Your search keyword '"CELL MODEL"' showing total 2,190 results

1. The Application of Duck Embryonic Fibroblasts CCL-141 as a Cell Model for Adipogenesis.

Author

Sun, Dan-Dan, Li, Xiao-Qin, Liu, Yong-Tong, Ge, Meng-Qi, and Hou, Zhuo-Cheng

Subjects

*STAINS & staining (Microscopy), *FAT cells, *GENE knockout, *GENE expression, *TRETINOIN, *ADIPOGENESIS

Abstract

Simple Summary: This study demonstrates that the duck embryo fibroblast cell line CCL-141 can undergo adipogenesis, vital for understanding fat cell development in ducks. Treatments with chicken serum, fatty acids, insulin, and all-trans retinoic acid induced fat cell formation, as evidenced by Oil Red O staining and a gene expression analysis. Moreover, the CRISPR/Cas9 knockout of the adipogenesis gene PPARγ in CCL-141 cells confirmed the cell line's utility for studying adipogenesis-related gene functions. These findings validate CCL-141 as a model for adipogenesis research, which will aid in uncovering its regulatory mechanisms. The duck embryo fibroblast cell line CCL-141, which is currently the only commercialized duck cell line, has been underexplored in adipogenesis research. (1) Background: This study establishes an experimental protocol to induce adipogenesis in CCL-141 cells, addressing the importance of understanding gene functions in this process. (2) Methods: Chicken serum, fatty acids, insulin, and all-trans retinoic acid were used to treat CCL-141 cells, with adipogenesis confirmed by Oil Red O staining and gene expression quantification. CRISPR/Cas9 technology was applied to knockout PPARγ, and the resulting adipogenic phenotype was assessed. (3) Results: The treatments promoted adipogenesis, and the knockout of PPARγ validated the cell line's utility for gene function studies. (4) Conclusions: CCL-141 cells are a suitable model for investigating duck adipogenesis, contributing to the understanding of regulatory factors in this biological process. [ABSTRACT FROM AUTHOR]

Published

2024

2. Implementing differentially pigmented skin models for predicting drug response variability across human ancestries.

Author

Zaaijer, Sophie and Groen, Simon C.

Abstract

Persistent racial disparities in health outcomes have catalyzed legislative reforms and heightened scientific focus recently. However, despite the well-documented properties of skin pigments in binding drug compounds, their impact on therapeutic efficacy and adverse drug responses remains insufficiently explored. This perspective examines the intricate relationships between variation in melanin-based skin pigmentation and pharmacokinetics and -dynamics, highlighting the need for considering diversity in skin pigmentation as a variable to advance the equitability of pharmacological interventions. The article provides guidelines on the selection of New Approach Methods (NAMs) to foster inclusive study designs in preclinical drug development pipelines, leading to an improved level of translatability to the clinic. [ABSTRACT FROM AUTHOR]

Published

2024

3. Deletion of exons 45 to 55 in the DMD gene: from the therapeutic perspective to the in vitro model.

Author

Poyatos-García, Javier, Soblechero-Martín, Patricia, Liquori, Alessandro, López-Martínez, Andrea, Maestre, Pilar, González-Romero, Elisa, Vázquez-Manrique, Rafael P., Muelas, Nuria, García-García, Gema, Ohana, Jessica, Arechavala-Gomeza, Virginia, and Vílchez, Juan J.

Subjects

*BECKER muscular dystrophy, *DUCHENNE muscular dystrophy, *DYSTROPHIN genes, *GENOME editing, *GENE therapy

Abstract

Background: Gene editing therapies in development for correcting out-of-frame DMD mutations in Duchenne muscular dystrophy aim to replicate benign spontaneous deletions. Deletion of 45–55 DMD exons (del45–55) was described in asymptomatic subjects, but recently serious skeletal and cardiac complications have been reported. Uncovering why a single mutation like del45–55 is able to induce diverse phenotypes and grades of severity may impact the strategies of emerging therapies. Cellular models are essential for this purpose, but their availability is compromised by scarce muscle biopsies. Methods: We introduced, as a proof-of-concept, using CRISPR-Cas9 edition, a del45–55 mimicking the intronic breakpoints harboured by a subset of patients of this form of dystrophinopathy (designing specific gRNAs), into a Duchenne patient's cell line. The edited cell line was characterized evaluating the dystrophin expression and the myogenic status. Results: Dystrophin expression was restored, and the myogenic defects were ameliorated in the edited myoblasts harbouring a specific del45–55. Besides confirming the potential of CRISPR-Cas9 to create tailored mutations (despite the low cleavage efficiency of our gRNAs) as a useful approach to generate in vitro models, we also generated an immortalized myoblast line derived from a patient with a specific del45–55. Conclusions: Overall, we provide helpful resources to deepen into unknown factors responsible for DMD-pathophysiology. [ABSTRACT FROM AUTHOR]

Published

2024

4. A simulation study on the effect of penetration of gold nanoparticles in the cytoplasm of healthy eye organs on dose enhancement of brachytherapy.

Author

Rasouli, Fatemeh S. and Masoudi, S. Farhad

Subjects

*GOLD nanoparticles, *MONTE Carlo method, *IRIS (Eye), *SCLERA, *RADIOISOTOPE brachytherapy

Abstract

Purpose: Special properties and recent advances in the synthesis and biomolecular functionalization of gold nanoparticles (GNPs) have led to the evolution of their use in biomedical applications such as photon radiotherapy. Simulation-based studies on the effect of various parameters that govern the dose enhancement due to utilizing GNPs have facilitated the progress of knowledge in this field. Due to their flexibility and easier accessibility compared with experimental works, simulations have the potential to be considered for pre-clinical tests and, therefore, should be close to the realistic conditions as much as possible. Materials and methods: To this aim, the present work investigates the effect of the presence of GNPs that are accumulated in the cytoplasm of the constituent cells in healthy tissues of a human eye phantom, inspired by the published experimental results which report that non-target tissues also receive the drugs containing GNPs. The GNPs' concentrations are assumed to decrease by moving from the tumor toward the depth of the phantom through a suggested pattern. The MCNPX Monte Carlo code is used for the simulations. Results: The results show that for four concentrations tested, the dose enhancement factor in the shallower layer reaches 6, and decreases to 1.2 in the last layer. The dose enhancements are also examined for critical structures of the iris, cornea, sclera, and lens, showing maximum deviations of about 3 to 200% compared with the absence of GNPs in the healthy tissue. Considering the reported doses to the lens by clinical institutions, the effect of penetration of GNPs to deep layers on treatment time is also investigated. Conclusions: The results show that the penetration of GNPs from the tumor toward healthy tissues strongly controls the dose enhancement over the various eye structures and emphasizes the importance of modeling the GNPs' distribution in the medium on the overall dose enhancement. Considering the current challenges in the clinical use of GNPs, more effort needs to be made to reach an effective endpoint in treatment. [ABSTRACT FROM AUTHOR]

Published

2024

5. Swelling of Spherical Polyelectrolyte Gels.

Author

Duan, Ming-Yu, Chen, Jia-Dong, Liu, Yi-Ming, Peng, Zhao-Feng, and Chen, Guang

Subjects

*DRUG adsorption, *ERYTHROCYTES, *FINITE element method, *ELECTROSTATIC interaction, *SOLUTION (Chemistry)

Abstract

Polyelectrolyte (PE) gels, distinguished by their unique stimuli-responsive swelling behavior, serve as the basis of broad applications, such as artificial muscles and drug delivery. In this work, we present a theoretical model to analyze the electrostatics and its contribution to the swelling behavior of PE gels in salt solutions. By minimizing the free energy of PE gels, we obtain two distinct scaling regimes for the swelling ratio at equilibrium with respect to the salt concentration. We compare our predictions for the swelling ratio with experimental measurements, which show excellent agreement. In addition, we employ a finite element method to assess the applicability range of our theoretical model and assumptions. We anticipate that our model will also provide valuable insights into drug adsorption and release, deformation of red blood cells, 4D printing and soft robotics, where the underlying mechanism of swelling remains enigmatic. [ABSTRACT FROM AUTHOR]

Published

2024

6. Enriched Environment Contributes to the Recovery from Neurotoxin-Induced Parkinson's Disease Pathology.

Author

Alcalá-Zúniga, Daphne, Espinoza-Torres, Erika, Das, Ranjit Kumar, Vargas, Magaly, Maldonado, Oscar, Benavides, Omar, Manojkumar, Arvind, de la Garza, Roberto, Davila, Natalia, Perez, Isaac, Martinez, Alejandro Hernandez, Roy, Deepa, López-Juárez, Alejandro, Zarei, Masoud M., Baker, Kelsey A., Gil, Mario, Rodrigo, Hansapani, de Erausquin, Gabriel A., and Roy, Upal

Abstract

Parkinson's disease (PD) is a neurological disorder that affects dopaminergic neurons. The lack of understanding of the underlying molecular mechanisms of PD pathology makes treating it a challenge. Several pieces of evidence support the protective role of enriched environment (EE) and exercise on dopaminergic neurons. The specific aspect(s) of neuroprotection after exposure to EE have not been identified. Therefore, we have investigated the protective role of EE on dopamine dysregulation and subsequent downregulation of DJ1 protein using in vitro and in vivo models of PD. Our study for the first time demonstrated that DJ1 expression has a direct correlation with dopamine downregulation in PD models and exposure to EE has a significant impact on improving the behavioral changes in PD mice. This research provides evidence that exercise in EE has a positive effect on PD without interfering with the current line of therapy. [ABSTRACT FROM AUTHOR]

