Proteolytic Pathways in Progression of Pre-Malignant Breast Disease

乳腺癌前病变进展中的蛋白水解途径

• 批准号: 8267714
• 负责人: RAYMOND R MATTINGLY
• 金额: $ 30.46万
• 依托单位: WAYNE STATE UNIVERSITY
• 依托单位国家: 美国
• 财政年份: 2008
• 资助国家: 美国
• 起止时间: 2008-08-01 至 2014-05-31
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/8267714
• 关键词: Algorithms; American Cancer Society; Architecture; Atypical hyperplasia; B-Lymphocytes; Biological Markers; Biopsy; Breast; Breast Diseases; Carcinoma; Cathepsins; Cathepsins B; Cell Line; Cell Surface Receptors; Cells; Characteristics; Coculture Techniques; Cysteine; Cysteine Protease; Diagnosis; Drug Industry; Dysplasia; Engineering; Exhibits; Fibroblasts; Genes; Goals; Human; In Situ Lesion; In Vitro; Indolent; Intervention; Lead; Lesion; Libraries; Malignant - descriptor; Malignant Neoplasms; Mammary Ductal Carcinoma; Mammary Gland Parenchyma; Mammary gland; Matrix Metalloproteinases; Mediating; Modeling; Monomeric GTP-Binding Proteins; Morphology; Myoepithelial; Myoepithelial cell; Noninfiltrating Intraductal Carcinoma; Pathway interactions; Peptide Hydrolases; Phenotype; Phosphotransferases; Premalignant; Process; Proteolysis; Proteomics; Reagent; Recurrence; Role; Sampling; Screening procedure; Signal Transduction; Specimen; Staging; Stromelysin 1; Testing; Therapeutic; Therapeutic Intervention; Woman; Work; Xenograft procedure; cathepsin F; cathepsin V; cell type; human disease; implantation; in vivo; infiltrating duct carcinoma; inhibitor/antagonist; macrophage; malignant breast neoplasm; malignant phenotype; neoplastic cell; p21-activated kinase 1; post gamma-globulins; public health relevance; research clinical testing; serial analysis of gene expression; stromelysin 3; treatment strategy; tumor

DESCRIPTION (provided by applicant): Mammographic screening leads to many women being diagnosed with ductal carcinoma in situ [DCIS], yet we cannot accurately predict which lesions will undergo malignant progression to invasive ductal carcinomas [IDC] or effectively block this transition. Studies of human breast biopsies have implicated in this process cysteine cathepsins V/L2 and B in tumor cells and macrophages and cathepsins F, K and L in myoepithelial cells/[myo]fibroblasts. Aberrant signal transduction, for example through p21-activated kinase 1 [PAK1], may contribute to increased pericellular proteolysis. Our working hypothesis is that the transition from pre-invasive DCIS to invasive carcinomas and the rapid progression of some DCIS lesions are mediated through alterations in proteolytic pathways in DCIS cells and DCIS-associated cells, and that dysregulated PAK1 contributes to the induction of these aberrant proteolytic pathways. To test this hypothesis, we will recapitulate the transition from pre-invasive DCIS to invasive carcinoma using in vitro and in vivo progression models that we have designated MAME for mammary architecture microenvironment engineering. In these models, we will use isogenic MCF10 cell lines [AT1, DCIS1 and CA1d] and two human DCIS cell lines [SUM-102 and SUM-225]. Our specific aims are to: 1. Modulate expression and activity of cysteine cathepsin V or B in the isogenic and SUM DCIS cell lines, both by direct targeting and through intervention at the level of PAK1, and determine using the in vitro MAME model whether the invasive phenotype is altered; 2. Determine using the in vitro MAME model whether the invasive phenotype can be altered by co-culturing modified cells from Aim 1 with myoepithelial cells, [myo]fibroblasts or both cell types, using wild-type cells and ones in which expression and activity of cysteine cathepsin F, K or L have been modulated; 3. Determine using the in vivo MAME model whether the malignant phenotype of xenografts of modified cells from Aim 1 can be altered by simultaneous implantation of myoepithelial cells, [myo]fibroblasts or both cell types, using wild-type cells and ones in which expression and activity of cysteine cathepsin F, K or L have been modulated; and 4. Screen [via our Hu/Mu ProtIn chip] the in vivo MAME model for proteolytic pathways that may contribute to the transition from DCIS to IDC and use the in vitro MAME model to define functional changes with libraries of reagents from the Center on Proteolytic Pathways. Validating, in the context both of the tumor and its microenvironment, proteases key to progression of DCIS to IDC, and kinase pathways that regulate them, should identify potential targets for therapeutic intervention as well as biomarkers to distinguish DCIS lesions that will rapidly progress to IDC. PUBLIC HEALTH RELEVANCE: Proteases and kinases are the subject of intensive efforts by the pharmaceutical industry to develop new treatment strategies for human diseases, including cancer. Our proposed studies will discover and validate protease pathways that are active in the tumor microenvironment and that mediate the transition to a full-blown malignancy, and kinase pathways that regulate these protease pathways. We anticipate that our studies will identify biomarkers to distinguish premalignant lesions that will progress to invasive cancers and define targets that will abrogate that progression.

