Background
Endothelial cells (EC) and smooth muscle cells (SMC) are two major cell types of blood vessels. EC and SMC are necessary for normal circulation and involved in different physiological processes, including angiogenesis, blood pressure control, coagulation, and inflammation [
1‐
4]. The study of EC and SMC is important for understanding the aetiology and treatment of cardiovascular and other diseases, including cancer and diabetes, since endothelial dysfunction is the basis of a broad range of pathologies [
5]. Both EC and SMC are considered promising resources for regenerative medicine and cell replacement therapy [
6‐
21].
Different cultures of endothelial and smooth muscle cells are used as models for studies of diseases. In vivo EC have high functional and structural heterogeneity depending on vessel type (artery, vein or lymphatic) and tissue [
3,
14,
22‐
25]. Endothelial heterogeneity manifests in embryonic development, and a cytokine-dependent signalling axis, along with the influence of the extracellular matrix and mechanical forces, drives this process further in the postnatal period. Indeed, it has been shown that EC and SMC isolated from various organs express defined patterns of transcription factors, angiogenic cytokines, adhesion molecules and chemokines [
3,
14,
22,
23,
26‐
28] that are essential to meet metabolic needs and adapt the cell to the organ environment. Therefore, isolation of EC and SMC from tissues relevant to the area of research is necessary for adequate study of specific pathologies [
29]. In addition, endothelial cells and their precursors are regarded as a promising source for regenerative medicine to treat pathological conditions such as cardiac infarction, muscle ischaemia, and bone fractures [
13]. Generation of sufficient vascular networks is also crucial for wound healing and successful tissue engineering.
It has been shown that the injection of EC and SMC in ischaemic organs leads to the formation of new blood vessels and promotes the recovery of the vascular network. The regenerative potential of endothelial cells is enhanced by smooth muscle cells [
30,
31]. Revascularization after injection of EC and SMC may be of a paracrine nature due to release of specific angiocrine factors that stimulate angiogenesis [
9,
15,
25].
Many researchers are currently seeking clinically relevant cell sources for the isolation of postnatal endothelial cells, endothelial progenitor cells [
6,
13,
29,
32‐
36] and smooth muscle cells [
7,
16,
17,
19‐
21]. However, sources of specialized human EC and SMC are limited, and the search for new sources is still relevant.
More than 20 years ago, two groups of authors developed methods for isolating human endothelial cells from the heart of the recipient during cardiac transplantation to study rejection of the donor organ [
37,
38]. However, this source is limited and may not be useful for regenerative purposes.
The aim of this study is to evaluate the use of primary human material rich in both EC and SMC, namely, right atrial appendage and ventricular cardiac tissues discarded during surgery. The atrial appendage is traditionally used as a source of c-kit-positive cardiac stem cells [
39,
40]. Additionally, in cultures derived from the atrial appendage, the presence of EC and SMC markers has been shown previously [
41]. The main goal of our study is to show that functional endothelial and smooth muscle cells can be obtained from an available source—surgical discarded cardiac tissue from right atrial appendage and right ventricular myocardium. We established a method for isolation, culture and enrichment of EC and SMC from cardiac tissues. This method yields a significant number of cells (up to 10
6) when they are cultured for 14 days in specific growth media for endothelial and smooth muscle cells. This amount is sufficient for magnetic sorting of CD31-positive endothelial cells. Endothelial and smooth muscle cells derived from human right atrial appendage and right ventricular myocardium may be a promising source of patient-specific cells for regenerative medicine purposes, especially for patients who face the prospect of surgical reoperation. For example, one application of endothelial cells is the development of cell-seeded vascular grafts, especially those under 6 mm in diameter [
8,
42]. As an example of what cells isolated by the proposed method may be used for tissue engineering, we seeded the cells on a biodegradable scaffold—a polycaprolactone/chitosan (PCL/CH) blended membrane.
We believe that the right atrial appendage and right ventricular myocardium can be used as a promising patient-specific source of EC and SMC. We think that our findings will be useful to scientists working towards improving techniques for therapeutic angiogenesis and tissue regeneration.