Published

2024

7. Deletion of exons 45 to 55 in the DMD gene: from the therapeutic perspective to the in vitro model

Author

Javier Poyatos-García, Patricia Soblechero-Martín, Alessandro Liquori, Andrea López-Martínez, Pilar Maestre, Elisa González-Romero, Rafael P. Vázquez-Manrique, Nuria Muelas, Gema García-García, Jessica Ohana, Virginia Arechavala-Gomeza, and Juan J. Vílchez

Subjects

Duchenne muscular dystrophy, Becker muscular dystrophy, CRISPR-Cas9, Gene therapy, Cell model, Dystrophin, Diseases of the musculoskeletal system, RC925-935

Abstract

Abstract Background Gene editing therapies in development for correcting out-of-frame DMD mutations in Duchenne muscular dystrophy aim to replicate benign spontaneous deletions. Deletion of 45–55 DMD exons (del45–55) was described in asymptomatic subjects, but recently serious skeletal and cardiac complications have been reported. Uncovering why a single mutation like del45–55 is able to induce diverse phenotypes and grades of severity may impact the strategies of emerging therapies. Cellular models are essential for this purpose, but their availability is compromised by scarce muscle biopsies. Methods We introduced, as a proof-of-concept, using CRISPR-Cas9 edition, a del45–55 mimicking the intronic breakpoints harboured by a subset of patients of this form of dystrophinopathy (designing specific gRNAs), into a Duchenne patient’s cell line. The edited cell line was characterized evaluating the dystrophin expression and the myogenic status. Results Dystrophin expression was restored, and the myogenic defects were ameliorated in the edited myoblasts harbouring a specific del45–55. Besides confirming the potential of CRISPR-Cas9 to create tailored mutations (despite the low cleavage efficiency of our gRNAs) as a useful approach to generate in vitro models, we also generated an immortalized myoblast line derived from a patient with a specific del45–55. Conclusions Overall, we provide helpful resources to deepen into unknown factors responsible for DMD-pathophysiology.

Published

2024

8. Creation of an in vitro model of GM1 gangliosidosis by CRISPR/Cas9 knocking‐out the GLB1 gene in SH‐SY5Y human neuronal cell line.

Author

Hosseini, Kamran, Fallahi, Jafar, Aligholi, Hadi, Heidari, Zahra, Nadimi, Elham, Safari, Fatemeh, Sisakht, Mohsen, Atapour, Amir, Khajeh, Sahar, Tabei, Seyed Mohammad Bagher, and Razban, Vahid

Subjects

*GENE expression, *NEURONS, *DIAGNOSTIC use of polymerase chain reaction, *MOLECULAR cloning, *GENETIC vectors

Abstract

GM1 gangliosidosis is one type of hereditary error of metabolism that occurs due to the absence or reduction of β‐galactosidase enzyme content in the lysosome of cells, including neurons. In vitro, the use of neural cell lines could facilitate the study of this disease. By creating a cell model of GM1 gangliosidosis on the SH‐SY5Y human nerve cell line, it is possible to understand the main role of this enzyme in breaking down lipid substrate and other pathophysiologic phenomena this disease. To knock‐out the human GLB1 gene, guides targeting exons 14 and 16 of the GLB1 gene were designed using the CRISPOR and CHOP‐CHOP websites, and high‐efficiency guides were selected for cloning in the PX458 vector. After confirming the cloning, the vectors were transformed into DH5α bacteria and then the target vector was extracted and transfected into human nerve cells (SH‐SY5Y cell line) by electroporation. After 48 h, GFP+ cells were sorted using the FACS technique and homozygous (compound heterozygous) single cells were isolated using the serial dilution method and sequencing was done to confirm them. Finally, gap PCR tests, X‐gal and Periodic acid‐Schiff (PAS) staining, and qPCR were used to confirm the knock‐out of the human GLB1 gene. Additionally, RNA sequencing data analysis from existing data of the Gene Expression Omnibus (GEO) was used to find the correlation of GLB1 with other genes, and then the top correlated genes were tested for further evaluation of knock‐out effects. The nonviral introduction of two guides targeting exons 14 and 16 of the GLB1 gene into SH‐SY5Y cells led to the deletion of a large fragment with a size of 4.62 kb. In contrast to the non‐transfected cell, X‐gal staining resulted in no blue color in GLB1 gene knock‐out cells indicating the absence of β‐galactosidase enzyme activity in these cells. Real‐time PCR (qPCR) results confirmed the RNA‐Seq analysis outcomes on the GEO data set and following the GLB1 gene knock‐out, the expression of its downstream genes, NEU1 and CTSA, has been decreased. It has been also shown that the downregulation of GLB1‐NEU1‐CTSA complex gene was involved in suppressed proliferation and invasion ability of knock‐out cells. This study proved that using dual guide RNA can be used as a simple and efficient tool for targeting the GLB1 gene in nerve cells and the knockout SH‐SY5Y cells can be used as a model investigation of basic and therapeutic surveys for GM1 gangliosidosis disease. Significance statement: This study concerns the modeling of GM1 gangliosidosis by knocking‐out the GLB1 gene in human nerve cells and using CRISPR/Cas9 technology. [ABSTRACT FROM AUTHOR]

Published

2024

9. Prinsepia utilis Royle polysaccharides promote skin barrier repair through the Claudin family.

Author

Wang, Bo, Wang, Feifei, Qu, Liping, Ma, Hongyu, Cheng, Yuying, Wu, Xinlang, Liu, Junxi, and He, Li

Subjects

*MONOSACCHARIDES, *CLAUDINS, *WESTERN immunoblotting, *POLYSACCHARIDES, *IMMUNOSTAINING, *GENE expression

Abstract

Background: Plant polysaccharides have various biological activities. However, few studies have been conducted on the skin barrier of Prinsepia utilis Royle polysaccharide extract (PURP). Materials and methods: The proportions of polysaccharides, monosaccharides and proteins were determined by extracting polysaccharides from fruit meal using water. The healing rate was measured by cell scratch assays. SDS‐damaged reconstructed human epidermal models, an acetone–ether‐induced mouse model and an IL‐4‐induced cellular inflammation model were used to detect the effects of polysaccharides on the phenotype, HA, TEWL, and TEER, with further characterizations performed using QRT‐PCR, Western blotting, immunofluorescence (IF) assays. Results: PURP contained 35.73% polysaccharides and 11.1% proteins. PURP promoted cell migration and increased skin thickness in a reconstructed human epidermis model. The TEWL significantly decreased, and the HA content significantly increased. PURP significantly increased the TEER and decreased the permeability of the SDS‐damaged reconstructed human epidermis model. Claudin‐3, Claudin‐4, and Claudin‐5 were significantly upregulated. IF and Western blot analysis revealed that the Claudin‐4 level significantly increased after treatment with PURP. Claudin‐1, Claudin‐3, Claudin‐4, and Claudin‐5 gene expression and IF and immunohistochemical staining were significantly increased in mice treated with acetone–ether. PURP promoted the expression of Claudin‐1, Claudin‐3, Claudin‐4, and Claudin‐5 after treatment with 100 ng/mL IL‐4. PURP also downregulated the expression of NO, IL6, TNFα and NFκB in Raw 264.7 cells and in a mouse model. Conclusion: We hypothesize that PURP may repair the skin barrier by promoting the expression of the claudin family and can assist in skin therapy. [ABSTRACT FROM AUTHOR]

Published

2024

10. MiR-21-5p modulates LPS-induced acute injury in alveolar epithelial cells by targeting SLC16A10

Author

Huanan Zeng, Yuqing Zhou, Zhi Liu, and Wei Liu

Subjects

ALI, LPS, Cell model, Inflammation, MiR-21-5p, SLC16A10, Medicine, Science

Abstract

Abstract Sepsis is a systemic inflammatory response syndrome resulting from the invasion of the human body by bacteria and other pathogenic microorganisms. One of its most prevalent complications is acute lung injury, which places a significant medical burden on numerous countries and regions due to its high morbidity and mortality rates. MicroRNA (miRNA) plays a critical role in the body's inflammatory response and immune regulation. Recent studies have focused on miR-21-5p in the context of acute lung injury, but its role appears to vary in different models of this condition. In the LPS-induced acute injury model of A549 cells, there is differential expression, but the specific mechanism remains unclear. Therefore, our aim is to investigate the changes in the expression of miR-21-5p and SLC16A10 in a type II alveolar epithelial cell injury model induced by LPS and explore the therapeutic effects of their targeted regulation. A549 cells were directly stimulated with 10 µg/ml of LPS to construct a model of LPS-induced cell injury. Cells were collected at different time points and the expression of interleukin 1 beta (IL-1β), tumor necrosis factor-α (TNF-α) and miR-21-5p were measured by RT-qPCR and western blot. Then miR-21-5p mimic transfection was used to up-regulate the expression of miR-21-5p in A549 cells and the expression of IL-1β and TNF-α in each group of cells was measured by RT-qPCR and western blot. The miRDB, TargetScan, miRWalk, Starbase, Tarbase and miR Tarbase databases were used to predict the miR-21-5p target genes and simultaneously, the DisGeNet database was used to search the sepsis-related gene groups. The intersection of the two groups was taken as the core gene. Luciferase reporter assay further verified SLC16A10 as the core gene with miR-21-5p. The expression of miR-21-5p and SLC16A10 were regulated by transfection or inhibitors in A549 cells with or without LPS stimulation. And then the expression of IL-1β and TNF-α in A549 cells was tested by RT-qPCR and western blot in different groups, clarifying the role of miR-21-5p-SLC16A10 axis in LPS-induced inflammatory injury in A549 cells. (1) IL-1β and TNF-α mRNA and protein expression significantly increased at 6, 12, and 24 h after LPS stimulation as well as the miR-21-5p expression compared with the control group (P

