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用蓝色发光二极管(455纳米)照射的成牙本质细胞样细胞的代谢活性。

Metabolic activity of odontoblast-like cells irradiated with blue LED (455 nm).

作者信息

de Almeida Leopoldina Fátima Dantas, Basso Fernanda Gonçalves, Turrioni Ana Paula Silveira, de-Souza-Costa Carlos Alberto, Hebling Josimeri

机构信息

Department of Restorative Dentistry, Araraquara Dental School, "Univ. Estadual Paulista-UNESP", Araraquara, SP, Brazil.

Department of Orthodontics and Pediatric Dentistry, Araraquara Dental School, "Univ. Estadual Paulista-UNESP", Rua Humaitá, 1680, Araraquara, SP, Brazil.

出版信息

Lasers Med Sci. 2016 Jan;31(1):119-25. doi: 10.1007/s10103-015-1837-z. Epub 2015 Nov 25.

Abstract

Blue light emitting diodes (LEDs) are frequently used in dentistry for light activation of resin-based materials; however, their photobiostimulatory effects have not yet been fully investigated. This study aimed to investigate the effect of blue LED (455 nm) on the metabolism of odontoblast-like cells MDPC-23. Energy doses of 2 and 4 J/cm(2) were used at 20 mW/cm(2) fixed power density. MDPC-23 cells were seeded at 10,000 cells/cm(2) density in Dulbecco's modified Eagle's medium (DMEM) containing 10 % fetal bovine serum (FBS). After 12 h, the culture medium was replaced with new DMEM supplemented with 0.5 % of FBS, and the cells were incubated for further 12 h. After that, single irradiation was performed to the culture, under selected parameters. Cell viability evaluations (Alamar Blue Assay, n = 12), number of viable cells (Trypan Blue Assay, n = 12), morphological analysis by scanning electron microscopy (SEM, n = 2), gene expression (n = 6) of alkaline phosphatase (Alp), collagen (Col-1a1), and dental matrix protein (Dmp-1) (quantitative polymerase chain reaction (qPCR)) were performed 72 h after irradiation. Data were analyzed by Kruskal-Wallis, ANOVA, and Tukey tests (p < 0.05). Direct light application at 4 J/cm(2) energy dose had no negative effects on cell viability, while irradiation with 2 J/cm(2) reduced cell metabolism. None of doses affected the number of viable cells compared with the control group. The two energy doses downregulated the expression of Alp; however, expression of Col-1a1 and Dmp-1 had no alteration. Cells presented change in the cytoskeleton only when irradiated with 2 J/cm(2). In conclusion, the blue LED (455 nm) irradiation, under the evaluated parameters, had no biostimulatory effects on MDPC-23 cells.

摘要

蓝色发光二极管(LED)在牙科领域常用于光激活树脂基材料;然而,其光生物刺激作用尚未得到充分研究。本研究旨在探讨蓝色LED(455纳米)对成牙本质细胞样细胞MDPC - 23代谢的影响。在固定功率密度为20毫瓦/平方厘米的条件下,使用了2焦耳/平方厘米和4焦耳/平方厘米的能量剂量。将MDPC - 23细胞以10000个细胞/平方厘米的密度接种于含有10%胎牛血清(FBS)的杜尔贝科改良伊格尔培养基(DMEM)中。12小时后,用添加了0.5% FBS的新鲜DMEM更换培养基,并将细胞再孵育12小时。之后,在选定参数下对培养物进行单次照射。照射72小时后进行细胞活力评估(alamar蓝测定法,n = 12)、活细胞数量(台盼蓝测定法,n = 12)、通过扫描电子显微镜进行形态分析(SEM,n = 2)以及碱性磷酸酶(Alp)、胶原蛋白(Col - 1a1)和牙基质蛋白(Dmp - 1)的基因表达(n = 6)(定量聚合酶链反应(qPCR))。数据通过Kruskal - Wallis检验、方差分析和Tukey检验进行分析(p < 0.05)。4焦耳/平方厘米能量剂量的直接光照对细胞活力没有负面影响,而2焦耳/平方厘米的照射降低了细胞代谢。与对照组相比,各剂量均未影响活细胞数量。两种能量剂量均下调了Alp的表达;然而,Col - 1a1和Dmp - 1的表达没有改变。仅在以2焦耳/平方厘米照射时细胞的细胞骨架出现变化。总之,在所评估的参数下,蓝色LED(455纳米)照射对MDPC - 23细胞没有生物刺激作用。

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