Abstract

Unspecialized cells that can renew themselves and give rise to multiple differentiated cell types are termed stem cells. The objective of this study was to characterize and investigate, through molecular and biochemical analyses, the stemness of cells derived from isolated mononucleated cells that originated from peripheral blood. The isolated mononucleated cells were separated according to their physical characteristics (adherent and suspension), after 4 to 7 days into a 14-day culturing period in complete medium. Our results revealed that adherent and suspension cells were positive for mesenchymal stem cell (MSC) and hematopoietic stem cell (HSC) markers, respectively. Differentiation of adherent cells into osteoblasts was associated with expression of the OPN gene and increasing ALP enzyme activity, while differentiation of suspension cells into osteoclasts was associated with expression of the TRAP gene and increasing TRAP enzyme activity. In conclusion, molecular and biochemical analyses showed that mononucleated cells consist of MSC (adherent) and HSC (suspension), and both cell types are able to differentiate into specialized cells from their respective lineage: osteoblast (MSC) and osteoclast (HSC).

1. Introduction

Stem cell research has been one of the most fascinating and controversial areas of contemporary biology. Progress in the area of stem cell research raises scientific questions as rapidly as it generates new discoveries. Stem cell research is hailed for the potential to revolutionize the future of medicine, with its ability to regenerate damaged and diseased organs. Stem cells can be defined by 3 main criteria: (1) the ability to self-renew for several cell divisions, which is a prerequisite for sustaining the stem cell pool, (2) the ability to generate at the single cell level differentiated progeny cells, generally of multiple lineages, and (3) the ability to functionally reconstitute a given tissue in vivo [1].

To date, several studies have shown that mesenchymal stem cells (MSCs) and hematopoietic stem cells (HSCs) are adult stem cells present in blood [2]. MSCs are generally defined as self-renewable, multipotent progenitor cells with the ability to differentiate into several mesenchymal lineages, including bone, cartilage, adipose, and muscle tissues [3]. These cells are usually identified by their plastic adherence and surface marker expression of CD73, CD90, CD105 and absence of CD34, CD45, HLA-DR [4]. Meanwhile, HSCs are defined by their ability to repopulate all of the hematopoietic lineage in vivo and sustain the production of these cells for the lifespan of the individual [5, 6]. Several laboratories have identified HSCs as cells that demonstrate specific positive markers such as KIT, Sca-1, SLAM family markers, and lineage negativity [4, 7].

However, the method used for obtaining HSCs and MSCs from peripheral blood mononucleated cells is still debated. Isolating small amounts of MSCs detectable in peripheral blood is difficult and depends on the method used. MSCs that have been isolated are adherent and display a fibroblastic appearance [8]. Therefore, in this study, we further separated the mixed population of isolated mononucleated cells according to their physical characteristics, which are nonadherent (suspension) and adherent, after several days of culture selection.

Stemness must be addressed before a cell is to be classified as a stem cell. In this study, the stemness of isolated mononucleated cells that we have further separated according to their physical characteristics was determined through the expression of stemness markers, gene expression profiles, and biochemical analysis of adherent and suspension mononucleated cells during osteoblast and osteoclast differentiation, respectively. Our results demonstrate that adherent and suspension mononucleated cells show expression of MSC markers and HSC markers, respectively. The gene expression profiles and biochemical analyses of adherent (MSC) and suspension (HSC) mononucleated cells during in vitro osteoblast and osteoclast differentiation indicate that these cells are also capable of fully differentiating into osteoblast and osteoclast cells. These studies demonstrate the possibility of obtaining HSC and MSC population from mononucleated blood. Our approach may lead to the improved ability to isolate HSCs and MSCs from mononucleated peripheral blood cells and it could lead to further research in cellular therapy.

