未分离的自体外周血干细胞和富含CD(34+)的自体移植物在多发性骨髓瘤中具有相似的长期培养启动能力。

A G Turhan, J H Bourhis, M L Bonnet, S Novault, C Bayle, A Bennaceur, W Vainchenker, J L Pico, F Beaujean
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引用次数: 2

摘要

富集CD(34+)的外周血干细胞(PBSC)越来越多地被用作多发性骨髓瘤(MM)患者的自体移植物。在MM中使用CD34+富集部分的基本原理是能够获得具有显著减少浆细胞污染的移植物。然而,这种操作对移植细胞增殖潜能的影响尚不清楚。作为一项随机试验的一部分,我们希望通过长期培养起始细胞(LTC-IC)测定7名MM患者自体移植物的原始造血细胞含量,比较移植CD(34+)富集细胞或未分离PBSC的MM患者的结果。在3例患者中,将CD(34+)细胞富集部分与未分离的PBSC进行比较,而在其余4例患者中,对总PBSC进行LTC-IC测定。在3例患者中,CD34+选择部分中CD34+细胞的平均百分比为82%(范围为71%-96%),而在4例患者中,PBSC中相同的百分比从0.6%到10%不等(平均:4.2%)。在三名移植了CD34+细胞片段的患者中,两名患者的CD34+与PBSC片段具有非常相似的LTC-IC生成潜力,这是通过在第5周每10(4)个CD34+细胞开始培养时的克隆生成细胞数量来评估的(PBSC: 92和168,CD34+片段:102和16),而一名患者的值略有不同(PBSC: 51和CD34+片段:103)。当比较所有7例患者的PBSC分数时,LTC-IC生成电位非常不均匀,从1.4到168不等。为了确定选择过程是否会影响两个部分中LTC-IC的数量,我们进行了限制性稀释试验,以确定两个患者中造血菌落分布的频率和LTC-IC的频率。造血集落的分布频率在CD34+和PBSC分数中都是线性的,当对培养物的CD34+细胞含量进行校正时,LTC-IC的频率也是线性的(1/20)。我们的研究结果表明,在所有3例患者中使用的CD34+选择程序(Ceprate)对LTC-IC的产生没有危害,这些发现支持了在多种情况下使用该程序以消除肿瘤的基本原理。
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Unfractionated peripheral blood stem cell autografts and CD(34+)-enriched autografts have similar long-term culture initiating capacity in multiple myeloma.

CD(34+)-enriched peripheral blood stem cells (PBSC) are increasingly being used as an autograft in patients with multiple myeloma (MM). The rationale for the use of the CD34+-enriched fraction in MM is the ability to obtain a graft with a significant reduction of contamination by plasma cells. However, the effect of such a manipulation on the proliferating potential of the engrafted cells is not known. We wished to study, as part of a randomized trial comparing the outcome in MM patients transplanted with either CD(34+)-enriched cells or unfractionated PBSC, the primitive hematopoietic cell content of the autografts using long-term culture initiating cell (LTC-IC) assays in 7 MM patients. In 3 patients CD(34+)cell-enriched fraction was compared to unfractionated PBSC whereas in the remaining 4 patients the LTC-IC assay was performed on total PBSC. The mean percentage of CD34+ cells of the CD34+ selected fraction in three patients was 82% (range 71%-96%) whereas the same percentage in PBSC varied from 0.6% to 10% in 4 patients (mean: 4.2%). Out of three patients transplanted with CD34+ cell fraction, two patients were found to have a very similar LTC-IC generating potential in their CD34+ versus PBSC fractions as this was assessed by the clonogenic cell output at week+5 per 10(4) CD34+ cells initiating the culture (PBSC: 92 and 168 and CD34+ fraction: 102 and 16, respectively) whereas one patient had a slightly different values (PBSC: 51 and CD34+ fraction: 103). When the PBSC fraction was compared in all 7 patients, the LTC-IC generation potential was very heterogenous, varying from 1.4 to 168. To determine if the selection procedure influences the numbers of LTC-IC's in both fractions, we have performed limiting dilution assays to determine both the frequency of distribution of hematopoietic colonies and the frequency of LTC-IC's in two patients. The frequency of distribution of hematopoietic colonies was linear in both CD34+ and PBSC fractions as was the frequency of LTC-IC when the corrections were made with regard to the CD34+ cell-content of the cultures (1/20). Our results indicate that the CD34+ selection procedure used in all three patients (Ceprate) is not deleterious for the generation of LTC-IC's and these findings support the rationale for the use of this procedure in multiple for the purposes of tumor depletion.

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