In vitro cell proliferation assay of demineralized dentin material membrane in osteoblastic MC3T3-E1 cells Defects: The Potential Application of Biological Forms of Bovine-Bone Filler

Pratiwi Soesilowati, - and Andra Rizqiawan, - and Retno Indrawati Roestamadji, - and Ahmad Rizal Arrosyad, - and Muhammad Alwino Bayu Firdauzy, - and Noor Hayaty Abu Kasim, - (2021) In vitro cell proliferation assay of demineralized dentin material membrane in osteoblastic MC3T3-E1 cells Defects: The Potential Application of Biological Forms of Bovine-Bone Filler. Clinical, Cosmetic and Investigational Dentistry, 13. pp. 1-7. ISSN 11791357

[img] Text (NASKAH)
15.In vitro cell proliferation.pdf
Download (841kB)
[img] Text (TURNITIN)
13. In vitro Cell Proliferation Assay of Demineralized Dentin.pdf
Download (1MB)
[img] Text (VALIDASI)
Artikel 15 Andra Riqiawan.pdf
Download (3MB)
[img] Text (VALIDASI2)
6.Dr.Pratiwi (In Vitro Cell Proliferasi...).pdf
Download (1MB)
[img] Text (KARIL)
16.In Vitro.pdf
Download (1MB)

Abstract

Aim: Demineralized dentin material membrane (DDMM) is a novel bioresorbable guided bone regeneration (GBR) which is derived from the demineralization process of bovine dentin. This material/process could be an alternative to resolve musculoskeletal dysfunction that harms the quality of human life. Purpose: To evaluate the cytotoxic effect of DDMM as GBR membrane on MC3T3-E1 osteoblast cell line. Methods: Cytotoxic effect was evaluated using the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay. Osteoblast MC3T3-E1 cell culture was used as a parameter of cell viability after reacting with GBR materials. The absorbance values were examined at each treatment to determine the percentage of cell viability. There were four groups created in the present study: two treatment groups and two control groups. The treatment groups consisted of a DDMM group and a bovine pericardium collagen membrane (BPCM) group. The control groups comprised a group containing cell culture medium as a negative control group and another positive control group that contained cell cultures. Results: The results revealed no significant difference in MC3T3-E1 cell viability between the treatment and control groups (p < 0.05). Moreover, as observed in the DDMM group, there was an increase in the number of osteoblast cells. Conclusion: DDMM is a suitable alternative biomaterial for GBR as it is non-cytotoxic and could potentially increase the rate of repair of craniofacial defects.

Item Type: Article
Subjects: R Medicine
R Medicine > RK Dentistry
Divisions: 02. Fakultas Kedokteran Gigi > Oral and Maxilofacial Surgery (Spesialis)
Creators:
CreatorsNIM
Pratiwi Soesilowati, -NIDN0030077901
Andra Rizqiawan, -NIDN0023098101
Retno Indrawati Roestamadji, -NIDN0012115903
Ahmad Rizal Arrosyad, --
Muhammad Alwino Bayu Firdauzy, -NIM021611133154
Noor Hayaty Abu Kasim, --
Depositing User: Rudy Febiyanto
Date Deposited: 16 Jun 2022 03:25
Last Modified: 08 Aug 2023 11:40
URI: http://repository.unair.ac.id/id/eprint/116765
Sosial Share:

Actions (login required)

View Item View Item