BM-MSCs Differentiated Insulin-Producing Cells Produce More Insulin in Presence of EGF than of FGF ()
1. Introduction
Diabetes Mellitus (DM) is a devastating disease affecting millions of people worldwide. In DM type1, destruction of pancreatic β cells by autoimmune attack results in decrease of insulin supply which leads to hyperglycemia and related serious complications. While DM type 2 is caused by insulin resistance and leads to hyperglycemia [1] [2] . Stem cells are important sources of insulin producing cells (IPCs) because of their multiple differentiation potential. IPCs can be generated from adult stem cells [3] .
Islet cell therapy (islet transplantation) is an important promising modality for diabetes therapy. Although some progress has been reported in islet transplantation, it has been hampered by immune rejection as well as by the limited availability of transplantable donor islets. On the other hand, mesenchymal stem cells possess broad differentiation ability. This has led to the investigation of the potentials of their therapeutic applications and their ability to differentiate into a number of cell types such as blood, liver, lung, skin, muscle, neuron and insulin producing cells [4] . Isolated adult mice bone marrow mesenchymal stem cells successfully induced to differentiate into insulin-producing cells. These cells had corrected the high blood glucose levels of chemically induced diabetic mice [5] .
This work aimed to evaluate IPC differentiation formulas, in presence of FGF or with EGF in regard to insulin production by using adult bone marrow-derived MSCs as a source of IPCs for β-cell replacement.
2. Materials and Methods
2.1. Isolation and Culture of Bone Marrow-Derived Mesenchymal Stem Cells
Bone marrow was isolated from tibiae and femur bones of adult mice after being euthanized according to the Iraqi Center for Cancer and Medical Genetic Research guidelines and approved by animal care committee. The bones were sterilized by immersion in 70% ethanol. The ends of the bones were cut and bone marrow was extruded by inserting a needle in one end through the bone shaft and injection of Tissue culture media (MEM, USbiological, USA) containing 10% fetal bovine serum (FBS, Capricorn-Scientific, Germany). The effluent was collected in sterile tubes. Gentle pipetting resulted in generation of a single cell suspension. Bone marrow cells were counted and plated with a concentration of 1 × 10−6/ml in T-25 flasks. The cells were then cultured in MEM containing 10% FBS and 1% penicillin and streptomycin at 37C in 5% CO2 Incubator.
2.2. Expansion of Bone Marrow-Derived Mesenchymal Stem Cells
After 24 hrs, the non-adherent cells were discarded. The adherent cells will be referred to as MSCs. These were fed for 7 days with complete MEM. When 80% confluence was reached as observed under inverted microscope (Olympus, Japan), the cells were washed with PBS and detached with a solution of 1 ml of trypsin/ EDTA. Cells were resuspended with complete MEM and tissue culture flask was used, this referred to as a first passage. This step was repeated for a second passage. Each passage was completed in 5 days.
2.3. Phenotyping of BM-MSCs
Bone marrow-derived MSCs (passage 2) were trypsinized and cultured in tissue culture dish with cover slip inside at density of 1 × 10−6 cells/ml. Cells grown on the cover slip to confluent after 3 - 4 days from the culture. Cells washed three times by PBS, dried and fixed with 4% formaldehyde for 9 - 10 minutes. Cells blocked and stained with anti-CD90 and anti-CD34 antibodies.
2.4. Differentiation of Mesenchymal Stem Cells to Insulin-Producing Cells
Mesenchymal stem cells (passage 2) were used for induction. After trypsinization cells were cultured at a density of 1 × 106 cells in 25 cm2 tissue culture flasks (Nunc, Denmark). After confluency, induction of differentiation was done by two different four steps formulas. Formula one: Step 1, the cell monolayer was treated for 24 hours with high glucose MEM (HMEM, 25 mol\Glucose) (US-biological, USA) supplemented with 10% FBS (Capricorn, Germany) and 106 mol/L retinoic acid (Santa Cruz Biotechnology, USA); Step 2, the medium was changed to H-DMEM with only 10% FBS for 48 hrs; Step 3, the medium was changed to low glucose Medium (LMEM), supplemented with 10% FBS, 10% mmol/L nicotinamide (Santa Cruz Biotechnology, USA) and 20 ng/ml fibroblast growth factor (US-biological, USA) for 6 days; Step 4, the low glucose medium was supplement with 10% FBS and 10 nmol/L exenden-4 (Santa Cruz Biotechnology, USA) for 6 days. Formula 2 was similar with modification of Step 3, by adding 20 ng/ml epidermal growth factor (US-biological, USA) instead of FGF.
