参与乳腺癌干细胞自我更新的信号因子

Kana Tominaga
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引用次数: 0

摘要

乳腺癌患者的术后或治疗后生存率高于其他类型的癌症患者。然而,在5-10年的潜伏期后,复发和转移到骨骼、肺和大脑是可能的。各种报道表明,在乳腺癌中发现了癌症干细胞(CSC),并被认为对肿瘤复发和转移等事件的预后有影响。推测肿瘤包括由CSC、转运扩增(TA)细胞、6、7和终末分化细胞组成的异质细胞群。CSC可以自我更新,进行对称细胞分裂,并通过不对称细胞分裂产生终末分化细胞和体细胞干细胞8,9。在这个异质性细胞群体中,CSC这个小细胞群体在肿瘤层级中占据最高位置。与非CSC相比,CSC具有较慢的细胞周期和较高的抗氧化能力,可抵抗针对增殖癌细胞的常规化疗和放疗10-12。尽管大量的癌细胞群通过化疗被消灭,但只有少数CSC可能存活并导致肿瘤复发和转移。因此,有必要阐明CSC的特征,规范CSC富集群体的评估方法和相关培养方法。使用已知的CSC特异性抗体进行流式细胞术分析是一种流行且简单的评估CSC的方法。由于CSC的细胞膜特性仅在活细胞中进行分析,因此可以通过流式细胞术对CSC群体进行富集和分离。在规范CSC培养方法中,肿瘤球培养和类器官培养16,17是评估CSC体外自我更新能力的有用工具。球培养已被用于评估培养的神经干细胞的存活和自我更新能力。摘要
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Signaling Factors Involved in Self-Renewal of Breast Cancer Stem-like Cells
Postoperative or post-treatment survival is greater among breast cancer patients than among those with other types of cancer. However, recurrence and metastasis to the bones, 1 lungs, and brain are possible after a latent period of 5–10 years. Various reports suggested that the cancer stem-like cells (CSC) are found in breast cancer and are considered to deter 2–5 the prognosis of events including tumor recurrence and metastasis. Tumors are speculated to comprise a heterogeneous cell population constituted by CSC, transit-amplifying (TA) cells, 6,7 and terminally differentiated cells. CSC can undergo self-renewal, symmetric cell division, and can yield terminally differentiated cells and somatic stem cells via asymmetric cell .8,9 division In this heterogeneous cell population, CSC, a small cell population, occupies the highest position in tumor hierarchy. With slow cell cycles and high anti-oxidative capacity compared with non-CSC, CSC are resistant to conventional chemoand radiotherapy 10–12 targeting proliferating cancer cells. Despite large cancer cell populations being eliminated through chemotherapy, only a few CSC may survive and cause tumor recurrence and metastasis. Hence, it is essential to elucidate the characteristics of CSC and standardize methods of assessing CSC-enriched populations and associated culture methods. Flow cytometry analysis using known CSC-specific antibodies is a popular and simple method for 13–15 assessing CSC. The CSC population can be enriched and fractionated through flow cytometry analysis because cell membrane characteristics of CSC is analyzed in only living cells. In standardizing culture methods for CSC, tumor sphere culture and organoid culture 16,17 are useful tools to assess the self-renewal capacity of CSC in vitro. Sphere culture has 18 been used to assess the survival and self-renewal capacity of neural stem cells in culture. Abstract
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