Achatina fulica mucous improves cell viability and increases collagen deposition in UVB-irradiated human fibroblast culture.

IF 1.1 Q4 CELL & TISSUE ENGINEERING
Journal of Stem Cells & Regenerative Medicine Pub Date : 2020-05-27 eCollection Date: 2020-01-01 DOI:10.46582/jsrm.1601005
Ch Tri Nuryana, Sofia Mubarika Haryana, Yohanes Widodo Wirohadidjojo, Nur Arfian
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引用次数: 4

Abstract

Introduction: Ultraviolet radiation induces skin photoaging by increasing matrix metalloproteinase-1 (MMP-1). MMP-1 degrades type I and III collagen that comprise the dermal connective tissue. Achatina fulica mucous (AFM) is a natural remedy that has protective effects on fibroblasts and collagen. Objective: To investigate the effects of AFM on cell viability and collagen deposition in UVB-irradiated human fibroblast culture. Methods: The mucous was extracted from 50 Achatina fulica snails that were stimulated by a 5-10 Volt electricity shock for 30-60 seconds and converted into powder by the freeze-drying process. The human dermal fibroblast culture was divided into six groups: group 1 were normal fibroblasts without UVB irradiation as normal control, groups 2-5 consisted of 100 mJ/cm2 UVB-irradiated fibroblasts. Group 2 had no treatment as negative control, group 3 was treated by PRP 10% as positive control group and groups 4-6 were treated by various concentrations of AFM (3.9; 15.625 and 62.5 μg/mL). At the end of the experiment, the proliferation was assessed with MTT assay, furthermore collagen deposition was measured by Sirius red assay. Real Time-PCR (RT-PCR) was performed to quantify Coll I, Coll III and MMP-1 mRNA expression, then to measured COL 1/COL III ratio. Results: UVB induced significant lower viability, upregulated MMP-1 and downregulated COL I and COL III mRNA expressions. Meanwhile AFM treated groups demonstrated higher cell viability with downregulation of MMP-1 and upregulation of COL I and COL III mRNA expressions. The ratio of COL I/ III expression was significantly (p<0.05) lower in the AFM treated groups compared to the UVB group. Among AFM treated groups, administration of 62.5 μg/mL AFM represented the best result. Conclusion: AFM may ameliorate viability of UVB-irradiated human fibroblast culture which associates with downregulating MMP-1, upregulating COL I and Col III, and reducing COL I/III ratio.

在uvb辐照的人成纤维细胞培养中,黄芩黏液提高细胞活力,增加胶原沉积。
紫外线照射通过增加基质金属蛋白酶-1 (MMP-1)诱导皮肤光老化。MMP-1降解构成真皮结缔组织的I型和III型胶原蛋白。黄芪黏液(AFM)是一种天然药物,对成纤维细胞和胶原蛋白有保护作用。目的:探讨AFM对uvb辐照人成纤维细胞细胞活力和胶原沉积的影响。方法:50只黄斑螺经5 ~ 10伏电击刺激30 ~ 60秒后,经冻干工艺转化成粉末,提取粘液。将人真皮成纤维细胞培养分为6组:1组为未受UVB照射的正常成纤维细胞,2-5组为受UVB照射100 mJ/cm2的成纤维细胞。2组不处理为阴性对照组,3组用10% PRP处理为阳性对照组,4 ~ 6组用不同浓度AFM (3.9;15.625和62.5 μg/mL)。实验结束时,采用MTT法检测细胞增殖情况,采用天狼星红法检测胶原沉积情况。采用Real Time-PCR (RT-PCR)检测Coll I、Coll III和MMP-1 mRNA的表达,并测定COL 1/COL III的比值。结果:UVB显著降低细胞活力,上调MMP-1表达,下调COL I和COL III mRNA表达。AFM处理组MMP-1表达下调,COL I和COL III mRNA表达上调,细胞活力增强。结论:AFM可能通过下调MMP-1,上调COL I和COL III,降低COL I/III比值来改善uvb照射下人成纤维细胞的培养活力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
3.40
自引率
0.00%
发文量
5
审稿时长
14 weeks
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