Serum‐free complete medium, an alternative medium to mimic androgen deprivation in human prostate cancer cell line models

Background Almost all men who present with advanced prostate cancer (CaP) and some men who fail therapy for clinically localized CaP are treated with androgen deprivation therapy (ADT). CaP cell lines are used to identify and characterize new agents for ADT or investigate mechanisms of ADT resistanc...

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Published in:The Prostate 2018-02, Vol.78 (3), p.213-221
Main Authors: Fiandalo, Michael V., Wilton, John H., Mantione, Krystin M., Wrzosek, Carol, Attwood, Kristopher M., Wu, Yue, Mohler, James L.
Format: Article
Language:English
Subjects:
androgen deprivation
Androgens
Androgens - metabolism
Cell culture
Cell growth
Cell Line, Tumor
Charcoal
charcoal‐stripped media
Culture media
Culture Media, Serum-Free
DHT
Fetal calf serum
Growth inhibition
Humans
Liquid chromatography
Male
mass spectrometry
Mass spectroscopy
Metabolism
Prostate cancer
Prostatic Neoplasms - metabolism
Tandem Mass Spectrometry
Testosterone
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Summary:Background Almost all men who present with advanced prostate cancer (CaP) and some men who fail therapy for clinically localized CaP are treated with androgen deprivation therapy (ADT). CaP cell lines are used to identify and characterize new agents for ADT or investigate mechanisms of ADT resistance. CaP cell lines are maintained in culture medium that contains fetal bovine serum, which contains testosterone (T). Androgen deprivation experiments are performed using media supplemented with androgen‐free serum, such as charcoal stripped fetal bovine serum (CS‐FBS). However, CS‐FBS composition varies from batch‐to‐batch and variations may impact experimental reproducibility. Serum free media (SFM) may provide a better defined alternative to media supplemented with CS‐FBS (CSM). Methods Cell growth of six human CaP cell lines was assessed using 3‐(4,5‐Dimethylthiazol‐2‐yl)‐2,5‐diphenyltetrazolium bromide (MTT). Androgen levels were measured using liquid chromatography‐tandem mass spectrometry (LC‐MS/MS). Results MTT assays showed 5 of 6 CaP cell lines grew after 6 days of culture in androgen‐ deprived SFM or CSM. LNCaP and VCaP growth was stimulated when cells were cultured in SFM or CSM supplemented with T. LNCaP, C4‐2, LAPC‐4, and VCaP cell growth was inhibited when cultured in SFM or CSM with T and bicalutamide. LC‐MS/MS data showed LAPC‐4 cells produced similar DHT levels when cultured in T‐supplemented SFM or CSM. Dutasteride impaired T to DHT metabolism in LAPC‐4. Conclusions Media composition contributed to growth differences observed between CaP cells cultured in SFM or CSM. However, the differences in media composition did not impair CaP cell response to T‐stimulated growth, bicalutamide growth inhibition, metabolism of T, or dutasteride efficiency. SFM can be used as a better defined alternative to CSM for androgen deprivation experiments.
ISSN:0270-4137
1097-0045
DOI:10.1002/pros.23459