C:\Users\JURNAL FKUSAKTI\Docume 164 *Postgraduate Biomedical Science Program, Medical Faculty, Sultan Agung Islamic University, Semarang, Indonesia **Department of Postgraduate Biomedical Science, Medical Faculty, Sultan Agung Islamic University, Semarang, Indonesia ***Department of Pathological Anatomy, Medical Faculty, Sultan Agung Islamic University, Semarang Indonesia †Stem Cell and Cancer Research Laboratory, Medical Faculty, Sultan Agung Islamic University Correspondence Dr. dr. H. Agung Putra, M. Si. Med. Chairman of Stem Cell and Cancer Research (SCCR) Laboratory, Medical Faculty, Universitas Islam Sultan Agung Semarang, Jl. Raya Kaligawe KM. 4 Semarang, Jawa Tengah 50112 Phone.+628164251646 Email: dr.agungptr@gmail.com ORCID ID : 0000-0003-4261-9437 Date of first submission, October 10, 2 01 8 Date of final revised submission, October 11, 2019 Date of acceptance, October 16, 2019 This open access article is distributed under a Creative Commons Attribution- Non Commercial-Share Alike 4.0 International License ABSTRACT UNIVERSA MEDICINA Hypoxia enhances self-renewal properties and markers of mesenchymal stem cells Vivi Yustianingsih*, Titiek Sumarawati**, and Agung Putra***,† BACKGROUND Mesenchymal stem cells (MSCs) are multipotent stromal cells that express CD73, CD90, and CD105 surface markers, but not CD14, CD45, CD34, CD11b, and HLA-DR. MSCs under hypoxic conditions have the essential role of maintaining the stemness capacity by releasing several growth factors into their medium, known as hypoxia conditioned medium (HCM). This study was performed to compare the effect of percentage of HCM to normoxic medium (NM) in increasing MSC proliferation marked by proliferation rate and surface marker expression. METHODS This study was of post-test only control group design using human umbilical cord-MSCs (hUC-MSCs) as subjects. The HCM treatment group was obtained by culturing MSCs under 5% O 2 , whereas the NM control group was grown under 20% O 2 . The hUC-MSCs were divided into 4 groups with different dose ratios of HCM to NM (25%:75%; 50%:50%; 75%:25% for P1, P2 and P3, respectively and 100% of NM for the controls). All of these groups were maintained at 37oC and the data was collected after 72 hours incubation. MSC marker expression of CD73, CD90 and CD105 was analyzed using flow cytometry and MSC proliferation by trypan blue assay. RESULT There were significant differences in MSC marker expression of CD73, CD90 and CD105 and proliferation at all dose ratios of HCM to NM (p<0.05). CONCLUSION Low oxygen concentration promotes MSC proliferation and stemness thus it might be beneficial for maintaining the MSC physiologic niche in-vitro. Keywords: MSC, MSC-HCM, proliferation, stemness ORIGINAL ARTICLE pISSN: 1907-3062 / eISSN: 2407-2230 DOI: http://dx.doi.org/10.18051/UnivMed.2019.v38.164-171 September-December, 2019 Vol.38- No.3 Cite this article as: Yustianingsih V, Sumara wati T, Putra A. Hypoxia en- hances self-renewal properties and mark- ers of mesenchymal stem cells. UnivMed 201 9;38 :1 6 4-7 1 . doi: 10 .18 05 1/ UnivMed.2019.v38.164-171 165 Univ Med Vol. 38 No.3 INTRODUCTION Mesenchymal stem ce lls (MSCs) are multipotent stromal cells with the capacity for self- renewal and differentiation into mesodermal lineages such as chondrocytes, osteoblasts, adipocytes, and neurons.(1) According to the International Society for Cellular Therapy (ISCT) MSCs’ main characteristics are adherence to plastic, expression of CD73, CD90, and CD105 and lack of expression of CD14, CD45, CD34, CD11b, and CD31 and HLA-DR. (2 ) Mesenchymal stem cells have been widely used for tissue engineer i ng and treatment of degenerative diseases and immune disorders, due to their trophic activity, immunomodulatory and angiogenic propertie s and multipotent differentiation capacity.(3) Mesenchymal stem cells can be isolated from a wide range of source tissues such as the umbilical cord, bone marrow, adipose tissue and dental pulp.(4-6) Moreover, an essential goal for expansion of MSCs in vitro is to obtain sufficient cell numbers for research and clinical application. This depends mainly on tissue source of MSCs and processing method. In umbilical cord-derived MSCs (UC-MSCs) the stemness is highest in comparison with bone marrow and adipose- derived MSCs, due in part to their higher telomerase activity, and pluripotent properties under certain conditions.