2.5. DTZ Staining
At day 15 of culture, the differentiated clusters were examined for insulin producing cells by staining with diphenylthiocarbazone (DTZ). Stock solution was prepared as previously described [6] , by dissolving 10 mg of STZ (Santa Cruz Biotechnology, USA) in 10 ml of dimethylsulfoxide (Santa Cruz Biotechnology, USA) and stored at −20˚C. At staining 1:10 dilution in PBS of stock solution were made and 2 ml of dithizon were added to cultured cells. Differentiated and undifferentiated cells were incubated at 37˚C for 30 minutes in DTZ containing medium.
2.6. Differentiation Detection
Cells were trypsinzed and reseeded on coverslips overnight. Cells were washed three times by PBS and fixed by 4% formaldehyde for 9 - 10 minutes, blocked with 4% hydrogen peroxide for 10 minutes. Serum blocking for 1 hour, and 1/100 diluted primary antibody was applied to slides, anti-insulin (Santa Cruz Biotechnology, USA) at 4˚C overnight. Biotinylated secondary antibody was added to slides for 30 minutes in room temperature following by Avidin-HRP. After washing (DAB) reagent incubated for 5 minutes (Santa Cruz Biotechnology, USA). Hematoxylin was used as a counter stain. Finally, mounted and examined under light microscope for brown positive cells.
2.7. Measurement of Insulin Secretion
Insulin secretion was induced by adding low glucose (3 Mm) serum free MEM and incubated at 37˚C for 12 h. Cells were washed with PBS twice and high glucose (17.5 Mm) were added and incubated at 37˚C for 2 h. The media were collected and stored in deep freeze −85˚C until measured using an insulin ELISA kit (Raybiotech, USA).
3. Results
3.1. Culture and Expansion of Bone Marrow-Derived Mesenchymal Stem Cells
The primary culture of BMSCs showed after 24 h a few cells attached and formed adherent cells while the non- adherent cells were discarded by the changing the culture media after 48 h (Figure 1(A) & Figure 1(B)).
The adherent cells began to proliferate and grow to form a monolayer after 5 - 6 days. Stem cells morphology described as spindle with oval body and flattened ends (Figure 1(C) & Figure 1(D)). The cells were subcultured once or twice as maximum every 5 - 7 days without visible morphologic changes (Figure 1(C) & Figure 1(D)).
3.2. Phenotyping of the Isolated BM-MSCs
Immunocytochemistry revealed that these cells expressed strong signal of CD90 (Figure 2(A)) when compared to negative control (Figure 2(B)) and absence of any CD34 expression (Figure 2(C)). H & E staining for the Bone Marrow Mesenchymal Stem cells monolayer confirm the morphological features recognized by the light microscope (Figure 2(D)).
3.3. Morphologic Changes and Phenotyping of Differentiated BM-MSCs
In the formula one, changes in the number of cell aggregation were colonies shaped like islet cells with regular structure (Figure 3(G) and Figure 3(J)). However, in the formula two, the number of cells aggregation was more with regular colonies (Figure 3(K) and Figure 3(L)). Differentiation of IPC was assessed by immunocytochemistry. After end stage at 15 days from differentiation, the presence of the insulin granules within IPC cytoplasm was highly detected by presence of brown positive cells in most of the differentiated cells. Moreover, to evaluate the insulin-producing cells in cultures, we stained the differentiated cells with zinc-chelating agent (DTZ) DTZ is binding substance, and pancreatic islets are stain crimson red after DTZ treatment. Differentiated cell clusters were distinctly stained crimson red by DTZ (Figure 4).
