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三维生物打印抗菌水凝胶对大鼠全层皮肤缺损创面的影响

[Effects of three-dimensional bioprinting antibacterial hydrogel on full-thickness skin defect wounds in rats].

作者信息

Jin R H, Zhang Z Z, Xu P Q, Xia S Z, Weng T T, Zhu Z K, Wang X G, You C G, Han C M

机构信息

Department of Burns and Wound Repair, the Second Affiliated Hospital of Zhejiang University School of Medicine, Zhejiang Key Laboratory for Diagnosis and Treatment of Severe Trauma and Burn, Hangzhou 310009, China.

Department of Burns, First People's Hospital of Hangzhou Xiaoshan District, Xiaoshan 311201, China.

出版信息

Zhonghua Shao Shang Yu Chuang Mian Xiu Fu Za Zhi. 2023 Feb 20;39(2):165-174. doi: 10.3760/cma.j.cn501120-20210809-00274.


DOI:10.3760/cma.j.cn501120-20210809-00274
PMID:36878526
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11630339/
Abstract

To explore the effects of three-dimensional (3D) bioprinting gelatin methacrylamide (GelMA) hydrogel loaded with nano silver on full-thickness skin defect wounds in rats. The experimental research method was adopted. The morphology, particle diameter, and distribution of silver nanoparticles in nano silver solution with different mass concentrations and the pore structure of silver-containing GelMA hydrogel with different final mass fractions of GelMA were observed by scanning electron microscope and the pore size was calculated. On treatment day 1, 3, 7, and 14, the concentration of nano silver released from the hydrogel containing GelMA with final mass fraction of 15% and nano silver with final mass concentration of 10 mg/L was detected by mass spectrometer. At 24 h of culture, the diameters of inhibition zone of GelMA hydrogel containing final mass concentration of 0 (no nano silver), 25, 50, and 100 mg/L nano silver against and were detected. Fibroblasts (Fbs) and adipose stem cells (ASCs) were isolated respectively by enzymatic digestion using the discarded prepuce after circumcision from a 5-year-old healthy boy who was treated in the Department of Urology of the Second Affiliated Hospital of Zhejiang University School of Medicine in July 2020, and the discarded fat tissue after liposuction from a 23-year-old healthy woman who was treated in the Department of Plastic Surgery of the Hospital in July 2020. The Fbs were divided into blank control group (culture medium only), 2 mg/L nano sliver group, 5 mg/L nano sliver group, 10 mg/L nano sliver group, 25 mg/L nano sliver group, and 50 mg/L nano sliver group, which were added with the corresponding final mass concentrations of nano sliver solution, respectively. At 48 h of culture, the Fb proliferation viability was detected by cell counting kit 8 method. The Fbs were divided into 0 mg/L silver-containing GelMA hydrogel group, 10 mg/L silver-containing GelMA hydrogel group, 50 mg/L silver-containing GelMA hydrogel group, and 100 mg/L silver-containing GelMA hydrogel group and then were correspondingly treated. On culture day 1, 3, and 7, the Fb proliferation viability was detected as before. The ASCs were mixed into GelMA hydrogel and divided into 3D bioprinting group and non-printing group. On culture day 1, 3, and 7, the ASC proliferation viability was detected as before and cell growth was observed by live/dead cell fluorescence staining. The sample numbers in the above experiments were all 3. Four full-thickness skin defect wounds were produced on the back of 18 male Sprague-Dawley rats aged 4 to 6 weeks. The wounds were divided into hydrogel alone group, hydrogel/nano sliver group, hydrogel scaffold/nano sliver group, and hydrogel scaffold/nano sliver/ASC group, and transplanted with the corresponding scaffolds, respectively. On post injury day (PID) 4, 7, 14, and 21, the wound healing was observed and the wound healing rate was calculated (=6). On PID 7 and 14, histopathological changes of wounds were observed by hematoxylin eosin staining (=6). On PID 21, collagen deposition of wounds was observed by Masson staining (=3). Data were statistically analyzed with one-way analysis of variance, analysis of variance for repeated measurement, Bonferroni correction, and independent sample test. The sliver nano particles in nano silver solution with different mass concentrations were all round, in scattered distribution and uniform in size. The silver-containing GelMA hydrogels with different final mass