靶向 SKP2 和 KDM5B 通过诱导衰老和凋亡来阻断 AKT 信号通路抑制前列腺癌的进展。

Co-targeting SKP2 and KDM5B inhibits prostate cancer progression by abrogating AKT signaling with induction of senescence and apoptosis.

机构信息

Department of Biomedical Sciences, School of Graduate Studies, Meharry Medical College, Nashville, Tennessee, USA.

Department of Biochemistry, Cancer Biology, Neuroscience and Pharmacology, Meharry Medical College, Nashville, Tennessee, USA.

出版信息

Prostate. 2024 Jun;84(9):877-887. doi: 10.1002/pros.24706. Epub 2024 Apr 11.

DOI:10.1002/pros.24706

PMID:38605532

Abstract

BACKGROUND

Prostate cancer (PCa) is the second-leading cause of cancer mortalities in the United States and is the most commonly diagnosed malignancy in men. While androgen deprivation therapy (ADT) is the first-line treatment option to initial responses, most PCa patients invariably develop castration-resistant PCa (CRPC). Therefore, novel and effective treatment strategies are needed. The goal of this study was to evaluate the anticancer effects of the combination of two small molecule inhibitors, SZL-P1-41 (SKP2 inhibitor) and PBIT (KDM5B inhibitor), on PCa suppression and to delineate the underlying molecular mechanisms.

METHODS

Human CRPC cell lines, C4-2B and PC3 cells, were treated with small molecular inhibitors alone or in combination, to assess effects on cell proliferation, migration, senescence, and apoptosis.

RESULTS

SKP2 and KDM5B showed an inverse regulation at the translational level in PCa cells. Cells deficient in SKP2 showed an increase in KDM5B protein level, compared to that in cells expressing SKP2. By contrast, cells deficient in KDM5B showed an increase in SKP2 protein level, compared to that in cells with KDM5B intact. The stability of SKP2 protein was prolonged in KDM5B depleted cells as measured by cycloheximide chase assay. Cells deficient in KDM5B were more vulnerable to SKP2 inhibition, showing a twofold greater reduction in proliferation compared to cells with KDM5B intact (p < 0.05). More importantly, combined inhibition of KDM5B and SKP2 significantly decreased proliferation and migration of PCa cells as compared to untreated controls (p < 0.005). Mechanistically, combined inhibition of KDM5B and SKP2 in PCa cells abrogated AKT activation, resulting in an induction of both cellular senescence and apoptosis, which was measured via Western blot analysis and senescence-associated β-galactosidase (SA-β-Gal) staining.

CONCLUSIONS

Combined inhibition of KDM5B and SKP2 was more effective at inhibiting proliferation and migration of CRPC cells, and this regimen would be an ideal therapeutic approach of controlling CRPC malignancy.

摘要

背景

前列腺癌（PCa）是美国癌症死亡的第二大原因，也是男性最常见的恶性肿瘤。虽然雄激素剥夺疗法（ADT）是初始反应的一线治疗选择，但大多数 PCa 患者最终都会发展为去势抵抗性 PCa（CRPC）。因此，需要新的有效治疗策略。本研究的目的是评估两种小分子抑制剂 SZL-P1-41（SKP2 抑制剂）和 PBIT（KDM5B 抑制剂）联合抑制 PCa 的抗癌作用，并阐明其潜在的分子机制。

方法

用小分子抑制剂单独或联合处理人 CRPC 细胞系 C4-2B 和 PC3，以评估对细胞增殖、迁移、衰老和凋亡的影响。

结果

在 PCa 细胞中，SKP2 和 KDM5B 在翻译水平上呈负相关调节。与表达 SKP2 的细胞相比，SKP2 缺陷细胞的 KDM5B 蛋白水平增加。相比之下，与 KDM5B 完整的细胞相比，KDM5B 缺陷细胞的 SKP2 蛋白水平增加。用环己酰亚胺追踪实验测量，KDM5B 耗竭细胞中 SKP2 蛋白的稳定性延长。与 KDM5B 完整的细胞相比，KDM5B 缺陷细胞对 SKP2 抑制更为敏感，增殖减少了两倍（p<0.05）。更重要的是，与未处理的对照组相比，联合抑制 KDM5B 和 SKP2 显著降低了 PCa 细胞的增殖和迁移（p<0.005）。从机制上讲，联合抑制 PCa 细胞中的 KDM5B 和 SKP2 阻断了 AKT 的激活，导致细胞衰老和凋亡的诱导，这通过 Western blot 分析和衰老相关β-半乳糖苷酶（SA-β-Gal）染色来测量。