The Impact of Indoles Activating the Aryl Hydrocarbon Receptor on Androgen Receptor Activity in the 22Rv1 Prostate Cancer Cell Line

The activation of the aryl hydrocarbon receptor (AhR) by xenobiotic compounds was demonstrated to result in the degradation of the androgen receptor (AR). Since prostate cancer is often dependent on AR, it has become a significant therapeutic target. As a result of the emerging concept of bacterial mimicry, we tested whether compounds with indole scaffolds capable of AhR activation have the potential to restrict AR activity in prostate cancer cells. Altogether, 22 indolic compounds were tested, and all of them activated AhR. However, only eight decreased DHT-induced AR luciferase activity. All indoles, which met the AhR-activating and AR-suppressing criteria, decreased the expression of DHT-inducible AR target genes, specifically KLK3 and FKBP5 mRNAs. The reduced AR binding to the KLK3 promoter was confirmed by a chromatin immunoprecipitation (ChIP) assay. In addition, some indoles significantly decreased AR protein and mRNA level. By using CRISPR/Cas9 AhR knockout technology, no relationship between AhR and AR, measured as target gene expression, was observed. In conclusion, some indoles that activate AhR possess AR-inhibiting activity, which seems to be related to the downregulation of AR expression rather than to AR degradation alone. Moreover, there does not seem to be a clear relationship that would connect AhR activation with AR activity suppression in 22Rv1 cells.


Introduction
Prostate cancer is one of the most common types of cancer in men, and the risk of developing it increases with advanced age. More than 75% of patients with prostate cancer are men over the age of 65 [1]. According to Siegel's statistic (2022), it is estimated that about 268,490 new cases of prostate cancer will be reported in the United States in 2022 [2]. In most deaths associated with prostate cancer, there is a predominant type known as castration-resistant prostate cancer (CRPC) [3]. Typical CRPC cellular mechanisms include androgen receptor (AR) overexpression, intratumoral synthesis of androgens, and the expression of shortened AR variants. [4]. These AR variants arise from alternative splicing of cryptic exons, and their activity is mostly ligand-independent [5]. The most abundant variant is AR-v7, which was indicated as a possible biological marker of prostate cancer development [6] since its levels have been reported to be significantly lower in normal prostate tissue than in prostate cancer tissue, or CRPC [5]. Prostate cancer with this splicing variant shows only a minor therapeutic response to commonly used anti-androgenic drugs (e.g., enzalutamide; ENZ) [7].
AR belongs to the nuclear receptor superfamily. Upon androgen (ligand) binding, AR translocates to the nucleus and binds to specific responsive elements in DNA. The most vital androgens are testosterone (T), dihydrotestosterone (DHT), and dehydroepiandrosterone (DHEA) [8]. Testosterone is the main male sex hormone and is converted to DHT by 5α-reductase enzyme. This process occurs in several target tissues, e.g., in the prostate [8,9].
Interestingly, the concept of AhR-mediated degradation of AR was described for other compounds, namely Icaritin [24] and Carbidopa [25]. Icaritin is one of the major metabolites of the compound Icariin [26,27]. Both of these substances are naturally occurring polyphenols, which can be found in plants of the genus Epimedium [27]. Carbidopa is a decarboxylase inhibitor used to treat Parkinson's disease [28]. Both of these compounds have been shown to induce AhR activation with consequent degradation of AR [24,25]. However, while Icaritin induced this effect in LNCaP, C4-2 and 22Rv1 cells, Carbidopa was demonstrated to have such an effect in LNCaP cells only. Moreover, these compounds suppressed the tumor proliferation of LNCaP implanted cells in nude mice [24,25].
Therefore, available studies strongly indicate the presence of AhR/AR crosstalk in prostate cancer cells, as various AhR ligands were reported to inhibit prostate cancer development, probably through several different mechanisms [22]. Published data suggest that only strong and potent AhR ligands are capable of inducing AR degradation through AhR activation [19].
Recently, our research team observed that the group of mostly synthetic compounds with an indole scaffold has the ability to activate AhR in hepatocarcinoma cells (AZ-AhR, derived from the parental HepG2 cell line) [29] with efficacy comparable to TCDD (5 nM).
Therefore, the objective of this study was to determine whether these indoles have the ability to suppress AR function through AhR activation and thus slow the proliferation of cancer cells.

