Kolster Moritz, Wilhelmi Mathias, Schrimpf Claudia, Hilfiker Andres, Haverich Axel, Aper Thomas
Division of Vascular and Endovascular Surgery, Department of Cardiothoracic, Transplantation and Vascular Surgery, Hannover Medical School, Hannover, Germany.
J Tissue Eng. 2017 Mar 15;8:2041731417698852. doi: 10.1177/2041731417698852. eCollection 2017 Jan-Dec.
In recent years, circulating progenitors of endothelial cells and smooth muscle cells were identified in the peripheral blood. In our study, we evaluated the utilization of both cell types isolated and differentiated from peripheral porcine blood in terms for their use for tissue engineering purposes. By means of density gradient centrifugation, the monocyte fraction from porcine blood was separated, split, and cultivated with specific culture media with either endothelial cell growth medium-2 or smooth muscle cell growth medium-2 for the differentiation of endothelial cells or smooth muscle cells. Obtained cells were characterized at an early stage of cultivation before the first passage and a late stage (fourth passage) on the basis of the expression of the antigens CD31, CD34, CD45, nitric oxide synthase, and the contractile filaments smooth-muscle alpha-actin (sm-alpha-actin) and smoothelin. Functional characterization was done based on the secretion of nitric oxide, the formation of a coherent monolayer on polytetrafluoroethylene, and capillary sprouting. During cultivation in both endothelial cell growth medium-2 and smooth muscle cell growth medium-2, substantially two types of cells grew out: early outgrown CD45-positive cells, which disappeared during further cultivation, and in 85% (n = 17/20) of cultures cultivated with endothelial cell growth medium-2 colony-forming late outgrowth endothelial cells. During cultivation with smooth muscle cell growth medium-2 in 80% (n = 16/20) of isolations colony-forming late outgrowth smooth muscle cells entered the stage. Cultivation with either endothelial cell growth medium-2 or smooth muscle cell growth medium-2 had selective effect on the late outgrown cells to that effect that the number of CD31-positive cells increased from 34.8% ± 13% to 83.9% ± 8% in cultures cultivated with endothelial cell growth medium-2 and the number of sm-α-actin+ cells increased from 52.6% ± 18% to 88% ± 5% in cultures cultivated with smooth muscle cell growth medium-2, respectively. Functional analyses revealed significantly higher levels of nitric oxide secretion, endothelialization capacity, and capillary formation in not expanded cultures cultivated with endothelial cell growth medium-2 in comparison to later stages of cultivation and mature aortic cells. Blood seems to be a reliable and feasible source for the isolation of both endothelial and smooth muscle cells for application in tissue engineering approaches. Whereas, early co-cultures of early and late outgrowth cells provide functional advantages, the differentiation of cells can be directed selectively by the used culture medium for the expansion of highly proliferative late outgrowth endothelial cells and late outgrowth smooth muscle cells, respectively.
近年来,在外周血中发现了内皮细胞和平滑肌细胞的循环祖细胞。在我们的研究中,我们评估了从猪外周血中分离和分化出的这两种细胞类型在组织工程中的应用。通过密度梯度离心法,分离出猪血液中的单核细胞部分,进行分割,并使用含有内皮细胞生长培养基-2或平滑肌细胞生长培养基-2的特定培养基进行培养,以分化出内皮细胞或平滑肌细胞。在首次传代前的培养早期阶段和后期(第四代),根据抗原CD31、CD34、CD45、一氧化氮合酶以及收缩丝平滑肌α-肌动蛋白(sm-α-肌动蛋白)和平滑肌肌动蛋白的表达对获得的细胞进行表征。基于一氧化氮的分泌、在聚四氟乙烯上形成连贯单层以及毛细血管形成进行功能表征。在用内皮细胞生长培养基-2和平滑肌细胞生长培养基-2培养期间,基本上长出了两种类型的细胞:早期长出的CD45阳性细胞,在进一步培养过程中消失,在用内皮细胞生长培养基-2培养的85%(n = 17/20)的培养物中,形成集落的晚期长出的内皮细胞。在用平滑肌细胞生长培养基-2培养期间,在80%(n = 16/20)的分离物中,形成集落的晚期长出的平滑肌细胞进入该阶段。用内皮细胞生长培养基-2或平滑肌细胞生长培养基-2培养对晚期长出的细胞有选择性作用,以至于在用内皮细胞生长培养基-2培养的培养物中,CD31阳性细胞的数量从34.8%±13%增加到83.9%±8%,在用平滑肌细胞生长培养基-2培养的培养物中,sm-α-肌动蛋白阳性细胞的数量从52.6%±18%增加到88%±5%。功能分析显示,与培养后期和成熟主动脉细胞相比,在用内皮细胞生长培养基-2培养的未扩增培养物中,一氧化氮分泌水平、内皮化能力和毛细血管形成明显更高。血液似乎是用于组织工程方法的内皮细胞和平滑肌细胞分离的可靠且可行的来源。虽然早期和晚期长出细胞的早期共培养具有功能优势,但可以通过使用的培养基分别选择性地引导细胞分化,以扩增高度增殖的晚期长出的内皮细胞和晚期长出的平滑肌细胞。
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