在HER2阳性乳腺癌细胞系中使用曲妥珠单抗恩杂鲁胺进行CRISPR筛选揭示了对耐药性的新见解。
CRISPR screens with trastuzumab emtansine in HER2-positive breast cancer cell lines reveal new insights into drug resistance.
作者信息
Lipert Barbara A, Siemens Kyla N, Khan Aziza, Airey Rebecca, Dam Gech Heng, Lu Man, Flinterman Marcella, Yong Queenie, Lee Tet Woo, Hunter Francis W, Jamieson Stephen M F
机构信息
Auckland Cancer Society Research Centre, University of Auckland, Auckland, New Zealand.
Maurice Wilkins Centre for Molecular Biodiscovery, University of Auckland, Auckland, New Zealand.
出版信息
Breast Cancer Res. 2025 Mar 31;27(1):48. doi: 10.1186/s13058-025-02000-1.
BACKGROUND
Trastuzumab emtansine (T-DM1) is an antibody-drug conjugate that is an effective therapy for HER2-positive breast cancer; however, its efficacy is limited by drug resistance. While multiple mechanisms of resistance have been proposed, these are not yet well understood. Greater understanding of T-DM1 sensitivity and resistance could provide new combination strategies to overcome resistance or predictive biomarkers to guide therapy.
METHODS
We have conducted CRISPR/Cas9 functional genomics modifier screens in HER2-positive breast cancer cell lines to allow for unbiased discovery of T-DM1 sensitivity and resistance genes. Whole-genome knockout screens were carried out in MDA-MB-361 and MDA-MB-453 cells treated with T-DM1 and its payload cytotoxin DM1. Hits were validated in secondary T-DM1 screens using a focused single-guide RNA (sgRNA) library and subsequently by individual gene knockout.
RESULTS
The whole-genome CRISPR screens with T-DM1 and DM1 identified 599 genes as potential modifiers of T-DM1 sensitivity and resistance. Of these, 17 genes were significantly enriched and 3 genes depleted at P < 0.001 in either or both MDA-MB-361 and MDA-MB-453 libraries in the secondary screens. Among the top hits, were known T-DM1 sensitivity genes ERBB2 and SLC46A3, in addition to negative regulators of mTOR complex 1: TSC1 and TSC2. MDA-MB-453 clones with knockout of TSC1 or partial knockout of TSC2 were more resistant to T-DM1 than wild type cells in competition growth assays and to T-DM1 and other HER2 targeting therapies (T-DXd, lapatinib and neratinib) in growth inhibition assays, and had increased internalisation of T-DM1 at 6 h. T-DM1 and the mTOR inhibitor everolimus demonstrated synergistic activity at inhibiting cell proliferation at multiple T-DM1 concentrations across four HER2-positive breast cancer cell lines.
CONCLUSIONS
Our CRISPR screening approach with T-DM1 in HER2-positive breast cancer cell lines identified genes not previously implicated in T-DM1 sensitivity or resistance, including TSC1 and TSC2. These genes may inform new strategies to enhance T-DM1 therapy in the clinic.
背景
曲妥珠单抗-美坦新(T-DM1)是一种抗体药物偶联物,是HER2阳性乳腺癌的有效治疗药物;然而,其疗效受到耐药性的限制。虽然已经提出了多种耐药机制,但对这些机制尚未完全了解。更深入地了解T-DM1的敏感性和耐药性可以提供新的联合策略来克服耐药性或预测性生物标志物以指导治疗。
方法
我们在HER2阳性乳腺癌细胞系中进行了CRISPR/Cas9功能基因组修饰筛选,以无偏见地发现T-DM1敏感性和耐药性基因。在用T-DM1及其有效载荷细胞毒素DM1处理的MDA-MB-361和MDA-MB-453细胞中进行全基因组敲除筛选。在使用聚焦单导向RNA(sgRNA)文库的二次T-DM1筛选中验证命中基因,随后通过单个基因敲除进行验证。
结果
用T-DM1和DM1进行的全基因组CRISPR筛选确定了599个基因作为T-DM1敏感性和耐药性的潜在修饰因子。其中,在二次筛选中,在MDA-MB-361和MDA-MB-453文库中的一个或两个文库中,17个基因在P<0.001时显著富集,3个基因显著减少。在最显著的命中基因中,除了mTOR复合物1的负调节因子TSC1和TSC2外,还有已知的T-DM1敏感性基因ERBB2和SLC46A3。在竞争生长试验中,敲除TSC1或部分敲除TSC2的MDA-MB-453克隆比野生型细胞对T-DM1更具抗性,在生长抑制试验中对T-DM1和其他HER2靶向治疗(T-DXd、拉帕替尼和来那替尼)更具抗性,并且在6小时时T-DM1的内化增加。在四种HER2阳性乳腺癌细胞系中,在多个T-DM1浓度下,T-DM1和mTOR抑制剂依维莫司在抑制细胞增殖方面表现出协同活性。
结论
我们在HER2阳性乳腺癌细胞系中用T-DM1进行的CRISPR筛选方法鉴定出了以前未涉及T-DM1敏感性或耐药性的基因,包括TSC1和TSC2。这些基因可能为临床上增强T-DM1治疗的新策略提供依据。
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