The Effects of Indoles on AhR and AR Transcription Activity
Firstly, the new reporter cell line 22AhRv1 was constructed, characterized (Supplement S1), and subsequently used to monitor AhR transcription activity in a prostate-specific environment. The AIZ-AR reporter cell line [30] was used to monitor AR transcription activity in the absence (agonist mode) or presence (antagonist mode) of DHT.
In the 22AhRv1 reporter cell line, the ability of tested indoles to activate AhR was measured after 4 h and 24 h. Significant AhR activation was observed for 1MI, 2MI, 4MI, 5MI, 6MI, 7MI, 2,5DMI, 6MeO, 4MeO1MI, and 7MeO4MI after 4 h ( Figure 1A). Interestingly, a positive control, TCDD, did not significantly activate AhR above the level of UT after 4 h, despite significant activation after 24 h (Supplementary S1 and Figure 1B). After 24 h, all indoles significantly and dose-dependently activated AhR with efficacy comparable to TCDD ( Figure 1B). An exception to this rule was 3MI (skatole), which had no effect at the highest concentration.
In the AIZ-AR reporter cell line, the ability of the tested indoles to affect AR was measured after 24 h. DHT-inducible AR-dependent luciferase activity reached approximately 7-fold induction next to UT (Figure 2A). True AhR ligands, TCDD and FICZ, were tested as well. While TCDD had no effect, FICZ significantly induced AR-mediated luciferase activity. Furthermore, the anti-androgen ENZ significantly decreased this activity. This was probably due to the use of regular serum in the medium, which contains certain levels of androgens. Of all the compounds tested, only 7MeO markedly and significantly increased AR activity (approximately 2.5 times). Interestingly, a concentration-dependent decrease in luciferase activity was observed for 3MI (with an IC 50 approx. 10 µM).
In antagonist mode, a positive control ENZ significantly inhibited DHT-inducible ARdependent luciferase activity to the level of UT. Interestingly, TCDD decreased luciferase activity by approximately 30%, while FICZ increased it above DHT by approximately 20%. This finding suggests that the impact of AhR activation on AR activity may be strongly dependent on the nature of the AhR ligand. A significant concentration-dependent decrease in AR activation was observed for 3MI, 4MI, 1,3DMI, 2,3DMI, 2,3,7TMI, 4,6DMI, 5,6DMI, and 7MeO4MI ( Figure 2B). A decrease in AR activity was most remarkable for 3MI (with IC 50~5 µM) and 4MI (IC 50~5 0 µM). Some compounds, such as 2,5DMI, 2,3,3TMI, 7MeO, or 5MeO2MI, were able to coactivate AR in combination with DHT (10 nM), but this was consistent with their activity observed in the agonist mode ( Figure 2A). Compounds that were able to significantly activate AhR and simultaneously inhibit DHT-activated AR were used for further experiments (Table 1).
Due to the decline in luciferase activity, we performed MTT and Crystal violet assays. After 24 h of incubation, most of the substances (concentration range 1-100 µM) have been described as nontoxic by both assays, since the decrease in cell viability was not less than 20% (Supplementary S2). However, an enormous decline was observed for 3MI and partially for 4MI by means of Crystal violet assay only (Supplementary S2B). We measured a decrease of 39% and 60% of untreated cells for 3MI and 4MI, respectively. A calculated inhibitory concentration for 3MI was estimated as IC 50~6 0 µM.