Published

2024

11. Modeling and Phenotyping Acute and Chronic Type 2 Diabetes Mellitus In Vitro in Rodent Heart and Skeletal Muscle Cells

Author

Kopp, Elena L, Deussen, Daniel N, Cuomo, Raphael, Lorenz, Reinhard, Roth, David M, Mahata, Sushil K, and Patel, Hemal H

Subjects

Biochemistry and Cell Biology, Medical Physiology, Biomedical and Clinical Sciences, Biological Sciences, Diabetes, Development of treatments and therapeutic interventions, 5.1 Pharmaceuticals, 2.1 Biological and endogenous factors, Aetiology, Metabolic and endocrine, Animals, Humans, Diabetes Mellitus, Type 2, Rodentia, Muscle Fibers, Skeletal, Glucose, Insulin, Insulin Resistance, Hyperglycemia, Palmitates, Adenosine Triphosphate, insulin resistance, type 2 diabetes, cell model, mitochondrial dysfunction, Biological sciences, Biomedical and clinical sciences

Abstract

Type 2 diabetes (T2D) has a complex pathophysiology which makes modeling the disease difficult. We aimed to develop a novel model for simulating T2D in vitro, including hyperglycemia, hyperlipidemia, and variably elevated insulin levels targeting muscle cells. We investigated insulin resistance (IR), cellular respiration, mitochondrial morphometry, and the associated function in different T2D-mimicking conditions in rodent skeletal (C2C12) and cardiac (H9C2) myotubes. The physiological controls included 5 mM of glucose with 20 mM of mannitol as osmotic controls. To mimic hyperglycemia, cells were exposed to 25 mM of glucose. Further treatments included insulin, palmitate, or both. After short-term (24 h) or long-term (96 h) exposure, we performed radioactive glucose uptake and mitochondrial function assays. The mitochondrial size and relative frequencies were assessed with morphometric analyses using electron micrographs. C2C12 and H9C2 cells that were treated short- or long-term with insulin and/or palmitate and HG showed IR. C2C12 myotubes exposed to T2D-mimicking conditions showed significantly decreased ATP-linked respiration and spare respiratory capacity and less cytoplasmic area occupied by mitochondria, implying mitochondrial dysfunction. In contrast, the H9C2 myotubes showed elevated ATP-linked and maximal respiration and increased cytoplasmic area occupied by mitochondria, indicating a better adaptation to stress and compensatory lipid oxidation in a T2D environment. Both cell lines displayed elevated fractions of swollen/vacuolated mitochondria after T2D-mimicking treatments. Our stable and reproducible in vitro model of T2D rapidly induced IR, changes in the ATP-linked respiration, shifts in energetic phenotypes, and mitochondrial morphology, which are comparable to the muscles of patients suffering from T2D. Thus, our model should allow for the study of disease mechanisms and potential new targets and allow for the screening of candidate therapeutic compounds.

Published

2023

12. A Simulation of the Mechanical Testing of the Cell Membrane and Cytoskeleton.

Author

Du, Yue, Cheng, Dai, Yang, Zhanli, Liu, Yaowei, Zhao, Qili, Sun, Mingzhu, Li, Haifeng, and Zhao, Xin

Subjects

CYTOSKELETON, CELLULAR mechanics, RHEOLOGY (Biology), CELL anatomy, YOUNG'S modulus, MODULUS of rigidity

Abstract

Cell models play a crucial role in analyzing the mechanical response of cells and quantifying cellular damage incurred during micromanipulation. While traditional models can capture the overall mechanical behavior of cells, they often lack the ability to discern among distinct cellular components. Consequently, by employing dissipative particle dynamics, this study constructed a triangular network-like representation of the cell membrane along with cross-linked cytoskeletal chains. The mechanical properties of both the membrane and cytoskeleton were then analyzed through a series of simulated mechanical tests, validated against real-world experiments. The investigation utilized particle-tracking rheology to monitor changes in the mean square displacements of membrane particles over time, facilitating the analysis of the membrane's storage and loss moduli. Additionally, the cytoskeletal network's storage and loss moduli were examined via a double-plate oscillatory shear experiment. The simulation results revealed that both the membrane and cytoskeleton exhibit viscoelastic behavior, as evidenced by the power-law dependency of their storage and loss moduli on frequency. Furthermore, indentation and microinjection simulations were conducted to examine the overall mechanical properties of cells. In the indentation experiments, an increase in the shear modulus of the membrane's WLCs correlated with a higher Young's modulus for the entire cell. Regarding the microinjection experiment, augmenting the microinjection speed resulted in reduced deformation of the cell at the point of membrane rupture and a lower percentage of high strain. [ABSTRACT FROM AUTHOR]

Published

2024

13. In Vitro Modelling of Osteogenesis Imperfecta with Patient-Derived Induced Mesenchymal Stem Cells.

Author

Claeys, Lauria, Zhytnik, Lidiia, Ventura, Laura, Wisse, Lisanne E., Eekhoff, Elisabeth M. W., Pals, Gerard, Bravenboer, Nathalie, Heine, Vivi M., and Micha, Dimitra

Subjects

*DYSPLASIA, *MESENCHYMAL stem cells, *PLURIPOTENT stem cells, *OSTEOGENESIS imperfecta, *FIBROBLASTS, *INDUCED pluripotent stem cells, *SKELETAL dysplasia, *CELL morphology

Abstract

(1) Mesenchymal stem cells (MSCs) are a valuable cell model to study the bone pathology of Osteogenesis Imperfecta (OI), a rare genetic collagen-related disorder characterized by bone fragility and skeletal dysplasia. We aimed to generate a novel OI induced mesenchymal stem cell (iMSC) model from induced pluripotent stem cells (iPSCs) derived from human dermal fibroblasts. For the first time, OI iMSCs generation was based on an intermediate neural crest cell (iNCC) stage. (2) Skin fibroblasts from healthy individuals and OI patients were reprogrammed into iPSCs and subsequently differentiated into iMSCs via iNCCs. (3) Successful generation of iPSCs from acquired fibroblasts was confirmed with changes in cell morphology, expression of iPSC markers SOX2, NANOG, and OCT4 and three germ-layer tests. Following differentiation into iNCCs, cells presented increased iNCC markers including P75NTR, TFAP2A, and HNK-1 and decreased iPSC markers, shown to reach the iNCC stage. Induction into iMSCs was confirmed by the presence of CD73, CD105, and CD90 markers, low expression of the hematopoietic, and reduced expression of the iNCC markers. iMSCs were trilineage differentiation-competent, confirmed using molecular analyses and staining for cell-type-specific osteoblast, adipocyte, and chondrocyte markers. (4) In the current study, we have developed a multipotent in vitro iMSC model of OI patients and healthy controls able to differentiate into osteoblast-like cells. [ABSTRACT FROM AUTHOR]

Published

2024

14. Establishing an ANO1-Based Cell Model for High-Throughput Screening Targeting TRPV4 Regulators.

Author

Zheng, Kai, Hu, Jiang, Hu, Cheng, Liu, Xueying, Wang, Yanyan, Han, Haojian, Xing, Wenzhu, Yang, Liu, Zhang, Junran, Hong, Qiyuan, Hao, Feng, and Li, Wenliang

Subjects

*TRPV cation channels, *HIGH throughput screening (Drug development), *CHLORIDE channels, *FLUORESCENT proteins, *FLUORESCENCE quenching

Abstract

Transient receptor potential vanilloid 4 (TRPV4) is a widely expressed cation channel that plays an important role in many physiological and pathological processes. However, most TRPV4 drugs carry a risk of side effects. Moreover, existing screening methods are not suitable for the high-throughput screening (HTS) of drugs. In this study, a cell model and HTS method for targeting TRPV4 channel drugs were established based on a calcium-activated chloride channel protein 1 Anoctamin 1 (ANO1) and a double mutant (YFP-H148Q/I152L) of the yellow fluorescent protein (YFP). Patch-clamp experiments and fluorescence quenching kinetic experiments were used to verify that the model could sensitively detect changes in intracellular Ca2+ concentration. The functionality of the TRPV4 cell model was examined through temperature variations and different concentrations of TRPV4 modulators, and the performance of the model in HTS was also evaluated. The model was able to sensitively detect changes in the intracellular Ca2+ concentration and also excelled at screening TRPV4 drugs, and the model was more suitable for HTS. We successfully constructed a drug cell screening model targeting the TRPV4 channel, which provides a tool to study the pathophysiological functions of TRPV4 in vitro. [ABSTRACT FROM AUTHOR]

Published

2024

15. Shionone Exhibits Anti-inflammatory and Antiproliferative Effects in Pulmonary Arterial Endothelial Cells and Smooth Muscle Cells via SIRT1 in Pulmonary Arterial Hypertension

Author

Jiang, Yunfei, Hei, Bingchang, Hao, Wenbo, Lin, Shudong, Liu, Xuzhi, Meng, Xianguo, Wang, Yuanyuan, Zhao, Mingyu, Yu, Haitao, Yang, Lei, and Guan, Zhanjiang

Published

2024

16. The Application of Duck Embryonic Fibroblasts CCL-141 as a Cell Model for Adipogenesis

Author

Dan-Dan Sun, Xiao-Qin Li, Yong-Tong Liu, Meng-Qi Ge, and Zhuo-Cheng Hou

Subjects

duck, adipogenesis, CCL-141, cell model, gene knockout, Veterinary medicine, SF600-1100, Zoology, QL1-991

Abstract

The duck embryo fibroblast cell line CCL-141, which is currently the only commercialized duck cell line, has been underexplored in adipogenesis research. (1) Background: This study establishes an experimental protocol to induce adipogenesis in CCL-141 cells, addressing the importance of understanding gene functions in this process. (2) Methods: Chicken serum, fatty acids, insulin, and all-trans retinoic acid were used to treat CCL-141 cells, with adipogenesis confirmed by Oil Red O staining and gene expression quantification. CRISPR/Cas9 technology was applied to knockout PPARγ, and the resulting adipogenic phenotype was assessed. (3) Results: The treatments promoted adipogenesis, and the knockout of PPARγ validated the cell line’s utility for gene function studies. (4) Conclusions: CCL-141 cells are a suitable model for investigating duck adipogenesis, contributing to the understanding of regulatory factors in this biological process.