Methods
Ethical statements
All procedures with human material were approved by the ethical board of the State Research Institute of Circulatory Pathology, Ministry of Healthcare of the Russian Federation (permit No. 45 by 26.12. 2014), and all donors signed an informed consent form. The animal tests were conducted in an SPF vivarium and were approved by the Institute of Cytology and Genetics of the Siberian Branch of the Russian Academy of Sciences (IC&G SD RAS) ethical board (permit No. 22.4 by 30.05.2014).
Cell isolation and culture
Cells were isolated from post-surgically discarded samples of human right atrial appendage and right ventricle myocardium as follows: the tissue was mechanically ground into pieces (1–3 mm3) and then enzymatically treated in 0.1% collagenase NB solution (Life Technologies, USA) at 37 °C for 30 min. After that, the resulting mixture of cells and debris was centrifuged at 300g for 5 min and seeded in plastic dishes coated with human collagen IV (Sigma, USA) in culture media specific for EC or SMC–EGM-2 (Endothelial Cell Growth Medium-2) or SmGM-2 (Smooth Muscle Growth Medium-2) (both—Lonza, Switzerland). Cell culture was maintained in 5% CO2 at 37 °C with 1:2–1:3 passaging using TrypLE Express enzyme (Life Technologies, Denmark). The medium was replaced completely every other day; half of the culture medium was replaced daily. When primary cell culture in EGM-2 reached a monolayer, 106 cells were sorted using magnetic MicroBeads (130-091-935, Miltenyi Biotec, Germany) conjugated with antibodies against human CD31. The procedure of magnetic-activated cell sorting (MACS) was conducted according to the manufacturer’s instructions.
Preparation of chitosan/PCL polymer membranes
Chitosan/PCL membranes for cell seeding were prepared as described earlier [
43‐
45] with certain modifications. Stock solutions were made: 1) 1 wt% chitosan with 85% deacetylation degree (Sigma–Aldrich, USA) in 0.5 M acetic acid, 2) 10 wt% PCL in glacial acetic acid, and 3) the additional dilutions of PCL listed below, also prepared in glacial acetic acid. Resulting PCL stock solutions were mixed with 3 ml of 1% chitosan to obtain the following combinations in a total volume of 10 ml:
PCL25 (PCL:chitosan 1:3) = 10 ml 0.1% PCL + 3 ml 1% chitosan
PCL50 (PCL:chitosan 1:1) = 10 ml 0.3% PCL + 3 ml 1% chitosan
PCL75 (PCL:chitosan 3:1) = 10 ml 0.9% PCL + 3 ml 1% chitosan
The obtained solutions (PCL25, PCL50, PCL75) were poured onto culture dishes (2 ml/10 cm2) and allowed to air-dry in a thermostat (55 °C) for 24 h until film formation. Membranes on dishes were neutralized for 30 min either with alkaline (0.5 M NaOH [2% w/v] for 30 min) or with alkaline/ethanol mixture (0.5 M NaOH in 80% ethanol followed by 3 washes in 80% ethanol). Finally, dishes with membranes were washed in PBS (phosphate-buffered saline), UV-sterilized for 40 min and placed in a CO2 incubator with 5% CO2 at 37 °C.
Immunofluorescent staining of cells
Passage 1 EC and SMC were grown to confluence on plastic dishes or on chitosan/PCL membranes. After that, they were fixed with 4% PFA (paraformaldehyde) for 10 min, permeabilized with 0.05% Triton X-100 for 10 min, and blocked with 1% BSA (bovine serum albumin). The cells were stained with primary antibodies overnight at 4 °C, washed with PBS and incubated with secondary antibodies for 1 h at room temperature. The stained cells were analysed with an inverted fluorescence microscope (Nikon Ti-E) using Nikon AR software.
