was higher than control group (21.2±3.2) respectively (both P0.05). With the increased concentration of ω-3 from 1 μmol/L to 10 μmol/L, the proliferation ability of HUVECs was inhibited, and the number of migration cells decreased from 15.8±2.0 to 11.0±2.1, which was lower than control group (22.1±3.0) respectively (both P0.05). In the angiogenesis assay, compared with control group (standard number: 43 721±4 654), the angiogenesis ability of HUVECs was significantly enhanced by ω-6 in concentration-dependent manner (1 μmol/L group: 63 238±4 795, 10 μmol/L group: 78 166±6 123, all P0.01). Meanwhile, with the increased concentration of ω-3 from 1 μmol/L to 10 μmol/L, the angiogenesis ability was significantly decreased from 30 129±3 102 to 20 012±1 541(all P0.01). The proliferation and migration ability of HUVECs were significantly promoted by ω-6 metabolites PGE2 (P0.05) in a concentration-dependent manner. In contrast, ω-3 metabolites PGE3 significantly inhibited the proliferation and migration ability of HUVECs in a concentration-dependent manner (all P0.05). After rofecoxib (a COX-2 specific inhibitor) inhibited the expression of COX-2, the expression level of PGE2 was significantly decreased in a dose-dependent manner. In co-culture system, whose gastric cancer cells expressed positive COX-2, ω-6 could increase angiogenesis of gastric cancer cells(P0.01), but ω-3 could inhibit such angiogenesis(P0.01). In co-culture system, whose gastric cancer cells did not express COX-2, ω-3 could inhibit the angiogenesis of gastric cancer cells (P0.05), but ω-6 had no effect on angiogenesis.The PUFA ω-6 can enhance the angiogenesis via the promotion of proliferation and migration of HUVECs, and COX-2 and PGE2 may play an important role in this process, whereas, the ω-3 can inhibit the angiogenesis through its middle metabolites PGE3 to inhibit the proliferation and migration of HUVECs. Results of this experiment may provide a new approach to inhibit and prevent the spread of gastric cancer.

Published

2017

242. A spleen tyrosine kinase inhibitor attenuates the proliferation and migration of vascular smooth muscle cells

Author

Hyang Hee Seo, Chang Youn Lee, Jiyun Lee, Kyu Hee Lim, Sang Woo Kim, Eunhyun Choi, Seahyoung Lee, Ki-Chul Hwang, and Soyeon Lim

Subjects

0301 basic medicine, Time Factors, Vascular smooth muscle, Cell, Proliferation, Drug Evaluation, Preclinical, Syk, Aorta, Thoracic, Muscle, Smooth, Vascular, Rats, Sprague-Dawley, Cell Movement, BAY61-3606, lcsh:QH301-705.5, Cells, Cultured, Migration, Medicine(all), Agricultural and Biological Sciences(all), Kinase, musculoskeletal system, medicine.anatomical_structure, cardiovascular system, Cell Migration Assays, tissues, Syk kinase inhibitor, Niacinamide, medicine.medical_specialty, Blotting, Western, Myocytes, Smooth Muscle, Short Report, Biology, BAY61-3606 VSMC, 03 medical and health sciences, In vivo, Internal medicine, medicine, Animals, Syk Kinase, Cell Proliferation, Wound Healing, Dose-Response Relationship, Drug, Biochemistry, Genetics and Molecular Biology(all), Cell growth, VSMC, Reproducibility of Results, Pyrimidines, 030104 developmental biology, Endocrinology, lcsh:Biology (General), Cancer research, Wound healing, Ex vivo

