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播散癌细胞的特异性分离:一种允许灵敏检测具有诊断和治疗价值的靶分子的新方法。

Specific isolation of disseminated cancer cells: a new method permitting sensitive detection of target molecules of diagnostic and therapeutic value.

作者信息

Tveito Siri, Maelandsmo Gunhild M, Hoifodt Hanne K, Rasmussen Heidi, Fodstad Oystein

机构信息

Department of Tumor Biology, Rikshospitalet-Radiumhospitalet Medical Center, Montebello, 0310, Oslo, Norway.

出版信息

Clin Exp Metastasis. 2007;24(5):317-27. doi: 10.1007/s10585-006-9052-8. Epub 2007 May 26.

Abstract

Molecular studies of rare cells, such as circulating cancer cells, require efficient pre-enrichment steps to obtain a pure population of target cells for further characterization. We have developed a two-step approach, starting with immunomagnetic enrichment, followed by specific isolation of individual, easily identifiable bead-rosetted target cells using a new semi-automated CellPick system. With this procedure, 1-50 live target cells can now be isolated. As a model system, we spiked a small number of tumor cells into millions of normal mononuclear cells (MNCs). Efficient isolation of pure target cells was obtained by use of the CellPick system, and the nature of isolated, bead-rosetted cells was verified by use of FISH. Single breast cancer cells were picked directly into an RNA preserving lysis buffer, reverse transcribed, and PCR amplified with two cDNA specific primer sets. With the isolated cells we consistently obtained both ubiquitously expressed and tumor cell specific PCR products. We also performed a successful mutation analysis of single cells using PCR and cycling temperature capillary electrophoresis (CTCE). This may have significant clinical implications in cancer and in other diseases, e.g. in characterizing micrometastatic cancer cells in blood and lymph nodes to help identifying patients who most likely will respond to therapies like tyrosine kinase inhibitors and compounds targeting specific mutations. By use of the CellPick system it is possible to specifically isolate bead-rosetted or otherwise labelled target cells from a heterogeneous cell population for further molecular characterization.

摘要

对罕见细胞(如循环癌细胞)进行分子研究,需要高效的预富集步骤,以获得纯的目标细胞群体用于进一步表征。我们开发了一种两步法,首先进行免疫磁珠富集,然后使用新型半自动CellPick系统对单个易于识别的珠状玫瑰花结目标细胞进行特异性分离。通过该程序,现在可以分离出1 - 50个活的目标细胞。作为一个模型系统,我们将少量肿瘤细胞混入数百万个正常单核细胞(MNC)中。使用CellPick系统可有效分离出纯的目标细胞,并通过荧光原位杂交(FISH)验证分离出的珠状玫瑰花结细胞的性质。将单个乳腺癌细胞直接挑选到RNA保存裂解缓冲液中,进行逆转录,并用两组cDNA特异性引物进行PCR扩增。利用分离出的细胞,我们始终能获得普遍表达的和肿瘤细胞特异性的PCR产物。我们还使用PCR和循环温度毛细管电泳(CTCE)对单个细胞进行了成功的突变分析。这可能在癌症和其他疾病中具有重要的临床意义,例如在表征血液和淋巴结中的微转移癌细胞以帮助识别最可能对酪氨酸激酶抑制剂和靶向特定突变的化合物等治疗产生反应的患者方面。通过使用CellPick系统,可以从异质细胞群体中特异性分离出珠状玫瑰花结或其他标记的目标细胞,用于进一步的分子表征。

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