Isolation, Characterization and Proliferation of Cancer Cells from Breast Cancer Patients

乳腺癌患者癌细胞的分离、鉴定和增殖

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作者:Wahyu Widowati, Yusuf Heriady, Dian Ratih Laksmitawati, Diana Krisanti Jasaputra, Teresa Liliana Wargasetia, Rizal Rizal, Fajar Sukma Perdana, Annisa Amalia, Annisa Arlisyah, Zakiyatul Khoiriyah, Ahmad Faried, Mawar Subangkit

Aim

This study aim to develop an isolation technique of breast cancer cell from patients as a cancer cell model. Material and

Conclusion

These cells belonged to a basal type of breast carcinoma and expressed CD44+/CD24+, then isolated BCCs can be used as model cancer cells for further research.

Discussion

The morphology of cancer cells was fibroblast like cells on the day 7th after isolation. Isolated breast cancer cells expressed 95.33±0.47% of CD44+/CD24+ and human epidermal growth factor receptor 2 (HER2) low expressions. Isolation of breast cancer cells can use In-house enzymatic protocol. Isolated breast cancer showed the same expression as MDA-MB468 (CD44+/CD24+) and HER2- compared to MCF-7 cell lines (CD44-/CD24+). Conclusion: These cells belonged to a basal type of breast carcinoma and expressed CD44+/CD24+, then isolated BCCs can be used as model cancer cells for further research.

Material and methods

Breast cancer cell isolation is performed by enzymatic methods using the collagen I and hyaluronidase. Then, breast cancer cells were characterized using flow cytometry based on the CD44/CD24 expression where MDA-MB468 and MCF-7 breast cancer cell lines were used as positive controls. Estrogen receptor (ER), progesterone receptor (PR), p53, HER2, and Ki67 expression were assessed using an immunohistochemistry assay. Result and

Methods

Breast cancer cell isolation is performed by enzymatic methods using the collagen I and hyaluronidase. Then, breast cancer cells were characterized using flow cytometry based on the CD44/CD24 expression where MDA-MB468 and MCF-7 breast cancer cell lines were used as positive controls. Estrogen receptor (ER), progesterone receptor (PR), p53, HER2, and Ki67 expression were assessed using an immunohistochemistry assay. Result and

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