Effects of Selected Indoles on the Target Gene Expression
All tested indoles increased concentration-dependent CYP1A1 mRNA expression, which is a marker of AhR activation [14]. The positive control, TCDD (10 nM), increased CYP1A1 expression by 106-fold ( Figure 3A). The weakest inducers of CYP1A1 were 4,6DMI and 5,6DMI, while 4MI was the strongest. Another AhR target gene, AhRR, was induced by TCDD, and only 4MI, 1,3DMI, and 7MeO4MI showed weak induction ( Figure 3B). Interestingly, 3 MI decreased AhRR mRNA levels.  activation was observed for 3MI, 4MI, 1,3DMI, 2,3DMI,  2,3,7TMI, 4,6DMI, 5,6DMI, and 7MeO4MI ( Figure 2B). A decrease in AR activity was most remarkable for 3MI (with IC50~5 µM) and 4MI (IC50~50 µM). Some compounds, such as 2,5DMI, 2,3,3TMI, 7MeO, or 5MeO2MI, were able to coactivate AR in combination with DHT (10 nM), but this was consistent with their activity observed in the agonist mode ( Figure 2A). Compounds that were able to significantly activate AhR and simultaneously inhibit DHT-activated AR were used for further experiments (Table 1). Due to the decline in luciferase activity, we performed MTT and Crystal violet assays. After 24 h of incubation, most of the substances (concentration range 1-100 µM) have been described as nontoxic by both assays, since the decrease in cell viability was not less than 20% (Supplementary S2). However, an enormous decline was observed for 3MI and partially for 4MI by means of Crystal violet assay only (Supplementary S2B). We measured a decrease of 39% and 60% of untreated cells for 3MI and 4MI, respectively. A calculated inhibitory concentration for 3MI was estimated as IC50~60 µM.     . The transcription activity of AR was evaluated using RGA. In agonist mode (A), the data obtained are expressed as fold inductions to UT. In antagonist mode (B), the results are expressed as a percentage, when DHT 10 nM is set to 100%. * represents a significant difference (p < 0.05) between untreated (UT) and compound-treated cells.   All tested indoles significantly reduced the DHT-inducible expression of AR target genes, namely KLK3 ( Figure 3C) and FKBP5 ( Figure 3D). Induction by DHT was approx. 1.5-fold and 4-fold for KLK3 and FKBP5, respectively. The expression of the UBE2C gene, which is regulated by AR-v7 only [31], was mildly decreased by all indoles ( Figure 3E). The strongest decrease (up to 60% of control cells) was observed for 3MI.

Binding of AR to the KLK3 Promoter after Treatment with Selected Indoles
In order to demonstrate whether the impact of the tested indoles started at the transcription level, we performed the ChIP assay. 22Rv1 cells were incubated with tested indoles (10 µM) and controls in antagonist mode (with DHT, 10 nM) for 90 min. The positive control DHT (10 nM) enriched the KLK3 promoter with AR by 2.8-4.9 fold ( Figure 4A). The presence of anti-androgen ENZ resulted in a significant reduction compared to DHT. Well known AhR ligands, TCDD and FICZ, were able to decrease a DHT-stimulated AR enrichment. A mild decrease has been observed for all tested indoles. The obtained data suggest that the observed decrease in KLK3 and FKBP5 mRNAs started already at the level of binding of AR to DNA, thus affecting AR functionality.
is set to 100% (for AR-target genes). * represents a significant difference (p < 0.05) between untreated (UT) and compound-treated cells (A,B) or DHT and compound+DHT-treated cells (C,D,E).

Binding of AR to the KLK3 Promoter after Treatment with Selected Indoles
In order to demonstrate whether the impact of the tested indoles started at the transcription level, we performed the ChIP assay. 22Rv1 cells were incubated with tested indoles (10 µM) and controls in antagonist mode (with DHT, 10 nM) for 90 min. The positive control DHT (10 nM) enriched the KLK3 promoter with AR by 2.8-4.9 fold ( Figure  4A). The presence of anti-androgen ENZ resulted in a significant reduction compared to DHT. Well known AhR ligands, TCDD and FICZ, were able to decrease a DHT-stimulated AR enrichment. A mild decrease has been observed for all tested indoles. The obtained data suggest that the observed decrease in KLK3 and FKBP5 mRNAs started already at the level of binding of AR to DNA, thus affecting AR functionality.

