Cosenza Lucia Carmela, Breda Laura, Breveglieri Giulia, Zuccato Cristina, Finotti Alessia, Lampronti Ilaria, Borgatti Monica, Chiavilli Francesco, Gamberini Maria Rita, Satta Stefania, Manunza Laura, De Martis Franca Rosa, Moi Paolo, Rivella Stefano, Gambari Roberto, Bianchi Nicoletta
Department of Life Sciences and Biotechnology, Section of Biochemistry and Molecular Biology, University of Ferrara, Via Fossato di Mortara 74, 44121, Ferrara, Italy.
Department of Hematology-Oncology, Weill Cornell Medical College, New York, NY, USA.
J Transl Med. 2016 Sep 2;14(1):255. doi: 10.1186/s12967-016-1016-4.
Cellular biobanking is a key resource for collaborative networks planning to use same cells in studies aimed at solving a variety of biological and biomedical issues. This approach is of great importance in studies on β-thalassemia, since the recruitment of patients and collection of specimens can represent a crucial and often limiting factor in the experimental planning.
Erythroid precursor cells were obtained from 72 patients, mostly β-thalassemic, expanded and cryopreserved. Expression of globin genes was analyzed by real time RT-qPCR. Hemoglobin production was studied by HPLC.
In this paper we describe the production and validation of a Thal-Biobank constituted by expanded erythroid precursor cells from β-thalassemia patients. The biobanked samples were validated for maintenance of their phenotype after (a) cell isolation from same patients during independent phlebotomies, (b) freezing step in different biobanked cryovials, (c) thawing step and analysis at different time points. Reproducibility was confirmed by shipping the frozen biobanked cells to different laboratories, where the cells were thawed, cultured and analyzed using the same standardized procedures. The biobanked cells were stratified on the basis of their baseline level of fetal hemoglobin production and exposed to fetal hemoglobin inducers.
The use of biobanked cells allows stratification of the patients with respect to fetal hemoglobin production and can be used for determining the response to the fetal hemoglobin inducer hydroxyurea and to gene therapy protocols with reproducible results.
细胞生物样本库是协作网络的关键资源,这些网络计划在旨在解决各种生物学和生物医学问题的研究中使用相同的细胞。这种方法在β地中海贫血研究中非常重要,因为患者的招募和样本的收集可能是实验计划中的关键且常常是限制因素。
从72名患者(大多数为β地中海贫血患者)中获取红系前体细胞,进行扩增和冷冻保存。通过实时RT-qPCR分析珠蛋白基因的表达。通过高效液相色谱法研究血红蛋白的产生。
在本文中,我们描述了由β地中海贫血患者扩增的红系前体细胞构成的地中海贫血生物样本库的建立和验证。对生物样本库中的样本进行了验证,以确保其在以下情况下保持表型:(a) 在独立采血过程中从同一患者分离细胞后;(b) 在不同的生物样本库冻存管中进行冷冻步骤后;(c) 解冻步骤以及在不同时间点进行分析后。通过将冷冻的生物样本库细胞运送到不同实验室进行验证,在这些实验室中,使用相同的标准化程序对细胞进行解冻、培养和分析。根据生物样本库细胞的胎儿血红蛋白产生基线水平进行分层,并使其暴露于胎儿血红蛋白诱导剂。
使用生物样本库中的细胞能够根据胎儿血红蛋白产生情况对患者进行分层,并且可用于确定对胎儿血红蛋白诱导剂羟基脲的反应以及对基因治疗方案的反应,结果具有可重复性。
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