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阿魏酸钠对人皮肤增生性瘢痕成纤维细胞增殖与凋亡的调控作用及信号机制

[Regulatory effects and signaling mechanism of sodium ferulate on the proliferation and apoptosis of human skin hypertrophic scar fibroblasts].

作者信息

Wang C, Chen W, Wang B J

机构信息

School of Basic Medicine, Chengdu University of Traditional Chinese Medicine, Chengdu 611137, China.

Internet Connections College of Education, Southwest Jiaotong University, Chengdu 610031, China.

出版信息

Zhonghua Shao Shang Yu Chuang Mian Xiu Fu Za Zhi. 2022 May 20;38(5):471-480. doi: 10.3760/cma.j.cn501120-20201120-00484.

DOI:10.3760/cma.j.cn501120-20201120-00484
PMID:35599423
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11705276/
Abstract

To investigate the regulatory effects and signaling mechanism of sodium ferulate on the proliferation and apoptosis of human skin hypertrophic scar fibroblasts (HSFbs). The experimental research methods were used. The 4-6 passage of HSFbs from human skin were used for the following experiments. HSFbs were co-cultured with sodium ferulate at final mass concentrations of 1, 1×10, 1×10, 1×10, 1×10, 1×10, and 1×10 mg/mL for 48 hours, and methyl thiazolyl tetrazolium method was used to determine the cell absorbance values and linear regression was used to analyze the half lethal concentration (LC50) of sodium ferulate (=6). HSFbs were co-cultured with sodium ferulate at final mass concentrations of 0.1, 0.2, 0.3, and 0.4 mg/mL for 24, 48, 72, and 96 hours, and methyl thiazolyl tetrazolium method was used to determine the cell absorbance values and the cell proliferation inhibition rate was calculated (=3). According to the random number table, the cells were divided into 0.300 mg/mL sodium ferulate group, 0.030 mg/mL sodium ferulate group, 0.003 mg/mL sodium ferulate group treated with sodium ferulate at corresponding final mass concentrations, and negative control group without any treatment. After 72 hours of culture, the cell absorbance values were determined by methyl thiazolyl tetrazolium method (=5), the microscopic morphology of cells was observed by transmission electron microscope (=3), the cell apoptosis was detected by TdT-mediated dUTP-biotin nick end labeling (TUNEL) assay and the apoptosis index was calculated (=4), the protein expressions of B lymphocystoma-2 (Bcl-2), Bcl-2-associated X protein (Bax), and cysteine aspartic acid specific protease-3 (caspase-3) were determined by immunohistochemistry (=4), and the protein expressions of transformed growth factor β (TGF-β), phosphorylated Smad2/3, phosphorylated Smad4, and phosphorylated Smad7 were detected by Western blotting (=4). Data were statistically analyzed with one-way analysis of variance and Dunnett test. The LC50 of sodium ferulate was 0.307 5 mg/mL. After being cultured for 24-96 hours, the cell proliferation inhibition rates of cells treated with sodium ferulate at four different mass concentrations tended to increase at first but decrease later, which reached the highest after 72 hours of culture, so 72 hours was chosen as the processing time for the subsequent experiments. After 72 hours of culture, the cell absorbance values in 0.003 mg/mL sodium ferulate group, 0.030 mg/mL sodium ferulate group, and 0.300 mg/mL sodium ferulate group were 0.57±0.06, 0.53±0.04, 0.45±0.05, respectively, which were significantly lower than 0.69±0.06 in negative control group <0.01). After 72 hours of culture, compared with those in negative control group, the cells in the three groups treated with sodium ferulate showed varying degrees of nuclear pyknosis, fracture, or lysis, and chromatin loss. In the cytoplasm, mitochondria were swollen, the rough endoplasmic reticulum was expanded, and local vacuolation gradually appeared. After 72 hours of culture, compared with that in negative control group, the apoptosis indexes of cells were increased significantly in 0.003 mg/mL sodium ferulate group, 0.030 mg/mL sodium ferulate group, and 0.300 mg/mL sodium ferulate group (<0.05 or <0.01). After 72 hours of culture, compared with those in negative control group, the protein expressions of Bcl-2 of cells in 0.300 mg/mL sodium ferulate group was significantly decreased (<0.01), the protein expressions of Bax of cells in 0.030 mg/mL sodium ferulate group and 0.300 mg/mL sodium ferulate group were significantly increased (<0.05), and the protein expression of caspase-3 of cells in 0.300 mg/mL sodium ferulate group was significantly increased (<0.01). After 72 hours of culture, compared with those in negative control group, the protein expression levels of TGF-β, phosphorylated Smad2/3, and phosphorylated Smad4 of cells in 0.030 mg/mL sodium ferulate group and 0.300 mg/mL sodium ferulate group were significantly decreased (<0.05 or <0.01), and the protein expression levels of phosphorylated Smad7 of cells in 0.003 mg/mL sodium ferulate group, 0.030 mg/mL sodium ferulate group, and 0.300 mg/mL sodium ferulate group were significantly increased (<0.01). Sodium ferulate can inhibit the proliferation of HSFbs of human skin and promote the apoptosis of HSFbs of human skin by blocking the expression of key proteins on the TGF-β/Smad signaling pathway and synergistically activating the mitochon- drial apoptosis pathway.

