采用三步法制备低温保存的无细胞抽取产物样本,进行解冻后分析,可获得高活细胞回收率。

IF 2.5 3区 医学 Q2 HEMATOLOGY
Transfusion Pub Date : 2024-11-07 DOI:10.1111/trf.18059
Rosalie M Sterner, Dustin J Strasburg, Sildane Va, Margaret A DiGuardo, Eapen K Jacob
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引用次数: 0

摘要

背景:由于低温保护剂的细胞毒性,对新鲜 CD34+ 细胞样本进行计数的流式细胞术方案并不适合低温保存的产品。对于低温保存的样本,通常要使用大量低渗溶液,以通过解冻后清洗去除低温保护剂,而低渗溶液会导致细胞死亡。我们最近开发了一种新颖的多步稀释法,随后进行流式细胞仪分析,以获得准确、可重复的结果。以前的方法涉及洗涤步骤,无法对细胞恢复情况进行计数,只能根据细胞活力来判断是否成功。新方法可评估总细胞回收率和有活力细胞回收率:研究设计和方法:将冷冻保存在10% DMSO中的血液制品的白细胞目标浓度为300×106/毫升。在 37°C 下解冻这些产品的冻存管,然后用 1%-人血白蛋白溶于右旋糖酐 40(10% 低分子量右旋糖酐溶于 0.9% 氯化钠),以 1:2 的比例稀释样本,每次加样间隔 5 分钟。进行 1:10 稀释以获得流式细胞仪分析所需的正确细胞浓度,稀释倍数为 1:20。最终白细胞浓度为 ~15 × 106/毫升,DMSO 稀释至 0.5%:结果:使用这种新方法检测了 52 份样本。总细胞回收率和存活细胞回收率是根据干细胞保存前的数据计算得出的。CD34 和 CD3 的总细胞回收率中位数大于 85%,而有活力细胞回收率中位数大于 75%:讨论:冷冻样本可通过逐步稀释的方法可靠地准备用于流式细胞仪检测,以保持细胞的完整性和可靠的回收率。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A three-step method for preparing cryopreserved samples of apheresis products for post-thaw analysis yields a high recovery of viable cells.

Background: Flow cytometry protocols for counting fresh CD34+ cell samples are not ideal for cryopreserved products due to cryoprotectant cytotoxicity. For cryopreserved samples, often large volumes of hypotonic solutions, which can cause cell death, are used to remove the cryoprotectant with a post-thaw wash. We recently developed a novel multistep dilution method with subsequent flow cytometry analysis to allow for accurate and reproducible results. The previous method involved washing steps which invalidate the ability to enumerate cell recovery, and success had to be gauged solely on viability. The new method allows for assessment of total cell recovery and viable cell recovery.

Study design and methods: Apheresis products were cryopreserved in 10% DMSO at a target WBC concentration of 300 × 106/mL. Cryovials from these products were thawed at 37°C, and samples were diluted 1:2 by three additions of 1/3 sample volume using 1%-Human Albumin in Dextran 40 (10% Low Molecular Weight Dextran in 0.9% NaCl) separated by 5 min between each addition. A 1:10 dilution was performed to obtain the correct cell concentration for flow cytometric analysis resulting in a 1:20 dilution. End WBC concentrations were ~15 × 106/mL with DMSO diluted to 0.5%.

Results: Fifty-two samples were tested with this new method. Total and viable cell recoveries were calculated based on pre-cryopreservation data. Median total cell recoveries for CD34 and CD3 were >85%, while median viable cell recoveries were >75%.

Discussion: Cryopreserved samples can be reliably prepared for flow cytometric testing using a step-wise dilution to preserve cell integrity and robust recoveries.

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来源期刊
Transfusion
Transfusion 医学-血液学
CiteScore
4.70
自引率
20.70%
发文量
426
审稿时长
1 months
期刊介绍: TRANSFUSION is the foremost publication in the world for new information regarding transfusion medicine. Written by and for members of AABB and other health-care workers, TRANSFUSION reports on the latest technical advances, discusses opposing viewpoints regarding controversial issues, and presents key conference proceedings. In addition to blood banking and transfusion medicine topics, TRANSFUSION presents submissions concerning patient blood management, tissue transplantation and hematopoietic, cellular, and gene therapies.
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