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Efficient Non-Viral Gene Modification of Mesenchymal Stromal Cells from Umbilical Cord Wharton’s Jelly with Polyethylenimine

机译:高效的非病毒基因改性来自脐带沃顿果冻的间充质基质细胞与聚乙烯菊花

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Mesenchymal stromal cells (MSC) derived from human umbilical cord Wharton’s jelly (WJ) have a wide therapeutic potential in cell therapy and tissue engineering because of their multipotential capacity, which can be reinforced through gene therapy in order to modulate specific responses. However, reported methodologies to transfect WJ-MSC using cationic polymers are scarce. Here, WJ-MSC were transfected using 25 kDa branched- polyethylenimine (PEI) and a DNA plasmid encoding GFP. PEI/plasmid complexes were characterized to establish the best transfection efficiencies with lowest toxicity. Expression of MSC-related cell surface markers was evaluated. Likewise, immunomodulatory activity and multipotential capacity of transfected WJ-MSC were assessed by CD2/CD3/CD28-activated peripheral blood mononuclear cells (PBMC) cocultures and osteogenic and adipogenic differentiation assays, respectively. An association between cell number, PEI and DNA content, and transfection efficiency was observed. The highest transfection efficiency (15.3 ± 8.6%) at the lowest toxicity was achieved using 2 ng/μL DNA and 3.6 ng/μL PEI with 45,000 WJ-MSC in a 24-well plate format (200 μL). Under these conditions, there was no significant difference between the expression of MSC-identity markers, inhibitory effect on CD3+ T lymphocytes proliferation and osteogenic/adipogenic differentiation ability of transfected WJ-MSC, as compared with non-transfected cells. These results suggest that the functional properties of WJ-MSC were not altered after optimized transfection with PEI.
机译:源自人脐带涡轮果冻(WJ)的间充质基质细胞(MSC)在细胞疗法和组织工程中具有宽的治疗潜力,因为它们的多电位能力可以通过基因治疗来加强,以调节特定的反应。然而,报告使用阳离子聚合物转染WJ-MSC的方法是稀缺的。这里,使用25kDa支链聚乙烯亚胺(PEI)和编码GFP的DNA质粒转染WJ-MSC。 PEI /质粒复合物的特征是建立具有最低毒性的最佳转染效率。评价MSC相关细胞表面标志物的表达。同样地,通过CD2 / CD3 / CD28活化外周血单核细胞(PBMC)培养和骨质发生和抗脂肪分化测定来评估转染的WJ-MSC的免疫调节活性和多电像能力。观察到细胞数,PEI和DNA含量和转染效率之间的关联。使用2ng /μLDNA和3.6ng /μlpe以24孔板格式(200μl)的45,000WJ-MSC为基础的最低毒性的最高转染效率(15.3±8.6%)。在这些条件下,与未转染的细胞相比,MSC - 识别标志物的表达与转染的WJ-MSC的抑制作用与转染的WJ-MSC的抑制作用与转染的WJ-MSC的抑制作用之间没有显着差异。这些结果表明,在用PEI优化转染后,WJ-MSC的功能性质没有改变。

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