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Figure 4. Immunocytochemical staining of differentiated cells for insulin (A: 25X). Differentiated cells detection with Cell clusters stained crimson red with DTZ (B: 40X) for both formula one and two where both stained positive.
3.4. Functional Evaluation for the Differentiated Cells (Insulin Release Assay)
Differentiated cells clusters released increasing amounts of insulin in presence of (17.5 Mm) glucose concentration. The mean insulin concentration secreted by the clusters was (0.3803 ± 0.002209 µIU/ml) for formula one. However, formula two was higher (0.4400 ± 0.005526 µIU/ml). These results represent the mean of this experiment; differences were statistically significant (P < 0.05). Cultured MSCs supernatants showed very low barely detectable amount of insulin, which can be neglected (0.004156 ± 0.0005547 µIU/ml).
4. Discussion
In our experiment, which is a preliminary study to evaluate insulin production from induced islet cells under influence of FGF and EGF. We were successful to isolate, culture and propagate mesenchymal stem cells, which were used for this evaluation. The morphological characterization of the cultured cells suggested being of stem cells in nature. We further tested the phenotype of bone marrow-derived mesenchymal stem cells and found it to be negative for CD34, which indicated they were unlikely to be hematopoietic stem cells. On the contrary, CD90 were positive indicating that the cultured bone marrow-derived cells were mesenchymal stem cells [7] . As proved by literatures, these cells were capable of generating IPCs [8] [9] .
Different protocols have been tried to induce bone marrow-derived MSCs to differentiate into IPCs in vitro [8] [9] . High glucose concentration is considered as a potent inducer for pancreatic islet differentiation [10] .
We tested a standard protocol [11] for IPC induction that utilized FGF as growth factor in final step and compared it to modified formula with replacing the FGF with EGF of differentiation protocol for induced BM- MSCs differentiation into islet cell in vitro. This protocol was developed as four-step protocol for differentiating stem cells into islet cells [12] . Both formula one and two found to be able to induce MSCs differentiation into insulin producing cells and secreting significant amount of insulin, however, presence of EGF shown to enhance insulin production in the induced cells as measured by quantitative ELISA assay. This was a result of cells proliferation in the media contain high glucose and growth factors. These factors are essential for supporting in vitro differentiation.
Mesenchymal stem cells were cultured in glucose rich medium. Glucose is a growth factor for β-cell replication in vitro and in vivo at 20 - 30 mol/lm concentrations. Glucose increases insulin content in cells derived from adult stem cells at a 5 mol/l mconcentration [13] . This supports the extra energy needed for cell division [14] . Retinoic acid, increasing proliferation and differentiation of beta cells, either from ducts or from islets, may be through up regulation or down regulation of factors or genes controlling these processes [15] . Epidermal growth factor increases cells differentiation because it is essential for proliferation into islets cells [16] . Fibroblast growth factor increases cell proliferation and early stages of clustering of pancreatic precursor cells [17] . On the other hand, nicotinamide is a poly ADP-ribose synthetase inhibitor and could induce pancreatic progenitor cells into insulin producing cells [18] . Whereas exendin-4 could also stimulate both β-cell replication and neogenesisto from ductal progenitor cells and inhibit apoptosis of β-cells [19] .
The induced IPCs were morphologically similar to pancreatic islet-like cells. More importantly, they not only produced insulin but also could secret insulin in response to different concentration of glucose stimulation in a regulated manner [20] . Therefore, we considered that bone marrow-derived MSCs as a good source of allograft for IPCs (β cells) replacement therapy, which could avoid immune rejection and ethical issue of embryonic origin. In conclusion, this study indicates that current published formulas can lead adult BM-MSCs to differentiate into insulin producing cells in vitro by using the four step protocol under appropriate conditions and EGF presence can enhance insulin production better than FGF as growth factor in Step 4. These results provide the strong evidence for our team to progress in testing feasibility of allograft transplantation utilizing bone marrow-derived MSCs IPC in the therapy of DM.
NOTES
*Corresponding author.