fractions of GelMA all showed pore structures of different sizes and interconnections. The pore size of silver-containing GelMA hydrogel with 10% final mass fraction was significantly larger than that of silver-containing GelMA hydrogels with 15% and 20% final mass fractions (with values both below 0.05). On treatment day 1, 3, and 7, the concentration of nano silver released from silver-containing GelMA hydrogel showed a relatively flat trend. On treatment day 14, the concentration of released nano silver in vitro increased rapidly. At 24 h of culture, the diameters of inhibition zone of GelMA hydrogel containing 0, 25, 50, and 100 mg/L nano silver against and were 0, 0, 0.7, and 2.1 mm and 0, 1.4, 3.2, and 3.3 mm, respectively. At 48 h of culture, the proliferation activity of Fbs in 2 mg/L nano silver group and 5 mg/L nano silver group was both significantly higher than that in blank control group (<0.05), and the proliferation activity of Fbs in 10 mg/L nano silver group, 25 mg/L nano silver group, and 50 mg/L nano silver group was all significantly lower than that in blank control group (<0.05). Compared with the that of Fbs in 0 mg/L silver-containing GelMA hydrogel group, the proliferation activity of Fbs in 50 mg/L silver-containing GelMA hydrogel group and 100 mg/L silver-containing GelMA hydrogel group was all significantly decreased on culture day 1 (<0.05); the proliferation activity of Fbs in 50 mg/L silver-containing GelMA hydrogel group was significantly increased (<0.05), while the proliferation activity of Fbs in 100 mg/L silver-containing GelMA hydrogel group was significantly decreased on culture day 3 (<0.05); the proliferation activity of Fbs in 100 mg/L silver-containing GelMA hydrogel group was significantly decreased on culture day 7 (<0.05). The proliferation activity of ASCs in 3D bioprinting group show no statistically significant differences to that in non-printing group on culture day 1 (>0.05). The proliferation activity of ASCs in 3D bioprinting group was significantly higher than that in non-printing group on culture day 3 and 7 (with values of 21.50 and 12.95, respectively, <0.05). On culture day 1, the number of dead ASCs in 3D bioprinting group was slightly more than that in non-printing group. On culture day 3 and 5, the majority of ASCs in 3D bioprinting group and non-printing group were living cells. On PID 4, the wounds of rats in hydrogel alone group and hydrogel/nano sliver group had more exudation, and the wounds of rats in hydrogel scaffold/nano sliver group and hydrogel scaffold/nano sliver/ASC group were dry without obvious signs of infection. On PID 7, there was still a small amount of exudation on the wounds of rats in hydrogel alone group and hydrogel/nano sliver group, while the wounds of rats in hydrogel scaffold/nano sliver group and hydrogel scaffold/nano sliver/ASC group were dry and scabbed. On PID 14, the hydrogels on the wound surface of rats in the four groups all fell off. On PID 21, a small area of wounds remained unhealed in hydrogel alone group. On PID 4 and 7, the wound healing rates of rats in hydrogel scaffold/nano sliver/ASC group were significantly higher than those of the other three groups (<0.05). On PID 14, the wound healing rate of rats in hydrogel scaffold/nano sliver/ASC group was significantly higher than the wound healing rates in hydrogel alone group and hydrogel/nano sliver group (all <0.05). On PID 21, the wound healing rate of rats in hydrogel alone group was significantly lower than that in hydrogel scaffold/nano sliver/ASC group (<0.05). On PID 7, the hydrogels on the wound surface of rats in the four groups remained in place; on PID 14, the hydrogel in hydrogel alone group was separated from the wounds of rats, while some hydrogels still existed in the new tissue of the wounds of rats in the other three groups. On PID 21, the collagen arrangement in the wounds of rats in hydrogel alone group was out of order, while the collagen arrangement in the wounds of rats in hydrogel/nano sliver group, and hydrogel scaffold/nano sliver/ASC group was relatively orderly. Silver-containing GelMA hydrogel has good biocompatibility and antibacterial properties. Its three-dimensional bioprinted double-layer structure can better integrate with new formed tissue in the full-thickness skin defect wounds in rats and promote wound healing.