Published

2024

17. Human Bone Marrow Derived-Mesenchymal Stem Cells Treatment for Autoimmune Premature Ovarian Insufficiency.

Author

Ma, Wen-Qing, Zhuo, Ai-Ping, Xiao, Yuan-Ling, Gao, Meng, Yang, Yu-Tao, Tang, Li-Chao, Wu, Yan-Hong, Tian, Dan, and Fu, Xia-Fei

Subjects

*PREMATURE ovarian failure, *OVARIAN follicle, *STEM cell treatment, *BONE marrow, *GRANULOSA cells, *HORMONE synthesis

Abstract

Background: Premature ovarian insufficiency (POI) is a relatively common gynecologic endocrine disorder, which is hypogonadism associated with amenorrhea, increased levels of gonadotropins, and hypoestrogenism. POI resulting from ovarian autoimmunity is a poorly understood clinical condition lacking effective treatments. This study is aimed to investigate the therapeutic effect of mesenchymal stem cells (MSCs) on autoimmune premature ovarian insufficiency. Methods: In this study, in vivo and in vitro experiments were conducted to clarify the therapeutic effects and possible mechanisms of human bone marrow-derived MSCs (hBMSCs) on autoimmune POI, and to provide an experimental evidence for the treatment of autoimmune POI by hBMSCs. Noteworthy, in this study, we used interferon-gamma (IFN-γ) to induce autoimmune inflammation in human granulosa cell line KGN, simulating the pathophysiological changes of granulosa cells in autoimmune POI, and therefore sought to establish an in vitro cell model of autoimmune POI, which is still lacking in experimental methodology. Results: And we found that, in vitro, co-culture of hBMSCs could promote granulosa cell proliferation, inhibit apoptosis, improve hormone synthesis capacity, and reduce the occurrence of pyroptosis; and in vivo, hBMSCs resulted in improved estrous cycle disorders in autoimmune POI mice, increased serum estradiol, decreased follicle-stimulating hormone, improved ovarian morphology, increased number of primordial and primary follicles, decreased number of atretic follicles, and decreased ovarian granulosa cell apoptosis. Conclusions: hBMSCs have therapeutic effects on autoimmune POI both in vitro and in vivo. [ABSTRACT FROM AUTHOR]

Published

2024

18. Modulation of TRPV1 and TRPA1 Channels Function by Sea Anemones' Peptides Enhances the Viability of SH-SY5Y Cell Model of Parkinson's Disease.

Author

Kolesova, Yuliya S., Stroylova, Yulia Y., Maleeva, Ekaterina E., Moysenovich, Anastasia M., Pozdyshev, Denis V., Muronetz, Vladimir I., and Andreev, Yaroslav A.

Subjects

*PARKINSON'S disease, *STRAITS, *SEA anemones, *ACID-sensing ion channels, *TRPV cation channels, *ION channels

Abstract

Cellular dysfunction during Parkinson's disease leads to neuroinflammation in various brain regions, inducing neuronal death and contributing to the progression of the disease. Different ion channels may influence the process of neurodegeneration. The peptides Ms 9a-1 and APHC3 can modulate the function of TRPA1 and TRPV1 channels, and we evaluated their cytoprotective effects in differentiated to dopaminergic neuron-like SH-SY5Y cells. We used the stable neuroblastoma cell lines SH-SY5Y, producing wild-type alpha-synuclein and its mutant A53T, which are prone to accumulation of thioflavin-S-positive aggregates. We analyzed the viability of cells, as well as the mRNA expression levels of TRPA1, TRPV1, ASIC1a channels, alpha-synuclein, and tyrosine hydroxylase after differentiation of these cell lines using RT-PCR. Overexpression of alpha-synuclein showed a neuroprotective effect and was accompanied by a reduction of tyrosine hydroxylase expression. A mutant alpha-synuclein A53T significantly increased the expression of the pro-apoptotic protein BAX and made cells more susceptible to apoptosis. Generally, overexpression of alpha-synuclein could be a model for the early stages of PD, while expression of mutant alpha-synuclein A53T mimics a genetic variant of PD. The peptides Ms 9a-1 and APHC3 significantly reduced the susceptibility to apoptosis of all cell lines but differentially influenced the expression of the genes of interest. Therefore, these modulators of TRPA1 and TRPV1 have the potential for the development of new therapeutic agents for neurodegenerative disease treatment. [ABSTRACT FROM AUTHOR]

Published

2024

19. Development and characterisation of mgTHP-1, a novel in vitro model for neural macrophages with microglial characteristics.

Author

Kodosaki, E, Daniels-Morgan, A, Hassan, N, Webb, R, Morris, K, and Kelly, CM

Subjects

MACROPHAGES, MICROGLIA, CYTOLOGY, REACTIVE oxygen species, CENTRAL nervous system

Abstract

Neuroinflammation is primarily characterised by activation of the brain's resident macrophages – the microglia. However, other central nervous system (CNS) cells also contribute to this response, including the astrocytes and endothelial cells. In addition, there is infiltration into the CNS of peripherally derived immune cells. Together these cells mediate inflammation by the production of cytokines, chemokines, reactive oxygen species, and secondary messengers, and enacting of the appropriate response to those signals. However, deciphering the specific contributions of each cell type has been challenging. Studying CNS cell biology is often challenging, as the isolation of primary cells is not always feasible, and differentiation towards microglia-like cells is complex. Here, we demonstrate a novel method whereby THP-1 monocytic cells are differentiated into neural macrophage cells with microglia-like cell characteristics. The cells, designated mgTHP-1, show typical morphological and gene expression patterns of resident CNS macrophages and functionally respond to inflammatory stimuli by producing inflammatory cytokines. Furthermore, with the addition of Vicenin-2 (an anti-inflammatory flavonoid) such responses can be reversed. This novel cell model will allow further investigations, and hence insights, into the neuroinflammatory mechanisms associated with CNS diseases. [ABSTRACT FROM AUTHOR]

Published

2024

20. A cell model for evaluating mitochondrial damage in cardiomyocytes.

Author

Zhang, Yingying, Chen, Yongxue, and Zhao, Senming

Abstract

Background: Various cellular models were used for assessment of mitochondrial damage in cardiomyocyte, but most of them are based on silent cells without contractility. The mitochondria in cells at working should be more sensitive to toxic or reperfusion damage due to their high level mitochondrial respiration. Therefore, contracting cells can represent inotropic agent-mediated high-energy demand states. Objective: To establish a cellular model to detect mitochondrial damage in cardiomyocytes at contraction. Method: Freshly isolated Sprague–Dawley rat cardiomyocytes were incubated with or without bupivacaine, in the presence or absence of isoprenaline, and electrically stimulated to induce rhythmic contractions. Results: Contraction under electrical field stimulation did not induce mitochondrial swelling or ROS production in DMEM; the silent cells in the presence of bupivacaine showed mild mitochondrial swelling, but contracting cells exhibited significantly higher mitochondrial swelling and increased ROS production (P < 0.05, vs. silent cells). Isoprenaline induced a further enhancement in mitochondrial swelling and ROS production in contracting cells. Conclusions: Contracting cells are more sensitive to bupivacaine toxicity and could be more accurately represent mitochondrial damage in vivo condition. [ABSTRACT FROM AUTHOR]

Published

2024

21. First insight into extracellular vesicle-miRNA characterization in a sheep in vitro model of inflammation.

Author

Ciliberti, Maria Giovanna, Santillo, Antonella, Sevi, Agostino, Albenzio, Marzia, De Leo, Vincenzo, Ingrosso, Chiara, Catucci, Lucia, and Caroprese, Mariangela

Subjects

MONONUCLEAR leukocytes, GENE expression, SHEEP, EXTRACELLULAR vesicles

Abstract

Extracellular vesicles (EVs) and their microRNA (miRNA) cargoes have garnered attention in the veterinary field for their regulatory role in various biological processes. This study aimed to (i) evaluate two techniques of EV isolation from sheep peripheral blood mononuclear cell (PBMC) supernatants using the ultracentrifugation (UC) and reagent (REA) methods and (ii) characterize the EV-miRNA profiles after an in vitro inflammatory environment mediated by lipopolysaccharides (LPS). Sheep peripheral blood was collected, and PBMCs were separated using a density gradient reagent. Subsequently, PBMCs were cultured at 37°C for 24 h (5% CO2), and the supernatants were collected to perform the EV isolation. The presence of CD81+ extracellular vesicle marker was determined, and the purity of isolated EVs was calculated as a ratio between the number of isolated EVs and the protein concentration. Moreover, the morphological characterization revealed mainly round-shaped structures with average sizes of 211 nm for EVs isolated by the UC method and 99 nm for EVs isolated by the REA method. Illumina NextSeq sequencing in a single-end mode was used to characterize the miRNA profile, and the differentially expressed (DE) miRNAs were analyzed using a combination of bioinformatics tools. The results revealed that the REA method is reliable for EV isolation from sheep supernatants. It was considered an improvement of the recovery rate and purity of EVs with the enhancement of the number and the expression levels of characterized miRNAs. The EVs isolated by the UC method after an LPS challenge showed 11 DE miRNAs, among which eight miRNAs were upregulated and three were downregulated. On the other hand, the REA method revealed an EV cargo in which eight DE miRNAs were upregulated and 21 DE miRNAs were downregulated. The master miRNA regulators of the biological process were identified by performing the MIRNA-mRNA network analysis, showing that, among the higher representative miRNAs based on the centrality and betweenness, the miR-26a-5p could have a crucial role in the resolution of inflammation. Moreover, the identification of the let-7 miRNA family in all the EVs showed potential targeted genes that regulate the inflammation and immune responses. [ABSTRACT FROM AUTHOR]