The following primary antibodies were used: anti-human CD31 (M0823, DAKO, 1:50), anti-α-SMA (DAKO, M0851, 1:50), anti-smooth muscle myosin heavy chain 11 (Abcam, ab82541, 1:500), anti-human CD90 (eBioscience, 14090982, 1:100), anti-Von Willebrand factor (Abcam, ab6994, 1:200), anti-fibronectin (Abcam, ab6328, 1:200), anti-elastin (Abcam, ab21610, 1:200), and anti-collagen IV (Life Span, 1:200).
The following secondary antibodies were used: Alexa Fluor 568 goat anti-mouse IgG1 (Life Technologies, A21124, 1:400), Alexa Fluor 488 goat anti-mouse IgG1 (Life Technologies, A21121, 1:400), Alexa Fluor 568 goat anti-mouse IgG2a (Life Technologies, A21134, 1:400), Alexa Fluor 568 goat anti-mouse IgG (H + L) (Life Technologies, A11031, 1:400), and Alexa Fluor 488 goat anti-mouse IgG (H + L) (Life Technologies, A11029, 1:400).
Flow cytometry quantitative analysis of cell populations
Cells in EGM-2 were used for fluorescence-activated cell sorting (FACS) analysis at the second passage before MACS and at the third passage after separation of CD31+ cells by MACS. Cells in SmGM-2 were used for FACS analysis at the second and fifth passages. The viability of cells was assessed by Trypan Blue (T10282, Invitrogen, USA) using a Countess Automated Cell Counter (C10227, Korea) and was more than 95%. The cells were detached with enzyme-free cell dissociation buffer (13151014, Gibco). Non-fixed cells were used for direct staining by fluorochrome-conjugated antibodies: anti-human CD31-APC (17-0319-42, eBioscience), anti-human VEGFR2-PE (560494, BD Biosciences), and anti-human CD90 (17-0909-42, eBioscience). Isotype-matched antibodies served as negative control. For indirect staining with anti-α-SMA antibodies (DAKO, M0851), cells were fixed with 4% PFA for 10 min, permeabilized with 0.1% TWEEN for 20 min, blocked with 1% BSA and incubated with primary antibodies overnight at 4 °C. Then, the cells were washed with PBS and incubated with Alexa Fluor 488 goat anti-mouse IgG (H + L) (Life Technologies, A11029) secondary antibody for 1 h at room temperature. The secondary antibody without the primary antibody was used as negative control. Cell populations were analysed on a FACS Canto II device using FACS Diva software. Assays were run in triplicate, and the data are presented as the mean ± standard deviation. Antibody dilutions and cell preparations were made according to the manufacturer’s instructions.
Analysis of endothelial cell ultrastructure
Endothelial cells from passage 2 were cultured on specific plastic films (Agar Scientific, Essex, UK) for 2, 4 and 8 days after MACS separation. EC attached to the films were fixed with 2.5% glutaraldehyde in cell culture medium for 15 min at room temperature and removed to a fresh solution of 2.5% glutaraldehyde in 0.1 M sodium cacodylate (pH 7.4) for 1 h incubation at room temperature with light agitation. Cells were washed three times for 5 min each in 0.1 M sodium cacodylate and post-fixed for 1 h in a 1% aqueous solution of osmium tetroxide containing 0.8% (w/v) of potassium ferricyanide (K3[Fe(CN)6]). After being washed with deionized water, the samples were incubated overnight at 4 °C in a 1% aqueous solution of uranyl acetate. The next day, the cells were washed once with deionized water, dehydrated in an ethanol series (30%, 50%—5 min, 70%, 96%—10 min, 100%—15 min) and acetone (twice, 20 min), and embedded in Agar 100 Resin (Agar Scientific, Essex, UK). Final polymerization of samples was induced by a 3-day incubation at 60 °C. Semi-thin sections were obtained with a Reichert-Jung Ultracut microtome, stained with methylene blue and analysed with a Zeiss Axioskop 40 light microscope. Ultra-thin sections were made using a Leica Ultracut microtome and stained with Reynolds lead citrate. Sections were examined with a JEOL JEM-100SX transmission electron microscope at the Interinstitutional Center for Microscopic Analysis of Biological Objects (IC&G SD RAS, Novosibirsk, Russia).