Effects of Selected Indoles on AR-fl and AR-v7 Protein Levels
In the context of the proposed hypothesis, we evaluated the AR protein level. A significant dose-dependent decrease was observed for both variants, AR-fl (110 kDa, Figure 5A,C) and AR-v7 (89 kDa, Figure 5B,C), exposed to 3MI, 4MI, 2,3,7TMI, and 7MeO4MI. Interestingly, 4MI in 1 µM increased the level of DHT-inducible AR-v7 protein by up to 200%. In order to verify the change in either degradation or transcription, we measured mRNA levels. And surprisingly, the mRNA levels of both AR variants decreased in a similar pattern, with the strongest effect shown by 3MI (IC50 approx. 10 µM), followed by 4MI, 2,3DMI, 2,3,7TMI, and 7MeO4MI ( Figure 5D,E). Thus, the tested indoles probably induce downregulation in AR mRNA, which is further reflected in a decrease of AR proteins.

Effects of Selected Indoles on AR-fl and AR-v7 Protein Levels
In the context of the proposed hypothesis, we evaluated the AR protein level. A significant dose-dependent decrease was observed for both variants, AR-fl (110 kDa, Figure 5A,C) and AR-v7 (89 kDa, Figure 5B,C), exposed to 3MI, 4MI, 2,3,7TMI, and 7MeO4MI. Interestingly, 4MI in 1 µM increased the level of DHT-inducible AR-v7 protein by up to 200%. In order to verify the change in either degradation or transcription, we measured mRNA levels. And surprisingly, the mRNA levels of both AR variants decreased in a similar pattern, with the strongest effect shown by 3MI (IC 50 approx. 10 µM), followed by 4MI, 2,3DMI, 2,3,7TMI, and 7MeO4MI ( Figure 5D,E). Thus, the tested indoles probably induce downregulation in AR mRNA, which is further reflected in a decrease of AR proteins.

CRISPR/Cas9 AhR Knockout
Finally, we tried to evaluate the connection between AhR, AR, and the strongest AhR activator in 22Rv1 cells, 4 MI, by genetic knockout. For this purpose, 22Rv1 cells were transiently transfected with the CRISPR/Cas9 plasmid for AhR-KO. In all experiments, a decrease in AhR mRNA was successfully observed between WT and KO samples ( Figure 6A). CYP1A1 mRNA expression in AhR KO cells decreased slightly after treatment with TCDD or 4MI in combination with or without DHT ( Figure 6B). However, the combined treatment of 4MI and DHT did not show any recurrent trend in KLK3 mRNA level ( Figure 6C) and had no impact on FKBP5 mRNA level ( Figure 6D) when comparing WT and AhR KO cells. The effect on AR mRNA levels is given in Supplementary S3. Finally, we tried to evaluate the connection between AhR, AR, and the strongest AhR activator in 22Rv1 cells, 4 MI, by genetic knockout. For this purpose, 22Rv1 cells were transiently transfected with the CRISPR/Cas9 plasmid for AhR-KO. In all experiments, a decrease in AhR mRNA was successfully observed between WT and KO samples ( Figure  6A). CYP1A1 mRNA expression in AhR KO cells decreased slightly after treatment with TCDD or 4MI in combination with or without DHT ( Figure 6B). However, the combined treatment of 4MI and DHT did not show any recurrent trend in KLK3 mRNA level ( Figure  6C) and had no impact on FKBP5 mRNA level ( Figure 6D) when comparing WT and AhR KO cells. The effect on AR mRNA levels is given in Supplementary S3.

Discussion
The main goal of this study was to demonstrate if AhR activation by certain indoles can result in the degradation or at least suppression of AR activity in prostate cancer cells. This assumption was based on the observations that strong AhR ligands degraded AR in the LNCaP prostate cell line [15,19] and that two other compounds, namely Icaritin [24] and Carbidopa [25], which could activate AhR, suppressed prostate cancer via AhRmediated degradation of AR. Effects of these compounds and indoles from our study on AhR and AR pathways are summarized in Table 2. The tested indoles were selected on the basis of a recent report by our research group, in which methyl-and methoxyindoles were identified as AhR agonists [29]. In the human hepatocarcinoma AZ-AhR cell line, all indoles activated AhR to some extent, and the strongest ones were reported to be 4 MI, 5