Published

2023

22. An optimised protocol for the investigation of insulin signalling in a human cell culture model of adipogenesis.

Author

Gamwell, Jonathan M., Paphiti, Keanu, Hodson, Leanne, Karpe, Fredrik, Pinnick, Katherine E., and Todorčević, Marijana

Subjects

*HUMAN cell culture, *CELL communication, *ADIPOGENESIS, *INSULIN, *HUMAN stem cells

Abstract

While there is no standardized protocol for the differentiation of human adipocytes in culture, common themes exist in the use of supra-physiological glucose and hormone concentrations, and an absence of exogenous fatty acids. These factors can have detrimental effects on some aspects of adipogenesis and adipocyte function. Here, we present methods for modifying the adipogenic differentiation protocol to overcome impaired glucose uptake and insulin signalling in human adipose-derived stem cell lines derived from the stromal vascular fraction of abdominal and gluteal subcutaneous adipose tissue. By reducing the length of exposure to adipogenic hormones, in combination with a physiological glucose concentration (5 mM), and the provision of exogenous fatty acids (reflecting typical dietary fatty acids), we were able to restore early insulin signalling events and glucose uptake, which were impaired by extended use of hormones and a high glucose concentration, respectively. Furthermore, the addition of exogenous fatty acids greatly increased the storage of triglycerides and removed the artificial demand to synthesize all fatty acids by de novo lipogenesis. Thus, modifying the adipogenic cocktail can enhance functional aspects of human adipocytes in vitro and is an important variable to consider prior to in vitro investigations into adipocyte biology. [ABSTRACT FROM AUTHOR]

Published

2023

23. Oral Galvanism Side Effects: Comparing Alloy Ions and Galvanic Current Effects on the Mucosa-like Model.

Author

Chepelova, Natalia, Antoshin, Artem, Voloshin, Sergei, Usanova, Anna, Efremov, Yuri, Makeeva, Maria, Evlashin, Stanislav, Stepanov, Mikhail, Turkina, Anna, and Timashev, Peter

Subjects

ELECTRICITY, DENTAL metallurgy, CORROSION in alloys, IONS, ALLOYS, ELECTROLYTIC corrosion

Abstract

The interaction of different dental alloys with the oral environment may cause severe side effects (e.g., burning sensation, inflammatory reactions, carcinogenesis) as a result of oral galvanism. However, the pathogenesis of side effects associated with oral galvanism is still unclear, and the effects of direct current and alloy corrosion ions are considered potentially contributing factors. Therefore, the aim of this study was to systemically compare the damaging effects of (1) galvanism as a synergistic process (direct current + corrosion ions), (2) direct current separately, and (3) corrosion ions separately on an in vitro mucosa-like model based on a cell line of immortalized human keratinocytes (HaCaTs) to reveal the factors playing a pivotal role in dental alloys side effects. For this, we chose and compared the dental alloys with the highest risk of oral galvanism: Ti64–AgPd and NiCr–AgPd. We showed that galvanic current may be the leading damaging factor in the cytotoxic processes associated with galvanic coupling of metallic intraoral appliances in the oral cavity, especially in the short-term period (28 days). However, the contribution of corrosion ions (Ni2+) to the synergistic toxicity was also shown, and quite possibly, in the long term, it could be no less dangerous. [ABSTRACT FROM AUTHOR]

Published

2023

24. Conditional reprogrammed human limbal epithelial cell model for anti-SARS-CoV-2 drug screening

Author

Yu Xiao, Ling Wang, Shi-xu Li, Shi-song Fang, Fan Luo, Shu-liang Chen, Xuan Zou, Lin Ye, and Wei Hou

Subjects

COVID-19, Limbal, Cell model, Drug screening, Science (General), Q1-390, Social sciences (General), H1-99

Abstract

To minimize the global pandemic COVID-19 spread, understanding the possible transmission routes of SARS-CoV-2 and discovery of novel antiviral drugs are necessary. We describe here that the virus can infect ocular surface limbal epithelial, but not other regions. Limbal supports wild type and mutant SARS-CoV-2 entry and replication depending on ACE2, TMPRSS2 and possibly other receptors, resulting in slight CPE and arising IL-6 secretion, which symbolizes conjunctivitis in clinical symptoms. With this limbal model, we have screened two natural product libraries and discovered several unreported drugs. Our data reveal important commonalities between COVID-19 and ocular infection with SARS-CoV-2, and establish an ideal cell model for drug screening and mechanism research.

Published

2024

25. Modelling α-synuclein processing in primary patient cells for pharmacological intervention

Author

Jessica K. Smith, George D. Mellick, and Alex M. Sykes

Subjects

α-synuclein, parkinson’s disease, protein trafficking, cell model, drug screen, Other systems of medicine, RZ201-999

Abstract

Aim: Parkinson’s disease (PD) is a complex, chronic neurodegenerative disorder with predominately sporadic etiology. Intricate genetic-environmental interactions lead to the hallmarks of the disease: degeneration of dopaminergic neurons and the deposition of α-synuclein aggregates. The aim of this study was to establish a novel primary patient cell model as an in vitro screen to study α-synuclein processing for drug screening. Methods: Primary patient olfactory neuroepithelial-derived cells (ONS) were exposed to α-synuclein and examined for cytotoxicity, processing, and solubility over 48 h. Epigallocatechin gallate (EGCG), which is known to destabilise α-synuclein fibrils, was used to investigate the solubilisation of α-synuclein in the model system. Results: Exposure to 0.1 μmol/L α-synuclein preformed fibrils was not toxic to ONS over 48 h. ONS processing of α-synuclein was observed to be different in PD cells by their increased accumulation in the cytoplasm. Processing deficits in the PD ONS were confirmed by immunoblotting with an increase in sodium dodecyl sulfate (SDS)-insoluble α-synuclein after 48 h. Conclusions: The data has illustrated the utility of primary patient ONS as a model system to understand the processing of α-synuclein. Considerable differences in α-synuclein processing were identified in PD ONS. Furthermore, the data suggests that primary patient ONS are a viable in vitro drug screening platform for α-synuclein pathology in PD.

Published

2023

26. Estimating Parameters of 3D Cell Model Using a Bayesian Recursive Global Optimizer (BaRGO)

Author

Miotti, Pietro, Filippi-Mazzola, Edoardo, Wit, Ernst C., Pivkin, Igor V., Goos, Gerhard, Founding Editor, Hartmanis, Juris, Founding Editor, Bertino, Elisa, Editorial Board Member, Gao, Wen, Editorial Board Member, Steffen, Bernhard, Editorial Board Member, Yung, Moti, Editorial Board Member, Mikyška, Jiří, editor, de Mulatier, Clélia, editor, Paszynski, Maciej, editor, Krzhizhanovskaya, Valeria V., editor, Dongarra, Jack J., editor, and Sloot, Peter M.A., editor

Published

2023

27. Establishment of a Burkholderia thailandensis invaded RAW264.7 cell model and underlying mechanism of infection

Author

LI Jin, LI Min, and LU Weiping

Subjects

burkholderia thailandensis, raw264.7 cells, cell model, inflammatory factors, infection mechanism, Medicine (General), R5-920

Abstract

Objective To establish a cell model of Burkholderia thailandensis (B. thailandensis, our isolated strain was named as BPM) infecting RAW264.7 cells in order to lay a foundation for further study on its pathogenic mechanism. Methods The bacterial solution containing same concentration of BPM was prepared to infect RAW264.7 cells with different diluted concentrations. The bacterial entry rate and intracellular survival status were analyzed by the bacterial uptake rate of BPM in RAW264.7 cells at different infection phases. The intracellular infection of bacteria and the ultra-structural pathological changes of host cells were dynamically observed by transmission electron microscopy (TEM) and Giemsa staining. The apoptosis induced by different phase points was detected by flow cytometry. The expression of inflammatory factors in cell supernatant was detected by LEGENDplexTM reagent. Results TEM displayed that some bacteria invaded into the cells 12 h after infection. The formation of typical multinucleate giant cells (MNGC) was observed at the earliest 8 h after BPM infection by Giemsa staining. With the elapse of infection time, MNGC formation rate and inflammatory factor expression were gradually increased. Conclusion The intracellular infection model of BPM is successfully constructed, and the inflammatory response of B. thailandensis infection in host cells is clarified, laying the experimental foundation for further study of the mechanism of B. thailandensis infection.

Published

2023

28. Research progress on immune function of food-derived bioactive peptides

Author

ZHANG Zhi-meng, NI Ce, OU Xiao-hui, CAO Tian-hong, CHENG Yun-hui, and WEN Li

Subjects

bioactive peptide, immune, immunopeptide, inflammatory response, cell model, animal models, Food processing and manufacture, TP368-456

Abstract

Food-derived bioactive peptides play an immunoregulation role by regulating signal pathways and influencing the expression of cytokines in vivo. This review summarizes immunoregulatory effects of the food-derived protein hydrolysates and bioactive peptides on cells, animal models and human beings, and the immune mechanism of food-derived bioactive peptides in different models is explained. Finally, the future application of bioactive peptides is prospected.

