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[氧化铈纳米酶-甲基丙烯酸酐明胶水凝胶对小鼠感染性全层皮肤缺损创面修复的影响]

[Effects of cerium oxide nanoenzyme-gelatin methacrylate anhydride hydrogel in the repair of infected full-thickness skin defect wounds in mice].

作者信息

Gu Y N, Xu X H, Wang Y P, Li Y T, Liang Z, Yu Z, Peng Y Z, Song B Q

机构信息

Xi'an Medical University, Xi'an 710021, China.

Department of Plastic Surgery, the First Affiliated Hospital, Air Force Medical University, Xi'an 710032, China.

出版信息

Zhonghua Shao Shang Yu Chuang Mian Xiu Fu Za Zhi. 2024 Feb 20;40(2):131-140. doi: 10.3760/cma.j.cn501225-20231120-00201.

DOI:10.3760/cma.j.cn501225-20231120-00201
PMID:38418174
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11630467/
Abstract

To investigate the effects of cerium oxide nanoenzyme-gelatin methacrylate anhydride (GelMA) hydrogel (hereinafter referred to as composite hydrogel) in the repair of infected full-thickness skin defect wounds in mice. This study was an experimental study. Cerium oxide nanoenzyme with a particle size of (116±9) nm was prepared by hydrothermal method, and GelMA hydrogel with porous network structure and good gelling performance was also prepared. The 25 μg/mL cerium oxide nanoenzyme which could significantly promote the proliferation of human skin fibroblasts and had high superoxide dismutase activity was screened out. It was added to GelMA hydrogel to prepare composite hydrogel. The percentage of cerium oxide nanoenzyme released from the composite hydrogel was calculated after immersing it in phosphate buffer solution (PBS) for 3 and 7 d. The red blood cell suspension of mice was divided into PBS group, Triton X-100 group, cerium oxide nanoenzyme group, GelMA hydrogel group, and composite hydrogel group, which were treated with corresponding solution. The hemolysis of red blood cells was detected by microplate reader after 1 h of treatment. The bacterial concentrations of methicillin-resistant (MRSA) and were determined after being cultured with PBS, cerium oxide nanoenzyme, GelMA hydrogel, and composite hydrogel for 2 h. The sample size in all above experiments was 3. Twenty-four 8-week-old male BALB/c mice were taken, and a full-thickness skin defect wound was prepared in the symmetrical position on the back and infected with MRSA. The mice were divided into control group without any drug intervention, and cerium oxide nanoenzyme group, GelMA hydrogel group, and composite hydrogel group applied with corresponding solution, with 6 mice in each group. The wound healing was observed on 3, 7, and 14 d after injury, and the remaining wound areas on 3 and 7 d after injury were measured (the sample size was 5). The concentration of MRSA in the wound exudation of mice on 3 d after injury was measured (the sample size was 3), and the blood flow perfusion in the wound of mice on 5 d after injury was observed using a laser speckle flow imaging system (the sample size was 6). On 14 d after injury, the wound tissue of mice was collected for hematoxylin-eosin staining to observe the newly formed epithelium and for Masson staining to observe the collagen situation (the sample size was both 3). After immersion for 3 and 7 d, the release percentages of cerium oxide nanoenzyme in the composite hydrogel were about 39% and 75%, respectively. After 1 h of treatment, compared with that in Triton X-100 group, the hemolysis of red blood cells in PBS group, GelMA hydrogel group, cerium oxide nanoenzyme group, and composite hydrogel group was significantly decreased (<0.05). Compared with that cultured with PBS, the concentrations of MRSA and cultured with cerium oxide nanoenzyme, GelMA hydrogel, and composite hydrogel for 2 h were significantly decreased (<0.05). The wounds of mice in the four groups were gradually healed from 3 to 14 d after injury, and the wounds of mice in composite hydrogel group were all healed on 14 d after injury. On 3 and 7 d after injury, the remaining wound areas of mice in composite hydrogel group were (29±3) and (13±5) mm, respectively, which were significantly smaller than (56±12) and (46±10) mm in control group and (51±7) and (38±8) mm in cerium oxide nanoenzyme group (with values all <0.05), but was similar to (41±5) and (24±9) mm in GelMA hydrogel group (with values both >0.05). On 3 d after injury, the concentration of MRSA on the wound of mice in composite hydrogel group was significantly lower than that in control group, cerium oxide nanoenzyme group, and GelMA hydrogel group, respectively (with values all <0.05). On 5 d after injury, the volume of blood perfusion in the wound of mice in composite hydrogel group was significantly higher than that in control group, cerium oxide nanoenzyme group, and GelMA hydrogel group, respectively (<0.05). On 14 d after injury, the wound of mice in composite hydrogel group basically completed epithelization, and the epithelization was significantly better than that in the other three groups. Compared with that in the other three groups, the content of collagen in the wound of mice in composite hydrogel group was significantly increased, and the arrangement was also more orderly. The composite hydrogel has good biocompatibility and antibacterial effect and . It can continuously sustained release cerium oxide nanoenzyme, improve wound blood perfusion in the early stage, and promote wound re-epithelialization and collagen synthesis, therefore promoting the healing of infected full-thickness skin defect wounds in mice.

