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Acellular Bi-Layer Silk Fibroin Scaffolds Support Functional Tissue Regeneration in a Rat Model of Onlay Esophagoplasty

机译:脱细胞双层丝素蛋白支架支持上皮食管成形术大鼠模型中的功能组织再生。

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摘要

Surgical management of long-gap esophageal defects with autologous gastrointestinal tissues is frequently associated with adverse complications including organ dysmotility, dysphagia, and donor site morbidity. In order to develop alternative graft options, bi-layer silk fibroin (SF) scaffolds were investigated for their potential to support functional tissue regeneration in a rodent model of esophageal repair. Onlay esophagoplasty was performed with SF matrices (N=40) in adult rats for up to 2 m of implantation. Parallel groups consisted of animals implanted with small intestinal submucosa (SIS) scaffolds (N=22) or sham controls receiving esophagotomy alone (N=20). Sham controls exhibited a 100% survival rate while rats implanted with SF and SIS scaffolds displayed respective survival rates of 93% and 91% prior to scheduled euthanasia. Animals in each experimental group were capable of solid food consumption following a 3 d post-op liquid diet and demonstrated similar degrees of weight gain throughout the study period. End-point μ-computed tomography at 2 m post-op revealed no evidence of contrast extravasation, fistulas, strictures, or diverticula in any of the implant groups. Ex vivo tissue bath studies demonstrated that reconstructed esophageal conduits supported by both SF and SIS scaffolds displayed contractile responses to carbachol, KCl and electrical field stimulation while isoproterenol produced tissue relaxation. Histological (Masson’s trichrome and hematoxylin and eosin) and immunohistochemical (IHC) evaluations demonstrated both implant groups produced de novo formation of skeletal and smooth muscle bundles positive for contractile protein expression [fast myosin heavy chain (MY32) and α-smooth muscle actin (α-SMA)] within the graft site. However, SF matrices promoted a significant 4-fold increase in MY32+ skeletal muscle and a 2-fold gain in α-SMA+ smooth muscle in comparison to the SIS cohort as determined by histomorphometric analyses. A stratified squamous, keratinized epithelium expressing cytokeratin 5 and involucrin proteins was also present at 2 m post-op in all experimental groups. De novo innervation and vascularization were evident in all regenerated tissues indicated by the presence of synaptophysin (SYP38)+ boutons and vessels lined with CD31 expressing endothelial cells. In respect to SIS, the SF group supported a significant 4-fold increase in the density of SYP38+ boutons within the implant region. Evaluation of host tissue responses revealed that SIS matrices elicited chronic inflammatory reactions and severe fibrosis throughout the neotissues, in contrast to SF scaffolds. The results of this study demonstrate that bi-layer SF scaffolds represent promising biomaterials for onlay esophagoplasty, capable of producing superior regenerative outcomes in comparison to conventional SIS scaffolds.
机译:具有自体胃肠道组织的长距离食管缺损的外科治疗通常与不良并发症相关,包括器官运动障碍,吞咽困难和供体部位发病。为了开发替代的移植选择,研究了双层丝素蛋白(SF)支架在食管修复啮齿动物模型中支持功能组织再生的潜力。在成年大鼠中用SF基质(N = 40)进行食管内成形术,植入时间最长为2 m。平行组由植入小肠粘膜下层(SIS)支架(N = 22)或仅接受食管切开术(N = 20)的假对照组组成的动物组成。假手术对照组的存活率为100%,而植入SF和SIS支架的大鼠在计划安乐死之前的存活率分别为93%和91%。每个实验组中的动物在术后3天流食后能够摄取固体食物,并且在整个研究期间显示出相似的体重增加程度。术后2 m进行终点μ计算机断层扫描,未发现任何植入物组存在造影剂外渗,瘘管,狭窄或憩室的证据。体外组织浸浴研究表明,由SF和SIS支架支撑的重建食管导管显示出对卡巴胆碱,KCl和电场刺激的收缩反应,而异丙肾上腺素则使组织松弛。组织学(Masson's trichrome,苏木精和曙红)和免疫组化(IHC)评估表明,两个植入物组均产生从头形成的骨骼肌和平滑肌束,对收缩蛋白表达呈阳性[快速肌球蛋白重链(MY32)和α-平滑肌肌动蛋白(α -SMA)]。然而,与组织形态分析相比,与SIS队列相比,SF矩阵促进MY32 +骨骼肌明显增加4倍,而α-SMA+平滑肌增加2倍。在所有实验组中,术后2 m均出现分层的鳞状上皮,角化上皮细胞角蛋白5和囊蛋白。从头开始神经支配和血管形成在所有再生组织中均明显存在,这表明存在突触素(SYP38)+钮扣和衬有CD31表达内皮细胞的血管。关于SIS,SF组支持植入区域内SYP38 +按键的密度显着增加4倍。对宿主组织反应的评估表明,与SF支架相反,SIS基质在整个新组织中引起了慢性炎症反应和严重的纤维化。这项研究的结果表明,双层SF支架代表有前途的食管成形术的有前途的生物材料,与常规SIS支架相比,能够产生优异的再生效果。

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