2. Materials and Methods

2.1. Isolation of Mononucleated Cells

Three samples of peripheral blood were obtained by venipuncture from each of 3 healthy volunteers (18–25 years old) after obtaining their informed consent and approval from the Ethical Committee of the Faculty of Science and Technology, Universiti Kebangsaan Malaysia (UKM). In each blood sample the cell culture experiment, gene expression, and biochemical analyses were performed. Human mononucleated peripheral blood cells were isolated using the Ficoll-Paque density-gradient separation method. Firstly, the blood samples were diluted three times with Hanks’ Balanced Salt Solution (Sigma, USA). The diluted blood samples were carefully layered 1 : 1.5 on Ficoll-Paque PLUS (GE Healthcare, Sweden) and centrifuged at 400 g for 20 min at room temperature. The mononucleated cell layer at the plasma-Ficoll interface was washed 3 times with phosphate buffer saline (PBS) and cultured in 6-well plates with complete medium containing α-Minimal Essential Medium (α-MEM) (Invitrogen, USA) supplemented with 10% (v/v) newborn calf serum (NBCS) (Invitrogen, USA) and 2% (v/v) penicillin-streptomycin solution (Invitrogen, USA) at 37°C in a humidified atmosphere containing 5% CO2. Approximately 8 ×105 mononuclear cells were isolated from 1 mL of peripheral blood samples. The isolated cells were cultured in complete medium for 14 days with complete medium exchange every 3 days. Cells were transferred into a new 6-well plate 4 to 7 days prior to separating them into plates of either adherent or suspension cells.

2.2. Cell Culture Morphology

The morphologies of adherent and suspension mononucleated cells were observed in vitro at days 0, 7, and 14 using an inverted microscope (Olympus, Model: CKX75). Images were obtained using a digital camera.

2.3. Differentiation of Adherent Mononucleated Cells into Osteoblasts

Approximately 1 × 105 cell/mL mononucleated cells cultured in suspension in complete medium were supplemented with differentiation factors, 50 μg/mL ascorbic acid (Sigma, USA) and 10 mM β-glycerophosphate (Sigma, USA), for 14 days to induce differentiation into osteoblasts. Cultures were maintained at 37°C with 5% CO2. Cells cultured in complete medium without differentiation factors were used as controls.

2.4. Differentiation of Suspension Mononucleated Cells into Osteoclasts

For osteoclast differentiation, 1 × 105 cell/mL of suspension mononucleated cells were cultured in complete medium supplemented with growth factors, 50 ng/mL recombinant sRANKL and 25 ng/mL macrophage-colony stimulating factor (M-CSF) and cultured for 10 days. Cultures were maintained at 37°C with 5% CO2. Cells cultured in complete medium without growth factors were used as controls.

2.5. Reverse-Transcriptase Polymerase Chain Reaction (RT-PCR) Amplification

Total RNA was extracted using TRI Reagent (Sigma, USA) following the manufacturer’s instructions. Total RNA was extracted from human adherent and suspension mononucleated cells that had been cultured for 14 days in complete medium, 10 and 14 days in osteoclast and osteoblast differentiation medium, respectively. One microgram total RNA was subjected to RT-PCR amplification using an Access RT-PCR System kit provided by Promega, USA. First-strand complementary DNA (cDNA) was synthesized by reverse transcription at 45°C for 45 min, followed by Avian Myeloblastosis Virus reverse transcriptase inactivation at 94°C for 2 min. Second-strand cDNA synthesis and PCR amplification consisted of 40 cycles of denaturation at 94°C for 30 sec, primer annealing for 1 min and extension at 68°C for 2 min, with a final cycle at 68°C for 7 min. The specific primer sequences used are shown in Table 1. Each RT-PCR product was then sequenced and analyzed.

2.6. Alkaline Phosphatase Assay

Biochemical analysis for osteoblast differentiation was conducted by Alkaline Phosphatase (ALP) enzyme assays of adherent cells cultured in osteoblast differentiation and complete medium on days 0, 3, 5, 7, 10, and 14. Adherent cells cultured in complete medium were used as the control. The cells were washed with PBS and then incubated in 0.1 M NaHCO3-Na2CO3 (pH 10.0), 0.1% (v/v) Triton X-100, 2 mM MgSO4 and 6 mM p-nitrophenyl phosphate (ρNPP) (Sigma, USA) for 30 min at 37°C. The reaction was stopped by adding 1 mL 1.5 M NaOH, and absorbance was measured at 405 nm. ALP activity is represented as the specific activity. The specific activity was determined by the unit activity (U) per total protein content (mg), and the protein content was measured using the Bradford method. One unit of activity is represented by the hydrolysis of 1 μM ρNPP per minute at 37°C. The ALP-specific activity was presented in a percentage value, which was compared to the ALP-specific activity in the control cells (cells cultured in complete medium). ALP-specific activity in the control cells was used to determine the basal activity rate (100%).