摘要

探讨三维(3D)生物打印负载纳米银的甲基丙烯酰化明胶(GelMA)水凝胶对大鼠全层皮肤缺损创面的影响。采用实验研究方法。通过扫描电子显微镜观察不同质量浓度纳米银溶液中银纳米颗粒的形态、粒径及分布,以及不同最终质量分数GelMA的含银GelMA水凝胶的孔隙结构,并计算孔径。在治疗第1、3、7和14天,用质谱仪检测最终质量分数为15%的含GelMA水凝胶和最终质量浓度为10 mg/L纳米银的水凝胶中释放的纳米银浓度。在培养24 h时,检测最终质量浓度为0(无纳米银)、25、50和100 mg/L纳米银的GelMA水凝胶对金黄色葡萄球菌和大肠杆菌的抑菌圈直径。分别采用酶消化法从2020年7月在浙江大学医学院附属第二医院泌尿外科接受治疗的1名5岁健康男孩包皮环切术后废弃的包皮,以及2020年7月在该医院整形外科接受治疗的1名23岁健康女性抽脂术后废弃的脂肪组织中分离成纤维细胞(Fbs)和脂肪干细胞(ASCs)。将Fbs分为空白对照组(仅培养基)、2 mg/L纳米银组、5 mg/L纳米银组、10 mg/L纳米银组、25 mg/L纳米银组和50 mg/L纳米银组,分别加入相应最终质量浓度的纳米银溶液。在培养48 h时,采用细胞计数试剂盒8法检测Fb增殖活力。将Fbs分为0 mg/L含银GelMA水凝胶组、10 mg/L含银GelMA水凝胶组、50 mg/L含银GelMA水凝胶组和100 mg/L含银GelMA水凝胶组,然后进行相应处理。在培养第1、3和7天,如前所述检测Fb增殖活力。将ASCs混入GelMA水凝胶中,分为3D生物打印组和非打印组。在培养第1、3和7天,如前所述检测ASC增殖活力,并通过活/死细胞荧光染色观察细胞生长情况。上述实验中的样本数均为3。在18只4至6周龄的雄性Sprague-Dawley大鼠背部制作4个全层皮肤缺损创面。将创面分为单纯水凝胶组、水凝胶/纳米银组、水凝胶支架/纳米银组和水凝胶支架/纳米银/ASC组,分别移植相应支架。在伤后第(PID)4、7、14和21天,观察创面愈合情况并计算创面愈合率(n = 6)。在PID 7和14天,通过苏木精-伊红染色观察创面组织病理学变化(n = 6)。在PID 21天,通过Masson染色观察创面胶原沉积情况(n = 3)。数据采用单因素方差分析、重复测量方差分析、Bonferroni校正和独立样本t检验进行统计学分析。不同质量浓度纳米银溶液中的银纳米颗粒均呈圆形,分布分散且大小均匀。不同最终质量分数GelMA的含银GelMA水凝胶均呈现出不同大小和相互连通的孔隙结构。最终质量分数为10%的含银GelMA水凝胶的孔径显著大于最终质量分数为15%和20%的含银GelMA水凝胶(P值均低于0.05)。在治疗第1、3和7天,含银GelMA水凝胶释放的纳米银浓度呈相对平稳趋势。在治疗第14天,体外释放的纳米银浓度迅速增加。在培养24 h时,含0、25、50和100 mg/L纳米银的GelMA水凝胶对金黄色葡萄球菌的抑菌圈直径分别为0、0、0.7和2.1 mm,对大肠杆菌的抑菌圈直径分别为0、1.4、3.2和3.3 mm。在培养48 h时,2 mg/L纳米银组和5 mg/L纳米银组Fbs的增殖活性均显著高于空白对照组(P < 0.05),10 mg/L纳米银组、25 mg/L纳米银组和50 mg/L纳米银组Fbs的增殖活性均显著低于空白对照组(P < 0.05)。与0 mg/L含银GelMA水凝胶组Fbs相比,50 mg/L含银GelMA水凝胶组和100 mg/L含银GelMA水凝胶组Fbs在培养第1天的增殖活性均显著降低(P < 0.05);50 mg/L含银GelMA水凝胶组Fbs在培养第3天的增殖活性显著升高(P < 0.05),而100 mg/L含银GelMA水凝胶组Fbs在培养第3天的增殖活性显著降低(P < 0.05);100 mg/L含银GelMA水凝胶组Fbs在培养第

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Zhonghua Shao Shang Yu Chuang Mian Xiu Fu Za Zhi. 2022-1-20

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