1. Generation of human umbilical cord vein CD146+ perivascular cell origined three-dimensional vascular construct
- Author
-
Betül Çelebi-Saltik, Petek Korkusuz, Beyza Gökçinar-Yagci, and Nilgün Yersal
- Subjects
0301 basic medicine ,Tunica media ,Pathology ,medicine.medical_specialty ,Myocytes, Smooth Muscle ,0206 medical engineering ,Dermatan Sulfate ,Tenascin ,CD146 Antigen ,Cell Communication ,02 engineering and technology ,Biochemistry ,Blood Vessel Prosthesis Implantation ,03 medical and health sciences ,Human Umbilical Vein Endothelial Cells ,medicine ,Humans ,Cells, Cultured ,Tissue Engineering ,Tissue Scaffolds ,biology ,Chemistry ,Tunica Adventitia ,Cell Biology ,Fibroblasts ,Tunica intima ,020601 biomedical engineering ,Blood Vessel Prosthesis ,Elastin ,Extracellular Matrix ,Fibronectin ,Phenotype ,030104 developmental biology ,medicine.anatomical_structure ,Cell Transdifferentiation ,cardiovascular system ,biology.protein ,CD146 ,Collagen ,Cardiology and Cardiovascular Medicine ,Blood vessel - Abstract
Small-diameter vascular grafts are needed for the treatment of coronary artery diseases in the case of limited accessibility of the autologous vessels. Synthetic scaffolds have many disadvantages so in recent years vascular constructs (VCs) made from cellularized natural scaffolds was seen to be very promising but number of studies comprising this area is very limited. In our study, our aim is to generate fully natural triple-layered VC that constitutes all the layers of blood vessel with vascular cells. CD146+ perivascular cells (PCs) were isolated from human umbilical cord vein (HUCV) and differentiated into smooth muscle cells (SMCs) and fibroblasts. They were then combined with collagen type I/elastin/dermatan sulfate and collagen type I/fibrin to form tunica media and tunica adventitia respectively. HUCV endothelial cells (ECs) were seeded on the construct by cell sheet engineering method after fibronectin and heparin coating. Characterization of the VC was performed by immunolabeling, histochemical staining and electron microscopy (SEM and TEM). Differentiated cells were identified by means of immunofluorescent (IF) labeling. SEM and TEM analysis of VCs revealed the presence of three histologic tunicae. Collagen and elastic fibers were observed within the ECM by histochemical staining. The vascular endothelial growth factor receptor expressing ECs in tunica intima; α-SMA expressing SMCs in tunica media and; the tenascin expressing fibroblasts in tunica adventitia were detected by IF labeling. In conclusion, by combining natural scaffolds and vascular cells differentiated from CD146+ PCs, VCs can be generated layer by layer. This study will provide a preliminary blood vessel model for generation of fully natural small-diameter vascular grafts.
- Published
- 2018
- Full Text
- View/download PDF