Growth factor release from platelet concentrates: analytic quantification and characterization for clinical applications

Background and Objectives Clinical use of plasma rich in growth factors requires biochemical product control. We aimed to measure and modulate concentrations of growth factors in solutions deriving from platelet apheresis or whole blood. Materials and Methods Growth factor concentrations were measur...

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Bibliographic Details
Published in:Vox sanguinis 2013-08, Vol.105 (2), p.129-136
Main Authors: Durante, C., Agostini, F., Abbruzzese, L., T. Toffola, R., Zanolin, S., Suine, C., Mazzucato, M.
Format: Article
Language:English
Subjects:
Adult
apheresis - platelets
Blood
Blood platelets
Blood Platelets - cytology
Blood Platelets - secretion
Blood Preservation
Calcium Chloride - pharmacology
Female
Humans
Intercellular Signaling Peptides and Proteins - secretion
Male
Middle Aged
Plasma
platelet concentrates
Platelet Transfusion
Plateletpheresis
quality control
regenerative medicine
Time Factors
Vascular endothelial growth factor
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Summary:Background and Objectives Clinical use of plasma rich in growth factors requires biochemical product control. We aimed to measure and modulate concentrations of growth factors in solutions deriving from platelet apheresis or whole blood. Materials and Methods Growth factor concentrations were measured 5’, 10’, 20’, 30’, 60’ after CaCl2 was added at 40°C to platelet‐apheresis products (n = 39) or after 60’ in platelet concentrates from whole blood (n = 13). Growth factor release was also obtained in platelet apheresis a) by incubation at 22°C or 40°C for 10’ or 30’ (n = 4); b) by repeated freeze–thaw (n = 9). Results Fibroblast growth factor (FGF), platelet‐derived growth factor (PDGF) isoforms AA and AB and transforming growth factor beta (TGF‐β) concentrations (pg/109 plt) were 25–60% higher in growth factors solutions from whole blood compared to platelet apheresis. Vascular endothelial growth factor (VEGF), TGF‐β and PDGF isoforms were released early (5–10’) during incubation: TGF‐β concentration increased also at 30’. FGF and epidermal growth factor (EGF) were released only after 30’. Incubation at 40°C/10’ increased VEGF (+70%) and decreased EGF (−30%) and PDGF‐BB (−50%) versus 22°C/30’. Shock significantly increased TGF‐β (1·6‐fold), EGF (1·5‐fold), FGF (4·5‐fold) and lowered PDGF isoforms (0·2‐ to 0·5‐fold) versus prolonged incubation at 40°C. Conclusion Platelets from platelet apheresis and whole‐blood release all investigated growth factors. The release can be regulated controlling incubation time and/or temperature and performing cell lysis.
ISSN:0042-9007
1423-0410
DOI:10.1111/vox.12039