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NanoLuc Binary Technology as a methodological approach: an important new tool for studying the localization of androgen receptor and androgen receptor splice variant V7 homo and heterodimers. | LitMetric

AI Article Synopsis

  • The androgen/androgen receptor signaling pathway is crucial in the development of prostate cancer, with most treatments relying on androgen deprivation therapy (ADT), but tumors often adapt by employing mechanisms like the AR-V7 splice variant that bypasses the need for androgens.
  • The study aimed to understand how full-length androgen receptors (AR-FL) and the AR-V7 variant interact in cells lacking androgens, using advanced NanoLuc technology.
  • Results suggested that while AR-FL dimers form in the cytoplasm and move to the nucleus after androgen exposure, AR-V7 dimers predominantly reside in the nucleus, indicating a different mechanism of action in the presence and absence of androgens.

Article Abstract

Background: The androgen/androgen receptor (AR)-signaling axis plays a central role in prostate cancer (PCa). Upon androgen-binding the AR dimerizes with another AR, and translocates into the nucleus where the AR-dimer activates/inactivates androgen-dependent genes. Consequently, treatments for PCa are commonly based on androgen deprivation therapy (ADT). The clinical benefits of ADT are only transitory and most tumors develop mechanisms allowing the AR to bypass its need for physiological levels of circulating androgens. Clinical failure of ADT is often characterized by the synthesis of a constitutively active AR splice variant, termed AR-V7. AR-V7 mRNA expression is considered as a resistance mechanism following ADT. AR-V7 no longer needs androgenic stimuli for nuclear entry and/or dimerization.

Methods: Our goal was to mechanistically decipher the interaction between full-length AR (AR-FL) and AR-V7 in AR-null HEK-293 cells using the NanoLuc Binary Technology under androgen stimulation and deprivation conditions.

Results: Our data point toward a hypothesis that AR-FL/AR-FL homodimers form in the cytoplasm, whereas AR-V7/AR-V7 homodimers localize in the nucleus. However, after androgen stimulation, all the AR-FL/AR-FL, AR-FL/AR-V7 and AR-V7/AR-V7 dimers were localized in the nucleus.

Conclusions: We showed that AR-FL and AR-V7 form heterodimers that localize to the nucleus, whereas AR-V7/AR-V7 dimers were found to localize in the absence of androgens in the nucleus.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10949640PMC
http://dx.doi.org/10.1186/s12885-024-12110-2DOI Listing

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