Discussion
The main goal of this study was to demonstrate if AhR activation by certain indoles can result in the degradation or at least suppression of AR activity in prostate cancer cells. This assumption was based on the observations that strong AhR ligands degraded AR in the LNCaP prostate cell line [15,19] and that two other compounds, namely Icaritin [24] and Carbidopa [25], which could activate AhR, suppressed prostate cancer via AhR-mediated degradation of AR. Effects of these compounds and indoles from our study on AhR and AR pathways are summarized in Table 2. The tested indoles were selected on the basis of a recent report by our research group, in which methyl-and methoxyindoles were identified as AhR agonists [29]. In the human hepatocarcinoma AZ-AhR cell line, all indoles activated AhR to some extent, and the strongest ones were reported to be 4 MI, 5 MI, 6 MI, 2,5 DMI, and 7MeO [29]. Similarly, all tested indoles activated AhR in the 22Rv1 prostate cell line after 24 h with efficacy comparable to TCDD, which drastically less activated AhR (5-fold, 10 nM) than AZ-AhR (1000-fold, 5 nM). A partial explanation of such a huge difference lies in the significantly lower amount of AhR protein in the prostate (22Rv1) than in AZ-AhR cells (personal observation). Table 2. Comparison of the effects of different compounds on AhR and AR receptors (↑ increase, ↓ decrease, -no effect; * only for certain compounds).
Further, next to the nature of a ligand/agonist of AhR, probably a specific environment plays a role since the study by Ohtake et al., 2007 [19] used LNCaP cells treated for 3 h in medium with 0.2% charcoal-stripped serum, while we used 22Rv1 cells in medium with 10% regular serum and added 10 nM DHT to mimic basal androgen secretion in the human body. Another difference between these two cell lines lies in the presence of AR variants, where LNCaP has one (AR-fl), while 22Rv1 has two (AR-fl, AR-v7) [5]. Furthermore, AR-v7 displays nuclear localization even in the absence of androgen and acts as a transcription factor [5].
Additionally, it seems that different types of prostate cancer cells have shown different sensitivity to affecting the AR pathways through AhR activation. The AR degradation process through AhR activation was not identified in all types of prostate cancer cells. In the androgen-sensitive LNCaP cell line, which was isolated from the left supraclavicular lymph [32], the mechanism of AR degradation through AhR activation by a strong ligand has been observed multiple times [20,22]. LNCaP cells are classified as AR and AhR-positive [21]. However, the same AhR ligand (TCDD) did not induce AR degradation in the castration-resistant C4-2 cell line [20], which was derived from the parental LNCaP [33]. This may be due to the fact that different types of prostate cancer are diverse in AhR and AR receptor content, and subcellular localization, and that AhR presence may affect AR phosphorylation status [34]. This is probably also reflected in our data, since ChIP results demonstrated a decrease in AR binding to the KLK3 promoter after 90 min (Figure 4), while AR protein levels ( Figure 5) were almost unaffected by most of the tested indoles after 24 h with the 10 µM concentrations used in ChIP. Thus, our results suggest a mix of potential post-translational modification of AR or affected interaction with other transcription partners. This consequently leads to a decrease in AR binding to the KLK3 promoter and a decrease in the mRNA levels of AR-target genes.
Probably the most interesting finding is the impact of 3MI (skatole) on AR activity and cell viability. Skatole is naturally a product of the intestinal microbiota and can be found in wide range of concentrations in the serum at least of patients with hepatic encephalopathy [35]. Unfortunately, it is not known what the average concentration of skatole in the serum of healthy individuals is. Therefore, our results may suggest a hypothesis that men with detectable skatole concentration in the serum are less likely to develop/have AR-dependent prostate cancer. The proposition of this hypothesis is based on the observation of a decline in all AR-mediated parameters we studied, as well as on the strongest decline in the Crystal violet assay, which is a reflection of the proliferative capacity of the cells.
Furthermore, we observed a visible morphological change in 22Rv1 cells at the end of skatole treatment (personal observation). Thus, it is likely that skatole triggers some sort of apoptotic event and apparently has more molecular targets inside the cells. Our assumption is based on the observation of different skatole action in relation to other indoles as it reduced rather than induced AhRR mRNA ( Figure 3B) and consistently induced concentration-dependently AhR mRNA (personal observation). The expression of AhRR and AhR is regulated by NF-kB [36], and the combination of genotoxic action, demonstrated for skatole in bronchial cells [37] (that is, activation of p53), and activation of NF-kB could explain these differences. However, this must be revealed in future research as a possible relationship (if any) between skatole blood level and prostate cancer incidence in men.
We believe that skatole deserves further investigation in the future in relation to prostate cancer.
The hypothesis of AR degradation through AhR activation by selected indolic compounds was tested. All 22 tested indoles displayed promising AhR-activating potential in the newly developed 22AhRv1 reporter cell line. However, only 8 of them were able to supress DHT-induced AR activation, namely 3MI, 4MI, 1,3DMI, 2,3DMI, 2,3,7TMI, 4,6DMI, 5,6DMI, and 7MeO4MI. At the mRNA level, 8 selected indoles increased CYP1A1 expression and significantly reduced DHT-inducible KLK3 and FKBP5 expression. Moreover, following ChIP analysis revealed reduced DHT-inducible binding of AR to the KLK3 promoter by selected indoles. The effect of the strongest AhR activator in this study, 4MI, was further monitored using transient transfection with the CRISPR/Cas9 AhR KO plasmid. However, after AhR KO, no change in AR-targets was observed. To conclude, some tested indoles showed the ability to suppress DHT-induced AR activation; however, this phenomenon does not seem to be associated with AhR activation. Therefore, the hypothesis of AR degradation via AhR activation for selected indoles has not been confirmed.

