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从临床骨髓样本中有效无标记分选多能间充质干细胞

Effective Label-Free Sorting of Multipotent Mesenchymal Stem Cells from Clinical Bone Marrow Samples.

作者信息

Zia Silvia, Cavallo Carola, Vigliotta Ilaria, Parisi Valentina, Grigolo Brunella, Buda Roberto, Marrazzo Pasquale, Alviano Francesco, Bonsi Laura, Zattoni Andrea, Reschiglian Pierluigi, Roda Barbara

机构信息

Stem Sel Ltd., Viale Giuseppe Fanin 48, 40127 Bologna, Italy.

Laboratory RAMSES, Research & Innovation Technology Department, IRCCS Istituto Ortopedico Rizzoli, 40136 Bologna, Italy.

出版信息

Bioengineering (Basel). 2022 Jan 22;9(2):49. doi: 10.3390/bioengineering9020049.

Abstract

Mesenchymal stem cells (MSC) make up less than 1% of the bone marrow (BM). Several methods are used for their isolation such as gradient separation or centrifugation, but these methodologies are not direct and, thus, plastic adherence outgrowth or magnetic/fluorescent-activated sorting is required. To overcome this limitation, we investigated the use of a new separative technology to isolate MSCs from BM; it label-free separates cells based solely on their physical characteristics, preserving their native physical properties, and allows real-time visualization of cells. BM obtained from patients operated for osteochondral defects was directly concentrated in the operatory room and then analyzed using the new technology. Based on cell live-imaging and the sample profile, it was possible to highlight three fractions (F1, F2, F3), and the collected cells were evaluated in terms of their morphology, phenotype, CFU-F, and differentiation potential. Multipotent MSCs were found in F1: higher CFU-F activity and differentiation potential towards mesenchymal lineages compared to the other fractions. In addition, the technology depletes dead cells, removing unwanted red blood cells and non-progenitor stromal cells from the biological sample. This new technology provides an effective method to separate MSCs from fresh BM, maintaining their native characteristics and avoiding cell manipulation. This allows selective cell identification with a potential impact on regenerative medicine approaches in the orthopedic field and clinical applications.

摘要

间充质干细胞(MSC)在骨髓(BM)中所占比例不到1%。有多种方法可用于其分离,如梯度分离或离心,但这些方法并非直接分离,因此需要通过塑料贴壁生长或磁性/荧光激活分选。为克服这一局限性,我们研究了一种新的分离技术用于从骨髓中分离间充质干细胞;该技术仅基于细胞的物理特性进行无标记分离,保留其天然物理特性,并能对细胞进行实时可视化。从接受骨软骨缺损手术的患者获取的骨髓在手术室直接浓缩,然后使用该新技术进行分析。基于细胞实时成像和样本概况,可突出显示三个组分(F1、F2、F3),并对收集的细胞的形态、表型、集落形成单位 - 成纤维细胞(CFU - F)和分化潜能进行评估。在F1中发现了多能间充质干细胞:与其他组分相比,其CFU - F活性更高,向间充质谱系的分化潜能更大。此外,该技术可去除死细胞,从生物样本中去除不需要的红细胞和非祖基质细胞。这种新技术提供了一种从新鲜骨髓中分离间充质干细胞的有效方法,保持其天然特性并避免细胞操作。这使得能够进行选择性细胞识别,对骨科领域的再生医学方法和临床应用具有潜在影响。

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