Abstract

Background Pathologic vascular smooth muscle cell (VSMC) proliferation and migration after vascular injury promotes the development of occlusive vascular disease. Therefore, an effective chemical agent to suppress aberrant proliferation and migration of VSMCs can be a potential therapeutic modality for occlusive vascular disease such as atherosclerosis and restenosis. To find an anti-proliferative chemical agent for VSMCs, we screened an in-house small molecule library, and the selected small molecule was further validated for its anti-proliferative effect on VSMCs using multiple approaches, such as cell proliferation assays, wound healing assays, transwell migration assays, and ex vivo aortic ring assay. Results Among 43 initially screened small molecule inhibitors of kinases that have no known anti-proliferative effect on VSMCs, a spleen tyrosine kinase (Syk) inhibitor (BAY61-3606) showed significant anti-proliferative effect on VSMCs. Further experiments indicated that BAY61 attenuated the VSMC proliferation in both concentration- and time-dependent manner, and it also significantly suppressed the migration of VSMCs as assessed by both wound healing assays and transwell assays. Additionally, BAY61 suppressed the sprouting of VSMCs from endothelium-removed aortic rings. Conclusion The present study identified a Syk kinase inhibitor as a potent VSMC proliferation and migration inhibitor and warrants further studies to elucidate its underlying molecular mechanisms, such as its primary target, and to validate its in vivo efficacy as a therapeutic agent for restenosis and atherosclerosis.

Published

2017

243. Anomalous diffusion and q-Weibull velocity distributions in epithelial cell migration

Author

Tatiane Souza Vilela Podestá, Tiago Venzel Rosembach, Anésia A. Santos, and Marcelo L. Martins

Subjects

0301 basic medicine, q-Weibull, Cell, Velocity, lcsh:Medicine, 01 natural sciences, Epithelium, Madin Darby Canine Kidney Cells, Mice, Mathematical and Statistical Techniques, Cell Movement, Animal Cells, Medicine and Health Sciences, lcsh:Science, Statistical Data, Weibull distribution, Physics, Multidisciplinary, Mathematical Models, Classical Mechanics, Cell migration, Random walk, Curve Fitting, Cell Motility, medicine.anatomical_structure, Physical Sciences, Epithelial cell migration, Cellular Types, Anatomy, Cell Migration Assays, Statistics (Mathematics), Statistical Distributions, Research Article, Anomalous diffusion, Motility, Cell Migration, Research and Analysis Methods, Time-Lapse Imaging, Motion, 03 medical and health sciences, Dogs, Cell Line, Tumor, 0103 physical sciences, medicine, Animals, 010306 general physics, Scaling, Wound Healing, lcsh:R, Biology and Life Sciences, Epithelial Cells, Cell Biology, Models, Theoretical, Biological Tissue, 030104 developmental biology, Random Walk, Biophysics, lcsh:Q, Mathematical Functions, Mathematics, Developmental Biology

Abstract

In multicellular organisms, cell motility is central in all morphogenetic processes, tissue maintenance, wound healing and immune surveillance. Hence, the control of cell motion is a major demand in the creation of artificial tissues and organs. Here, cell migration assays on plastic 2D surfaces involving normal (MDCK) and tumoral (B16F10) epithelial cell lines were performed varying the initial density of plated cells. Through time-lapse microscopy quantities such as speed distributions, velocity autocorrelations and spatial correlations, as well as the scaling of mean-squared displacements were determined. We find that these cells exhibit anomalous diffusion with q-Weibull speed distributions that evolves non-monotonically to a Maxwellian distribution as the initial density of plated cells increases. Although short-ranged spatial velocity correlations mark the formation of small cell clusters, the emergence of collective motion was not observed. Finally, simulational results from a correlated random walk and the Vicsek model of collective dynamics evidence that fluctuations in cell velocity orientations are sufficient to produce q-Weibull speed distributions seen in our migration assays.

