Volume 37 Issue 4
Apr.  2021
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Guo Bingyu, Lin Feng, Hui Qiang, et al. Expression and effect of microRNA-627 in human hypertrophic scar[J]. Chin j Burns, 2021, 37(4): 369-376. DOI: 10.3760/cma.j.cn501120-20200225-00090
Citation: Guo Bingyu, Lin Feng, Hui Qiang, et al. Expression and effect of microRNA-627 in human hypertrophic scar[J]. Chin j Burns, 2021, 37(4): 369-376. DOI: 10.3760/cma.j.cn501120-20200225-00090

Expression and effect of microRNA-627 in human hypertrophic scar

doi: 10.3760/cma.j.cn501120-20200225-00090
  • Received Date: 2020-02-25
    Available Online: 2021-10-28
  • Publish Date: 2021-04-20
  • Objective To investigate the expression and effect of microRNA-627 (miR-627) in human hypertrophic scar. Methods The experimental research method was used. From October 2019 to January 2020, hypertrophic scar tissue from 6 patients with hypertrophic scar (2 males and 4 females, aged (34±11) years) and the remaining normal skin tissue from 6 trauma patients (3 males and 3 females, aged (35±13) years) after flap transplantation were collected. The above-mentioned 12 patients were admitted to the General Hospital of Northern Theater Command and met the inclusion criteria. The mRNA expression of miR-627 was detected by real-time fluorescent quantitative reverse transcription polymerase chain reaction. The 3rd to 5th passages of fibroblasts (Fbs) were isolated from hypertrophic scar tissue and cultured for subsequent experiments after identification. Fbs from hypertrophic scar were divided into miR-627 negative control group, miR-627 mimic group, and miR-627 inhibitor group. The corresponding sequences were transfected respectively. At 0 (immediately), 12, 24, 36, and 48 h after transfection, the cell viability was detected by thiazolyl blue method; at 24 h after transfection, the apoptosis was detected by flow cytometry; at 24 h after transfection, the protein expression levels of insulin-like growth factor Ⅰ (IGF-Ⅰ), type Ⅰ collagen, and α smooth muscle actin (α-SMA) were detected by Western blotting. Two batches of Fbs from hypertrophic scar were used, one batch was divided into IGF-Ⅰ wild type+miR-627 negative control group and IGF-Ⅰ wild type+miR-627 mimic group, and the other batch was divided into IGF-Ⅰ mutant+miR-627 negative control group and IGF-Ⅰ mutant+miR-627 mimic group. The corresponding sequences were transfected respectively. At 48 h after transfection, the expressions of luciferase and renal luciferase were detected by luciferase reporter gene detection kit, and the ratio of the two was calculated to reflect the activity of IGF-Ⅰ. Fbs from hypertrophic scar were divided into miR-627 negative control group, miR-627 mimic alone group, and miR-627 mimic+IGF-Ⅰ group, and were transfected with the corresponding sequences respectively. At 24 h after transfection, the protein expression levels of IGF-Ⅰ, type Ⅰ collagen, and α-SMA were detected by Western blotting. The number of samples in cell experiment was 3. Data were statistically analyzed with analysis of variance for factorial design, one-way analysis of variance, independent sample

    t

    test, and chi-square test. Results The expression of miR-627 mRNA in hypertrophic scar tissue was 0.47±0.06, which was significantly lower than 1.12±0.23 in normal skin tissue (

    t

    =15.090,

    P

    <0.01). At 12, 24, 36, and 48 hours after transfection, the cell viability of miR-627 mimic group was significantly lower than that of miR-627 negative control group (

    t

    =9.918, 34.370, 13.580, 61.550,

    P

    <0.05 or

    P

    <0.01); the cell viability of miR-627 inhibitor group was significantly higher than that of miR-627 negative control group (

    t

    =4.722, 8.616, 13.330, 14.000,

    P

    <0.05 or

    P

    <0.01). At 24 h after transfection, compared with the apoptosis rate (8.42±0.47)% in miR-627 negative control group, (10.89±0.35)% in miR-627 mimic group was significantly higher (

    t

    =7.301,

    P

    <0.01), and (5.00±0.22)% in miR-627 inhibitor group was significantly lower (

    t

    =11.510,

    P

    <0.01). At 24 h after transfection, compared with the cell protein expressions of IGF-Ⅰ, type Ⅰ collagen, and α-SMA in miR-627 negative control group, those in miR-627 mimic group were significantly lower (

    t

    =25.470, 5.282, 7.415,

    P

    <0.01), and those in miR-627 inhibitor group were significantly higher (

    t

    =15.930, 8.857, 9.763,

    P

    <0.01). At 48 h after transfection, the luciferase/renal luciferase ratio of IGF-Ⅰ of cells in IGF-Ⅰ wild type+miR-627 mimic group was 0.463±0.061, which was significantly lower than 0.999±0.011 in IGF-Ⅰ wild type+miR-627 negative control group (

    t

    =16.852,

    P

    <0.01); the luciferase/renal luciferase ratio of IGF-Ⅰ of cells in IGF-Ⅰ mutant+miR-627 mimic group was 0.934±0.021, which was similar to 0.930±0.023 in IGF-Ⅰ mutant+miR-627 negative control group (

    t

    =1.959,

    P>

    0.05). At 24 h after transfection, the protein expressions of IGF-Ⅰ, type Ⅰ collagen, and α-SMA of cells in miR-627 mimic alone group were 1.623±0.070, 1.363±0.042, and 1.617±0.025, which were significantly lower than 2.723±0.045, 2.147±0.067, and 2.533±0.055 in miR-627 negative control group (

    t

    =22.831, 7.280, 26.220,

    P

    <0.01); the protein expressions of IGF-Ⅰ, type Ⅰ collagen, and α-SMA of cells in mimic+IGF-Ⅰ group were 2.477±0.102, 1.760±0.046, and 2.387±0.049, which were significantly higher than those of miR-627 mimic alone group (

    t

    =3.830, 8.286, 3.436,

    P

    <0.05 or

    P

    <0.01). Conclusions miR-627 expression in human hypertrophic scars is down-regulated; miR-627 can inhibit the proliferation and promote the apoptosis of Fbs in human hypertrophic scar by targeted inhibition of IGF-Ⅰ expression.

     

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