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1. DCAF16-Based Covalent Degradative Handles for the Modular Design of Degraders

   https://doi.org/10.1101/2025.04.25.650514  

   Orr, Lauren M; Tomlinson, Sydney J; Grupe, Hannah R; Lim, Melissa; Ho, Emily; Yilmaz, Halime; Zhou, Grace; Leon, Barbara; Olzmann, James A; Nomura, Daniel K (April 2025, bioRxiv)

   Abstract Targeted protein degradation (TPD) is a powerful strategy for targeting and eliminating disease-causing proteins. While heterobifunctional Proteolysis-Targeting Chimeras (PROTACs) are more modular, the rational design of monovalent or molecular glue degraders remains challenging. In this study, we generated a small library of BET-domain inhibitor JQ1 analogs bearing elaborated electrophilic handles to identify permissive covalent degradative handles and E3 ligase pairs. We identified an elaborated fumaramide handle that, when appended onto JQ1, led to the proteasome-dependent degradation of BRD4. Further characterization revealed that the E3 ubiquitin ligase CUL4^DCAF16—a common E3 ligase target of electrophilic degraders—was responsible for BRD4 loss by covalently targeting C173 on DCAF16. While this original fumaramide handle, when appended onto other protein-targeting ligands, did not accommodate the degradation of other neo-substrates, a truncated version of this handle attached to JQ1 was still capable of degrading BRD4, now through targeting both C173 and C178. This truncated fumaramide handle, when appended on various protein targeting ligands, and was also more permissive in degrading other neo-substrates, including CDK4/6, SMARCA2/4, and the androgen receptor (AR). We further demonstrated that this optimized truncated fumaramide handle, when transplanted onto an AR DNA binding domain-targeting ligand, could degrade both AR and the undruggable truncation variant of AR, AR-V7, in androgen-independent prostate cancer cells in a DCAF16-dependent manner. Overall, we have identified a unique DCAF16-targeting covalent degradative handle that can be transplanted across several protein-targeting ligands to induce the degradation of their respective targets for the modular design of monovalent or bifunctional degraders. 

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2. Sulfinyl Aziridines as Stereoselective Covalent Destabilizing Degraders of the Oncogenic Transcription Factor MYC

   https://doi.org/10.1101/2025.02.24.639755  

   Rosen, Hannah T; Li, Kelvin; Li, Erin L; Currier, Brynne; Brittain, Scott M; Garcia, Francisco J; Beard, Diana C; Haenni-Holzinger, Sandra; Dovala, Dustin; McKenna, Jeffrey M; et al (February 2025, bioRxiv)

   Abstract While MYC is a significant oncogenic transcription factor driver of cancer, directly targeting MYC has remained challenging due to its intrinsic disorder and poorly defined structure, deeming it “undruggable.” Whether transient pockets formed within intrinsically disordered and unstructured regions of proteins can be selectively targeted with small molecules remains an outstanding challenge. Here, we developed a bespoke stereochemically-paired spirocyclic oxindole aziridine covalent library and screened this library for degradation of MYC. Through this screen, we identified a hit covalent ligand KL2-236, bearing a unique sulfinyl aziridine warhead, that engaged MYCin vitroas pure MYC/MAX protein complex andin situin cancer cells to destabilize MYC, inhibit MYC transcriptional activity and degrade MYC in a proteasome-dependent manner through targeting intrinsically disordered C203 and D205 residues. Notably, this reactivity was most pronounced for specific stereoisomers of KL2-236 with a diastereomer KL4-019 that was largely inactive. Mutagenesis of both C203 and D205 completely attenuated KL2-236-mediated MYC degradation. We have also optimized our initial KL2-236 hit compound to generate a more durable MYC degrader KL4-219A in cancer cells. Our results reveal a novel ligandable site within MYC and indicate that certain intrinsically disordered regions within high-value protein targets, such as MYC, can be interrogated by isomerically unique chiral small molecules, leading to destabilization and degradation. 

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3. Abstract P2386: Androgen Receptor Signaling Promotes YAP1 Nuclear Localization

   Cinar, B: Al-Mathkour; Khan, S. and (January 2019, ASCB-EMBO 2018 Annual Meeting)