Published

2017

244. Development of a Kinetic Assay for Late Endosome Movement

Author

Michael Kuhn, Melissa Thomas, Felix Meyenhofer, Marc Bickle, Yannis Kalaidzidis, and Milan Ešner

Subjects

Endosome, Movement, Green Fluorescent Proteins, Endocytic cycle, Motility, Endosomes, Biology, Biochemistry, Analytical Chemistry, Automation, RNA interference, Cell Line, Tumor, Organelle, Image Processing, Computer-Assisted, Combinatorial Chemistry Techniques, Humans, Late endosome, Principal Component Analysis, LAMP1, Nocodazole, Reproducibility of Results, Phenotype, Cell biology, Microscopy, Fluorescence, Multivariate Analysis, Molecular Medicine, RNA Interference, Cell Migration Assays, Biotechnology

Abstract

Automated imaging screens are performed mostly on fixed and stained samples to simplify the workflow and increase throughput. Some processes, such as the movement of cells and organelles or measuring membrane integrity and potential, can be measured only in living cells. Developing such assays to screen large compound or RNAi collections is challenging in many respects. Here, we develop a live-cell high-content assay for tracking endocytic organelles in medium throughput. We evaluate the added value of measuring kinetic parameters compared with measuring static parameters solely. We screened 2000 compounds in U-2 OS cells expressing Lamp1-GFP to label late endosomes. All hits have phenotypes in both static and kinetic parameters. However, we show that the kinetic parameters enable better discrimination of the mechanisms of action. Most of the compounds cause a decrease of motility of endosomes, but we identify several compounds that increase endosomal motility. In summary, we show that kinetic data help to better discriminate phenotypes and thereby obtain more subtle phenotypic clustering.

Published

2014

245. Pulp Fibroblasts Synthesize Functional Complement Proteins Involved in Initiating Dentin–Pulp Regeneration

Author

F. Chmilewsky, Charlotte Jeanneau, Imad About, Patrick Laurent, Institut des Sciences du Mouvement Etienne Jules Marey (ISM), and Aix Marseille Université (AMU)-Centre National de la Recherche Scientifique (CNRS)

Subjects

Lipopolysaccharides, [SDV]Life Sciences [q-bio], Complement Membrane Attack Complex, Dental Caries, Biology, Pathology and Forensic Medicine, stomatognathic system, Humans, Regeneration, Progenitor cell, Complement Activation, Cells, Cultured, Dental Pulp, Stem Cells, Regeneration (biology), Chemotaxis, Fibroblasts, Blood proteins, Culture Media, Complement system, Teichoic Acids, stomatognathic diseases, Biochemistry, Dentin, Pulp (tooth), Lipoteichoic acid, Cell Migration Assays, Complement membrane attack complex

Abstract

International audience; The complement system is an efficient plasma immune surveillance system that controls tissue injury and infection. Although the liver constitutes the primary circulating complement protein synthesis site, extrahepatic synthesis is known to optimize local tissue inflammatory reaction. Because dentin–pulp regeneration is known to be regulated locally, we investigated activation of the local complement system within the dental pulp and its role in initiating the regeneration process. Membrane attack complex (C5b-9) formation and Gram's staining revealed that complement activation is correlated with the presence of Gram-positive bacteria in carious human teeth. RT-PCR analysis demonstrated that cultured human pulp fibroblasts stimulated with lipoteichoic acid produce all the proteins required for efficient complement activation. This was demonstrated in vitro by C5b-9 formation and C5a active fragment production in the absence of plasma proteins. Finally, the dynamic migration assays performed in μ-Slide chemotaxis chambers and use of a C5aR-specific antagonist (W54011) demonstrated that the activation of complement proteins synthesized by pulp fibroblasts and the subsequent release of C5a specifically induced pulp progenitor cell recruitment. Our study reveals human pulp fibroblasts as the first nonimmune cell type capable of synthesizing all complement proteins. These fibroblasts cells contribute significantly to tissue regeneration by recruiting pulp progenitors via complement activation, which suggests to a potential therapeutic strategy of targeting pulp fibroblasts in dentin–pulp regeneration.