摘要

为研究氧化铈纳米酶 - 甲基丙烯酸酐明胶(GelMA)水凝胶(以下简称复合水凝胶)对小鼠感染性全层皮肤缺损创面的修复作用。本研究为实验性研究。采用水热法制备粒径为(116±9)nm的氧化铈纳米酶,同时制备具有多孔网络结构且凝胶性能良好的GelMA水凝胶。筛选出能显著促进人皮肤成纤维细胞增殖且具有高超氧化物歧化酶活性的25μg/mL氧化铈纳米酶,将其添加到GelMA水凝胶中制备复合水凝胶。将复合水凝胶浸泡于磷酸盐缓冲液(PBS)中3天和7天后,计算氧化铈纳米酶从复合水凝胶中的释放百分比。将小鼠红细胞悬液分为PBS组、Triton X - 100组、氧化铈纳米酶组、GelMA水凝胶组和复合水凝胶组,分别用相应溶液处理。处理1小时后,用酶标仪检测红细胞溶血情况。将耐甲氧西林金黄色葡萄球菌(MRSA)与PBS、氧化铈纳米酶、GelMA水凝胶和复合水凝胶共培养2小时后,测定其细菌浓度值。上述所有实验的样本量均为3。取24只8周龄雄性BALB/c小鼠,在背部对称位置制备全层皮肤缺损创面并感染MRSA。将小鼠分为无任何药物干预的对照组,以及分别涂抹相应溶液的氧化铈纳米酶组、GelMA水凝胶组和复合水凝胶组,每组6只。在损伤后3天、7天和14天观察伤口愈合情况,并测量损伤后3天和7天的剩余伤口面积(样本量为5)。测定损伤后3天小鼠伤口渗出液中MRSA的浓度(样本量为3),并使用激光散斑血流成像系统观察损伤后5天小鼠伤口的血流灌注情况(样本量为6)。在损伤后14天,收集小鼠伤口组织进行苏木精 - 伊红染色以观察新形成的上皮组织,进行Masson染色以观察胶原情况(样本量均为3)。浸泡3天和7天后,复合水凝胶中氧化铈纳米酶的释放百分比分别约为39%和75%。处理1小时后,与Triton X - 100组相比,PBS组、GelMA水凝胶组、氧化铈纳米酶组和复合水凝胶组的红细胞溶血率显著降低(P<0.05)。与用PBS培养相比,用氧化铈纳米酶、GelMA水凝胶和复合水凝胶培养2小时后的MRSA浓度显著降低(P<0.05)。四组小鼠的伤口在损伤后3天至14天逐渐愈合,复合水凝胶组小鼠的伤口在损伤后14天全部愈合。在损伤后3天和7天,复合水凝胶组小鼠的剩余伤口面积分别为(29±3)和(13±5)mm,显著小于对照组的(56±12)和(46±10)mm以及氧化铈纳米酶组的(51±7)和(38±8)mm(P值均<0.05),但与GelMA水凝胶组的(41±5)和(24±9)mm相似(P值均>0.05)。在损伤后3天,复合水凝胶组小鼠伤口处的MRSA浓度分别显著低于对照组、氧化铈纳米酶组和GelMA水凝胶组(P值均<0.05)。在损伤后5天,复合水凝胶组小鼠伤口的血流灌注量分别显著高于对照组、氧化铈纳米酶组和GelMA水凝胶组(P<0.05)。在损伤后14天,复合水凝胶组小鼠的伤口基本完成上皮化,且上皮化程度显著优于其他三组。与其他三组相比,复合水凝胶组小鼠伤口中的胶原含量显著增加,且排列也更有序。复合水凝胶具有良好的生物相容性和抗菌作用,它能持续缓释氧化铈纳米酶,在早期改善伤口血流灌注,促进伤口再上皮化和胶原合成,从而促进小鼠感染性全层皮肤缺损创面的愈合。

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