EFFECT OF CHITOSAN ON PROTEIN CONTENT IN THE MEDIUM CULTURE OF OSTEOBLASTS EXPOSED TO OXIDATIVE STRESS

Abstract

Chitosan is a derivative of chitin which has potential for use in bone regeneration and has been reported can stimulate
bone formation. Oxidative stress as one cause of bone damage, was found increased in osteoporosis, periodontitis and
arthritis. One of the species oxygen reactive (ROS), hydrogen peroxide, has been reported can inhibit osteoblast proliferation. This study was aimed to investigate the effect of various chitosan concentrations on protein content in the
culture medium of human osteoblast-like cell line, MG 63, which was exposed to hydrogen peroxide. MG 63 cells were
exposed to various chitosan concentrations (% w/v) 0.1, 0.2, 0.4, and 1.6%. Culture cells without chitosan were used as a
control. Cells were growth with α-MEM medium (37ºC, 5% CO2) until they became confluent, then they were exposed to
hydrogen peroxide for 4 hours. The protein content in the culture medium was measured by using Bradford protein assay
at 655 nm wavelength. The result showed that hydrogen peroxide decreased protein concentration in the medium culture
compared with group without hydrogen peroxide. Treatment group with chitosan concentration 0.4% and 1.6% exhibited
a significant increasing of protein concentration in osteoblast culture medium compared with control. In conclusion, in
osteoblast culture medium chitosan can inhibit the decreasing of total protein concentration which was caused by
oxidative stress.