Published

2023

29. Metabolomics comparison of metabolites and functional pathways in the SH-SY5Y cell model of Parkinson's disease under PEMF exposure

Author

Li-na Zhu, Deng Chen, and Chengqi He

Subjects

PEMF, Metabolomics, PD, SH-SY5Y, Cell model, Science (General), Q1-390, Social sciences (General), H1-99

Abstract

Objective: PEMF is an emerging technique in the treatment of Parkinson's disease (PD) due to its potential improvement of movement speed. The aim of this study was to investigate the metabolic profiles of pulsed electromagnetic fields (PEMFs) in an SH-SY5Y cell model of PD. Methods: The SH-SY5Y cell model of PD was induced by 1-methyl-4-phenylpyridinium (MPP+). Liquid chromatography mass spectrometry (LC‒MS)-based untargeted metabolomics was performed to examine changes in the PD cell model with or without PEMF exposure. We conducted KEGG pathway enrichment analysis to explore the potentially related pathways of the differentially expressed metabolites. Results: A total of 275 metabolites were annotated, and 27 significantly different metabolites were found between the PEMF treatment and control groups (VIP >1, P

Published

2024

30. Models of gouty nephropathy: exploring disease mechanisms and identifying potential therapeutic targets

Author

Lin Wang, Xiaoyu Zhang, Jiayan Shen, Yuanyuan Wei, Ting Zhao, Niqin Xiao, Xiaoman Lv, Dongdong Qin, Yundong Xu, Yang Zhou, Jing Xie, Zhaofu Li, and Zhaohu Xie

Subjects

gouty nephropathy, pathogenesis, animal models, cell model, uric acid, Medicine (General), R5-920

Abstract

Gouty nephropathy (GN) is a metabolic disease with persistently elevated blood uric acid levels. The main manifestations of GN are crystalline kidney stones, chronic interstitial nephritis, and renal fibrosis. Understanding the mechanism of the occurrence and development of GN is crucial to the development of new drugs for prevention and treatment of GN. Currently, most studies exploring the pathogenesis of GN are primarily based on animal and cell models. Numerous studies have shown that inflammation, oxidative stress, and programmed cell death mediated by uric acid and sodium urate are involved in the pathogenesis of GN. In this article, we first review the mechanisms underlying the abnormal intrinsic immune activation and programmed cell death in GN and then describe the characteristics and methods used to develop animal and cell models of GN caused by elevated uric acid and deposited sodium urate crystals. Finally, we propose potential animal models for GN caused by abnormally high uric acid levels, thereby provide a reference for further investigating the methods and mechanisms of GN and developing better prevention and treatment strategies.

Published

2024

31. MiR-21-5p modulates LPS-induced acute injury in alveolar epithelial cells by targeting SLC16A10

Author

Zeng, Huanan, Zhou, Yuqing, Liu, Zhi, and Liu, Wei

Published

2024

32. Tanshinol inhibits trophoblast cell migration and invasion by regulating Gadd45a in preeclampsia

Author

Yanlin Yang, Haixia Shang, Jingfen Sun, Xiaofeng Shi, and Bohui Zhou

Subjects

Tanshinol, preeclampsia, Gadd45a, HTR-8/SVneo, cell model, Gynecology and obstetrics, RG1-991

Abstract

AbstractObjective Tanshinol is an active constituent of Salvia miltiorrhiza that possesses anti-inflammatory, antioxidant, and antibacterial activities. Therefore, this study attempted to detect whether it has a role in the treatment of preeclampsia (PE).Methods In this study, we explored the effect of tanshinol on the development of PE at the cellular level. The effect of tanshinol on cell proliferation was measured by colony formation and EdU assays. The migration, invasion, and in vitro angiogenesis of HTR-8/SVneo cells were detected by wound-healing, transwell, and tube formation assays, respectively. In addition, a PE cell model was established by overexpression of Gadd45a, and this cell model was assessed with the optimal concentration of tanshinol.Results The results show that tanshinol enhanced proliferation, migration, invasion, and tube formation of HTR-8/SVneo cells in vitro. Furthermore, the reduction in proliferation, migration, invasion, and tube formation of cells by Gadd45a overexpression was partially reversed by tanshinol treatment. Tanshinol also inhibited the apoptosis of HTR-8/SVneo cells transfected with Gadd45a.Conclusions In summary, tanshinol promoted proliferation, migration, invasion, and tube formation and inhibited the apoptosis of HTR-8/SVneo cells. It may be a novel therapeutic compound to attenuate the development of PE.

Published

2023

33. An optimised protocol for the investigation of insulin signalling in a human cell culture model of adipogenesis

Author

Jonathan M. Gamwell, Keanu Paphiti, Leanne Hodson, Fredrik Karpe, Katherine E. Pinnick, and Marijana Todorčević

Subjects

Adipogenic cocktail, adipose stem cell, adipocyte, cell model, insulin signalling, glucose uptake, Diseases of the endocrine glands. Clinical endocrinology, RC648-665, Cytology, QH573-671, Physiology, QP1-981

Abstract

ABSTRACTWhile there is no standardized protocol for the differentiation of human adipocytes in culture, common themes exist in the use of supra-physiological glucose and hormone concentrations, and an absence of exogenous fatty acids. These factors can have detrimental effects on some aspects of adipogenesis and adipocyte function. Here, we present methods for modifying the adipogenic differentiation protocol to overcome impaired glucose uptake and insulin signalling in human adipose-derived stem cell lines derived from the stromal vascular fraction of abdominal and gluteal subcutaneous adipose tissue. By reducing the length of exposure to adipogenic hormones, in combination with a physiological glucose concentration (5 mM), and the provision of exogenous fatty acids (reflecting typical dietary fatty acids), we were able to restore early insulin signalling events and glucose uptake, which were impaired by extended use of hormones and a high glucose concentration, respectively. Furthermore, the addition of exogenous fatty acids greatly increased the storage of triglycerides and removed the artificial demand to synthesize all fatty acids by de novo lipogenesis. Thus, modifying the adipogenic cocktail can enhance functional aspects of human adipocytes in vitro and is an important variable to consider prior to in vitro investigations into adipocyte biology.

Published

2023

34. Evaluate the Protective Effect of Antioxidants on Retinal Pigment Cell Hazard Induced by Blue Light: A Mini-Review.

Author

Lu, Yujing and Qi, Hang

Subjects

*BLUE light, *RHODOPSIN, *CHROMATOPHORES, *MACULAR degeneration, *MONOCHROMATIC light, *MELANOPSIN, *LIGHT sources

Abstract

In recent years, with the emergence of complex lighting technology, people are more exposed to artificial light sources, and people are more concerned about the damage of light to eyes. While the eyes have adapted several mechanisms to protect themselves from this damage, certainly exposure to light can still cause temporary or permanent damage. Blue light has been reported to be more damaging than white and green light. Blue light can cause retinal degeneration and is a major cause of the onset and development of severe age-related macular degeneration (AMD). This review introduces the protective effects of various antioxidants on blue light-induced retinal damage based on cell models in a more realistic biological environment and points out the direction for the prevention of retinal blue light damage and future research. [ABSTRACT FROM AUTHOR]

Published

2023

35. N-acetylcysteine modulates rotenone-induced mitochondrial Complex I dysfunction in THP-1 cells.

Author

Kwok, Winston Tse-Hou, Kwak, Haejin Angela, and Andreazza, Ana Cristina

Subjects

*MITOCHONDRIA, *ACETYLCYSTEINE, *PARKINSON'S disease, *ROTENONE

Abstract

• N-acetylcysteine modulates rotenone-induced mitochondrial Complex I dysfunction. • N-acetylcysteine can ameliorate the rotenone-induced increase of cell-free mitochondrial DNA. • Rotenone exposure affect complex I protein glutathionylation. • N-acetylcysteine may help to preserve the normal function of mitochondria in THP-1 cells. Mitochondrial Complex I dysfunction and oxidative stress have been part of the pathophysiology of several diseases ranging from mitochondrial disease to chronic diseases such as diabetes, mood disorders and Parkinson's Disease. Nonetheless, to investigate the potential of mitochondria-targeted therapeutic strategies for these conditions, there is a need further our understanding on how cells respond and adapt in the presence of Complex I dysfunction. In this study, we used low doses of rotenone, a classical inhibitor of mitochondrial complex I, to mimic peripheral mitochondrial dysfunction in THP-1 cells, a human monocytic cell line, and explored the effects of N-acetylcysteine on preventing this rotenone-induced mitochondrial dysfunction. Our results show that in THP-1 cells, rotenone exposure led to increases in mitochondrial superoxide, levels of cell-free mitochondrial DNA, and protein levels of the NDUFS7 subunit. N-acetylcysteine (NAC) pre-treatment ameliorated the rotenone-induced increase of cell-free mitochondrial DNA and NDUFS7 protein levels, but not mitochondrial superoxide. Furthermore, rotenone exposure did not affect protein levels of the NDUFV1 subunit but induced NDUFV1 glutathionylation. In summary, NAC may help to mitigate the effects of rotenone on Complex I and preserve the normal function of mitochondria in THP-1 cells. [ABSTRACT FROM AUTHOR]

Published

2023

36. The Mitochondrial m.3243A>G Mutation on the Dish, Lessons from In Vitro Models.

Author

Ryytty, Sanna and Hämäläinen, Riikka H.