2.7. Tartrate-Resistant Acid Phosphatase Assay

Biochemical analysis for osteoclast differentiation was conducted by Tartrate-Resistant Acid Phosphatase (TRAP) enzyme assays of suspension cells cultured in osteoclast differentiation and complete medium on days 0, 3, 5, 7 and 10. Suspension cells cultured in complete medium were used as the control. The cells were washed with PBS. The TRAP enzyme was assayed in cell extracts and complete medium using ρNPP as a substrate in an incubation medium (1 mL) containing the following components: 10 mM ρNPP, 0.1 M Na-acetate (pH 5.8), 0.15 M KCl, 0.1% (v/v) Triton X-100, 10 mM Na-tartrate, 1 mM ascorbic acid, and 0.1 mM FeCl3. The mixture was incubated for 1 hour and the reaction was stopped by adding 500 μL of 0.3 M NaOH and immediately read at a wavelength of 405 nm. TRAP activity is expressed as the hydrolysis of 1 μM pNPP per min at 37°C. The specific activity was determined by unit activity (U) per total protein content (mg), as mentioned previously. The TRAP-specific activity was presented in a percentage value, which was compared to TRAP-specific activity in the control cells (suspension cells cultured in complete medium). TRAP-specific activity in the control cells was used to determine the basal activity rate (100%).

2.8. Statistical Analysis

Data were statistically analyzed using paired t-tests. Data were considered statistically significant at .

3. Results

3.1. Morphology and Characteristics of Isolated Cells

The freshly isolated mononucleated cells from human peripheral blood (Figure 1(a)) were morphologically heterogeneous. Further culturing of these cells in complete medium for 7-day produced two different types of cells. One cell type was round and floated in the medium or loosely attached to the culture dish (suspension cells); another cell type firmly attached with a different morphological appearance (adherent cells) (Figures 1(b) and 2(b)). The adherent and suspension mononucleated cells were then separated; mononucleated cells that already attached were left to expand in the same dishes, while suspension mononucleated cells were transferred into new 6-well plates.

Adherent and suspension mononucleated cells were separated after 7 days in vitro culture selection. Both adherent and suspension mononucleated cells were maintained in complete medium for 14 days of culture, to deplete most of the unwanted cells and allow time for proliferation prior to enriching the cells for analysis. After 14 days in culture, the adherent and suspension cells became more morphologically homogeneous; most of the cells in suspension were morphologically round (Figure 1(c)), while the adherent mononucleated cells showed a spindle-shaped fibroblast-like morphology (Figure 1(d)). However, morphological characteristics alone are insufficient to demonstrate the presence of mononucleated stem cells. Thus, the mononucleated cells were further characterized by a molecular approach (RT-PCR analysis), using human-specific stem cell markers.

3.2. Expression of Mesenchymal Stem Cell (MSC) and Hematopoietic Stem Cell (HSC) Markers

Adherent and suspension mononucleated cells from human peripheral blood (Figure 3(a)) were analyzed by RT-PCR for the presence of MSC and HSC markers. In this study, we used CD105 as an MSC marker, SLAM F1 as an HSC marker, and KIT as stem cell marker. Adherent and suspension mononucleated cells (Figure 2) were shown to express MSC and HSC markers, respectively. Furthermore, adherent and suspension mononucleated cells were negative for the presence of HSC and MSC markers, respectively. RT-PCR showed amplification of products of the expected size for the MSC marker: CD105 (290 bp), HSC marker: SLAM F1 (403 bp), and stem cell marker: KIT (316 bp).

3.3. Gene Expression Profiles during Osteoblast and Osteoclast Differentiation

Gene expression profiles of adherent and suspension mononucleated cells during osteoblast and osteoclast differentiation were carried out to evaluate the capacities of MSCs from adherent and HSCs from suspension mononucleated cells to differentiate into specialized cells from their expected lineage. RT-PCR was performed to examine how gene expression of MSC, HSC, osteoblast and osteoclast marker profiles changes during osteoblast and osteoclast differentiation. RT-PCR analyses were conducted simultaneously at days 0, 5, 10, and 14 for osteoblast differentiation and at days 0, 3, 7, and 10 for osteoclast differentiation. RT-PCR analyses showed different levels of gene expression in (Figure 3) mononucleated cells during osteoblast and osteoclast differentiation. The markers for MSCs (CD105), HSCs (SLAM F1), osteoblasts (OPN), and osteoclasts (TRAP) were used. As seen in Figure 3(a), the expression of the osteoblast marker was low during early osteoblast differentiation but increased over time, similar to osteoclast differentiation of mononucleated cells and increased osteoclast marker expression throughout the differentiation period. The increases in osteoblast and osteoclast marker transcription suggest that the mononucleated cells differentiated into mature osteoblast and osteoclast cells, respectively. Moreover, the expression of stemness markers in both adherent and suspension suspension mononucleated cells decreased over the time in differentiation media, which indicates that the unspecialized mononucleated stem cells have successfully differentiated.