Cell Lines
Human prostate carcinoma epithelial cell lines 22Rv1 (ECACC No. 105092802) and AIZ-AR [30] were cultured in Rosewell Park Memorial Institute (RPMI) 1640 medium supplemented with 10% fetal bovine serum (FBS), 1% non-essential amino acids, and 2 mM L-glutamine (Sigma-Aldrich, Missouri, USA). At the beginning of the experiments, GENERI BIOTECH s.r.o. (Hradec Králové, Czech Republic) performed the authentication of the 22Rv1 cell line. Cells were maintained in a humidified incubator at 37 • C and 5% CO 2 . Cell lines were regularly tested for the presence of mycoplasma using the MycoAlert TM Mycoplasma Detection Kit (Lonza, Basilej, Switzerland).

Compounds and Reagents
The tested indoles were selected based on previous research [29] in our laboratory and are listed in Table 3. The table contains key structures of tested indoles is given in Supplementary S4. The chemicals used are listed in Supplementary S5.

Reporter Gene Assay (RGA)
Initially, a cellular system was established to monitor AhR transcription activity in the 22Rv1 cell line (Supplementary S1). AIZ-AR reporter cell line [30] was used for evaluation of AR transcription activity. Cells were seeded in 96-well plates at a density of 2 × 10 4 cells per well in a volume of 200 µL and stabilized overnight. 22AhRv1 cells were incubated with tested indoles for 4 h and 24 h. AIZ-AR cells were treated with indoles for 24 h in agonist and antagonist mode (in the presence of DHT 10 nM). DMSO (untreated; 0.1%; v/v) was used as the vehicle/negative control, TCDD (10 nM) was used as the positive control in 22AhRv1 and DHT (10 nM) was used as the AIZ-AR positive control. Furthermore, anti-androgen ENZ (10 µM) was used as AR suppression control in AIZ-AR cells, and the effects of TCDD (10 nM) and FICZ (10 µM) in the presence or absence of DHT (10 nM) were also evaluated. After treatments, cells were lysed with 1x Reporter Lysis Buffer (Promega, Wisconsin, USA) and luciferase activity was measured with the Infinite M200.

