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Intact microglia are cultured and non-invasively harvested without pathological activation using a novel cultured cell recovery method.

机译:培养完整的小胶质细胞,并使用新型培养的细胞回收方法进行非病理性激活,无需病理激活。

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摘要

Because spontaneous host regeneration of damaged tissues is limited, novel therapeutics utilizing cultured cells with the aid of tissue engineering methods are promising alternatives for tissue replacement. One critical shortcoming is current requirement for invasive cell harvest from culture to fabricate cell-based devices. Although microglia that secrete neurotrophic factors are attractive candidates for novel cell transplantation therapy for damaged central nervous system tissue, the intact harvest of cultured microglia is presently not achievable. Therefore, primary microglia were plated onto culture surfaces grafted with the temperature-responsive polymer, poly(N-isopropylacrylamide) (PIPAAm). This surface undergoes rapid, reversible temperature-dependent changes in its hydration state and surface hydrophilicity. Microglia attached and proliferated on PIPAAm-grafted dishes at 37 degrees C. By reducing culture temperature, more than 90% of the cells spontaneously detached from the dishes within several minutes without trypsin or EDTA treatment. Recovered and replated microglia exhibited phenotypic properties comparable to those of primary microglia freshly isolated from brain. By contrast, less than 60% of the cells were harvested by trypsin digestion, and exhibited significant alteration of characteristic cellular properties as monitored by pathological states in vivo. This new technology exhibits utility for the preparation of cell sources required for cell transplantation as well as microglial function analysis.
机译:由于受损组织的自发宿主再生受到限制,因此在组织工程方法的帮助下利用培养细胞的新型治疗方法有望成为组织替代的替代方法。一个关键的缺点是当前需要从培养到制造基于细胞的装置进行侵入性细胞收获。尽管分泌神经营养因子的小胶质细胞是用于受损中枢神经系统组织的新型细胞移植治疗的诱人候选物,但目前仍无法完整培养培养的小胶质细胞。因此,将原代小胶质细胞接种到接有温度响应性聚合物聚(N-异丙基丙烯酰胺)(PIPAAm)的培养表面上。该表面的水合状态和表面亲水性经历快速,可逆的温度依赖性变化。小胶质细胞在37摄氏度的PIPAAm移植皿上附着并增殖。通过降低培养温度,无需胰蛋白酶或EDTA处理,几分钟内有90%以上的细胞自发地从皿上分离。恢复和重新植入的小胶质细胞表现出的表型特性可与新鲜从脑中分离出的原发性小胶质细胞相媲美。相比之下,通过胰蛋白酶消化收获的细胞不到60%,并且表现出明显的细胞特征改变,如通过体内的病理状态所监测的。这项新技术展示了用于准备细胞移植以及小胶质细胞功能分析所需的细胞来源的实用性。

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