Cytokine pattern analysis
A total of 106 sorted and unsorted EC were grown in EGM-2 for 24 h on 10 cm dishes. After that, the medium was removed, the cells were washed with PBS three times, and unsupplemented basal EBM was added for 120 h to obtain conditioned medium. Cytokine pattern (vascular endothelial growth factor, VEGF; stromal cell-derived factor 1α, SDF1α; hepatocyte growth factor, HGF; epidermal growth factor, EGF; fibroblast growth factor 2, FGF2) was analysed by enzyme-linked immunosorbent assay (ELISA) using Quantikine kits (R&D Systems, USA).
Functional characteristics of EC and SMC in a Matrigel plug model
An in vivo Matrigel angiogenesis assay was conducted as previously described [
25,
46]. Female immunodeficient (severe combined immunodeficiency, SCID) mice (6–8 weeks, 22–28 g) were used for experiments. Animals were kept in the SPF vivarium of the IC&G SD RAS (Novosibirsk, Russia). EC and SMC were used at passage 5–7, and 5 × 10
5 cells in 50 µl PBS were mixed with 50 µl of Matrigel (BD Biosciences, USA) immediately before injection. A total of 100 µl of suspension was injected subcutaneously into the abdominal area of the animal. The animals (n = 15) were divided into three groups: a control group receiving only PBS (n = 5), a Matrigel + EC group (n = 5) and a group that received a Matrigel + EC/SMC 1:1 mixture injection (n = 5). The endothelial cells were labelled with vital MitoTracker Deep Red FM (M22426, Molecular Probes, USA). The animals were sacrificed after 14 days. The Matrigel plug was isolated and frozen in TissueTek (Sakura, USA), and 10 µm sections of the vascularized implant were obtained on a Leica HM550 cryotome (Leica, Germany). Prepared sections were stained with fluorescently tagged isolectin B4 to visualize the vasculature, and isolectin-positive structures were captured in 10 fields of view (FOVs) on a Nikon Ti-E microscope. Structure counts were obtained using Angio Tool software [
47], and the results were analysed using a Wilcoxon test with the Bonferroni correction in R version 3.3.1 (R Core Team, Austria) [
48]. Representative photos were performed using confocal microscope LSM 780 NLO (Zeiss) at the Microscopy Center of the Institute of Cytology and Genetics, SB RAS, Russia.
Fluorescent in situ hybridization (FISH)
Pretreatment of cryosections before FISH
Slides with cryosections were incubated in xylene for 10 min followed by rehydration in 100% ethanol 2 times for 5 min and 90, 80, 70–75, 50% ethanol for 5 min each. Then, the slides were washed in PBS for 15 min and incubated in 1% Triton X-100 overnight. The next day, the slides were washed in PBS for 15 min, transferred into a Coplin jar with prewarmed (80 °C) 10 mM sodium citrate buffer in a water bath, and incubate for 1 h. The slides were washed by soaking into a Coplin jar with PBS followed by incubation in prewarmed (37 °C) 0.01% pepsin for 10 min. Then, the slides were transferred into a Coplin jar with 1% BSA and washed in 2X SSC (saline-sodium citrate) 2 times for 5 min followed by incubation in Triton X-100 (0.7%)/HCl (0.1 N). Finally, the slides were washed in 2X SSC 2 times for 5 min.
Probe preparation
Human Cot-1 DNA (15279011, Thermo Fisher Scientific) and mouse Cot-1 DNA (18440016, Thermo Fisher Scientific) were labelled with biotin 16-dUTP (11093070910, Roche) or digoxigenin-11-dUTP (11558706910, Roche) in 30 PCR cycles by DOP-PCR (degenerate oligonucleotide-primed PCR) with MW6 primer [
49]. Human and mouse Cot-1 DNA and labelled probes (100 ng of each) were mixed with 1 mg/ml salmon sperm DNA, followed by addition of 2 volumes of 100% ethanol and complete desiccation in a speed vac. The desiccated probes were dissolved in 10 µl of hybridization solution containing 50% formamide, 10% dextran sulphate, 2X SSC (1X SSC: 0.15 M NaCl, 0.015 M sodium citrate, pH 7.0), and 1% TWEEN 20 for 1 h at 37 °C in a water bath. The probes were denatured in the hybridization solution for 5 min at 75 °C and transferred to ice quickly.
