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冷冻保存后心脏瓣膜的间质细胞和基质修复

Interstitial cellular and matrix restoration of cardiac valves after cryopreservation.

作者信息

Messier R H, Bass B L, Domkowski P W, Hopkins R A

机构信息

Department of Surgery of the Washington, DC, Veterans Affairs Medical Center, Georgetown University Medical Center, Washington, DC, USA.

出版信息

J Thorac Cardiovasc Surg. 1999 Jul;118(1):36-49. doi: 10.1016/S0022-5223(99)70139-X.

Abstract

OBJECTIVES

We previously characterized the porcine aortic leaflet interstitial cell phenotype as having both synthetic and contractile characteristics; that is, it is a myofibroblast. In this study we hypothesized (1) that the cryopreservation of aortic valves causes a significant reduction in cell density, (2) that it simultaneously causes alterations in representative components of extracellular matrix, and (3) that both of these processes are reversible.

METHODS

Seventy-two leaflets from 24 porcine aortic valves were studied. Whole valves were subjected to variable lengths of preharvest ischemia (group 1), ischemia followed by processing analogous to clinical methods (group 2), and ischemia followed processing with an organ culture type of resuscitation (group 3). Vital dye exclusion by cells enzymatically dispersed from leaflets was used to quantify viability. Electron and light microscopy, immunohistochemical assay, and a silicone rubber substratum contractility assay were used both in dispersed cell preparations and in leaflet cross sections to examine structural, ultrastructural, and functional changes across the 3 groups through a range of preharvest ischemic times.

RESULTS

Results indicated that harvest ischemic periods between 2 and 24 hours after donor death were not responsible for cell number reductions. During this interval overt dissolution of chondroitin sulfate simultaneous with a relative sparing of fibronectin was evidenced by immunohistochemical staining. Although not reduced in number, ischemic interstitial cells did show significant ultrastructural evidence of injury and suppressed monoclonal binding to vimentin and alpha-smooth muscle actin. After cryopreservation, viable cell numbers were always markedly reduced at all ischemic intervals and damage to both soluble extracellular matrix components and cell ultrastructure was increased. At all time and processing points, however, some retention of matrix secretory and cellular contractile capabilities was observed among the surviving cells. After the extended periods of preharvest ischemia (2-24 hours) followed by processing, a restitution of functioning cells was accomplished by means of whole-leaflet incubation in 15% fetal bovine serum.

CONCLUSIONS

After application of the described methods, new cells within restored intact leaflets as well as in single-cell preparations demonstrated normal ultrastructure and contractile and synthetic functions (normal phenotypic expression). If functioning leaflet interstitial cells can contribute to homograft durability, bioengineering methods for pretransplantation cell repopulation could be refined with these techniques and applied to clinical valve transplantation.

摘要

目的

我们之前已将猪主动脉瓣小叶间质细胞的表型特征描述为具有合成和收缩特性,即它是一种肌成纤维细胞。在本研究中,我们假设:(1)主动脉瓣的冷冻保存会导致细胞密度显著降低;(2)它同时会引起细胞外基质代表性成分的改变;(3)这两个过程都是可逆的。

方法

对来自24个猪主动脉瓣的72个瓣叶进行了研究。将整个瓣膜进行不同时长的收获前缺血处理(第1组)、缺血后采用类似临床方法进行处理(第2组)以及缺血后采用器官培养类型的复苏处理(第3组)。通过对从瓣叶中酶解分散出的细胞进行活染排斥试验来量化细胞活力。在分散的细胞制剂和瓣叶横切面上,利用电子显微镜和光学显微镜、免疫组织化学分析以及硅橡胶基质收缩试验,通过一系列收获前缺血时间来检查三组之间的结构、超微结构和功能变化。

结果

结果表明,供体死亡后2至24小时的收获缺血期并非导致细胞数量减少的原因。在此期间,免疫组织化学染色显示硫酸软骨素明显溶解,同时纤连蛋白相对保留。尽管缺血间质细胞数量未减少,但确实显示出明显的超微结构损伤证据,且与波形蛋白和α-平滑肌肌动蛋白的单克隆结合受到抑制。冷冻保存后,在所有缺血间隔期,活细胞数量总是显著减少,并且可溶性细胞外基质成分和细胞超微结构的损伤均增加。然而,在所有时间点和处理点,在存活细胞中均观察到一些基质分泌和细胞收缩能力的保留。在收获前长时间缺血(2 - 24小时)后再进行处理,通过将整个瓣叶在15%胎牛血清中孵育实现了功能细胞的恢复。

结论

应用所述方法后,恢复完整的瓣叶内以及单细胞制剂中的新细胞表现出正常的超微结构以及收缩和合成功能(正常的表型表达)。如果有功能的瓣叶间质细胞有助于同种异体移植物的耐久性,那么可利用这些技术改进移植前细胞再填充的生物工程方法,并应用于临床瓣膜移植。

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