Matthew D Poskus, Jacob McDonald, Matthew Laird, Ruxuan Li, Kyle Norcoss, Ioannis K Zervantonakis
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Candidate targets for combination therapy were identified using differential expression and multivariate regression modeling. Follow-up experiments were performed to evaluate the effects of HER2 kinase combination therapies in fibroblast-protected cancer cell lines and fibroblasts.</p><p><strong>Results: </strong>Compared to monoculture, fibroblast-conditioned medium increased the expression of plasminogen activator inhibitor-1 (PAI1) and cell cycle regulator polo like kinase 1 (PLK1) in lapatinib-treated breast cancer cells. Combination therapy of lapatinib with inhibitors targeting either PAI1 or PLK1, eliminated fibroblast-protected cancer cells, under both conditions of direct coculture with fibroblasts and protection by fibroblast-conditioned medium. Analysis of publicly available, clinical transcriptomic datasets revealed that HER2-targeted therapy fails to suppress PLK1 expression in stroma-rich HER2+ breast tumors and that high PAI1 gene expression associates with high stroma density. Furthermore, we showed that an epigenetics-directed approach using a bromodomain and extraterminal inhibitor to globally target fibroblast-induced proteomic adaptions in cancer cells, also restored lapatinib sensitivity.</p><p><strong>Conclusions: </strong>Our data-driven framework of proteomic profiling in breast cancer cells identified the proteolytic degradation regulator PAI1 and the cell cycle regulator PLK1 as predictors of fibroblast-mediated treatment resistance. Combination therapies targeting HER2 kinase and these fibroblast-induced signaling adaptations eliminates fibroblast-protected HER2+ breast cancer cells.</p><p><strong>Supplementary information: </strong>The online version contains supplementary material available at 10.1007/s12195-024-00823-0.</p>","PeriodicalId":9687,"journal":{"name":"Cellular and molecular bioengineering","volume":"17 5","pages":"491-506"},"PeriodicalIF":2.3000,"publicationDate":"2024-10-11","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC11538110/pdf/","citationCount":"0","resultStr":"{\"title\":\"Rational Design of HER2-Targeted Combination Therapies to Reverse Drug Resistance in Fibroblast-Protected HER2+ Breast Cancer Cells.\",\"authors\":\"Matthew D Poskus, Jacob McDonald, Matthew Laird, Ruxuan Li, Kyle Norcoss, Ioannis K Zervantonakis\",\"doi\":\"10.1007/s12195-024-00823-0\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><strong>Introduction: </strong>Fibroblasts, an abundant cell type in the breast tumor microenvironment, interact with cancer cells and orchestrate tumor progression and drug resistance. 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引用次数: 0
摘要
导言:成纤维细胞是乳腺肿瘤微环境中一种丰富的细胞类型,它与癌细胞相互作用,并协调肿瘤的进展和耐药性。然而,人们对成纤维细胞衍生因子影响药物敏感性的机制仍知之甚少。在此,我们根据蛋白质组学分析结果开发出合理的联合疗法,以克服成纤维细胞介导的 HER2+ 乳腺癌细胞的耐药性:方法:在单培养和暴露于乳腺成纤维细胞调节培养基的条件下,研究了HER2激酶抑制剂拉帕替尼的药物敏感性。使用反相蛋白质阵列测量蛋白质表达。利用差异表达和多变量回归模型确定了联合疗法的候选靶点。后续实验评估了HER2激酶联合疗法在成纤维细胞保护癌细胞株和成纤维细胞中的效果:结果:与单培养相比,成纤维细胞条件培养基增加了拉帕替尼治疗的乳腺癌细胞中纤溶酶原激活物抑制剂-1(PAI1)和细胞周期调节剂polo like kinase 1(PLK1)的表达。拉帕替尼与针对PAI1或PLK1的抑制剂联合治疗,在与成纤维细胞直接共培养和成纤维细胞调节培养基保护两种条件下,都能消除成纤维细胞保护的癌细胞。对公开的临床转录组数据集的分析表明,HER2靶向疗法无法抑制富含基质的HER2+乳腺肿瘤中PLK1的表达,PAI1基因的高表达与基质密度高有关。此外,我们还发现了一种以表观遗传学为导向的方法,该方法使用溴链和外膜抑制剂来全面靶向成纤维细胞诱导的癌细胞蛋白质组适应性,也能恢复拉帕替尼的敏感性:我们以数据为驱动的乳腺癌细胞蛋白质组学分析框架确定了蛋白水解降解调节因子PAI1和细胞周期调节因子PLK1是成纤维细胞介导的治疗耐药性的预测因子。针对HER2激酶和这些成纤维细胞诱导的信号适应性的联合疗法可消除成纤维细胞保护的HER2+乳腺癌细胞:在线版本包含补充材料,可在10.1007/s12195-024-00823-0上获取。
Rational Design of HER2-Targeted Combination Therapies to Reverse Drug Resistance in Fibroblast-Protected HER2+ Breast Cancer Cells.