Slide preparation, in situ hybridization and washes
The slide-mounted cryosections were denatured in prewarmed 70% formamide/2X SSC for 20 min at 70 °C followed by incubation in 2X SSC for 2 min. The slides were dried at room temperature (r.t.). Ten microliters of probe was pipetted onto a prewarmed coverslip and picked up with a slide followed by incubation in a humid chamber in a water bath at 37 °C overnight. The next day, the slides were washed in 2X SSC/50% formamide 4 × 3 min at 37 °C in a water bath, then in 2X SSC 4 × 3 min at 37 °C and transferred to 4X SSC/0.1% TWEEN 20 at r.t.
Detection
Biotinylated probes were detected with a fluorescein-avidin (A-2011, Vector Laboratories)/biotinylated anti-avidin system (BA-0300, Vector Laboratories) and digoxigenin-labelled DNA was visualized with anti-digoxigenin rhodamine Fab fragments (11207750910, Roche). The nuclei were counterstained with 40,6-diamino-2-phenylindol in antifade (Vectashield, H-1200, Vector Laboratories) and then visualized using a Nikon Ni-E microscope.
XTT proliferation assay
Endothelial cells were seeded at a density of 2.5*104/cm2 in EGM-2 on plastic or chitosan/PCL membranes. Endothelial cell proliferation on chitosan/PCL was estimated by an XTT test (2,3-bis-(2-methoxy-4-nitro-5-sulfophenyl)-2H-tetrazolium-5-carboxanilide) (11465015001, Roche, USA) according to the manufacturer’s instructions at 22 h after the reagents were added. The results were estimated using a scanning spectrophotometer 2030 Multilabel Reader Victor X3 (Perkin-Elmer, USA) at 490 nm wavelength.
Evaluation of EC angiogenic potential in 3D Matrigel tubulogenesis assay
CD31+ (positive) sorted EC were stained with the vital mitochondrial dye TMRM (tetramethylrhodamine, methyl ester) (Life Technologies, USA) and cultured until 40–60% confluence. After that, the growth medium was aspirated and a 1:1 mixture of Matrigel (BD Biosciences, USA) with growth medium was prepared on ice. The obtained mixture was poured on top of the cells, and after 24 h of incubation, the formation of capillary-like structures was observed. Pictures were obtained on an inverted fluorescence microscope (Nikon Ti-E) by the Z-stack method, applying the Advanced Research software 6D module.
Cell seeding and viability assay
The proliferation of EC on different surface types was estimated by cell counts obtained at 1, 8 and 12 days after seeding on different matrices. The cells were labelled with TMRM vital mitochondrial dye (Life Technologies, USA) or NucBlue vital nuclear dye (Life Technologies, USA). Cells were counted in 5 random FOVs with a 10× objective using an inverted fluorescence microscope (Nikon Ti-E, Nikon, Japan) and NIS Advanced Research software (Nikon, Japan). All experiments were conducted in triplicate for statistical analysis.
Preparation of sections from membranes seeded with endothelial cells
For histological study, we chose CD31+ EC cultured on PCL75 membranes, which were fixed with 4% PFA as described above. The membrane with fixed cells was separated from the dish with tweezers and frozen in TissueTek; after that, 10 µm sections were prepared on a Cryostat Microm HM 550 (Microm International GmbH, Germany) in the Multiple-access Center for Microscopy of Biological Subjects (Institute of Cytology and Genetics, Novosibirsk, Russia).
