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Freeze drying of red blood cells: The use of directional freezing and a new radio frequency lyophilization device

机译:冷冻干燥红细胞:使用定向冷冻和新型射频冻干设备

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摘要

Red blood cell (RBC) units are administered routinely into patients expressing a wide range of acute and chronic conditions (e.g., anemia, traumatic bleeding, chronic diseases, and surgery). The modern blood banking system has been designed to answer this need and assure a continuous, high quality blood supply to patients. However, RBCs units can be stored under hypothermic conditions for only up to 42 days, which leads to periodic shortages. Cryopreservation can solve these shortages, but current freezing methods employ high glycerol concentrations, which need to be removed and the cells washed prior to transfusion, resulting in a long (more than 1 hour) and cumbersome washing step. Thus, frozen RBCs have limited use in acute and trauma situations. In addition, transportation of frozen samples is complicated and costly. Freeze drying (lyophilization) of RBCs has been suggested as a solution for these problems, since it will allow for a low weight sample to be stored at room temperature, but reaching this goal is not a simple task. We studied the effect of different solutions (IMT2 and IMT3) containing trehalose and antioxidants or trehalose and human serum albumin, respectively, on freezing/thawing and freeze drying of RBCs. In addition, we evaluated the effect of cells concentrations and cooling rates on the post thaw and post rehydration recoveries of the RBCs. Finally, we developed a new radio frequency (RF) lyophilization device for a more rapid and homogeneous sublimation process of the frozen RBCs samples. Recovery and free Hb were measured as well as oxygen association/dissociation and cell's deformability. We found that IMT3 (0.3 M trehalose and 10% HSA) solution that was directionally frozen at a rapid interface velocity of 1 mm/sec (resulting in a cooling rate of 150°C/min) yielded the best results (better than IMT2 solution and slow interface velocity). Freeze thawing gave 100% survival, while freeze drying followed by rehydration with 20% dextran-40kDa solution resulted in 75% survival. However, recovery following freeze drying was possible only when 20% Dextran-40 solution was used as the rehydration medium. The rehydrated cells were not stable upon an eight-fold dilution. The RF lyophilization system increased the sublimation rate more than twice compared to conventional drying and maintained a high survival rate of the RBCs after partial drying.
机译:红细胞(RBC)单元通常用于表达多种急性和慢性疾病(例如贫血,创伤性出血,慢性疾病和手术)的患者。现代血液储存系统旨在满足这一需求,并确保为患者提供持续,高质量的血液。但是,RBCs单元在低温条件下最多只能存储42天,这会导致周期性短缺。冷冻保存可以解决这些不足,但是当前的冷冻方法使用高浓度的甘油,需要将其去除,然后在输血之前洗涤细胞,这导致漫长(超过1小时)且麻烦的洗涤步骤。因此,冷冻的红细胞在急性和创伤情况下用途有限。另外,冷冻样品的运输是复杂且昂贵的。已建议将RBC冷冻干燥(冻干)作为解决这些问题的方法,因为它可以将低重量的样品保存在室温下,但要达到这一目标并非易事。我们研究了分别含有海藻糖和抗氧化剂或海藻糖和人血清白蛋白的不同溶液(IMT2和IMT3)对RBC的冷冻/解冻和冷冻干燥的影响。此外,我们评估了细胞浓度和冷却速率对红细胞解冻后和补液后回收率的影响。最后,我们开发了一种新的射频(RF)冻干设备,用于冷冻RBC样品的更快,更均匀的升华过程。测量回收率和游离Hb以及氧缔合/解离和细胞的可变形性。我们发现以1mm / sec的快速界面速度定向冻结的IMT3(0.3M海藻糖和10%HSA)溶液(导致冷却速度为150°C / min)产生了最佳结果(比IMT2溶液更好)和缓慢的界面速度)。冷冻解冻给出100%的存活率,而冷冻干燥然后用20%葡聚糖-40kDa溶液再水化得到75%的存活率。但是,冷冻干燥后的恢复只有在使用20%Dextran-40溶液作为补液介质时才有可能。再水化的细胞在八倍稀释后不稳定。与常规干燥相比,RF冻干系统将升华速率提高了两倍以上,并在部分干燥后保持了RBC的高存活率。

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