3.4. Biochemical Analysis during Osteoblast and Osteoclast Differentiation

Biochemical analyses during osteoblast and osteoclast differentiation were carried out by two different enzyme assays: ALP and TRAP assays. ALP is a relative marker of osteoblast differentiation, while TRAP is a biochemical marker for osteoclasts. Figure 4 shows the percentage of ALP-specific activity during 14 days of osteoblast differentiation. The percentage of ALP-specific activities in adherent mononucleated cells cultured in osteoblast differentiation medium gradually increased from day 3 to day 14 of osteoblast differentiation. This was statistically significant () starting from days 7, 10, and 14 of osteoblast differentiation (Figure 4). Therefore, adherent cells, which consist of MSCs, were successfully differentiated into osteoblasts.

Meanwhile, biochemical analysis using TRAP enzyme assays during osteoclast differentiation showed that the percentage of TRAP-specific activities increased in suspension mononucleated cells cultured in osteoclast differentiation medium starting from day 3 to day 10 of the induction of differentiation (Figure 5). Statistical analysis using a paired t-test for TRAP enzyme assays showed a significant increase () at days 5, 7, and 10 of differentiation. These results indicate that the suspension cells were successfully differentiated into osteoclasts, as TRAP is used as a biochemical marker for osteoclasts.

4. Discussion

The isolation of mononucleated cells was based on density gradient centrifugation using Ficoll-Paque, in which differences in density separate mononucleated cells from other blood cells. As shown in Figure 1(a), the isolated mononucleated cells are in a heterogeneous population. After 7 days of culture in complete medium, we obtained a mixed population with a low number of fibroblast-like cells (adherent) and suspension cells that have one round nucleus (e.g., lymphocytes, monocytes, and macrophages) (Figure 1(b)). Both adherent and suspension cells were cultured separately for additional 7 days. After a total of 14 days of in vitro culture selection, the adherent and suspension cells became more morphologically homogenous (Figures 1(c) and 1(d)) as we suspect that a majority of differentiated and precursor cells died due to their short lifespan, for example, granulocytes (30–40 minutes in the peripheral blood with a total lifespan of 7–13 days that varied under certain pathological conditions), monocytes (5–7 days), and platelets (3–5 days) [9].

For a particular cell type to be classified as a stem cell, proof of stemness through proper and accepted characterization tests must be addressed. Stemness refers to the stem cell properties of having a certain gene or genes whose expression makes possible both the potential for self-renewal and multilineage differentiation [10]. In our study, CD105 was used as an MSC marker, SLAM F1 as an HSC marker, and KIT as stem cell marker (Figure 3(a)). KIT or c-Kit or CD117 is a Stem Cell Factor (SCF) receptor and expression of KIT in both types of stem cells is important as it acts on migration, adhesion, survival, proliferation, and differentiation [11]. KIT expression was reported in adult bone marrow hematopoietic and mesenchymal stem cells [12, 13] as well as fetal and umbilical cord hematopoietic stem cells [14, 15]. According to Hassan [16], its expression correlates with the self-renewal function of these fetal and adult stem cells. Moreover, KIT was found expressed in both human and mouse undifferentiated embryonic stem cells with a role in maintaining their undifferentiated state and correlation with functional measures of their pluripotency [1721]. CD105 or endoglin is a type I membrane glycoprotein, which is located on the cell surface and is also part of the TGF-β receptor complex [22]. CD105 is involved in regulating the proliferation of MSCs [23]. SLAMF1 is a cell surface receptor important in the self-renewal of HSCs [24] and is the founding member of the SLAM family of cell surface receptors [25, 26]. SLAM family members regulate the proliferation and activation of lymphocytes [27, 28].

This study revealed that adherent cells were positive for the expression of MSC markers, with an absence of HSC marker expression. By contrast, suspension cells were positive for the presence of HSC markers, while MSC marker expression was absent (Figure 2). These data indicate that adherent mononucleated cells with fibroblast-like morphology are MSCs, while HSCs are suspension mononucleated cells with round nuclear morphology.

The ability to generate differentiated progeny is one stem cell property (stemness). The stemness of adherent and suspension mononucleated cells was further determined by gene expression profiles and biochemical analysis during osteoblast and osteoclast differentiation. MSCs have the ability to differentiate into all of the mesenchymal lineages, while HSCs have the ability to repopulate the hematopoietic lineages. Thus, adherent cells (MSCs) were differentiated into osteoblast cells that originated from mesenchymal lineages, while suspension cells (HSCs) were induced to differentiate into osteoclast cells that originated from hematopoietic lineages.

