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雌激素受体阳性且对雌激素有反应的正常人乳腺细胞在培养中的增殖。

Propagation of oestrogen receptor-positive and oestrogen-responsive normal human breast cells in culture.

作者信息

Fridriksdottir Agla J, Kim Jiyoung, Villadsen René, Klitgaard Marie Christine, Hopkinson Branden M, Petersen Ole William, Rønnov-Jessen Lone

机构信息

Department of Cellular and Molecular Medicine, Faculty of Health Sciences, University of Copenhagen, DK-2200 Copenhagen N, Denmark.

Danish Stem Cell Centre, Faculty of Health Sciences, University of Copenhagen, DK-2200 Copenhagen N, Denmark.

出版信息

Nat Commun. 2015 Nov 13;6:8786. doi: 10.1038/ncomms9786.

Abstract

Investigating the susceptibility of oestrogen receptor-positive (ER(pos)) normal human breast epithelial cells (HBECs) for clinical purposes or basic research awaits a proficient cell-based assay. Here we set out to identify markers for isolating ER(pos) cells and to expand what appear to be post-mitotic primary cells into exponentially growing cultures. We report a robust technique for isolating ER(pos) HBECs from reduction mammoplasties by FACS using two cell surface markers, CD166 and CD117, and an intracellular cytokeratin marker, Ks20.8, for further tracking single cells in culture. We show that ER(pos) HBECs are released from growth restraint by small molecule inhibitors of TGFβ signalling, and that growth is augmented further in response to oestrogen. Importantly, ER signalling is functionally active in ER(pos) cells in extended culture. These findings open a new avenue of experimentation with normal ER(pos) HBECs and provide a basis for understanding the evolution of human breast cancer.

摘要

为了临床应用或基础研究而探究雌激素受体阳性(ER(pos))正常人乳腺上皮细胞(HBECs)的易感性,需要一种成熟的基于细胞的检测方法。在此,我们着手鉴定用于分离ER(pos)细胞的标志物,并将看似处于有丝分裂后阶段的原代细胞扩增为指数生长的培养物。我们报告了一种强大的技术,通过荧光激活细胞分选(FACS)从缩乳术中分离ER(pos) HBECs,使用两种细胞表面标志物CD166和CD117,以及一种细胞内细胞角蛋白标志物Ks20.8,以便在培养中进一步追踪单个细胞。我们表明,ER(pos) HBECs可被TGFβ信号通路的小分子抑制剂解除生长抑制,并且对雌激素的反应会进一步促进生长。重要的是,ER信号在长期培养的ER(pos)细胞中具有功能活性。这些发现为使用正常ER(pos) HBECs开展新的实验开辟了一条途径,并为理解人类乳腺癌的演变提供了基础。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/954c/4660059/8c88ae2f6483/ncomms9786-f1.jpg

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