Method Article
Cancer Associated Fibroblasts (CAFs) facilitate tumor initiation, growth and progression through signaling that promotes proliferation, angiogenesis, and inflammation. Here we describe a method to isolate pure populations of normal fibroblasts and CAFs from fresh mouse and human tissues by cell sorting, using PDGFRα as a surface marker VSports在线直播.
Cancer-associated fibroblasts (CAFs) are the most prominent cell type within the tumor stroma of many cancers, in particular breast carcinoma, and their prominent presence is often associated with poor prognosis1,2. CAFs are an activated subpopulation of stromal fibroblasts, many of which express the myofibroblast marker α-SMA3. CAFs originate from local tissue fibroblasts as well as from bone marrow-derived cells recruited into the developing tumor and adopt a CAF phenotype under the influence of the tumor microenvironment4. CAFs were shown to facilitate tumor initiation, growth and progression through signaling that promotes tumor cell proliferation, angiogenesis, and invasion5-8. We demonstrated that CAFs enhance tumor growth by mediating tumor-promoting inflammation, starting at the earliest pre-neoplastic stages9. Despite increasing evidence of the key role CAFs play in facilitating tumor growth, studying CAFs has been an on-going challenge due to the lack of CAF-specific markers and the vast heterogeneity of these cells, with many subtypes co-existing in the tumor microenvironment10. Moreover, studying fibroblasts in vitro is hindered by the fact that their gene expression profile is often altered in tissue culture11,12 . To address this problem and to allow unbiased gene expression profiling of fibroblasts from fresh mouse and human tissues, we developed a method based on previous protocols for Fluorescence-Activated Cell Sorting (FACS)13,14. Our approach relies on utilizing PDGFRα as a surface marker to isolate fibroblasts from fresh mouse and human tissue V体育2025版. PDGFRα is abundantly expressed by both normal fibroblasts and CAFs9,15 . This method allows isolation of pure populations of normal fibroblasts and CAFs, including, but not restricted to α-SMA+ activated myofibroblasts. Isolated fibroblasts can then be used for characterization and comparison of the evolution of gene expression that occurs in CAFs during tumorigenesis. Indeed, we and others reported expression profiling of fibroblasts isolated by cell sorting16. This protocol was successfully performed to isolate and profile highly enriched populations of fibroblasts from skin, mammary, pancreas and lung tissues. Moreover, our method also allows culturing of sorted cells, in order to perform functional experiments and to avoid contamination by tumor cells, which is often a big obstacle when trying to culture CAFs.
1. Dissecting Mammary or Skin Tissue from Mice
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Using PDGFRα as a marker for fibroblasts results in isolation of highly enriched populations of tissue fibroblasts. The level of purity after sorting was 99%, as quantified by post-sort analysis (Figure 2A). Estimating the percentage of contaminating non-fibroblast cells by the relative expression of cell-specific control genes (Figure 2B) typically shows 0. 1-0. 6% contamination VSports app下载. This level of purity allows high quality transcriptome profiling of isolated fibroblasts9.
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While experiments performed in tissue culture can be informative and suggest functional principles that can be verified in vivo, it is known that large changes occur in gene expression of cells in culture11,12 VSports手机版. In order to avoid a tissue culture step when profiling gene expression in fibroblasts, we developed a protocol that allows isolation of normal, as well as cancer-associated fibroblasts from fresh mouse or human tissue. This protocol was successfully applied with skin, pancreas and breast tissu.
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No conflicts of interest declared.
We thank Dr. Yitzchak Oschry and Dr. Orit Sagi-Asif for their help with FACS sorting V体育ios版. This research was supported by grants to NE from the European Union Seventh Framework Programme (FP7/2007-2013) under grant agreement n ° [276890], from the Israel Cancer Association (#20110078), and from the Israel Cancer Research Fund (Research Career Development Award).
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| Name | Company | Catalog Number | Comments |
|---|---|---|---|
| DMEM | Gibco | 41965 | |
| PBS | Biological Industries | 02-023-1A | |
| Collagenase II | Worthington | LS4176 | |
| Collagenase IV | Worthington | LS4188 | |
| Deoxyribonuclease | Worthington | LS2007 | |
| PharmLyse | BD | 555899 | |
| Cell strainer 70 μm | SPL | 93070 | |
| Purified anti-mouse CD16/CD32 | BD Pharmingen | 553142 | |
| Via probe (7AAD) | e-Bioscience | 00-6993-50 | |
| Anti-mouse CD140a-PE (PDGFRa) | e-Bioscience | 12-1401-81 | |
| Anti-mouse F4/80- FITC | Cederlane | CL8940F | |
| DMEM w/o Phenol Red | Gibco | 31053 | |
| Collagen Type I | BD Biosciences | 354236 |
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