   The transcriptional coactivator YAP1 (yes-associated protein 1) is a critical nuclear effector of the Hippo pathway. The serine/threonine protein kinases STK3/4 and LATS1/2, core components of the Hippo pathway, phosphorylate and inhibit YAP1 nuclear localization. Previously, we reported that the interaction of nuclear YAP1 with androgen receptor (AR) might play a critical role in prostate cancer progression and therapeutic relapse (Kuser-Abali et al., Nat. Commun. 2015). Here, we investigated the regulation of YAP1 by androgens in isogenic, androgen-responsive LNCaP and androgen non-responsive C4-2 prostate cancer cell models. We demonstrated that androgen suppressed the inhibitory phospho-Ser127 site on YAP1 in LNCaP cells, but the effects of androgen on phospho-Ser127 was modest in C4-2 cells. In agreement with this observation, androgen increased the presence of nuclear YAP1 in LNCaP cells, whereas regardless of androgen exposure the YAP1 protein was primarily expressed in C4-2 cell nuclei. We also demonstrated that androgen exposure suppressed the levels of phospho-Ser127 induced by okadaic acid, which is a potent inhibitor of the Ser/Thr phosphatases PP1 and PP2A. Moreover, the pharmacological inhibition of androgen receptor (AR) signaling by enzalutamide reversed the inhibitory effects of androgen on phospho-Ser127, which coincided with the inhibition of YAP1 nuclear localization. Similarly, the genetic inhibition of AR signaling by small interfering RNA (siRNA) reduced phospho-Ser127 levels. Additionally, the silencing of the STK3/4 and LATS1/2 signaling by siRNA resulted in increases in YAP1 protein levels. Furthermore, our analysis of the TCGA (The Cancer Genome Atlas) prostate adenocarcinoma data set indicates that the levels of YAP1 and AR mRNA expression were positively correlated in prostate cancer clinical samples. These observations suggest that AR signaling promotes YAP1 nuclear localization by suppressing phospho-Ser127, possibly through the protein phosphatases PP1 and PP2A, and supporting a new mechanism of YAP1 regulation and YAP1-mediated cancer cell growth and survival. 

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4. Aurora Kinase A-YBX1 Synergy Fuels Aggressive Oncogenic Phenotypes and Chemoresistance in Castration-Resistant Prostate Cancer

   https://doi.org/10.3390/cancers12030660  

   Nikhil, Kumar; Raza, Asif; Haymour, Hanan S.; Flueckiger, Benjamin V.; Chu, Jiachong; Shah, Kavita (March 2020, Cancers)

   Multifunctional protein YBX1 upregulation promotes castration-resistant prostate cancer (CRPC). However, YBX1 protein abundance, but not its DNA status or mRNA levels, predicts CRPC recurrence, although the mechanism remains unknown. Similarly, the mechanism by which YBX1 regulates androgen receptor (AR) signaling remains unclear. We uncovered the first molecular mechanism of YBX1 upregulation at a post-translational level. YBX1 was identified as an Aurora Kinase-A (AURKA) substrate using a chemical screen. AURKA phosphorylates YBX1 at two key residues, which stabilizes it and promotes its nuclear translocation. YBX1 reciprocates and stabilizes AURKA, thereby initiating a synergistic loop. Notably, phospho-resistant YBX1 is dominant-negative and fully inhibits epithelial to mesenchymal transition, chemoresistance, drug-resistance and tumorigenesis in vivo. Unexpectedly, we further observed that YBX1 upregulates AR post-translationally by preventing its ubiquitylation, but not by increasing its transcription as reported before. Uncovering YBX1-mediated AR stabilization is highly significant due to AR’s critical role in both androgen-sensitive prostate cancer and CRPC. As YBX1 inhibitors are unknown, AURKA inhibitors provide a potent tool to degrade both YBX1 and AR simultaneously. Finally, this is the first study to show a reciprocal loop between YBX1 and its kinase, indicating that their concomitant inhibition will be act synergistically for CRPC therapy. 

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5. Coupled Feedback Loops Involving PAGE4, EMT and Notch Signaling Can Give Rise to Non-Genetic Heterogeneity in Prostate Cancer Cells

   https://doi.org/10.3390/e23030288  

   Singh, Divyoj; Bocci, Federico; Kulkarni, Prakash; Jolly, Mohit Kumar (March 2021, Entropy)

   null (Ed.)

   Non-genetic heterogeneity is emerging as a crucial factor underlying therapy resistance in multiple cancers. However, the design principles of regulatory networks underlying non-genetic heterogeneity in cancer remain poorly understood. Here, we investigate the coupled dynamics of feedback loops involving (a) oscillations in androgen receptor (AR) signaling mediated through an intrinsically disordered protein PAGE4, (b) multistability in epithelial–mesenchymal transition (EMT), and (c) Notch–Delta–Jagged signaling mediated cell-cell communication, each of which can generate non-genetic heterogeneity through multistability and/or oscillations. Our results show how different coupling strengths between AR and EMT signaling can lead to monostability, bistability, or oscillations in the levels of AR, as well as propagation of oscillations to EMT dynamics. These results reveal the emergent dynamics of coupled oscillatory and multi-stable systems and unravel mechanisms by which non-genetic heterogeneity in AR levels can be generated, which can act as a barrier to most existing therapies for prostate cancer patients. 

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