描述（由申请人提供）：乳腺X线筛查导致许多女性被诊断为导管原位癌[DCIS]，但我们无法准确预测哪些病变将恶性进展为浸润性导管癌[IDC]或有效阻止这种转变。 对人乳腺活检的研究表明，肿瘤细胞和巨噬细胞中的半胱氨酸组织蛋白酶V/L2和B以及肌上皮细胞/[肌]成纤维细胞中的组织蛋白酶F、K和L与该过程有关。 异常信号转导，例如通过p21激活激酶1 [PAK 1]，可能有助于增加细胞周围蛋白水解。 我们的工作假设是，从浸润性前DCIS到浸润性癌的转变和一些DCIS病变的快速进展是通过DCIS细胞和DCIS相关细胞中蛋白水解途径的改变介导的，并且PAK 1失调有助于诱导这些异常的蛋白水解途径。 为了验证这一假设，我们将使用体外和体内进展模型来概括从浸润前DCIS到浸润性癌的转变，我们将MAME指定为乳腺结构微环境工程。 在这些模型中，我们将使用等基因MCF 10细胞系[AT 1、DCIS 1和CA 1d]和两种人DCIS细胞系[SUM-102和SUM-225]。 我们的具体目标是：1.通过直接靶向和通过在PAK 1水平上的干预来调节半胱氨酸组织蛋白酶V或B在同基因和SUM DCIS细胞系中的表达和活性，并使用体外MAME模型确定侵袭性表型是否改变; 2.使用体外MAME模型确定是否可以通过将来自Aim 1的修饰细胞与肌上皮细胞、[肌]成纤维细胞或两种细胞类型共培养来改变侵袭性表型，使用野生型细胞和其中半胱氨酸组织蛋白酶F、K或L的表达和活性已被调节的细胞; 3.使用体内MAME模型确定来自Aim 1的修饰细胞的异种移植物的恶性表型是否可以通过同时植入肌上皮细胞、[肌]成纤维细胞或两种细胞类型来改变，使用野生型细胞和其中半胱氨酸组织蛋白酶F、K或L的表达和活性已经被调节的细胞;和4. [通过我们的Hu/Mu ProtIn芯片]筛选体内MAME模型中可能有助于从DCIS转变为IDC的蛋白水解途径，并使用体外MAME模型来定义来自蛋白水解途径中心的试剂库的功能变化。 在肿瘤及其微环境的背景下，验证DCIS进展为IDC的关键蛋白酶和调节它们的激酶途径，应该确定治疗干预的潜在靶点以及区分将快速进展为IDC的DCIS病变的生物标志物。 公共卫生相关性：蛋白酶和激酶是制药工业为开发人类疾病（包括癌症）的新治疗策略而密集努力的主题。 我们提出的研究将发现并验证在肿瘤微环境中具有活性并介导向完全恶性肿瘤转变的蛋白酶途径，以及调节这些蛋白酶途径的激酶途径。 我们预计，我们的研究将确定生物标志物，以区分癌前病变，将进展为浸润性癌症，并确定目标，将废除这种进展。