Martin V M, Siewert C, Scharl A, Harms T, Heinze R, Ohl S, Radbruch A, Miltenyi S, Schmitz J
Miltenyi Biotec GmbH, Bergisch Gladbach, Germany.
Exp Hematol. 1998 Mar;26(3):252-64.
Disseminated epithelial tumor cells have been detected in the bone marrow and blood of cancer patients by means of immunocytochemical or immunofluorescent staining of cytocentrifuge slides, multiparameter flow cytometry, and reverse transcriptase-polymerase chain reaction. However, it is hardly possible using such methods to detect tumor cells at a frequency below 10(-6). To increase the sensitivity of these detection techniques we have developed a new technology for the enrichment of disseminated epithelial tumor cells from hematopoietic cell samples by high-gradient magnetic cell sorting (MACS). Cells are permeabilized and fixed and carcinoma cells are magnetically labeled specifically with an anti-cytokeratin 8 monoclonal antibody (mAb) directly conjugated to superparamagnetic microbeads. Magnetically labeled cells are enriched on high-gradient magnetic columns. Tumor cells are detected in the enriched cell fraction by flow cytometry, fluorescence microscopy, or immunocytochemisty. In this study we demonstrated the method using a model system in which five to 5,000 cells from a breast cancer cell line were seeded into blood cell samples from a healthy donor containing 1.2 x 10(8) leukocytes. Tumor cells were 10,477+/-4242 (n=25)-fold magnetically enriched, and 57.7%+/-16.9% (n=33) of the initially seeded tumor cells were recovered. Applying the method to 20-40 mL blood samples from patients with advanced carcinomas of the breast, prostate, colon, rectum, or lung, we were able to detect between one and 6.8 x 10(4) cytokeratin-expressing tumor cells in 21 of 34 patients. This corresponds to frequencies of tumor cells between 6.8 x 10(-9) and 1.1 x 10(-3) among nucleated cells in the original sample. Enriched tumor cells were further analyzed for expression of tissue-specific and prognostic markers such as breast mucin glycoproteins, erbB2, and CD44v6 for additional characterization and to confirm their tumor origin. The technique described could become a valuable tool for the quantification and molecular characterization of metastatic carcinoma cells in hematopoietic tissue, and may ultimately prove useful in the diagnosis, prognosis, and monitoring of patients with carcinoma.
通过对细胞离心涂片进行免疫细胞化学或免疫荧光染色、多参数流式细胞术以及逆转录聚合酶链反应,已在癌症患者的骨髓和血液中检测到播散性上皮肿瘤细胞。然而,使用这些方法几乎不可能检测到频率低于10^(-6)的肿瘤细胞。为了提高这些检测技术的灵敏度,我们开发了一种新技术,通过高梯度磁性细胞分选(MACS)从造血细胞样本中富集播散性上皮肿瘤细胞。细胞经通透处理和固定后,癌细胞用直接与超顺磁性微珠偶联的抗细胞角蛋白8单克隆抗体(mAb)进行特异性磁性标记。磁性标记的细胞在高梯度磁性柱上富集。通过流式细胞术、荧光显微镜或免疫细胞化学在富集的细胞组分中检测肿瘤细胞。在本研究中,我们使用一个模型系统演示了该方法,即将来自乳腺癌细胞系的5至5000个细胞接种到含有1.2×10^8个白细胞的健康供体的血细胞样本中。肿瘤细胞经磁性富集10477±4242倍(n = 25),回收了最初接种肿瘤细胞的57.7%±16.9%(n = 33)。将该方法应用于来自晚期乳腺癌、前列腺癌、结肠癌、直肠癌或肺癌患者的20 - 40 mL血液样本,我们在34例患者中的21例中检测到1至6.8×10^4个表达细胞角蛋白的肿瘤细胞。这对应于原始样本中有核细胞中肿瘤细胞的频率在6.8×10^(-9)至1.1×10^(-3)之间。对富集的肿瘤细胞进一步分析组织特异性和预后标志物如乳腺粘蛋白糖蛋白、erbB2和CD44v6的表达,以进行进一步表征并确认其肿瘤来源。所描述的技术可能成为定量和分子表征造血组织中转移性癌细胞的有价值工具,并最终可能证明对癌症患者的诊断、预后和监测有用。
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