Literature DB >> 12124795

Formation of three-dimensional cell/polymer constructs for bone tissue engineering in a spinner flask and a rotating wall vessel bioreactor.

Vassilios I Sikavitsas1, Gregory N Bancroft, Antonios G Mikos.   

Abstract

The aim of this study is to investigate the effect of the cell culture conditions of three-dimensional polymer scaffolds seeded with rat marrow stromal cells (MSCs) cultured in different bioreactors concerning the ability of these cells to proliferate, differentiate towards the osteoblastic lineage, and generate mineralized extracellular matrix. MSCs harvested from male Sprague-Dawley rats were culture expanded, seeded on three-dimensional porous 75:25 poly(D,L-lactic-co-glycolic acid) biodegradable scaffolds, and cultured for 21 days under static conditions or in two model bioreactors (a spinner flask and a rotating wall vessel) that enhance mixing of the media and provide better nutrient transport to the seeded cells. The spinner flask culture demonstrated a 60% enhanced proliferation at the end of the first week when compared to static culture. On day 14, all cell/polymer constructs exhibited their maximum alkaline phosphatase activity (AP). Cell/polymer constructs cultured in the spinner flask had 2.4 times higher AP activity than constructs cultured under static conditions on day 14. The total osteocalcin (OC) secretion in the spinner flask culture was 3.5 times higher than the static culture, with a peak OC secretion occurring on day 18. No considerable AP activity and OC secretion were detected in the rotating wall vessel culture throughout the 21-day culture period. The spinner flask culture had the highest calcium content at day 14. On day 21, the calcium deposition in the spinner flask culture was 6.6 times higher than the static cultured constructs and over 30 times higher than the rotating wall vessel culture. Histological sections showed concentration of cells and mineralization at the exterior of the foams at day 21. This phenomenon may arise from the potential existence of nutrient concentration gradients at the interior of the scaffolds. The better mixing provided in the spinner flask, external to the outer surface of the scaffolds, may explain the accelerated proliferation and differentiation of marrow stromal osteoblasts, and the localization of the enhanced mineralization on the external surface of the scaffolds. Copyright 2002 Wiley Periodicals, Inc.

Entities:  

Keywords:  NASA Discipline Cell Biology; Non-NASA Center

Mesh:

Substances:

Year:  2002        PMID: 12124795     DOI: 10.1002/jbm.10150

Source DB:  PubMed          Journal:  J Biomed Mater Res        ISSN: 0021-9304


  58 in total

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4.  Bioreactor strategy in bone tissue engineering: pre-culture and osteogenic differentiation under two flow configurations.

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5.  Enhanced cell ingrowth and proliferation through three-dimensional nanocomposite scaffolds with controlled pore structures.

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6.  Evaluation of bioreactor-cultivated bone by magnetic resonance microscopy and FTIR microspectroscopy.

Authors:  Ingrid E Chesnick; Francis A Avallone; Richard D Leapman; William J Landis; Naomi Eidelman; Kimberlee Potter
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7.  Biological response to pre-mineralized starch based scaffolds for bone tissue engineering.

Authors:  A J Salgado; J E Figueiredo; O P Coutinho; R L Reis
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8.  Transplantation of engineered bone tissue using a rotary three-dimensional culture system.

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Review 9.  Tissue engineered bone grafts: biological requirements, tissue culture and clinical relevance.

Authors:  Mirjam Fröhlich; Warren L Grayson; Leo Q Wan; Darja Marolt; Matej Drobnic; Gordana Vunjak-Novakovic
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10.  The effect of hydrostatic pressure on three-dimensional chondroinduction of human adipose-derived stem cells.

Authors:  Rei Ogawa; Shuichi Mizuno; George F Murphy; Dennis P Orgill
Journal:  Tissue Eng Part A       Date:  2009-10       Impact factor: 3.845

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