Gene expression profiles demonstrated that the stemness markers were downregulated upon the induction of differentiation, resulting in decreased marker expression. All of the stemness markers, such as CD105 and SLAM F1, which have been used to examine gene expression profiles, play a significant role in the maintenance of the undifferentiated state of cells by stimulating proliferation [23, 24, 29]. Therefore, the downregulated of these genes might play important roles in the initiation of the differentiation process in mononucleated cells. By contrast, osteoblast and osteoclast markers were upregulated during differentiation, which resulted in the increased expression of these markers.

ALP [30], osteopontin (OPN), and osteocalcin (OC) [31] genes have been widely used as osteoblast markers, while cathepsin K (CATK) and TRAP are used as osteoclast markers [32]. The increase in OPN gene transcription (Figure 3(a)) shows that mononucleated cells differentiate into mature osteoblast cells [9], while increased expression of TRAP (Figure 3(b)) indicates that mononucleated cells have differentiated into osteoclast cells [33, 34]. The housekeeping gene (GAPDH) is constitutively expressed at the same level throughout differentiation. This finding is in agreement with previous findings by Barber et al. [35], which showed that GAPDH is constitutively expressed at a relatively constant level in mammalian cells or tissues (Figure 3).

Biochemical analysis was performed to further confirm that adherent and suspension mononucleated cells were able to differentiate into osteoblast and osteoclast cells, respectively, when exposed to the appropriate induction medium. In addition to the increased expression of OPN, osteoblasts also actively produce the ALP enzyme [32]. Therefore, ALP enzyme activity assays were carried out to detect the presence of active osteoblast cells, when adherent cells were cultured in the differentiation osteoblast medium that contains ascorbic acid and β-glycerophosphate. As seen in Figure 4, ALP enzyme activity was significantly higher from day 7 until day 14 of osteoblast differentiation in the presence of these two differentiation factors. This finding is in agreement with previous findings in which Zainal Ariffin et al. [9], Zainol Abidin et al. [33, 34], and Yazid et al. [36] showed that ALP activity increased during osteoblast differentiation. The ALP enzyme is associated with bone formation of osteoblast cells [37] as it is involved in producing high levels of local phosphate ions that provide the chemical conditions needed for mineral deposition, which induces the mineralization of osteoblast cells [38].

TRAP enzyme activity assays were carried out to detect the presence of osteoclast cells when suspension cells were cultured in the differentiation osteoclast medium, which contains RANKL and M-CSF. TRAP enzymes were secreted at the highest levels at day 10 of osteoclast differentiation (Figure 5). These data are also in accord with the findings of Zainal Ariffin et al. [9], Zainol Abidin et al. [33, 34], and Yazid et al. [36], who reported that TRAP enzyme activity was highest at day 10 of osteoclast differentiation from mouse cells in suspension. Furthermore, the increased activity of TRAP enzymes was concurrent with increased expression of the TRAP gene in the gene expression profile analyses. The adherent and suspension mononucleated cells, therefore, had the capacity to differentiate into osteoclasts and osteoblasts, respectively, when exposed to the appropriate induction medium. Thus, in this study, the gene expression profile and biochemical analyses of mononucleated cells during differentiation revealed that both adherent and suspension mononucleated cells were successfully differentiated into more specialized cells.

5. Conclusions

Using the expression of stem cell markers, adherent and suspension mononucleated cells were shown to have MSC and HSC characteristics, respectively. Observation of the gene expression profiles and biochemical analyses of adherent and suspension mononucleated cells during osteoblast and osteoclast differentiation, respectively, indicates that these cells are also capable of fully differentiating into their respective cell types. Therefore, our isolation procedure could be useful as the first step in isolating more homogeneous populations of MSCs and HSCs, which are essential for functional and molecular investigations into mechanisms that regulate their self-renewal, lineage restriction, and differentiation.

Acknowledgments

This study was supported by grants from the Ministry of Higher Education, Malaysia (UKM-ST-06-FRGS0099-2009 and UKM-ST-08-FRGS0004–2010), the Ministry of Science, Technology and Innovation (MOSTI), Malaysia (09-05-MGI-GMB002), and Universiti Kebangsaan Malaysia (UKM-GUP-BTK-07–15-197).