Different Proliferative Properties of Smooth Muscle Cells of Human Arterial and Venous Bypass Vessels

Author:

Yang Zhihong1,Oemar Barry S.1,Carrel Thiery1,Kipfer Beat1,Julmy Friedgard1,Lüscher Thomas F.1

Affiliation:

1. From Cardiovascular Research (Z.Y., B.S.O., T.F.L.), Institute for Physiology, University Zürich-Irchel, Switzerland; Cardiology (F.J.), Cardiovascular and Thoracic Surgery (T.C., B.K.), Inselspital Bern, Switzerland; and Cardiology (Z.Y., B.S.O., T.F.L.), University Hospital Zürich, Switzerland.

Abstract

Background —Internal mammary artery (IMA) bypass grafts have a higher patency than saphenous vein (SV) grafts. Intimal hyperplasia of SV grafts is due to smooth muscle cell (SMC) proliferation and migration. We hypothesized that different SMC growth activity exists in IMA and SV, which may explain the different patencies of arterial and venous grafts. Methods and Results —SMCs were isolated from IMA and SV by explant culture and stimulated with serum or platelet-derived growth factor-BB (PDGF-BB). Cell growth was analyzed by explant outgrowth rate, 3 H-thymidine incorporation, or cell counting. PDGF receptor expression and autophosphorylation, regulation of mitogen-activated protein kinases (MAPKs), and cyclin-dependent kinase inhibitors (p27 Kip1 and p21 Cip1 ) were analyzed by molecular techniques. SMC outgrowth from explants by serum (20%) over a 20-day period was more pronounced in SV (37±5%) than in IMA (4±3%; P <.001) of the same patients. Serum (10%) increased cell number more rapidly in SV (2×10 4 /well to 18±4×10 4 /well; P <.05) than in IMA (2×10 4 /well to 9±4×10 4 /well; P <.05) over an 8-day period. PDGF-BB (0.01 to 10 ng/mL) stimulated 3 H-thymidine incorporation (1347±470% above control levels) and increased cell number in SV (2×10 4 /well to 5±1×10 4 /well; P <.05) but not in IMA. PDGF α- and β-receptors were similarly expressed and were activated in both SV and IMA. PDGF-BB induced a similar MAPK activation (kinetics and maximal activity) in both SV and IMA cells but increased MAPK protein level only in SV. Furthermore, PDGF-BB markedly downregulated the cell cycle inhibitor p27 Kip1 in SV, but this was much less pronounced in IMA. Conclusions —SMCs from SVs exhibit enhanced proliferation compared with IMA in spite of functional growth factor receptor expression and MAPK activation. However, PDGF increased MAPK protein level only in SV and downregulated cell cycle inhibitor (p27 Kip1 ) more potently in SV than in IMA. This may explain the resistance to growth stimuli of IMA SMCs and may contribute to the longer patency of arterial versus venous grafts.

Publisher

Ovid Technologies (Wolters Kluwer Health)

Subject

Physiology (medical),Cardiology and Cardiovascular Medicine

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