Statistical analysis
RStudio version 3.3.1 [
48] and Microsoft Excel version 14.0.6023.1000 were used for data analysis. Data are presented as the mean ± SD. The Wilcoxon test, with Bonferroni correction where required, was used for comparison between the two groups. p < 0.05 was considered significant.
Discussion
Methods for isolation of cardiac EC and SMC have been described for many animal models, namely, mouse, rat, guinea pig, and rabbit [
69‐
78]. All of them are based on either a perfusion technique or enzymatic hydrolysis of myocardial samples, excised from the isolated heart from sacrificed animals. Isolation of human cardiac endothelial cells was described by Gräfe et al. and McDouall et al. [
37,
38]. As a source of endothelial cells, they used explanted human hearts of recipients who underwent cardiac transplantation. The first method requires a specialized perfusion system; the second was based on fermentative hydrolysis of chunks of ventricle from an explanted human heart followed by sorting with an anti-HLADR antibody or Ulex lectin-coated magnetic beads. The authors emphasize the importance of studying cardiac endothelial cells to investigate the pathophysiology/pharmacology of cardiovascular disease [
37].
The atrial appendage as a post-operative by-product is widely used for producing c-kit-positive cardiac stem cells (CSC), whose regenerative potential has been the focus of extensive research, including clinical trials (SCIPIO, CADUCEUS—see clinicaltrials.gov) [
79‐
82]. We propose to use this source as well as post-operative myocardial material to isolate human EC and SMC, which can be a source of patient-specific therapeutic cell populations in patients who face the prospect of surgical reoperation.
We introduced a technique for functional endothelial and smooth muscle cell extraction from post-operative myocardial specimens taken from the right atrial appendage and right ventricle. The proposed method includes the following stages: enzymatic tissue hydrolysis, culture of isolated cells on specific media on the surface of human collagen IV, enrichment by means of magnetic sorting for an endothelial population with antibodies against the mature endotheliocyte marker CD31, and further cultivation on a surface processed with collagen IV in specific culture media.
After enrichment by means of magnetic sorting, the content of CD31-positive cells increases more than fourfold, and the content of VEGFR2-positive cells increases almost tenfold in medium for endotheliocyte growth. Along with that, the content of CD90-positive cells non-specific for an endothelial population decreases up to 2.1 ± 2.8%, and αSMA-positive cells are lost. It is worth noting that in the process of primary culture in medium without added growth factors, endothelial markers are completely lost after 2–3 passages, and the fraction of CD90-positive cells increases up to 80% (data not presented). It is confirmed by a number of further tests that the population enriched for the endothelial marker CD31 represents functional endotheliocytes.
One important aspect of the functional characterization of an endothelial population is an ultrastructural study for the presence of typical granules. WPBs are distinctive cigar-shaped granules specific to functional endothelial cells [
83]. WPBs contain molecules of vWF protein, P-selectin, and the other functional molecules secreted by endothelial cells in response to shifting microenvironment conditions [
84,
85]. Thus, ultrastructural study of these cells reveals the presence and formation dynamics of WPBs (Fig.
3). In mature WPBs, folded structures of vWF—one of the basic components contained in the granules—are detected. The ability of derived endothelial cells to produce the extracellular matrix components fibronectin and collagen IV, to form capillary-like structures in Matrigel and to metabolize the acetylated form of low density lipoprotein is shown in the present study.
