ABSTRACT
BACKGROUND: Hematopoietic stem cell (HSC) transplantation is considered a possible treatment option capable of curing various diseases. The aim of this study was the co-culturing of mesenchymal stem cell (MSC) spheres with HSCs under hypoxic condition to enhance the proliferation, self-renewal, stemness, and homing capacities of HSCs. METHODS AND RESULTS: HSCs were expanded after being subjected to different conditions including cytokines without feeder (Cyto), co-culturing with adherent MSCs (MSC), co-culturing with adherent MSCs + hypoxia (MSC + Hyp), co-culturing with MSCs spheres (Sph-MSC), co-culturing with MSCs spheres + hypoxia (Sph-MSC + Hyp), co-culturing with MSC spheres + cytokines (Sph-MSC + Cyto). After 10 days, total nucleated cell (TNC) and CD34+/CD38- cell counts, colony-forming unit assay (CFU), long-term culture initiating cell (LTC-IC), the expression of endothelial protein C receptor (EPCR), nucleostemin (NS), nuclear factor I/X (Nfix) CXCR4, and VLA-4 were evaluated. The TNC, CD34+/CD38- cell count, CFU, and LTC-IC were higher in the Sph-MSC + Hyp and Sph-MSC + Cyto groups as compared with those of the MSC + Hyp group (P < 0.001). The expanded HSCs co-cultured with MSC spheres in combination with hypoxia expressed more EPCR, CXCR4, VLA-4, NS, and Nfix mRNA. The protein expression was also more up-regulated in the Sph-MSC + Cyto and Sph-MSC + Hyp groups. CONCLUSION: Co-culturing HSCs with MSC spheres under hypoxic condition not only leads to higher cellular yield but also increases the expression of self-renewal and homing genes. Therefore, we suggest this approach as a simple and non-expensive strategy that might improve the transplantation efficiency of HSCs.
Subject(s)
Coculture Techniques/methods , Hematopoietic Stem Cells/metabolism , Mesenchymal Stem Cells/metabolism , Antigens, CD34/metabolism , Cell Culture Techniques , Cell Differentiation , Cell Hypoxia/physiology , Cell Proliferation , Cells, Cultured , Coculture Techniques/economics , Cost-Benefit Analysis , Cytokines/metabolism , Fetal Blood/cytology , Humans , Receptors, CXCR4ABSTRACT
Bone marrow stromal cells (BMSCs, also known as bone marrow mesenchymal stem cells) are a plastic-adherent heterogeneous cell population that contain inherent skeletal progenitors and a subset of multipotential skeletal stem cells (SSCs). Application of BMSCs in therapeutic protocols implies its isolation and expansion under good manufacturing practices (GMP). Here we describe the procedures we have found to successfully generate practical BMSCs numbers, with preserved biological potency.
Subject(s)
Biomedical Technology/standards , Bone Marrow Cells/cytology , Bone and Bones/cytology , Primary Cell Culture/methods , Antigens, CD34/genetics , Antigens, CD34/metabolism , Biomedical Technology/methods , Cells, Cultured , Coculture Techniques/economics , Coculture Techniques/methods , Coculture Techniques/standards , Costs and Cost Analysis , Culture Media, Serum-Free/chemistry , Humans , Practice Guidelines as Topic , Primary Cell Culture/economics , Primary Cell Culture/standards , Stromal Cells/cytology , Stromal Cells/metabolismABSTRACT
There is an increasing interest in studying the crosstalk between tumor-associated adipose tissue and tumor progression. In proximity to the primary site of kidney tumors, perinephric adipose tissue has direct contact with cancer cells when kidney cancer becomes invasive. To mimic the perinephric adipose tissue microenvironment, we applied the liquid overlay-based technique, which cost-effectively generated functional adipocyte spheroids using mesenchymal stem cells isolated from human perinephric adipose tissue. Thereafter, we co-cultured adipocyte spheroids with unpolarized macrophages and discovered an M2 phenotype skew in macrophages. Moreover, we discovered that, in the presence of adipocyte spheroids, M2 macrophages exhibited stronger invasive capacity than M1 macrophages. We further showed that the perinephric adipose tissue sampled from metastatic kidney cancer exhibited high expression of M2 macrophages. In conclusion, the liquid overlay-based technique can generate a novel three-dimensional platform enabling investigation of the interactions of adipocytes and other types of cells in a tumor microenvironment.
Subject(s)
Adipocytes/cytology , Adipogenesis , Adipose Tissue/cytology , Cell Culture Techniques/instrumentation , Mesenchymal Stem Cells/cytology , Adipocytes/pathology , Adipose Tissue/pathology , Cell Culture Techniques/economics , Cells, Cultured , Cellular Microenvironment , Coculture Techniques/economics , Coculture Techniques/instrumentation , Humans , Kidney Neoplasms/pathology , Macrophages/cytology , Macrophages/pathology , Mesenchymal Stem Cells/pathology , Spheroids, Cellular/cytology , Spheroids, Cellular/pathology , Tumor Cells, CulturedABSTRACT
Current methods to study angiogenesis in cancer growth and development can be difficult and costly, requiring extensive use of in vivo methodologies. Here, we utilized an in vitro adipocyte derived stem cell and endothelial colony forming cell (ADSC/ECFC) co-culture system to investigate the effect of lentiviral-driven shRNA knockdown of target genes compared to a non-targeting shRNA control on cord formation using High Content Imaging. Cord formation was significantly reduced following knockdown of the VEGF receptor VEGFR2 in VEGF-driven cord formation and the FGF receptor FGFR1 in basic FGF (bFGF)-driven cord formation. In addition, cord formation was significantly reduced following knockdown of the transcription factor forkhead box protein O1 (FOXO1), a protein with known positive effects on angiogenesis and blood vessel stabilization in VEGF- and bFGF-driven cord formation. Lentiviral shRNA also demonstrated utility for stable knockdown of VEGFR2 and FOXO1 in ECFCs, allowing for interrogation of protein knockdown effects on in vivo neoangiogenesis in a Matrigel plug assay. In addition to interrogating the effect of gene knockdown in endothelial cells, we utilized lentiviral shRNA to knockdown specificity protein 1 (SP1), a transcription factor involved in the expression of VEGF, in U-87 MG tumor cells to demonstrate the ability to analyze angiogenesis in vitro in a tumor-driven transwell cord formation system and in tumor angiogenesis in vivo. A significant reduction in tumor-driven cord formation, VEGF secretion, and in vivo tumor angiogenesis was observed upon SP1 knockdown. Therefore, evaluation of target gene knockdown effects in the in vitro co-culture cord formation assay in the ADSC/ECFC co-culture, ECFCs alone, and in tumor cells translated directly to in vivo results, indicating the in vitro method as a robust, cost-effective and efficient in vitro surrogate assay to investigate target gene involvement in endothelial or tumor cell function in angiogenesis.