摘要

探讨阿魏酸钠对人皮肤增生性瘢痕成纤维细胞(HSFbs)增殖和凋亡的调控作用及信号机制。采用实验研究方法。取人皮肤来源的4 - 6代HSFbs进行以下实验。将HSFbs与终质量浓度分别为1、1×10、1×10、1×10、1×10、1×10和1×10 mg/mL的阿魏酸钠共培养48小时,采用甲基噻唑基四氮唑法测定细胞吸光度值,并通过线性回归分析阿魏酸钠的半数致死浓度(LC50)(=6)。将HSFbs与终质量浓度为0.1、0.2、0.3和0.4 mg/mL的阿魏酸钠共培养24、48、72和96小时,采用甲基噻唑基四氮唑法测定细胞吸光度值并计算细胞增殖抑制率(=3)。根据随机数字表,将细胞分为分别用相应终质量浓度阿魏酸钠处理的0.300 mg/mL阿魏酸钠组、0.030 mg/mL阿魏酸钠组、0.003 mg/mL阿魏酸钠组,以及未作任何处理的阴性对照组。培养72小时后,采用甲基噻唑基四氮唑法测定细胞吸光度值(=5),用透射电子显微镜观察细胞微观形态(=3),采用TdT介导的dUTP - 生物素缺口末端标记法(TUNEL)检测细胞凋亡并计算凋亡指数(=4),用免疫组织化学法检测B淋巴细胞瘤 - 2(Bcl - 2)、Bcl - 2相关X蛋白(Bax)和半胱氨酸天冬氨酸特异性蛋白酶 - 3(caspase - 3)的蛋白表达(=4),用蛋白质印迹法检测转化生长因子β(TGF - β)、磷酸化Smad2/3、磷酸化Smad4和磷酸化Smad7的蛋白表达(=4)。数据采用单因素方差分析和Dunnett检验进行统计学分析。阿魏酸钠的LC50为0.307 5 mg/mL。在培养24 - 96小时后,用四种不同质量浓度阿魏酸钠处理的细胞的细胞增殖抑制率起初呈上升趋势,但随后下降,在培养72小时时达到最高,因此选择72小时作为后续实验的处理时间。培养72小时后,0.003 mg/mL阿魏酸钠组、0.030 mg/mL阿魏酸钠组和0.300 mg/mL阿魏酸钠组的细胞吸光度值分别为0.57±0.06、0.53±0.04、0.45±0.05,均显著低于阴性对照组的0.69±0.06(<0.01)。培养72小时后,与阴性对照组相比,用阿魏酸钠处理的三组细胞均出现不同程度的核固缩、断裂或溶解,以及染色质丢失。在细胞质中,线粒体肿胀,粗面内质网扩张,局部逐渐出现空泡化。培养72小时后,与阴性对照组相比,0.003 mg/mL阿魏酸钠组、0.030 mg/mL阿魏酸钠组和0.300 mg/mL阿魏酸钠组的细胞凋亡指数显著升高(<0.05或<0.01)。培养72小时后,与阴性对照组相比,0.300 mg/mL阿魏酸钠组细胞的Bcl - 2蛋白表达显著降低(<0.01),0.030 mg/mL阿魏酸钠组和0.300 mg/mL阿魏酸钠组细胞的Bax蛋白表达显著升高(<0.05),0.300 mg/mL阿魏酸钠组细胞的caspase - 3蛋白表达显著升高(<0.01)。培养72小时后,与阴性对照组相比,0.030 mg/mL阿魏酸钠组和0.300 mg/mL阿魏酸钠组细胞的TGF - β、磷酸化Smad2/3和磷酸化Smad4蛋白表达水平显著降低(<0.05或<0.01),0.003 mg/mL阿魏酸钠组、0.030 mg/mL阿魏酸钠组和0.300 mg/mL阿魏酸钠组细胞的磷酸化Smad7蛋白表达水平显著升高(<0.01)。阿魏酸钠可通过阻断TGF - β/Smad信号通路关键蛋白的表达并协同激活线粒体凋亡通路,抑制人皮肤HSFbs的增殖并促进其凋亡。