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移植到视网膜下间隙的微加工聚甲基丙烯酸甲酯支架上的视网膜祖细胞的存活、迁移和分化。

Survival, migration and differentiation of retinal progenitor cells transplanted on micro-machined poly(methyl methacrylate) scaffolds to the subretinal space.

作者信息

Tao Sarah, Young Conan, Redenti Stephen, Zhang Yiqin, Klassen Henry, Desai Tejal, Young Michael J

机构信息

Department of Physiology, University of California, San Francisco, 1700 4th Street, San Francisco, California, USA.

出版信息

Lab Chip. 2007 Jun;7(6):695-701. doi: 10.1039/b618583e. Epub 2007 Mar 28.

Abstract

Stem and progenitor cells can be combined with polymer substrates to generate tissue equivalents in culture. The replacement of retinal tissue lost to disease or trauma using retinal progenitor cells (RPCs) delivered on polymer scaffolds and transplanted into the sub-retinal space of the damaged retina is a promising therapeutic strategy. Micromachining-based, ultra-thin PMMA poly(methyl methacrylate) scaffolds may provide a suitable cytoarchitectural environment for tissue engineering and transplantation to the diseased eye. Here, adhesion of RPCs to polymer, as well as migration and differentiation in the host retina were compared for PMMA scaffolds (6 microm thickness) with either smooth or porous (11 microm diameter) surface topography. RPCs were cultured under identical conditions on smooth or porous laminin-coated polymer scaffolds and transplanted into the subretinal space of C57BL/6 mice. RPCs could be cultured on both scaffolds with similar results, although transplantation with non-porous scaffolds showed limited RPC retention. Porous scaffolds demonstrated enhanced RPC adherence during transplantation and allowed for greater process outgrowth and cell migration into the host retinal layers. Integrated cells expressed the mature neuronal marker neurofilament-200 (nf-200), the glial marker glial fibrillary acidic protein (GFAP) and the retinal-specific marker recoverin. No host foreign body response was seen. In conclusion, ultra-thin film PMMA scaffolds micromachined to contain through pores retain adherent RPCs to a considerably greater extent than unmachined versions during the transplantation process and can serve as a biocompatible substrate for cell delivery in vivo.

摘要

干细胞和祖细胞可与聚合物基质结合,在培养中生成组织等效物。使用聚合物支架递送并移植到受损视网膜的视网膜下间隙中的视网膜祖细胞(RPC)来替代因疾病或创伤而丧失的视网膜组织,是一种很有前景的治疗策略。基于微加工的超薄聚甲基丙烯酸甲酯(PMMA)支架可为组织工程和移植到患病眼睛提供合适的细胞结构环境。在此,比较了具有光滑或多孔(直径11微米)表面形貌的PMMA支架(厚度6微米)上RPC与聚合物的粘附以及在宿主视网膜中的迁移和分化情况。RPC在相同条件下培养在光滑或多孔的层粘连蛋白包被的聚合物支架上,并移植到C57BL/6小鼠的视网膜下间隙。RPC可在两种支架上培养,结果相似,尽管无孔支架移植后RPC保留有限。多孔支架在移植过程中显示出增强的RPC粘附,并允许更大程度的突起生长和细胞迁移到宿主视网膜层。整合的细胞表达成熟神经元标志物神经丝-200(nf-200)、胶质标志物胶质纤维酸性蛋白(GFAP)和视网膜特异性标志物恢复蛋白。未观察到宿主异物反应。总之,通过微加工制成的含有通孔的超薄PMMA支架在移植过程中比未加工的版本能在更大程度上保留粘附的RPC,并且可作为体内细胞递送的生物相容性基质。

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