Subject(s)
Adipocytes/cytology , Coculture Techniques/methods , Neovascularization, Pathologic/metabolism , RNA, Small Interfering/pharmacology , Sp1 Transcription Factor/genetics , Animals , Cell Line, Tumor , Coculture Techniques/economics , Endothelial Cells/metabolism , Female , Gene Expression Regulation, Neoplastic , Gene Knockdown Techniques , Genetic Vectors/administration & dosage , Genetic Vectors/genetics , Humans , Indoles/administration & dosage , Lentivirus/genetics , Mice, Nude , Neoplasm Transplantation , Pyrroles/administration & dosage , RNA, Small Interfering/genetics , Stem Cells/metabolism , SunitinibABSTRACT
In this paper, we report a simultaneous realization of both efficient ethanol production and saving medium nutrient (corn steep liquor [CSL]) during bioethanol fermentation of overliming-treated hydrolysate of waste house wood (WHW) using ethanologenic Escherichia coli KO11. In cultivation using WHW hydrolysate supplemented with 4% (v/v) CSL and 0.2 g-dry cell weight (DCW)/l E. coli KO11 cells, the overall ethanol yield reached 84% of the theoretical value at 61 h. When we conducted the cultivation with 1% CSL to reduce the supplemental medium cost, the overall ethanol yield remained in the range of 66-72% even at 90 h. We proposed two alternative methods for increasing the overall yield even with 1% CSL. The first method involved increasing the inoculum size of E. coli KO11 up to 0.8 g-DCW/l, where 83% of the overall yield was attained at 60 h of cultivation. The second method involved the coculture of 0.2 g-DCW/l E. coli KO11 together with 0.02 g-DCW/l of Saccharomyces cerevisiae TJ1, and the overall yield reached 81% at 47 h of cultivation.
Subject(s)
Escherichia coli/metabolism , Ethanol/economics , Ethanol/metabolism , Industrial Waste/economics , Saccharomyces cerevisiae/metabolism , Wood/economics , Wood/microbiology , Coculture Techniques/economics , Coculture Techniques/methods , Cost Savings/methods , Hydrolysis , Industrial Waste/prevention & control , JapanABSTRACT
Intercellular interactions are studied using different co-culture systems. Tumor conditioned medium-based systems, filter inserts and direct contact co-culture systems are often used according to research needs. In this article we present a new co-culture technique, using negatively-charged slides (NCS) as the culture surface. The technique was developed on a human-derived endothelial cell line-breast cancer interaction model. Two variations of this model are presented: In the first variation co-culture is achieved by using one NCS and a standard tissue culture treated dish as growing surfaces for the two cell populations respectively, while in the second variation the two cell populations are grown on two NCS. No significant difference was found between cell culture on the NCS compared to regular culture plasticware and staining was not only successfully but also easily performed. The suggested co-culture model has the advantage of allowing real time studies regarding cellular interactions. Additionally the two cell populations can be independently studied. Morphology is maintained throughout the procedure allowing morphological observation. Moreover, low cost is a factor permitting the application of the suggested model even in low budget laboratories. The features of the co-culture model that we developed are presented in relation to the salient features of other models.
Subject(s)
Cell Communication , Coculture Techniques/instrumentation , Coculture Techniques/methods , Models, Biological , Biomarkers/analysis , Cell Line, Tumor , Coculture Techniques/economics , Endothelial Cells/cytology , Endothelial Cells/metabolism , Humans , ImmunohistochemistryABSTRACT
To select an insert suitable for human umbilical vein endothelial cell (HUVEC) culture, we compared several available inserts of 0.2 to 0.45 micron porosity: Cellagen (ICN), Transwell-COL (Costar), Millicell-HA and CM (Millipore), Anopore (Nunc), Cyclopore (Falcon) in comparison with a control surface (Thermanox). The requirements were: (i) to promote attachment, adhesion and proliferation of HUVEC (judged by [3H]thymidine incorporation into DNA at days 1, 3, 7); (ii) to allow HUVEC visualization by inverted, fluorescence microscopy for uptake of DiI-Ac-LDL and scanning electron microscopy, performed at day 9 after seeding. Because Transwell and Cellagen are collagen precoated and CM has to be coated for cell culture, we performed collagen coating (types I + III or IV) for non-pretreated inserts for the purpose of comparison. Our preferences comprise Transwell-COL, Cyclopore not coated or coated (whatever the collagen type), and Cellagen. However, on a quality/price ratio criterion, Cyclopore, even uncoated, is the insert of choice. The HA, CM and Anopore inserts, even coated, do not allow HUVEC growth but do not alter positive uptake of acetylated LDL.
