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首页> 外文期刊>Transfusion: The Journal of the American Association of Blood Banks >Isolation and flow cytometric analysis of T-cell-depleted CD34+ PBPCs.
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Isolation and flow cytometric analysis of T-cell-depleted CD34+ PBPCs.

机译:去除T细胞的CD34 + PBPC的分离和流式细胞仪分析。

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摘要

BACKGROUND: To extend allogeneic HPC transplantation to a greater range of patients, the use of partially matched related donors is under development. Because of the inherently higher degree of histoincompatibility in such transplants, there is increased risk of GVHD as well as of graft failure. Ex vivo depletion of donor-derived T-lymphocytes from PBPCs is one of the most effective methods of preventing GVHD. Thus far, individual centers have used custom-developed procedures to deplete the graft of T cells that are responsible for alloreactivity, often employing relatively impure, nonstandardized reagents such as soybean agglutinin and complement. In addition, with improved methods of T-cell depletion, it has been difficult to accurately assess the number of T cells remaining. Because different centers have used different protocols to assay T cells, it has been difficult to reproduce and validate the results between institutions, and this has limited direct comparison of data between centers. STUDY DESIGN AND METHODS: A standardized approach for T-cell depletion was developed by using a Good Manufacturing Practice-manufactured magnetic cell separator (Isolex 300i, Nexell Therapeutics) and commercially available OKT3 antibody. T-cell depletion was performed on PBPCs from six haploidentical donors. RESULTS: CD34+ cell recovery was 47 percent (range, 31-63%) with a median purity of 94 percent (range, 75-99%) and median T-cell log depletion of 4.72 (range, 3.90-5.83). Because this high degree of depletion makes it challenging to accurately quantitate the remaining T cells, two highly sensitive flow cytometric protocols were developed, each of which accurately detects T cells with a sensitivity of 2 per 10,000 (0.02%). The purified CD34+ cells administered to the patients (dose range, 6.13-13.50 x 10(6)/kg) provided rapid neutrophil and platelet engraftment. CONCLUSION: With the Isolex 300i and a MoAb directed against T cells, a high degree of T-cell depletion is obtained. Sensitive, accurate, and reproducible assays have now been developed for T-cell enumeration in these highly purified cell populations.
机译:背景:为了将同种异体HPC移植扩大到更大范围的患者,正在开发使用部分匹配的相关供体的方法。由于在此类移植中固有的较高的组织相容性程度,因此GVHD和移植失败的风险增加。从PBPC体内离体去除供体来源的T淋巴细胞是预防GVHD的最有效方法之一。到目前为止,各个中心已使用定制开发的程序来耗尽负责同种反应的T细胞移植,通常使用相对不纯的非标准化试剂,例如大豆凝集素和补体。另外,利用改进的T细胞耗竭方法,难以准确评估剩余的T细胞数量。由于不同的中心使用了不同的实验方案来检测T细胞,因此很难在机构之间复制和验证结果,这限制了中心之间对数据的直接比较。研究设计和方法:使用Good Manufacturing Practice制造的磁性细胞分离器(Isolex 300i,Nexell Therapeutics)和可商购的OKT3抗体,开发了T细胞耗竭的标准化方法。 T细胞耗竭是对来自六个单性供体的PBPC进行的。结果:CD34 +细胞回收率为47%(范围31-63%),中位纯度为94%(范围75-99%),T细胞对数耗竭中位数为4.72(范围3.90-5.83)。由于这种高度的消耗使得准确定量剩余的T细胞具有挑战性,因此开发了两种高度灵敏的流式细胞术方案,每种方案都能准确检测T细胞,其灵敏度为每10,000个中有2个(0.02%)。给予患者的纯化CD34 +细胞(剂量范围6.13-13.50 x 10(6)/ kg)提供了快速的中性粒细胞和血小板移植。结论:使用Isolex 300i和针对T细胞的MoAb,可以获得高度的T细胞耗竭。对于这些高度纯化的细胞群中的T细胞计数,现已开发出灵敏,准确和可重复的测定方法。

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