Objective: To explore the effects and possible molecular mechanism of histone deacetylase 6 (HDAC6) inhibitor Tubastatin A on the proliferation and movement of human skin fibroblasts (HSFs). Methods: The experimental research method was used. HSFs in logarithmic growth phase were taken and divided into negative control group, 1 μmol/L Tubastatin A group, 5 μmol/L Tubastatin A group, and 10 μmol/L Tubastatin A group according to the random number table. The HSFs in negative control group were added with Dulbecco's modified eagle medium with the final volume fraction of 0.1% dimethyl sulfoxide (hereinafter referred to as the complete medium), and the other three groups were added with the complete medium with the corresponding final molarity of Tubastatin A. After 24 h of conventional culture, the cell proliferation activity was detected using cell counting kit 8 (CCK-8) method and 5-ethynyl-2'-deoxyuridine (EdU) staining; the range of motion of cells within 3 h was observed under the living cell workstation, and the curve movement velocity of the cells was calculated. The protein expressions of extracellular signal-regulated kinase 1/2 (ERK1/2) and phosphorylated ERK1/2 (p-ERK1/2) were detected by Western blotting, and the ratio of p-ERK1/2 to ERK1/2 was calculated to represent the activity of ERK1/2. The sample number in cell proliferation activity detection with CCK-8 method was 6, while the sample numbers in other experiments were 3. Data were statistically analyzed with one-way analysis of variance and least significant difference test. Results: After 24 h of culture, CCK-8 method and EdU staining showed that compared with negative control group, the cell proliferation activities in 1 μmol/L Tubastatin A group, 5 μmol/L Tubastatin A group, and 10 μmol/L Tubastatin A group were significantly decreased (P<0.01). After 24 h of culture, CCK-8 method showed that compared with 1 μmol/L Tubastatin A group, the cell proliferation activity in 10 μmol/L Tubastatin A group was significantly decreased (P<0.05); EdU staining showed that compared with 1 μmol/L Tubastatin A group, the cell proliferation activities in 5 μmol/L Tubastatin A group and 10 μmol/L Tubastatin A group were significantly decreased (P<0.05 or P<0.01). Within 3 h of observation, the ranges of cell motion in 1 μmol/L Tubastatin A group, 5 μmol/L Tubastatin A group, and 10 μmol/L Tubastatin A group were obviously reduced compared with that in negative control group. Within 3 h of observation, the curve movement velocity of cells in negative control group was (0.780±0.028) μm/min, which was obviously faster than (0.594±0.023), (0.469±0.028), and (0.391±0.021) μm/min of 1 μmol/L Tubastatin A group, 5 μmol/L Tubastatin A group, and 10 μmol/L Tubastatin A group (P<0.01); the curve movement velocity of cells in 1 μmol/L Tubastatin A group was obviously faster than those in 5 μmol/L Tubastatin A group and 10 μmol/L Tubastatin A group (P<0.01); the curve movement velocity of cells in 5 μmol/L Tubastatin A group was obviously faster than that in 10 μmol/L Tubastatin A group (P<0.05). After 24 h of culture, compared with negative control group, the activities of ERK1/2 of cells in 1 μmol/L Tubastatin A group, 5 μmol/L Tubastatin A group, and 10 μmol/L Tubastatin A group were decreased significantly (P<0.01); compared with 1 μmol/L Tubastatin A group, the activities of ERK1/2 of cells in 5 μmol/L Tubastatin A group and 10 μmol/L Tubastatin A group were decreased significantly (P<0.01); compared with 5 μmol/L Tubastatin A group, the activity of ERK1/2 of cells in 10 μmol/L Tubastatin A group was decreased significantly (P<0.05). Conclusions: HDAC6 inhibitor Tubastatin A may mediate the inhibitory effect on proliferation and movement of HSFs by inhibiting the activity of ERK1/2.
目的: 探讨组蛋白脱乙酰酶6(HDAC6)抑制剂Tubastatin A对人皮肤成纤维细胞(HSF)增殖及运动性的影响及其可能的分子机制。 方法: 采用实验研究方法。取对数生长期HSF,按随机数字表法分为阴性对照组及1 μmol/L Tubastatin A组、5 μmol/L Tubastatin A组、10 μmol/L Tubastatin A组。阴性对照组加入含终体积分数0.1%二甲基亚砜的DMEM培养液(以下简称完全培养液),其余3组分别加入含相应终物质的量浓度Tubastatin A的完全培养液。常规培养24 h后,采用细胞计数试剂盒8(CCK-8)法和5-乙炔基-2'-脱氧尿嘧啶核苷(EdU)染色检测细胞增殖活力;在活细胞工作站下观察细胞3 h内运动范围,计算细胞曲线运动速度;采用蛋白质印迹法检测胞外信号调节激酶1/2(ERK1/2)及磷酸化ERK1/2(p-ERK1/2)的蛋白表达量,并计算p-ERK1/2与ERK1/2比值,以此表示ERK1/2活性。CCK-8法行细胞增殖活力检测样本数为6,其余实验样本数为3。对数据行单因素方差分析及LSD检验。 结果: 培养24 h后,CCK-8法和EdU染色显示,与阴性对照组比较,1 μmol/L Tubastatin A组、5 μmol/L Tubastatin A组、10 μmol/L Tubastatin A组细胞增殖活力均显著下降(P<0.01)。培养24 h后,CCK-8法显示,与1 μmol/L Tubastatin A组比较,10 μmol/L Tubastatin A组细胞增殖活力显著下降(P<0.05);EdU染色显示,与1 μmol/L Tubastatin A组比较,5 μmol/L Tubastatin A组、10 μmol/L Tubastatin A组细胞增殖活力显著下降(P<0.05或P<0.01)。观察3 h内,1 μmol/L Tubastatin A组、5 μmol/L Tubastatin A组、10 μmol/L Tubastatin A组细胞运动范围较阴性对照组明显缩小。观察3 h内,阴性对照组细胞曲线运动速度为(0.780±0.028)μm/min,明显快于1 μmol/L Tubastatin A组、5 μmol/L Tubastatin A组、10 μmol/L Tubastatin A组细胞的(0.594±0.023)、(0.469±0.028)、(0.391±0.021)μm/min(P<0.01);1 μmol/L Tubastatin A组细胞曲线运动速度明显快于5 μmol/L Tubastatin A组和10 μmol/L Tubastatin A组(P<0.01);5 μmol/L Tubastatin A组细胞曲线运动速度明显快于10 μmol/L Tubastatin A组(P<0.05)。培养24 h后,与阴性对照组比较,1 μmol/L Tubastatin A组、5 μmol/L Tubastatin A组、10 μmol/L Tubastatin A组细胞ERK1/2的活性显著下降(P<0.01);与1 μmol/L Tubastatin A组比,5 μmol/L Tubastatin A组和10 μmol/L Tubastatin A组细胞ERK1/2的活性显著下降(P<0.01);与5 μmol/L Tubastatin A组比较,10 μmol/L Tubastatin A组细胞ERK1/2的活性显著下降(P<0.05)。 结论: HDAC6抑制剂Tubastatin A可能通过抑制ERK1/2活性,从而抑制HSF增殖及运动。.