In terms of the investigation of cells’ functional properties by means of ELISA, cytokine quantities were estimated in conditioned medium obtained from primary unsorted culture, grown in EGM-2, as well as enriched endotheliocyte culture. The discovered decrease of VEGF165 in conditioned medium obtained from sorted cells compared to unsorted can be associated with two factors. First, cytokines are expressed not only by endothelial cells but by a number of other cell types (macrophages, activated T-lymphocytes and others) [
86,
87], which can be present in primary unsorted population. Direct enrichment of endothelial cells leads to the loss of a significant portion of other VEGF-secreting cells. For example, the fraction of CD90-positive cells decreases more than 20-fold. Second, the decrease of VEGF165 content in conditioned medium from sorted endotheliocytes can be associated with the almost tenfold increase of cells containing the VEGF receptor VEGFR2. FACS data indicate that the VEGFR2-positive portion elevates from 6.2 ± 1.6% in an unsorted population to 60.4 ± 2.5% in a sorted one. An analogous tendency to decrease in conditioned medium from enriched endotheliocytes is observed for HGF. Additionally, an insignificant drop of FGF-2 level is detected. The opposite tendency is revealed for SDF-1α and EGF. Their content in conditioned medium from sorted endothelial cells is reliably higher than in medium obtained from an unsorted cell population. A higher content of the given chemokines indicates the endothelial cells’ paracrine potential.
Functional characteristics in vitro were confirmed by functional testing in vivo on an abdominal Matrigel implant model in immunodeficient SCID mice. It has been shown by Japanese authors [
9,
15], that combined transplantation of human EC and mural cells (MC, both smooth muscle cells and pericytes) could markedly increase vascular regeneration compared to single-fraction transplantation of EC or MC. However, a transplantation of mural cells leads to less pronounced revascularization compared to endothelial cells. Therefore, to test in vivo the functional properties of the derived endothelial and smooth muscle cells, we had three experimental groups of SCID-mice: injection of endothelial cells, injection of both smooth muscle endothelial cells, and PBS as a control. Injection of endothelial cells leads to fivefold multiplication of vascular structures detected on Matrigel implant cryosections in comparison with control PBS injection. After cooperative injection of endothelial and smooth muscle cells derived from human myocardium, the quantity of vascular structures increases 15-fold compared to the control (Fig.
4d).
We have shown by fluorescent in situ hybridization that cryosections of Matrigel implants contain not only human cells but also mouse cells, the latter to a larger extent (Fig.
4e). This is affirmed by paracrine factor action, which facilitates the development of vascular structures composed of mouse cells in response to the introduction of human endothelial cells.
Thus, we proposed a new source for functional endothelial and smooth muscle cells isolation—post-operational material from the human right atrial appendage and right ventricle myocardium. These cells can be used for the development of cell-seeded tissue-engineered constructs for the purposes of vascular surgery. As an example of the application of both types of cells, we seeded them on a biodegradable scaffold—a polycaprolactone/chitosan (PCL/CH) blended membrane. We characterized the morphological and functional properties of those cells and evaluated their biological behaviour after seeding to chitosan/PCL membranes.
Blood vessel substitutes from biological and synthetic materials have been extensively developed in recent years [
66,
88]. Vascular grafts made of polytetrafluoroethylene (PTFE), polyethylene terephthalate (PET), and polyurethanes have been widely tested, and in spite of synthetic materials’ positive features (accurate sizing, permeability, controlled structure and mechanical properties), their application brought unsatisfactory long-term results [
88]. The latter is especially an issue when synthetic prostheses of small diameter are used. The complications include stenosis, thrombosis, neointimal hyperplasia, lack of vascularization and inflammation induced by polymer degradation products resulting in loss of structural integrity [
89,
90]. This problem drew researchers’ attention to biodegradable materials, among which chitosan and polycaprolactone (PCL) found wide medical application [
60]. Using a mixture of natural (chitosan) and synthetic (PCL) polymers made it possible to combine positive features of both materials [
91]. Furthermore, this approach increases feasibility and reduces expense compared to standard PCL-monomer synthesis followed by polymerization. In a number of works, both chitosan and PCL separately were found to be inferior to their combination, with optimal proportions of these components established and tested in membranes that were successfully seeded with mouse fibroblasts [
45], bovine corneal endothelial cells [
43] or human dermal microvascular EC [
44]. The possibility of using material consisting of a mixture of polycaprolactone and chitosan, seeded with autologous peripheral blood mononuclear cells, to create a small diameter vessel has been demonstrated in vivo in a canine model [
8]. However, even combined chitosan/PCL material has been shown to have much room for improvement, and as a mixture of 2 polymers gave better functional properties, seeding these with several ex vivo cultured cell types can provide more reliable reproduction of the properties of blood vessels.
