多发性骨髓瘤中的实时聚合酶链反应：干细胞采集物肿瘤污染的定量分析

Real-time polymerase chain reaction in multiple myeloma: quantitative analysis of tumor contamination of stem cell harvests.

作者信息

Ladetto Marco, Omedè Paola, Sametti Selina, Donovan John W, Astolfi Monica, Drandi Daniela, Volpato Federica, Giaccone Luisa, Giaretta Fulvia, Palumbo Antonio, Bruno Benedetto, Pileri Alessandro, Gribben John G, Boccadoro Mario

机构信息

Divisione Universitaria di Ematologia, Azienda Ospedaliera S. Giovanni Battista, Torino, Italy.

出版信息

Exp Hematol. 2002 Jun;30(6):529-36. doi: 10.1016/s0301-472x(02)00794-4.

DOI:10.1016/s0301-472x(02)00794-4

PMID:12063019

Abstract

OBJECTIVE

Autologous transplantation of bone marrow (BM) and peripheral blood progenitor cells (PBPC) is commonly used for treatment of multiple myeloma (MM). Although both stem cell sources harbor residual clonal cells, a quantitative evaluation of their level of tumor contamination (LTC) still needs to be performed through highly accurate and reproducible approaches. In this study, we used a validated real-time polymerase chain reaction (PCR) strategy to evaluate LTC of BM and PBPC samples obtained from MM patients.

MATERIALS AND METHODS

The patients underwent two different mobilization courses (defined as early or late course) following two cycles of cyclophosphamide 5 g/m(2). LTC was evaluated by measuring the number of clonal immunoglobulin heavy-chain rearrangements followed by normalization of samples using the GAPDH gene.

RESULTS

Overall, 26 PBPC and 12 BM samples were analyzed. Main results are as follows. 1) PBPC harvests are less contaminated than BM samples taken immediately after each mobilization course (median difference 2.68 logs; range 1.7 to 4.6) (p < 0.0001). 2) LTC of PBPC harvests has only minimal variation among different leukaphereses performed during the same mobilization course (median difference 0.45 logs; range 0.22 to 1.2). 3) No difference was observed among PBPC and BM samples obtained after the late mobilization course as compared to the early mobilization course (median reduction 0.21 logs; range -0.39 to 1.3) (p = 0.84). 4) In PBPC but not in BM samples, there is a clear overestimation of the percentage of plasma cells when flow cytometric evaluation of CD38(bright) cells is compared to real-time PCR results. This suggests that in PBPC, most CD38(bright) cells do not belong to the neoplastic clone.

CONCLUSIONS

Real-time PCR using the IgH rearrangement proved an effective tool for monitoring LTC in stem cell harvests from MM patients. The smaller LTC of PBPC harvests supports the role of PBPC as stem cell rescue for MM patients compared to BM cells.

摘要

目的

自体骨髓（BM）和外周血祖细胞（PBPC）移植常用于治疗多发性骨髓瘤（MM）。尽管这两种干细胞来源都含有残留的克隆细胞，但仍需要通过高度准确且可重复的方法对其肿瘤污染水平（LTC）进行定量评估。在本研究中，我们使用经过验证的实时聚合酶链反应（PCR）策略来评估从MM患者获得的BM和PBPC样本的LTC。

材料与方法

患者在接受两个周期5 g/m²环磷酰胺治疗后，经历了两种不同的动员疗程（定义为早期或晚期疗程）。通过测量克隆性免疫球蛋白重链重排的数量，随后使用甘油醛-3-磷酸脱氢酶（GAPDH）基因对样本进行标准化来评估LTC。

结果

总体而言，分析了26个PBPC样本和12个BM样本。主要结果如下：1）每次动员疗程后立即采集的PBPC收获物的污染程度低于BM样本（中位数差异2.68对数；范围1.7至4.6）（p < 0.0001）。2）在同一动员疗程中进行的不同白细胞分离术中，PBPC收获物的LTC变化极小（中位数差异0.45对数；范围0.22至1.2）。3）与早期动员疗程相比，晚期动员疗程后获得的PBPC和BM样本之间未观察到差异（中位数减少0.21对数；范围 -0.39至1.3）（p = 0.84）。4）在PBPC样本中，但在BM样本中未观察到，当将CD38（明亮）细胞的流式细胞术评估与实时PCR结果进行比较时，浆细胞百分比明显高估。这表明在PBPC中，大多数CD38（明亮）细胞不属于肿瘤克隆。