(7–9) A previous study has shown that the major concerns of in vitro MSC propagation are poor growth kinetics, early senescence and DNA damage during expansion.(6) Therefore, isolation techniques, culture medium, oxygen tension, supplements, cell seeding density and their modification such as under hypoxia and TNF-α are essential for MSC propagation.(10,11) One previous study reported that oxygen concentration is a critical environmental factor for maintaining in vitro stem cell plasticity and proliferation.(12) Other studies also demonstrated that hypoxic conditions (O 2 pressure under 5% have positive effects on MSCs in terms of in vitro survival and self-renewal, particularly in prese rving the stemness and enhancing proliferation.(13–15) There was an enhancement of MSC proliferation in hypoxic conditions compared to normoxia even following 2 weeks of incubation of the cultures.(16) However, this study did not report the use of the hypoxia chamber as a culture device. In contrast, another study reported that continued hypoxia reduced the clonogenic ability and differentiation potential of MSCs.(7) Another study described that 24-h hypoxia is beneficial for the functional properties of MSCs.(17) Since hypoxia is the most similar to the physiological conditions occurring in living organisms, we decided to examine MSC culture both in normoxic and hypoxic conditions. In this study, we analyzed the comparative effect of hypoxia-conditioned medium (HCM) obtained after 24-h hypoxia incubation to NM (with HCM:NM ratios of about 25%:75%; 50%:50% and 75%:25%, respectively) in enhancing MSC stemness through analyzing MSC proliferation and CD73, CD90 and CD105 expression for 72 hours incubation. METHODS Research design This post-test only control group design was conducted in the Stem Cell and Cancer Research Laboratory, Faculty of Medicine, Universitas Islam Sultan Agung (Unissula), Semarang from July-September 2018. Research subjects Human umbilical cord-MSCs (hUC-MSC) were used as the subjects and divided into 4 groups with different doses of MSC-HCM. The total number of hUC-MSCs was 1.2 x 106 cells and was equally divided into 4 groups. The control group was treated with normal medium, whereas the treatment groups were supplemented with 25% HCM (P1), 50% HCM (P2) and 75% HCM (P3), respectively. Mesenchymal stem cell isolation Mononuclear ce ll s (MNCs) from an umbilical cord were collected and separated by 166 Ficoll-Paque solution (density 1.077 g/mL; GE) in centrifuge tubes (15 mL). The mononuclear cells were transferred to a new tube and washed twice through centrifugation at 2000 rpm for 10 minutes. They were then seeded into 25-cm2 flasks at a density of 1 × 107–108 cells/cm2. The flasks contained Dulbecco’s modified Eagle’s Medium– Low Glucose (DMEM-LG, GIBCO Invitrogen) supplemented with 1% L-Glutamine 200 mM, 1% Antibiotic—Antimycotic comprising 10.000 U/mL sodium penicillin, 1% 10.000 μg/mL streptomycin sulfate, 25 μg/mL amphotericin B (GIBCO/ Invitrogen Corporation), and 10% Fetal Bovine Serum ( GIBCO/Invitr oge n Corporation). Umbilical cord blood (UCB)-MSC cultures were maintained at 37 °C in 5% CO 2 and non-adherent cells were removed after 48 h. The medium was changed every other day. The experiments were performed at the fourth passage of the cultures with approximately 80–90% confluence. UCB- MSC lineages were established in culture up to the fourth passage. Characterization of MSCs T he c h a ra c t e r i s t ic s o f MSCs w e r e analyzed by flow cytometric analysis at the fourth passage. The cells were subsequently incubated at room temperature and in the dark wi th f lu or e s c ei n i sot h i ocya n a te ( FITC) - conjugated, allophycocyanin (APC)-conjugated or phycoerythrin (PE)-conjugated monoclonal antibodies, including CD73, CD90 and CD105. APC-, PE-, and FITC-conjugated isotypes were used as negative controls. The analysis used BD PharmingenTM (BD Biosciences, Franklin Lakes, NJ, USA) at 4°C for 30 min. The cells were washed twice with 1% BSA/PBS, resuspended in 200 µL 1% BSA/PBS and analyzed using a flow cytometer (BD Biosciences, San Jose, CA, USA). In-vitro differentiation For the differentiation test, MSCs were grown on 24-well plates at densities of 1x104 cells/ well, with