Protein kinase D1 mitigation against etoposide induced DNA damage in prostate cancer is associated with increased α-Catenin.

IF 2.6 3区医学 Q3 ENDOCRINOLOGY & METABOLISM Prostate Pub Date : 2024-10-20 DOI:10.1002/pros.24812

Sanjeev Shukla, Teruko Osumi, Mohammed Al-Toubat, Samuel Serrano, Pankaj Kumar Singh, Mario Mietzsch, Robert McKenna, Jonathan Chardon-Robles, Sunil Krishnan, K C Balaji

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Abstract

Background: The E-cadherin, α- and β-Catenin interaction at the cell adherens junction plays a key role in cell adhesion; alteration in the expression and function of these genes are associated with disease progression in several solid tumors including prostate cancer. The membranous β-Catenin is dynamically linked to the cellular cytoskeleton through interaction with α-Catenin at amino acid positions threonine 120 (T120) to 151 of β-Catenin. Nuclear presence of α-Catenin modulates the sensitivity of cells to DNA damage. The objective of this study is to determine the role of α-Catenin and protein kinase D1 (PrKD1) in DNA damage response.

Methods: Prostate cancer cells; LNCaP, LNCaP (Sh-PrKD1; silenced PrKD1), C4-2 and C4-2 PrKD1 were used for various sets of experiments to determine the role of DNA damage in PrKD1 overexpression and silencing cells. These cells were treated with compound-10 (100 nM) and Etoposide (30 µM), total cell lysates, cytosolic and nuclear fractions were prepared to observe various protein expressions. We performed single cell gel electrophoresis (COMET assay) to determine the etoposide induce DNA damage in C4-2 and C4-2 PrKD1 cells. The animal experiments were carried out to determine the tolerability of compound-10 by mice and generate preliminary data on efficacy of compound-10 in modulating the α-Catenin and PrKD1 expressions in inhibiting tumor progression.

Results: PrKD1, a novel serine threonine kinase, phosphorylates β-Catenin T120. In silico analysis, confirmed that T120 phosphorylation alters β- to α-Catenin binding. Forced expression of PrKD1 in prostate cancer cells increased β- and α-Catenin protein levels associated with reduced etoposide induced DNA damage. Downregulation of α-Catenin abrogates the PrKD1 mitigation of DNA damage. The in vitro results were corroborated in vivo using mouse prostate cancer patient derived xenograft model by inhibition of PrKD1 kinase activity with compound-10, a selective PrKD inhibitor, demonstrating decreased total β- and α-Catenin protein levels, and β-Catenin T120 phosphorylation.

Conclusions: Alteration in DNA damage response pathways play major role in prostate cancer progression. The study identifies a novel mechanism of α-Catenin dependent DNA damage mitigation role for PrKD1 in prostate cancer.

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蛋白激酶 D1 对依托泊苷诱导的前列腺癌 DNA 损伤的缓解与 α-Catenin 的增加有关。

背景：细胞粘附连接处的E-cadherin、α-和β-Catenin相互作用在细胞粘附中起着关键作用；这些基因表达和功能的改变与包括前列腺癌在内的几种实体瘤的疾病进展有关。膜β-Catenin通过在β-Catenin的苏氨酸120（T120）至151的氨基酸位置与α-Catenin相互作用而与细胞骨架动态连接。α-Catenin的核存在可调节细胞对DNA损伤的敏感性。本研究旨在确定α-Catenin和蛋白激酶D1（PrKD1）在DNA损伤反应中的作用：方法：使用前列腺癌细胞LNCaP、LNCaP（Sh-PrKD1；沉默PrKD1）、C4-2和C4-2 PrKD1进行多组实验，以确定DNA损伤在PrKD1过表达和沉默细胞中的作用。用化合物-10（100 nM）和依托泊苷（30 µM）处理这些细胞，制备总细胞裂解液、细胞膜和核分馏物以观察各种蛋白质的表达。我们对 C4-2 和 C4-2 PrKD1 细胞进行了单细胞凝胶电泳（COMET 检测），以确定依托泊苷诱导的 DNA 损伤。我们还进行了动物实验，以确定小鼠对化合物-10的耐受性，并得出化合物-10在抑制肿瘤进展过程中调节α-Catenin和PrKD1表达的初步数据：结果：PrKD1是一种新型丝氨酸苏氨酸激酶，能使β-Catenin T120磷酸化。硅学分析证实，T120磷酸化改变了β与α-Catenin的结合。在前列腺癌细胞中强制表达 PrKD1 可提高 β- 和 α-Catenin 蛋白水平，并减少依托泊苷诱导的 DNA 损伤。下调α-Catenin会减弱PrKD1对DNA损伤的缓解作用。使用选择性PrKD抑制剂化合物-10抑制PrKD1激酶的活性，显示总β和α-Catenin蛋白水平降低，β-Catenin T120磷酸化减少，从而在小鼠前列腺癌患者衍生的异种移植模型中证实了体外实验结果：结论：DNA损伤应答通路的改变在前列腺癌的进展中起着重要作用。结论：DNA损伤应答通路的改变在前列腺癌的进展中起着重要作用。该研究发现了PrKD1在前列腺癌中依赖于α-Catenin的DNA损伤缓解作用的新机制。

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来源期刊

Prostate 医学-泌尿学与肾脏学

CiteScore

5.10

自引率

3.60%

发文量

180

审稿时长

1.5 months

期刊介绍： The Prostate is a peer-reviewed journal dedicated to original studies of this organ and the male accessory glands. It serves as an international medium for these studies, presenting comprehensive coverage of clinical, anatomic, embryologic, physiologic, endocrinologic, and biochemical studies.