Subjects

*MITOCHONDRIAL DNA, *PLURIPOTENT stem cells, *GENETIC mutation, *MITOCHONDRIA

Abstract

The m.3243A>G mutation in the tRNA Leu(UUR) gene (MT-TL1) is one of the most common pathogenic point mutations in human mtDNA. Patient symptoms vary widely and the severity of the disease ranges from asymptomatic to lethal. The reason for the high heterogeneity of m.3243A>G-associated disease is still unknown, and the treatment options are limited, with only supportive interventions available. Furthermore, the heteroplasmic nature of the m.3243A>G mutation and lack of specific animal models of mtDNA mutations have challenged the study of m.3243A>G, and, besides patient data, only cell models have been available for studies. The most commonly used cell models are patient derived, such as fibroblasts and induced pluripotent stem cell (iPSC)-derived models, and cybrid models where the mutant DNA is transferred to an acceptor cell. Studies on cell models have revealed cell-type-specific effects of the m.3243A>G mutation and that the tolerance for this mutation varies between cell types and between patients. In this review, we summarize the literature on the effects of m.3243A>G in cell models. [ABSTRACT FROM AUTHOR]

Published

2023

37. Effect of Cell Generations on t-BHP-induced Oxidative Stress Model of Caco-2 Cells

Author

Jun NI, Cailian YUAN, Rong SHE, Chengfa ZHAO, Lijuan LI, Xu YANG, and Xiaoyan YANG

Subjects

caco-2 cells, tert-butyl hydrogen peroxide, oxidative stress, cell model, cell passage number, 8-hydroxydeoxyguanosine, Food processing and manufacture, TP368-456

Abstract

Objective: To investigate the effects of cell passage number on the establishment of an oxidative stress model in human colon adenocarcinoma cells (Caco-2) caused by tert-butyl hydroperoxide (t-BHP). Methods: First, by applying various t-BHP concentrations (1, 2 and 3 mmol/L) to the F15 generation of Caco-2 cells for 1, 2, 3, 4, 5 and 6 hours, the content of malondialdehyde (MDA) and 8-hydroxydeoxyguanosine (8-OHdG) in different treatment groups were measured to determine the basic conditions for constructing the oxidative stress model of Caco-2 cells. Then, based on the fundamental parameters, the effect of cell passage number (F14, F15, F18, F19 and F20) on the development of oxidative stress model was investigated using the content of 8-OHdG as an index. Results: When exposed to 1, 2 and 3 mmol/L of t-BHP for 3 to 6 hours, the oxidative stress model of Caco-2 cells from the F15 generation could be established steadily. The content of 8-OHdG in Caco-2 cells of the F14, F15 and F18 generations was significantly higher than that in control group (which had not been treated with t-BHP) after being exposed to 2.0 mmol/L t-BHP for 5 hours (P

Published

2023

38. A Simulation of the Mechanical Testing of the Cell Membrane and Cytoskeleton

Author

Yue Du, Dai Cheng, Zhanli Yang, Yaowei Liu, Qili Zhao, Mingzhu Sun, Haifeng Li, and Xin Zhao

Subjects

cell model, DPD, bulk rheology, indentation, cell penetration, cytoskeleton, Mechanical engineering and machinery, TJ1-1570

Abstract

Cell models play a crucial role in analyzing the mechanical response of cells and quantifying cellular damage incurred during micromanipulation. While traditional models can capture the overall mechanical behavior of cells, they often lack the ability to discern among distinct cellular components. Consequently, by employing dissipative particle dynamics, this study constructed a triangular network-like representation of the cell membrane along with cross-linked cytoskeletal chains. The mechanical properties of both the membrane and cytoskeleton were then analyzed through a series of simulated mechanical tests, validated against real-world experiments. The investigation utilized particle-tracking rheology to monitor changes in the mean square displacements of membrane particles over time, facilitating the analysis of the membrane’s storage and loss moduli. Additionally, the cytoskeletal network’s storage and loss moduli were examined via a double-plate oscillatory shear experiment. The simulation results revealed that both the membrane and cytoskeleton exhibit viscoelastic behavior, as evidenced by the power-law dependency of their storage and loss moduli on frequency. Furthermore, indentation and microinjection simulations were conducted to examine the overall mechanical properties of cells. In the indentation experiments, an increase in the shear modulus of the membrane’s WLCs correlated with a higher Young’s modulus for the entire cell. Regarding the microinjection experiment, augmenting the microinjection speed resulted in reduced deformation of the cell at the point of membrane rupture and a lower percentage of high strain.

Published

2024

39. In Vitro Modelling of Osteogenesis Imperfecta with Patient-Derived Induced Mesenchymal Stem Cells

Author

Lauria Claeys, Lidiia Zhytnik, Laura Ventura, Lisanne E. Wisse, Elisabeth M. W. Eekhoff, Gerard Pals, Nathalie Bravenboer, Vivi M. Heine, and Dimitra Micha

Subjects

induced mesenchymal stem cells, cell model, osteoblast, bone, skeletal dysplasia, Osteogenesis Imperfecta, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

(1) Mesenchymal stem cells (MSCs) are a valuable cell model to study the bone pathology of Osteogenesis Imperfecta (OI), a rare genetic collagen-related disorder characterized by bone fragility and skeletal dysplasia. We aimed to generate a novel OI induced mesenchymal stem cell (iMSC) model from induced pluripotent stem cells (iPSCs) derived from human dermal fibroblasts. For the first time, OI iMSCs generation was based on an intermediate neural crest cell (iNCC) stage. (2) Skin fibroblasts from healthy individuals and OI patients were reprogrammed into iPSCs and subsequently differentiated into iMSCs via iNCCs. (3) Successful generation of iPSCs from acquired fibroblasts was confirmed with changes in cell morphology, expression of iPSC markers SOX2, NANOG, and OCT4 and three germ-layer tests. Following differentiation into iNCCs, cells presented increased iNCC markers including P75NTR, TFAP2A, and HNK-1 and decreased iPSC markers, shown to reach the iNCC stage. Induction into iMSCs was confirmed by the presence of CD73, CD105, and CD90 markers, low expression of the hematopoietic, and reduced expression of the iNCC markers. iMSCs were trilineage differentiation-competent, confirmed using molecular analyses and staining for cell-type-specific osteoblast, adipocyte, and chondrocyte markers. (4) In the current study, we have developed a multipotent in vitro iMSC model of OI patients and healthy controls able to differentiate into osteoblast-like cells.

Published

2024

40. INCREASED EXPRESSION OF AKR1C2 AND AKR1B1 GENES IS ASSOCIATED WITH THE DEVELOPMENT OF RESISTANCE TO DOCETAXEL IN PROSTATE CANCER

Author

Pudova Е.A.

Subjects

рак предстательной железы, химиотерапия, доцетаксел, резистентность, клеточная модель, экспрессия, prostate cancer, chemotherapy, docetaxel, resistance, cell model, expression, Genetics, QH426-470

Abstract

Drug resistance is one of the most pressing issues in modern oncology and is a result of the combination of various molecular events in tumor cells under the influence of a drug, the full understanding of which is yet to be determined. The present study focused mainly on evaluating the expressionof genesfrom the aldo-keto reductase family during the development of chemoresistance in prostate cancer (PC) – one of the most common and socially significant types of cancer in men worldwide. Using transcriptomic profiling of a PC cell model during the development of resistance to the taxane docetaxel, a statistically significant increase in the expression of two genes from the aldo-keto reductase family, AKR1C2 and AKR1B1, was demonstrated, which was also confirmed by quantitative PCR. The obtained results emphasize the high potential of these genes for further research as promising markers of resistance, as well as therapeutic targets.

Published

2023

41. First insight into extracellular vesicle-miRNA characterization in a sheep in vitro model of inflammation

Author

Maria Giovanna Ciliberti, Antonella Santillo, Agostino Sevi, Marzia Albenzio, Vincenzo De Leo, Chiara Ingrosso, Lucia Catucci, and Mariangela Caroprese

Subjects

biomarkers, LPS, cell model, livestock, immune system, small ruminant, Veterinary medicine, SF600-1100

Abstract

Extracellular vesicles (EVs) and their microRNA (miRNA) cargoes have garnered attention in the veterinary field for their regulatory role in various biological processes. This study aimed to (i) evaluate two techniques of EV isolation from sheep peripheral blood mononuclear cell (PBMC) supernatants using the ultracentrifugation (UC) and reagent (REA) methods and (ii) characterize the EV-miRNA profiles after an in vitro inflammatory environment mediated by lipopolysaccharides (LPS). Sheep peripheral blood was collected, and PBMCs were separated using a density gradient reagent. Subsequently, PBMCs were cultured at 37°C for 24 h (5% CO2), and the supernatants were collected to perform the EV isolation. The presence of CD81+ extracellular vesicle marker was determined, and the purity of isolated EVs was calculated as a ratio between the number of isolated EVs and the protein concentration. Moreover, the morphological characterization revealed mainly round-shaped structures with average sizes of 211 nm for EVs isolated by the UC method and 99 nm for EVs isolated by the REA method. Illumina NextSeq sequencing in a single-end mode was used to characterize the miRNA profile, and the differentially expressed (DE) miRNAs were analyzed using a combination of bioinformatics tools. The results revealed that the REA method is reliable for EV isolation from sheep supernatants. It was considered an improvement of the recovery rate and purity of EVs with the enhancement of the number and the expression levels of characterized miRNAs. The EVs isolated by the UC method after an LPS challenge showed 11 DE miRNAs, among which eight miRNAs were upregulated and three were downregulated. On the other hand, the REA method revealed an EV cargo in which eight DE miRNAs were upregulated and 21 DE miRNAs were downregulated. The master miRNA regulators of the biological process were identified by performing the MIRNA-mRNA network analysis, showing that, among the higher representative miRNAs based on the centrality and betweenness, the miR-26a-5p could have a crucial role in the resolution of inflammation. Moreover, the identification of the let-7 miRNA family in all the EVs showed potential targeted genes that regulate the inflammation and immune responses.

Published

2023

42. Study of the Thermochemical Effect on the Transport and Structural Characteristics of Heterogeneous Ion-Exchange Membranes by Combining the Cell Model and the Fine-Porous Membrane Model.