DMEM supplemented with osteogenic- induction medium containing 10-7 mol/L/0.1 μM dexamethasone, 10 mmol/L β-glycerophosphate, 50μmol/L ascorbate-2-phosphate (Sigma-Aldrich, Louis St, MO) and 10% fetal bovine serum (FBS). The cells were rinsed in PBS and fixed with cold 70% ethanol (v/v) for 1 hour at room temperature, then rinsed three times with twice- distilled water after 21 days of induction. A volume of 1 ml 2% Alizarin Red solution (w/v) (pH 4.1- 4.3) was added and the cells incubated for 30 minutes at room temperature, then rinsed four times in twice-distilled water. Hypoxia conditioned medium (HCM) A previous protocol (18) was adapted for use in this study. Briefly, hMSCs were incubated until confluent, after which they were seeded in a T25 flask (2 × 106 cells), washed twice with endothelial basal medium (EBM-2; Lonza), and then placed in a hypoxic chamber (Anaerobic Environment; ThermoForma, Waltham, MA, USA) containing 5 ml EBM-2 for 12 hours. The airtight humidified hypoxic chamber was maintained at 37°C and continuously supplied with 5% CO 2 , 10% H 2 , and 85% N 2 . The oxygen level in the chamber was ~0.5%. After incubation, the medium was collected and centrifuged at 1000 rpm for 10 minutes at 4°C. Then the HCM was added to the treatment groups at concentrations of 25, 50% and 75%, respectively. Mesenchymal stem cell proliferation essay and stemness The cells were counted in a hemocytometer for analyzing cell proliferation. In brief, following treatment, the cells are harvested and an aliquot of cells is combined with trypan blue dye solution and loaded into the hemocytometer chamber. The cells are then viewed under the microscope and the number of live cells present within a specific area are counted. The number of cells counted per area multiplied by the dilution factor will determine the number of live cells per milliliter. The stemness of MSCs was analyzed after 72-h induction using a BD PharmingenTM flow cytometer (BD Biosciences, Franklin Lakes, NJ, USA). Yustianingsih, Sumarawati, Putra Effect Of MSC-HCM on MSC self-renewal 167 Univ Med Vol. 38 No.3 Statistical analysis All values are expressed as the mean ± SD. Comparisons between the four groups were analyzed using ANOVA and then followed by posthoc Fisher’s LSD. A p value of <0.05 was considered significant. All analyses were performed with SPSS 16.0. Ethical clearance All research activities were approved by the Commission on Test Animal Ethics (Komisi Etik Hewan Uji), Faculty of Medicine, Universitas Islam Sultan Agung, Semarang, under No. 233/ VII/2018/Komisi Bioetik. A B C RESULTS Mesenchymal stem cell characterization The MSCs were successfully isolated from the umbilical cord, based on their adherence to plastic. After reaching 80% confluence, the cells were harvested for 4 passages. The MSCs showed a fusiform appearance, became confluent after 5-7 days in culture and were regularly passaged. Flow cytometry analysis showed that the MSCs were positively expressing 75.8% of CD73, 84.1% of CD90 and 55.2% of CD105 (Figure 1). Figure 1. Characteristics of UC-MSCs expressing CD73, CD90 and CD105 by flow cytometry 168 In vitro differentiation The MSC differentiation assay was done by means of osteogenic medium. The results s ho we d tha t M SCs w e r e c ap a b l e of differentiating into osteogenic cells as indicated by their red color from Alizarin red staining (Figure 2b). MSCs self-renewal and stemness The MSC appearance was analyzed using the light microscope at 24, 48, and 72 hours after MSC-HCM induction (Figure 3). The results showed significant between-group differences in MSC self-renewal appearance (p=0.000). The highest result was shown by P3 with a high concenteration of MSC-HCM (75%) (Table 1). This is in line with the expression of MSC positive markers (CD 73, CD90, CD105). DISCUSSION Several studies have reported that hypoxic conditions may modulate the paracrine activity of MSCs by up-regulating the various secretable factors into a medium such as HCM. These soluble molecules are associated with the Figure 2. (a) UC-MSC-like from in vitro culture showing fibroblast-like and polygonal cells, at 40x magnifica- tion, (b) osteogenic differentiation test with Alizarin Red staining appearing in MSC population 0 hours 24 hours 48 hours 72 hours Control P1 P2 P3 Figure 3. Appearance