Quantitative Reverse Transcriptase PCR (RT-qPCR)
Only indoles capable of activating AhR and simultaneously suppressing AR activity were selected for PCR analysis. Cells were seeded in 6-well plates at a density of 1.5 × 10 6 cells per well in a volume of 1.5 mL and stabilized overnight. Cells were treated with 8 selected indoles in 4 concentrations (1, 10, 50, and 100 µM) in antagonist conditions (with DHT at 10 nM). After 24 h of treatment, cells were washed with PBS, and total mRNA was isolated using TRI Reagent ® (Molecular Research Centre, Ohio, USA), according to protocol. Quality was monitored in the A260/A280 ratio. cDNA was synthesized from 1000 ng of total RNA using M-MuLV Reverse Transctiptase (New England BioLabs, Massachusetts, USA) at 42 • C for 60 min in the presence of Random Primer 6 (100 pmol/µL; New England BioLabs). Subsequently, enzyme activity was inactivated when incubated at 65 • C for 10 min in Dry Bath Incubator (Major Science, California, USA). The mRNA expression was evaluated with KiCqStart ® Probe Assays (Sigma-Aldrich) or with SYBR ® Green (Roche Diagnostics, Prague, Czech Republic) according to the manufacturer's recommendations. The expression of genes related to the AhR pathway (AhR, AhRR, CYP1A1) and AR-target genes (AR-fl, AR-v7, FKBP5, KLK3, UBE2C) was monitored. The list of used probes and primers is given in Table 4. qRT-PCR was performed on the Light Cycler 480 II apparatus (Roche Diagnostic), and the reaction settings for KiCqStart ® Probe Assays analysis are shown in Table 5. The reaction by SYBR ® Green analysis was performed according to the manufacturer s recommendations. Sample measurements, including the non-template control (NTC), were performed in triplicate, and gene expression was normalized to the housekeeping gene GAPDH. The data obtained were evaluated by the delta-delta method. Table 4. Sequences of used primers and probes.

Western Blot
Cells were seeded in 6-well plates at a density of 1.5 × 10 6 cells per well in a 1.5 mL volume and stabilized. The treatment was similar to that for RT-qPCR. Total protein extracts were isolated for each sample after 24 h of treatment. Cells were washed with 1× PBS, scraped into 1 mL of PBS (cold) and centrifuged (4000 rpm/1500 rcf, 3 min, 4 • C). Pellet was re-suspended in 80 µL protein lysis buffer (pH 7.5; 50 mM HEPES, 5 mM EDTA, 150 mM NaCl, 1% Triton X-100 with anti-protease and anti-phosphatase cocktail) and centrifuged at 13 000 rpm (14,500 rcf), 15 min, 4 • C. The supernatant was collected, and the protein concentration in each sample was determined by 1x Bradford reagent (Sigma Aldrich). Protein samples were separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE; 10% running gel, 4% stacking gel) in the BioRad Miniprotean system (California, USA), according to the manufacturer's recommendations. SDS-PAGE was followed by semi-dry protein transfer onto a polyvinylidene difluoride (PVDF) membrane. The membranes were stained with Ponceau S Rouge solution (0.1% w/v in 5% acetic acid), washed with 1xTBS/Tween, and incubated with 5% non-fat dried milk for 1 h at room temperature (RT). Membranes were incubated overnight with appropriate antibody diluted in 5% solution of bovine serum albumin (BSA) in 1xTBS/Tween at 4 • C. After incubation, the membranes were washed with 1xTBS/Tween and incubated with secondary horseradish peroxidase-conjugated antibody diluted in 5% non-fat dried milk for 1 h at RT. List of used antibodies and their concentrations is given in Table 6. Membranes were analyzed using WesternSure ® PREMIUM Chemiluminiscent Substrate (Li-Cor, Nebraska USA) and the C-DiGit Chemiluminiscence Western Blot Scanner (Li-Cor). Obtained results were processed by Image Studio 5.0 for C-DiGit Scanner software. Protein expression was normalized per β-actin (43 kDa). 22Rv1 cells were seeded in a 60-mm plate at a density of 4 × 10 6 cells per plate in a 4 mL volume and stabilized overnight. The following day, cells were incubated with selected indoles in antagonist mode (only 10 µM concentration with DHT 10 nM) and controls (DMSO in a ratio of 1:1000; DHT 10 nM). Furthermore, the effect of some other compounds (TCDD 10 nM; FICZ 10 µM; ENZ 10 µM) in combination with DHT 10 nM was evaluated. Cells were incubated with the tested compounds for 90 min at 37 • C. Subsequently, ChIP was performed according to the manufacturer's recommendations in the manual for the Simple ChIP Plus Enzymatic Chromatin IP Kit (Cell Signaling Technology, Danvers, MA, USA) as previously described, with minor modifications [29]. Briefly, an aliquot of 15 µg of digested chromatin was resuspended in ChIP buffer in total volume of 500 µL for each sample and incubated overnight with ChIP validated antibody (4 µL of anti-AR antibody; Cell Signalling Technology). Also, a control sample with normal rabbit IgG was prepared (1 µL of IgG antibody). The following day, 25 µL of Protein G magnetic beads were added to each sample and incubated with rotation for 45 min at 4 • C. The beads were separated in the Magnetic Separation Rack, and subsequently several washing steps (using low-and high-salt buffer, according to the manufacturer) were performed. Then, 150 µL of ChIP elution buffer was added to each sample. The elution was achieved with incubation at 65 • C for 30 min with shaking (1200 rpm/100 rcf). Magnetic beads were separated, and eluted chromatin was transferred into a clear tube. After that, 6 µL of NaCl (5 M) and 2 µL of proteinase K were added to each sample and incubated at 65 • C for 15 min with shaking (1200 rpm/100 rcf). Thus, 750 µL of DNA binding buffer were added to each sample, which was briefly vortexed and centrifuged. Samples were transferred to spin columns and washed with 600 µL of DNA wash buffer. Chromatin was eluted from columns by adding 45 µL of DNA elution buffer and collected in new tubes. The result analysis was performed using RT-qPCR in Light Cycler 480. For each well, the reaction mix contained 2 µL of eluted ChIP sample, 5 µL SYBR Green (Roche), 2 µL of PCR grade H 2 O (Roche) and 1 µL of KLK3 Promoter Primers (SimpleChIP, Cell Signaling). The setting of this reaction is given in Table 7. For the purpose of agarose gel analysis, the next PCR run was performed with elongation for 30 cycles only. The product of such a reaction was analyzed using agarose electrophoresis (4% gel, 65 V, 1.5 h). Samples were dyed with GelRed ® nucleic acid stain (Biotium, California, USA). The result was visualized with the Syngene G:BOX gel documentation system (Cambridge, UK).