Author

Filippov, Anatoly N., Akberova, Elmara M., and Vasil'eva, Vera I.

Subjects

*ION-permeable membranes, *POLYMERIC membranes, *ION exchange resins, *ELECTRIC conductivity, *PERMEABILITY

Abstract

For the first time, based on the joint application of the fine-porous and cell models, a theoretical analysis of the changing transport and structural characteristics of heterogeneous polymeric ion-exchange membranes (IEMs) MK-40, MA-40, and MA-41 after exposure to elevated temperatures in water and aggressive media (H2SO4 and NaOH solutions), as well as after long-term processing in electrodialyzers of various types, was carried out. The studied membranes are composites of ion-exchange polymers with polyethylene and nylon reinforcing mesh. The external influences provoke the aging of IEMs and the deterioration of their characteristics. The transport properties of IEMs are quantitatively described using five physicochemical parameters: counterion diffusion and equilibrium distribution coefficients in the membrane, characteristic exchange capacity, which depends on the microporosity of ion-exchanger particles, and macroscopic porosity at a known exchange capacity of IEMs. Calculations of the physicochemical parameters of the membranes were performed according to a specially developed fitting technique using the experimental concentration dependences of integral diffusion permeability and specific electrical conductivity, and their model analogs. This made it possible to identify and evaluate changes in the membrane micro- and macrostructure and examine the process of artificial aging of the IEM polymer material due to the abovementioned external impacts. [ABSTRACT FROM AUTHOR]

Published

2023

43. 基于氧化应激的固态发酵白酒抑制肝癌HepG2细胞增殖.

Author

周琦, 管祺杰, and 耿燕

Subjects

NUCLEAR factor E2 related factor, INHIBITION of cellular proliferation, ALCOHOL dehydrogenase, XANTHINE oxidase, REACTIVE oxygen species, CHO cell, ETHANOL, QUINONE compounds

Abstract

Copyright of Journal of Chinese Institute of Food Science & Technology is the property of Journal of Chinese Institute of Food Science & Technology Periodical Office and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2023

44. Leukemogenic SHP2 mutations lead to erythropoietin independency of HCD-57 cells: a novel model for preclinical research of SHP2-mutant JMML

Author

Yuming Zhao, Chunxiao He, Dengyang Zhang, Yao Guo, Zhiyong Peng, Liuting Yu, Na Li, Chun Chen, Zhizhuang Joe Zhao, and Yun Chen

Subjects

SHP2, Cell model, JMML, HCD-57, Diseases of the blood and blood-forming organs, RC633-647.5, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Abstract Leukemogenic SHP2 mutations occur in 35% of patients with juvenile myelomonocytic leukemia (JMML), a rare but fatal hematopoietic malignancy without representative cell models, which are urgently needed to investigate the pathogenesis and to develop novel therapeutic strategies. In this study, we established stable cell lines with aberrant signaling resembling SHP2-mutant JMML through retroviral expression of SHP2-D61Y/E76K in HCD-57 cells, a murine erythroleukemia cell line that depends on erythropoietin (EPO) for survival. SHP2-D61Y/E76K drives the survival and proliferation of HCD-57 cells in the absence of EPO, but not in Ba/F3 cells in the absence of IL-3. Transformed HCD-57 cells showed activated MAPK signaling that is consistent with SHP2-mutant JMML. Transformed HCD-57 cells were sensitive to dasatinib and trametinib, two targeted drugs previously reported to inhibit SHP2-mutant JMML cells. Furthermore, we injected mutant SHP2-transformed HCD-57 cells into immune-deficient mice intravenously and found that these cells rapidly proliferated in the spleen and bone marrow, providing an excellent model for in vivo testing of drugs targeting the aberrant signaling of mutant SHP2. In conclusion, we established the novel cell lines HCD-57/SHP2-E76K and -D61Y that depended on signaling of mutant SHP2 for survival, thus resembling SHP2-mutant JMML. Our model is a valuable tool to investigate the pathogenic mechanisms of mutant SHP2 and targeted drugs for SHP2-mutant JMML.

Published

2023

45. A discussion of 'unsaturated cell model of effective thermal conductivity of soils'

Author

Hans Janssen

Subjects

Cell model, Unsaturated soils, Thermal conductivity, Maxwell-Eucken, Hashin-Shtrickman, Science, Technology

Abstract

Article highlights This post-publication review voices a number of concerns on an article previously published in the journal. It reveals a number of hidden weaknesses that are considered of interest to the readers of the commented article. It moreover argues that the correction of the used model voids the presented analysis of impact on the research field.

Published

2022

46. Nutritional assessment models for diabetes and aging

Author

Yuxi Wen, Yuanyuan Liu, Qihui Huang, Mohamed A. Farag, Xiaoqing Li, Xuzhi Wan, and Chao Zhao

Subjects

aging, animal model, assessment, cell model, diabetes, food nutrition, Nutrition. Foods and food supply, TX341-641, Food processing and manufacture, TP368-456

Abstract

Abstract Diabetes is a chronic disease, and its complexity and its various complications complicate studies in diabetes management. Aging is one of the main risk factors for diabetes, and elderly are a high‐risk group for developing the disease. In recent years, increasing evidence has revealed the underlying molecular basis for aging diabetes and its connection to related signal pathways. Several key pathways in the aging process can affect insulin secretion and induce diabetes. In this review, we propose a possible connection between diabetes and aging in terms of development timeline and molecular pathology to better understand this interaction between two diseases, especially aging diabetes. Additionally, cell and animal models associated with diabetes are summarized, as well as a summary of models currently being used to study aging diabetes, and their strengths and limitations are also presented. The explanation of these types of models would help us to better understand the relationship between type 2 diabetes and aging and provide a basis for subsequent research on disease mechanisms and/or drug development.

Published

2022

47. Slow Flow Past a Slip Sphere in Cell Model: Magnetic Effect

Author

Prasad, Madasu Krishna, Sarkar, Priya, Cavas-Martínez, Francisco, Series Editor, Chaari, Fakher, Series Editor, di Mare, Francesca, Series Editor, Gherardini, Francesco, Series Editor, Haddar, Mohamed, Series Editor, Ivanov, Vitalii, Series Editor, Kwon, Young W., Series Editor, Trojanowska, Justyna, Series Editor, Bharti, Ram P., editor, and Gangawane, Krunal M., editor

Published

2022

48. Holistic Equivalent Circuit Model for Capacitive Extracellular Stimulation

Author

Polz Mathias, Rath Thomas, Trimmel Gregor, Stoppacher Sara, Nowakowska Marta, Kornmüller Karin, Shestha Niroj, Baumgartner Christian, and Rienmüller Theresa

Subjects

extracellular stimulation, electrode-cell interaction, cell model, patch clamp simulation, oepc, Medicine

Abstract

Capacitive extracellular stimulation is a common method in implanted stimulation electrodes. The basis for investigating the transmission of stimuli from an electrode to adhered cells are in vitro experiments using calcium imaging or patch clamp measurements. Computational spatial models are used to simulate the mechanism of signal transmission at the cell-electrode interface but require high computing power. In this work, the Stern model to characterize the electrochemical double-layer (EDL) formation and a modified two-domain model are combined into a holistic equivalent circuit modelling capacitive cell stimulation. The described parameters can be directly associated with physicochemical effects. A simulation of the involved control and measurement systems allows the validation of the model with in vitro patch clamp recordings. The relationship of the cell’s distance to the electrode and efficacy of signal transmission could be observed. With this concept we aim to convert different complex approaches into a simple model and thus give an overview of the mechanisms of stimulation. We want to facilitate the interpretation of measured signals especially in voltage clamp measurements.

Published

2022

49. Strategies for understanding the role of cellular heterogeneity in the pathogenesis of lung cancer: a cell model for chronic exposure to cigarette smoke extract

Author

Dong Xia, Jieyi Liu, Juanjuan Yong, Xiang Li, Weidong Ji, Zhiqiang Zhao, Xiaohui Wang, Chen Xiao, Sai Wu, Huaixiang Liu, Heping Zhao, and Yun He

Subjects

Cell model, Cell heterogeneity, Malignant transformation, Invasion-phenotype, Chronic exposure, Diseases of the respiratory system, RC705-779

Abstract

Abstract Background Human tumors are highly heterogeneous at the cellular, molecular, genetic and functional levels. Tumor heterogeneity has tremendous impact on cancer progression and treatment responses. However, the mechanisms for tumor heterogeneity have been poorly understood due to the lack of experimental models. Methods This study provides a novel exploration and analysis of the impacts of cellular and molecular heterogeneity of human lung epithelial cells on their malignant transformation following chronic exposure to cigarette smoke extracts. Results The ability of cigarette smoke extract (CSE) to cause malignant transformation of the human bronchial epithelial cells (16HBE) is dependent on the sizes of the cells. Epithelial-mesenchymal transition (EMT) plays an important role in this process. Mechanistically, CSE-induced malignant transformation of 16HBE cells was closely linked to the reduced relative telomere length of the larger 16HBE cells, thereby up-regulation of the expression of stemness genes. Conclusions These findings provide novel insights for understanding the impact of cellular heterogeneity in lung cancer development. The in vitro transformation model described in this study could be extrapolated to studying the pathogenesis of other malignancies, as well as for mechanistic studies that are not feasible in vivo.

Published

2022

50. 食源性生物活性肽的免疫功能研究进展.

Author

张芷萌, 倪 策, 欧晓晖, 曹天红, 程云辉, and 文 李

Subjects

PROTEIN hydrolysates, HUMAN beings, PEPTIDES, CELLULAR signal transduction, ANIMAL models in research

Abstract

Copyright of Food & Machinery is the property of Food & Machinery Editorial Office and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2023