The proliferation dynamics and retention of specific functional properties of endothelial and smooth muscle cells of human cardiac explants, contained in tissue-engineered constructs made on a base of polycaprolactone and chitosan, were analysed in vitro. We have shown that a mixture of polycaprolactone and chitosan is advantageous for endothelial cell proliferation in comparison with 100% chitosan. The proliferation indices of the endothelial cells tends to be higher upon alkaline-ethanol solution neutralization compared to alkaline aqueous solution (Fig.
5b). Cells proliferate on PCL25 surfaces more effectively than on PCL50 or PCL75 surfaces. Therefore, it is preferable to use membranes with a 25:75 ratio of PCL and chitosan, neutralized with a mixture of alkaline and ethanol, when creating tissue-engineered constructs with endothelial cells from human cardiac explants.
An important aspect to confirm the functionality of the cells growing on the scaffold is the retention of a typical pattern of cell antigens. It has been shown that, depending on the composition of the scaffold, the pattern of markers may change, even to the point that some of them are lost entirely. For example, the integral membrane protein Na–K ATPase in bovine corneal endothelium, growing on substrates of mixtures with different ratios of PCL/CH, was only weakly detected on PCL5 and PCL10, while levels appeared to be normal on PCL15 and PCL25 [
43]. It is reported that, when cells are grown on 100% chitosan, this marker is completely lost in the cells. It has been shown that, if human dermal microvascular endothelial cells (HDMEC) are grown on the surface of the metal alloy Co28Cr6Mo, endothelial cells acquire an aberrant pattern of intracellular distribution of CD31, VE-cadherin, ZO-1 and F-actin [
92]. In experiments conducted in vivo, implants of CoCrMo-alloy disrupted the integrity of the microvascular endothelium in the surrounding tissues and caused extensive oedema [
93], whereas the cultivation of HDMEC on the surface of a titanium alloy does not lead to changes in the pattern of intracellular distribution of these markers [
92].
We have shown in vitro retention of specific markers contained in endothelial and smooth muscle cells in tissue-engineered constructs on a PCL and chitosan mixture. For endothelial cells grown on membranes made of given polymer mixtures, retention of CD31 and vWF was shown, along with the capacity to metabolize low-density lipoproteins, to yield the extracellular matrix components collagen IV and fibronectin, and to form capillary-like structures in Matrigel poured onto cells sitting on the membrane. For smooth muscle cells, αSMA and SMMHC retention was shown. Retention of cell functional properties in the composition of tissue-engineered constructs in vitro gives grounds for the assumption that populating a mixed polymer membrane would facilitate adequate integration to surrounding tissues and minimize negative remote results for vascular transplant. Thus, in the year 2013, a group of investigators demonstrated the possibility of using material composed of a mixture of PCL and chitosan for cell-seeded vessels of small diameter (less than 6 mm) [
8]. The nano-fibres utilized in scaffold formation were obtained by electro-spinning of given polymer mixture, and then they were populated by autologous mononuclear cells from canine peripheral blood and implanted in the carotid arteries of 6 dogs. Histological and immunohistochemical analysis of the tissue-engineered constructs, obtained after 3 months, showed the regeneration of endothelium and the presence of collagen and elastin [
8]. In work on bovine corneal endothelium growing on membranes prepared from PCL-chitosan mixture by means of evaporation in a convection oven, the authors demonstrated the high proliferative capacities and preservation of morphophysiological and functional properties of endothelial cells in the constructs [
43].
Authors’ contributions
Conception and design: ZIS, SAI, PEA, ILN, ZSM; data analysis and interpretation: ZIS, ZMK, SShB, SAI, SAM, SA, MPI, AE; contribution of reagents/materials/analysis tools/administrative and financial support: KAA, PEA, ILN, PYV, AE, ZSM; manuscript writing: ZIS, MPI, SAI, SAM. All authors read and approved the final manuscript.