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冷冻保存前后脐带血造血细胞参数的评估。

Assessment of cord blood hematopoietic cell parameters before and after cryopreservation.

作者信息

Kurtz James, Seetharaman Shalini, Greco Nicholas, Moroff Gary

机构信息

American Red Cross, Jerome H. Holland Laboratory for the Biomedical Sciences, Rockville, Maryland 20855, USA.

出版信息

Transfusion. 2007 Sep;47(9):1578-87. doi: 10.1111/j.1537-2995.2007.01327.x.

Abstract

BACKGROUND

The testing of cord blood (CB) progenitor and stem cell units for transplantation suitability involves enumeration of total nucleated cells before freezing. CD34+ cell counts may also be a means of determining suitability. Studies have been conducted to evaluate how specific storage conditions influence cell counts.

STUDY DESIGN AND METHODS

CB units were processed by hydroxyethyl starch volume reduction. Cryopreserved-thawed samples were diluted 1:3 without washing. CD34+ cells were measured with three commercially available assay methods. In specific studies, apoptosis-indicating reagents were included. CB units were analyzed for nucleated cells, aldehyde dehydrogenase-containing cells, and progenitor colonies.

RESULTS

CD34+ cell levels and nucleated cells were retained during storage in test tubes at 1 to 6 degrees C for 3 days. Cryopreserved-thawed samples showed a reduction in CD34+ cells relative to prefreeze levels with the largest decrease with the Stem-Kit (Beckman Coulter) restricted gating procedure. Prefreeze samples contained minimal numbers of presumed apoptotic cells detected with 7-aminoactinomycin D or SYTO16, but after cryopreservation-thawing there was an increase. Nucleated cell levels determined with a hematology analyzer or flow cytometry were reduced after thawing. Cryopreservation-thawing reduced the percentage of CD34+ cells positive for the presence of aldehyde dehydrogenase and the number of progenitor colonies. These differences were significant.

CONCLUSION

These studies indicate that CD34+ cell counts were maintained when CB samples were stored at 1 to 6 degrees C in test tubes for 3 days. Cryopreservation-thawing resulted in changes in a number of parameters including the percentage of CD34+ cells that were aldehyde dehydrogenase(+) and the number of 7-aminoactinomycin D(+) cells and SYTO16(low) cells.

摘要

背景

对用于移植的脐带血(CB)祖细胞和干细胞单位进行适用性检测,需要在冷冻前对总核细胞进行计数。CD34+细胞计数也可能是确定适用性的一种方法。已经开展了多项研究来评估特定的储存条件如何影响细胞计数。

研究设计与方法

采用羟乙基淀粉体积减少法处理CB单位。冻融后的样品不洗涤,按1:3稀释。使用三种市售检测方法测量CD34+细胞。在特定研究中,加入了凋亡指示试剂。对CB单位进行核细胞、含醛脱氢酶细胞和祖细胞集落分析。

结果

CB单位在1至6摄氏度的试管中储存3天时,CD34+细胞水平和核细胞得以保留。冻融后的样品相对于冻前水平,CD34+细胞减少,其中使用Stem-Kit(贝克曼库尔特公司)限制门控程序时减少最多。冻前样品中,用7-氨基放线菌素D或SYTO16检测到的假定凋亡细胞数量极少,但冻融后数量增加。用血液分析仪或流式细胞术测定的核细胞水平在解冻后降低。冻融降低了醛脱氢酶阳性的CD34+细胞百分比和祖细胞集落数量。这些差异具有统计学意义。

结论

这些研究表明,CB样品在1至6摄氏度的试管中储存3天时,CD34+细胞计数得以维持。冻融导致多项参数发生变化,包括醛脱氢酶阳性的CD34+细胞百分比、7-氨基放线菌素D阳性细胞和SYTO16(低表达)细胞数量。

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