CRISPR/Cas9 AhR Knock-Out
To verify the relationship between AhR and AR, 22Rv1 cells were transiently transfected with an AhR CRISPR/Cas9 KO plasmid according to the manufacturer's protocol (Santa cruz Biotechnology, Texas, USA), with minor modifications. Briefly, 22Rv1 cells were seeded in a 6-well plate (2 × 10 5 cells and 3 mL of medium per well) and stabilized for 24 h in a humidified incubator (80% confluence). Subsequently, cells were transfected with the CRISPR/Cas9 AhR KO plasmid or with the control CRISPR/Cas9 plasmid, as a negative control. Solution A, 1 µg of plasmid DNA in Plasmid Transfection Medium in a total volume of 150 µL, and solution B, 5 µL of UltraCruz ® Transfection Reagent in Plasmid Transfection Medium in a total volume of 150 µL, were prepared for each well and let stand for 5 min at RT. Subsequently, solution A was added to solution B, vortexed, and incubated for 20 min at RT.
Plates with stabilized cells were transferred to the flow box, and the growth medium was replaced by a fresh one. To each well, 300 µL of transfection solution A + B was added dropwise. The plate was gently mixed by swirling, and cells were incubated with transfection reagents for 48 h. After incubation, the transfection process was visually confirmed by fluorescence microscopy by detection of green fluorescence protein (GFP). Subsequently, transiently transfected cells were exposed to the tested compounds (UT, DHT 10 nM, TCDD 10 nM with or without DHT 10 nM, 4 MI 100 µM with or without DHT 10 nM) for 24 h. Total mRNA was isolated, and the expression of genes (AhR, CYP1A1, AR-fl, KLK3, and FKBP5) was evaluated as described earlier (Section 4.4). For evaluating AhR mRNA levels, specific primers were designed for exon 5, which is the target DNA sequence for the CRISPR/Cas9 AhR KO plasmid.

Statistical Analysis
The obtained data were processed using GraphPad Prism Version 9.4.1 (GraphPad Software, San Diego, CA, USA). Significant values in all experiments were determined by two-way ANOVA (symbol * in the charts). Western blot results were analysed using Image Studio 5.0 for C-DiGit Scanner software (Li-cor, Nebraska, USA).