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Purpose. Tricalcium phosphate (TCP)/chitosan composite microgranules were developed as bone substitutes and tissue engineering scaffolds with the aim of obtaining a high bone forming efficacy. The microgranules have the ability to fill various types o...
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RISS 인기검색어
Transforming Growth Factor (TGF)-β1 Releasing Tricalcium Phosphate/Chitosan Microgranules as Bone Substitutes
한글로보기https://www.riss.kr/link?id=E873567
- 저자
- 발행기관
-
발행연도
2004년
-
작성언어
English
-
자료형태
dCollection
-
수록면
88-94
-
0
상세조회 -
0
다운로드
부가정보
다국어 초록 (Multilingual Abstract)
Purpose. Tricalcium phosphate (TCP)/chitosan composite microgranules were developed as bone substitutes and tissue engineering scaffolds with the aim of obtaining a high bone forming efficacy. The microgranules have the ability to fill various types of defect sites with closer packing. In addition. the transforming growth factor-beta I(TGF-β1) was added to the microgranules in order to improve bonehealing efficacy.
Methods. TCP/chitosan microgranules were fabricated by dropping a TCP suspended chitosan solution into a NaOH/ethanol solution. TGF-β1 was incorporated into the TCP/chitosan microgranules by soaking the microgranules into the TGF-β1 solution. Scanning electron microscopy(SEM) observations as well as experiments examining the release of TGF-β1 from chitosan and TCP/chitosan microgranules were performed. SEM was used to examine the cell morphologies on the microgranules, and the extent of cell proliferation was evaluated using a dimethyl-thiazol tetrazolium bromide (MTT) assay. The differentiated cell function was assessed by measuring the alkaline phosphatase activity as well as performing an osteocalcin assay.
Results. The size of the prepared microgranules was 350-500㎛ and TCP powders were observed on the surface of the microgranules. TGF-β1 was released from the TCP/chitosan microgranules at a therapeutic concentration for 4 weeks. The proliferation of osteoblasts on the TGF-β1 loaded microgranules was the highest among the microgranules. SEM indicated that the seeded osteoblastice cells were firmly attached to the microgranules and proliferated in a multilayer fashion. The ALPase activity and osteocalcin content of all the samples increased during the culture period
Conclusions. These results suggest that the TCP/chitosan microgranules are potential bone substitutes with a drug releasing capacity and a osteoblastic cells culture scaffold.
Methods. TCP/chitosan microgranules were fabricated by dropping a TCP suspended chitosan solution into a NaOH/ethanol solution. TGF-β1 was incorporated into the TCP/chitosan microgranules by soaking the microgranules into the TGF-β1 solution. Scanning electron microscopy(SEM) observations as well as experiments examining the release of TGF-β1 from chitosan and TCP/chitosan microgranules were performed. SEM was used to examine the cell morphologies on the microgranules, and the extent of cell proliferation was evaluated using a dimethyl-thiazol tetrazolium bromide (MTT) assay. The differentiated cell function was assessed by measuring the alkaline phosphatase activity as well as performing an osteocalcin assay.
Results. The size of the prepared microgranules was 350-500㎛ and TCP powders were observed on the surface of the microgranules. TGF-β1 was released from the TCP/chitosan microgranules at a therapeutic concentration for 4 weeks. The proliferation of osteoblasts on the TGF-β1 loaded microgranules was the highest among the microgranules. SEM indicated that the seeded osteoblastice cells were firmly attached to the microgranules and proliferated in a multilayer fashion. The ALPase activity and osteocalcin content of all the samples increased during the culture period
Conclusions. These results suggest that the TCP/chitosan microgranules are potential bone substitutes with a drug releasing capacity and a osteoblastic cells culture scaffold.
Purpose. Tricalcium phosphate (TCP)/chitosan composite microgranules were developed as bone substitutes and tissue engineering scaffolds with the aim of obtaining a high bone forming efficacy. The microgranules have the ability to fill various types of defect sites with closer packing. In addition. the transforming growth factor-beta I(TGF-β1) was added to the microgranules in order to improve bonehealing efficacy.
Methods. TCP/chitosan microgranules were fabricated by dropping a TCP suspended chitosan solution into a NaOH/ethanol solution. TGF-β1 was incorporated into the TCP/chitosan microgranules by soaking the microgranules into the TGF-β1 solution. Scanning electron microscopy(SEM) observations as well as experiments examining the release of TGF-β1 from chitosan and TCP/chitosan microgranules were performed. SEM was used to examine the cell morphologies on the microgranules, and the extent of cell proliferation was evaluated using a dimethyl-thiazol tetrazolium bromide (MTT) assay. The differentiated cell function was assessed by measuring the alkaline phosphatase activity as well as performing an osteocalcin assay.
Results. The size of the prepared microgranules was 350-500㎛ and TCP powders were observed on the surface of the microgranules. TGF-β1 was released from the TCP/chitosan microgranules at a therapeutic concentration for 4 weeks. The proliferation of osteoblasts on the TGF-β1 loaded microgranules was the highest among the microgranules. SEM indicated that the seeded osteoblastice cells were firmly attached to the microgranules and proliferated in a multilayer fashion. The ALPase activity and osteocalcin content of all the samples increased during the culture period
Conclusions. These results suggest that the TCP/chitosan microgranules are potential bone substitutes with a drug releasing capacity and a osteoblastic cells culture scaffold.
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