Published

2014

246. Methods for Studying Tumor Cell Migration and Invasiveness

Author

Lucia Knopfová, Petra Kovaříková, Pavel Bouchal, and Eva Michalová

Subjects

ved/biology, ved/biology.organism_classification_rank.species, Cancer, Cell migration, Chemotaxis, In Vitro Techniques, Biology, medicine.disease, Metastasis, Oncology, Cell Movement, In vivo, Cancer research, medicine, Humans, Neoplasm Invasiveness, Hepatocyte growth factor, Neoplasm Metastasis, Cell Migration Assays, Wound healing, Model organism, medicine.drug

Abstract

Migration and invasiveness are phenotypic characteristics of cells that contribute to physiological processes, such as wound healing or embryogenesis and they are involved in serious pathological processes, namely in tumor cell metastasis. Availability of methods for studying migration and invasiveness of the cells is important for understanding molecular basis of these processes. In the case of cancer, migration, invasiveness and metastatic potential of tumor cells are key factors that determine clinical prognosis of the patients. This communication provides an overview of in vitro and in vivo methods which are used to study cell migration, invasion and metastasis. In vitro meth-ods for studying cell migration include simple two dimensional assays (scratch - wound assay and the assay based on the effect of hepatocyte growth factor) and methods based on chemotaxis (Dunns chamber, videomicroscopy of cells, the use of carriers with chemoattractants). Methods for studying both cell migration and invasiveness in vitro include more complex systems based on the principle of the Boyden chamber (transwell migration/ invasive test, analysis of cell migration and invasion in xCELLigence system, confocal microscopy based approaches) as well as analysis of cell migration in microchannels. Our overview of in vivo methods provides an introduction into model organisms and methods used in this field, with an emphasis on the study of cancer metastasis in mouse models. The methods described in this review are mainly involved in larger research projects aiming at developing new diagnostic and therapeutic approaches in oncology.

Published

2014

247. Quantitative Assessment of the Relationship Between Cellular Morphodynamics and Signaling Events by Stochastic Analysis of Fluorescent Images

Author

Marco De Spirito, Massimiliano Papi, Giovambattista Pani, Alessandro Maiorana, and Giuseppe Maulucci

Subjects

Yellow fluorescent protein, Motility, Time-Lapse Imaging, Settore FIS/07 - FISICA APPLICATA (A BENI CULTURALI, AMBIENTALI, BIOLOGIA E MEDICINA), Mice, Cell Movement, Settore MED/04 - PATOLOGIA GENERALE, Cell Line, Tumor, Animals, Instrumentation, Event (probability theory), reactive oxygen species, Staining and Labeling, Pixel, biology, Chemistry, Stochastic process, imaging, Fluorescence, Order (biology), Microscopy, Fluorescence, motility, biology.protein, Cell Migration Assays, signaling, Biological system, Intracellular, Signal Transduction

Abstract

Cell motility involves a number of strategies that cells use in order to seek nutrients, escape danger, and fulfill morphogenetic roles. Here we present a methodology to quantify morphological changes and their relationship with signaling events from time-lapse imaging microscopy experiments, in order to characterize physiological and pathological processes. To this aim, the stationary spatial pattern of signaling events is determined through an intracellular fluorescent probe, and it is related with the frequency and entity of morphodynamic events, which are in turn quantified through a stochastic approach: two pseudoimages are obtained from a time series of moving cells that describe the probability that a pixel belongs to the cell, and the probability that a pixel is subject to a dynamic event. The simultaneous construction of these maps permits visualization of hot spots of dynamic events, i.e., zones of formation of membrane protrusions and retractions and their relationship with the signaling events reported by the specific probe employed. The method is tested on spontaneous movement of cells, trasfected with redox-sensitive yellow fluorescent protein, in which the distribution of the hot spots and its change upon expression of constitutively active Rac (V12-Rac), is related to the distribution of oxidized spots.