Introduction: Fibroblasts, an abundant cell type in the breast tumor microenvironment, interact with cancer cells and orchestrate tumor progression and drug resistance. However, the mechanisms by which fibroblast-derived factors impact drug sensitivity remain poorly understood. Here, we develop rational combination therapies that are informed by proteomic profiling to overcome fibroblast-mediated therapeutic resistance in HER2+ breast cancer cells.
Methods: Drug sensitivity to the HER2 kinase inhibitor lapatinib was characterized under conditions of monoculture and exposure to breast fibroblast-conditioned medium. Protein expression was measured using reverse phase protein arrays. Candidate targets for combination therapy were identified using differential expression and multivariate regression modeling. Follow-up experiments were performed to evaluate the effects of HER2 kinase combination therapies in fibroblast-protected cancer cell lines and fibroblasts.
Results: Compared to monoculture, fibroblast-conditioned medium increased the expression of plasminogen activator inhibitor-1 (PAI1) and cell cycle regulator polo like kinase 1 (PLK1) in lapatinib-treated breast cancer cells. Combination therapy of lapatinib with inhibitors targeting either PAI1 or PLK1, eliminated fibroblast-protected cancer cells, under both conditions of direct coculture with fibroblasts and protection by fibroblast-conditioned medium. Analysis of publicly available, clinical transcriptomic datasets revealed that HER2-targeted therapy fails to suppress PLK1 expression in stroma-rich HER2+ breast tumors and that high PAI1 gene expression associates with high stroma density. Furthermore, we showed that an epigenetics-directed approach using a bromodomain and extraterminal inhibitor to globally target fibroblast-induced proteomic adaptions in cancer cells, also restored lapatinib sensitivity.
Conclusions: Our data-driven framework of proteomic profiling in breast cancer cells identified the proteolytic degradation regulator PAI1 and the cell cycle regulator PLK1 as predictors of fibroblast-mediated treatment resistance. Combination therapies targeting HER2 kinase and these fibroblast-induced signaling adaptations eliminates fibroblast-protected HER2+ breast cancer cells.
Supplementary information: The online version contains supplementary material available at 10.1007/s12195-024-00823-0.
期刊介绍:
The field of cellular and molecular bioengineering seeks to understand, so that we may ultimately control, the mechanical, chemical, and electrical processes of the cell. A key challenge in improving human health is to understand how cellular behavior arises from molecular-level interactions. CMBE, an official journal of the Biomedical Engineering Society, publishes original research and review papers in the following seven general areas:
Molecular: DNA-protein/RNA-protein interactions, protein folding and function, protein-protein and receptor-ligand interactions, lipids, polysaccharides, molecular motors, and the biophysics of macromolecules that function as therapeutics or engineered matrices, for example.
Cellular: Studies of how cells sense physicochemical events surrounding and within cells, and how cells transduce these events into biological responses. Specific cell processes of interest include cell growth, differentiation, migration, signal transduction, protein secretion and transport, gene expression and regulation, and cell-matrix interactions.
Mechanobiology: The mechanical properties of cells and biomolecules, cellular/molecular force generation and adhesion, the response of cells to their mechanical microenvironment, and mechanotransduction in response to various physical forces such as fluid shear stress.
Nanomedicine: The engineering of nanoparticles for advanced drug delivery and molecular imaging applications, with particular focus on the interaction of such particles with living cells. Also, the application of nanostructured materials to control the behavior of cells and biomolecules.
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