under light microscope of MSCs after HCM induction Yustianingsih, Sumarawati, Putra Effect Of MSC-HCM on MSC self-renewal 169 Univ Med Vol. 38 No.3 increased proliferation rate and stemness properties of MSCs. Whereas the effects of hypoxia have been investigated previously, the comparison between HCM and NM in enhancing MSC prolif eration in vitro by constantly maintaining stemness pr ope rties rema ins unknown. In this study we introduced various HCM to NM dose ratios in MSCs using the hypoxic condition chamber as in a previous study,(17) then analyzed the increase in MSC proliferation rate and their expression of CD73, CD90, and CD105. Our results showe d that there were significant differences between all HCM to NM dose ratios in cell proliferation rate after 72 hours. This is in accordance with a previous study that found that hypoxic conditions may increase the proliferation and stemness in MSCs.(18) We suggest that the hypoxic state induces hypoxia- inducible factor-1a (HIF-1a) as transcription factor for inducing HIF-1a survival target genes including self-renewal and proliferation.(19) This is in line with one other study reporting that MSCs under hypoxic conditions also have the ability to express the transcription embryonic factors such as Sox2.(18) In undifferentiated mouse and human embryonic stem cells (ES), Oct3/4 and Sox2 also interact with the Nanog promoter to strengthen the stemness of the cells.(18,20) These factors serve as candidate molecules for mastering the regulation of initiation, maintenance, and differentiation of pluripotent cells. This is also in accordance with our finding that there are significant differences between all HCM to NM dose ratios in MSC positive markers (CD73, CD90, CD105) with the highest result in group P3 (75%:25%). We suggest that the secretome released by MSCs under hypoxic conditions may induce the in vitro MSC progeny cells to grow over with maintaining their stemness. Variable Treatment groups p value Control (n=3) P1 (n=3) P2 (n=3) P3 (n=3) Proliferation (cell) 411666.67 ± 12583.05 461666.67 ± 10408.33 535000.00 ± 13228.75 571666.67 ± 10606.60 0.000* CD73 (%) 76.41 ± 0.70 86.5 ± 1.20 90.86 ± 0.40 99.26 ± 0.50 0.000* CD90 (%) 84.16 ± 0.30 90.83 ± 0.45 93.73 ± 0.45 96.43 ± 0.55 0.000* CD105 (%) 55.41 ± 0.26 60.81 ± 0.45 63.86 ± 0.40 66.80 ± 0.30 0.000* Table 1. Distribution of MSC proliferation and stemness after 72 hour incubation by treatment groups Note: P1 medium with 25% HCM, P2 medium with 50% HCM, P3 medium with 75% HCM. *Significant at p<0.05 Groups Mean differences p value Proliferation Control P1 P2 P3 P1 P2 P3 P2 P3 CD73 Control P1 P2 P3 P1 P2 P3 P2 P3 CD90 Control P1 P2 P3 P1 P2 P3 P2 P3 CD105 Control P1 P2 P3 P1 P2 P3 P2 P3 -50000.00 -123333.33 -155833.33 -73333.33 -105833.33 -32500.00 -10.033 -14.43 -22.83 -4.40 -12.80 -8.40 -6.66 -9.56 -12.26 -2.90 -5.60 -2.70 -5.40 -8.46 -11.40 -3.06 -6.00 -2.93 0.001 0.000 0.000 0.000 0.000 0.020 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 0.000 Table 2. Multiple comparisons of MSC proliferation and stemness Note: P1 medium with 25% HCM, P2 medium with 50% HCM, P3 medium with 75% HCM 170 Our findings indicate that HCM plays an important role in stemness potentials of the adult stem cell (ASC) including UC-MSC under hypoxic conditions. The limitation of this study is that we did not analyze the transcription marker molecules such as Sox2, Oct3/4 and Nanog. CONCLUSIONS Low oxygen c once ntra tion in M SCs promotes cell proliferation and stemness, thus it might be beneficial for maintaining the MSC physiologic niche in-vitro. CONFLICT OF INTEREST Co mp e t i ng i n t e r e s t s : N o r e l e va nt disclosures. ACKNOWLEDGEMENT We would like to thank the Stem Cell and Cancer Research Laboratory, Medical Faculty, Universitas Islam Sultan Agung, Semarang and the Department of Postgraduate Biomedical Science, Medical Faculty, Universitas Islam Sultan Agung, Semarang for all the facilities needed to finish this research. CONTRIBUTORS VY, AP and TS contributed to the basic concept and design of the study. VY and AP contributed to writing the manuscript and p e r f o r mi ng th e e x pe r i me nt . V Y a nd A P contributed to sample preparation and data collection. VY contributed to the statistical analysis. 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