Published

2014

248. A truncating mutation in the laminin-332α chain highlights the role of the LG45 proteolytic domain in regulating keratinocyte adhesion and migration

Author

Daniele Castiglia, M. El Hachem, Eugenia Piccinni, Giovanna Zambruno, Renata Boldrini, Paola Fortugno, Valentina Calabresi, Andrea Diociaiuti, Francesca Cianfarani, and G. Di Zenzo

Subjects

Keratinocytes, Male, Mutant, Dermatology, Cell Movement, Laminin, Gene expression, Cell Adhesion, medicine, Humans, Keratinocyte migration, Frameshift Mutation, Cell adhesion, Genetics, biology, Middle Aged, medicine.disease, Reverse transcriptase, Cell biology, medicine.anatomical_structure, biology.protein, Epidermolysis bullosa, Cell Migration Assays, Epidermolysis Bullosa, Junctional, Keratinocyte, Cell Adhesion Molecules

Abstract

Summary Background Altered function of laminin-332 (α3β3γ2) consequent to mutations in the LAMA3, LAMB3 and LAMC2 genes causes junctional epidermolysis bullosa non-Herlitz (JEB-nH). JEB-nH patients suffer from skin blistering and have an increased risk of developing aggressive skin carcinomas in adulthood. Laminin-332 is proteolytically processed and its extracellular mature form lacks the α3 chain C-terminal globules 4 and 5 (LG45). The LG45 tandem has cell adhesion and protumorigenic properties. However, mutations that affect this domain are very rare and their functional effects in patients have not been explored to date. Objective To characterize molecularly an adult patient with JEB-nH and altered laminin-332 expression presenting multiple skin carcinomas, and to analyse LG45-mediated biological functions using keratinocytes from the patient. Methods A mutational search in laminin-332 genes was performed by hetero-duplex analysis. LAMA3 mRNA and laminin-332 protein levels in patient keratinocytes were investigated by real-time reverse transcriptase polymerase chain reaction and radioimmunoprecipitation assay, respectively. Keratinocyte migration was examined by scratch and Boyden chamber assays. Results We identified a homozygous LAMA3 mutation, p.Leu1648TrpfsX32, which truncates the last 45 amino acids of the carboxyl terminal LG5 subdomain. Gene expression studies revealed that the mutant transcripts were stable and even increased, precursor laminin-332 molecules were retained intracellularly and the amount of mature extracellular heterotrimers was reduced to about 50%. Finally, the patient's keratinocytes migrated faster than normal keratinocytes. Conclusions Structural disruption of LG5 highlights the critical functions of the LG45 proteolytic region in precursor laminin-332 secretion and keratinocyte adhesion and migration. Perturbation of LG45 function might explain the non-aggressive behaviour of carcinomas in this patient.

Published

2014

249. Antiapoptotic Effects of Anthocyanin from the Seed Coat of Black Soybean Against Oxidative Damage of Human Lens Epithelial Cell Induced by H2O2

Author

Jee Won Mok, Choun-Ki Joo, and Dong-Jin Chang

Subjects

Programmed cell death, Cell Survival, Swine, Blotting, Western, Apoptosis, Cell Count, Biology, medicine.disease_cause, Anthocyanins, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Western blot, Annexin, Lens, Crystalline, In Situ Nick-End Labeling, medicine, Animals, Humans, Cytotoxicity, Cells, Cultured, bcl-2-Associated X Protein, TUNEL assay, Dose-Response Relationship, Drug, medicine.diagnostic_test, Caspase 3, food and beverages, Epithelial Cells, Hydrogen Peroxide, Molecular biology, Sensory Systems, Oxidative Stress, Ophthalmology, Proto-Oncogene Proteins c-bcl-2, chemistry, Anthocyanin, Seeds, bcl-Associated Death Protein, Soybeans, Tumor Suppressor Protein p53, Cell Migration Assays, Oxidative stress

Abstract

To describe the protective effect of anthocyanin from black soybean in human lens epithelial cell line (HLE-B3) under H2O2-induced oxidative stress.Cytotoxicity of anthocyanin and H2O2 were determined by Cell Counting Kit-8 test. Viability of HLE-B3 cells under various H2O2 concentration (0, 50 and 100 μM) with or without pretreatment of anthocyanin (0, 50, 100 and 200 μg/ml) was measured. After quantifying the percentage of the apoptosis by Annexin V assay and APO-BrdU TUNEL assay, we conducted western blot and immunostaining of apoptosis-related molecules; Bcl2, BAD, BAX, p53 and caspase-3. To confirm the effect of anthocyanin on an ex vivo model, its effect on cultures of the lenses of porcine were examined.Anthocyanin reduced cell death of HLE-B3 under H2O2-induced oxidative stress in a dose-dependent manner. In Annexin V analysis, anthocyanin protected HLE-B3 cells from apoptosis. H2O2 increased the expression of BAX, BAD, p53 and caspase-3 in a time-dependent manner, those of which anthocyanin significantly decreased. On the other hand, Bcl2 was increased from anthocyanin-treated lens cells. And in anthocyanin-treated lens organ culture, transparency was maintained.This study showed that anthocyanin protects HLE-B3 cells under oxidative stress from apoptosis, and the mechanism of the effect is related to the intrinsic pathway of apoptosis. Anthocyanin has a potential in prevention of cataract.

Published

2014

250. High proliferative potential endothelial colony-forming cells contribute to hypoxia-induced pulmonary artery vasa vasorum neovascularization

Author

Aftab Ahmad, Hala Nijmeh, Evgenia V. Gerasimovskaya, Vivek Balasubramaniam, Kurt R. Stenmark, and Nana Burns

Subjects

Male, Pulmonary and Respiratory Medicine, CD31, Pathology, medicine.medical_specialty, Physiology, Angiogenesis, Hypertension, Pulmonary, Pulmonary Artery, Biology, Colony-Forming Units Assay, Neovascularization, Antigens, CD, Physiology (medical), medicine, Animals, Hypoxia, Telomerase, Cell Proliferation, Tube formation, Neovascularization, Pathologic, Vasa Vasorum, Articles, Cell Biology, Endoglin, Hypoxia (medical), medicine.disease, Pulmonary hypertension, Platelet Endothelial Cell Adhesion Molecule-1, Proto-Oncogene Proteins c-kit, medicine.anatomical_structure, Animals, Newborn, Vasa vasorum, Cancer research, Cattle, medicine.symptom, Cell Migration Assays

Abstract

Angiogenic expansion of the vasa vasorum (VV) is an important contributor to pulmonary vascular remodeling in the pathogenesis of pulmonary hypertension (PH). High proliferative potential endothelial progenitor-like cells have been described in vascular remodeling and angiogenesis in both systemic and pulmonary circulations. However, their role in hypoxia-induced pulmonary artery (PA) VV expansion in PH is not known. We hypothesized that profound PA VV neovascularization observed in a neonatal calf model of hypoxia-induced PH is due to increased numbers of subsets of high proliferative cells within the PA adventitial VV endothelial cells (VVEC). Using a single cell clonogenic assay, we found that high proliferative potential colony-forming cells (HPP-CFC) comprise a markedly higher percentage in VVEC populations isolated from the PA of hypoxic (VVEC-Hx) compared with control (VVEC-Co) calves. VVEC-Hx populations that comprised higher numbers of HPP-CFC also demonstrated markedly higher expression levels of CD31, CD105, and c-kit than VVEC-Co. In addition, significantly higher expression of CD31, CD105, and c-kit was observed in HPP-CFC vs. the VVEC of the control but not of hypoxic animals. HPP-CFC exhibited migratory and tube formation capabilities, two important attributes of angiogenic phenotype. Furthermore, HPP-CFC-Co and some HPP-CFC-Hx exhibited elevated telomerase activity, consistent with their high replicative potential, whereas a number of HPP-CFC-Hx exhibited impaired telomerase activity, suggestive of their senescence state. In conclusion, our data suggest that hypoxia-induced VV expansion involves an emergence of HPP-CFC populations of a distinct phenotype with increased angiogenic capabilities. These cells may serve as a potential target for regulating VVEC neovascularization.

Published

2014