CYSTATIN C EFFECT ON B16 MELANOMA METASTASIS

胱抑素 C 对 B16 黑色素瘤转移的影响

• 批准号: 6376512
• 负责人: JAMES Lewis COX
• 金额: $ 13.93万
• 依托单位: A.T. STILL UNIVERSITY OF HEALTH SCIENCES
• 依托单位国家: 美国
• 财政年份: 1999
• 资助国家: 美国
• 起止时间: 1999-07-01 至 2003-06-30
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/6376512
• 关键词: antineoplastics; cathepsin B; confocal scanning microscopy; cysteine endopeptidases; enzyme activity; fluorescence microscopy; gene expression; injection /infusion; laboratory mouse; melanoma; metastasis; neoplastic cell; neoplastic growth; protease inhibitor; respiratory infections; tissue /cell culture; transfection /expression vector

The metastatic spread of cancer is primarily responsible for the intractable nature of the disease. Interference of cancer metastasis with chemical or biologic agents could perhaps bring about increased survival times in cancer patients. The overall goal of this project is to elucidate steps by which natural cysteine proteinase inhibitors, the cystatins, may act as antimetastatic agents. The long term goal is to target cysteine proteinases as a therapeutic adjunct to traditional treatments for malignant neoplasms. The model to be used in these studies are highly metastatic B 16 mouse melanoma cell lines which have been genetically modified to overproduce cystatin C. In addition, a number of experiments will explore the effect of purified cystatin C on metastatic melanoma cell characteristics such as motility, invasion in vitro, growth and metastasis in vivo. Motility and in vitro invasion will be conducted with modified Boyden chambers. Metastasis studies (in vivo) will be carried out by tail-vein injections of labeled cells or dermal injections of melanoma cells so that tumor growth and metastasis can be measured. Localization studies with antibodies specific for cystatin C and cathepsin B, together with cathepsin B activity measurements will help define the role of cysteine proteinases in metastasis. Specific genetic constructs involving cystatin C will be created to allow marker activities to aid in localization studies. Both conventional fluorescence microscopy and confocal microscopy will be used in localization studies. The specific aims for this project are to determine: l. Does cystatin C overexpression inhibit an early stage of lung colonization? 2. Whether cystatin C inhibits tumor growth, either in clones overexpressing cystatin C or when cystatin C is administered to melanoma tumors in vivo. 3. What effects occur upon exogenous addition of cystatin C to B16 melanoma cells in vitro? 4. Localization of cystatin C by transfection of melanoma cells with gene fusions or modified cystatin in expression vectors. These specific aims will help advance our knowledge of the role of cysteine proteinase inhibitors as anti-metastatic agents. The therapeutic value of this class of inhibitors will be revealed in studies of this nature because the target enzyme and inhibitor are well defined and the B16 melanoma are among the best of characterized metastatic cell lines.

癌症的转移性扩散是该疾病难治性的主要原因。用化学或生物制剂干扰癌症转移可能会增加癌症患者的生存时间。该项目的总体目标是阐明天然半胱氨酸蛋白酶抑制剂，即胱抑素，可能作为抗转移剂的步骤。长期目标是将半胱氨酸蛋白酶作为恶性肿瘤传统治疗的辅助治疗手段。这些研究中使用的模型是高转移性的b16小鼠黑色素瘤细胞系，这些细胞系经过基因修饰，过量产生胱抑素C。此外，许多实验将探索纯化的胱抑素C对转移性黑色素瘤细胞的运动、体外侵袭、体内生长和转移等特性的影响。运动和体外侵袭将用改良的博伊登腔进行。转移研究（体内）将通过尾静脉注射标记细胞或真皮注射黑色素瘤细胞进行，以便测量肿瘤的生长和转移。半胱氨酸蛋白酶C和组织蛋白酶B特异性抗体定位研究，以及组织蛋白酶B活性测量将有助于确定半胱氨酸蛋白酶在转移中的作用。将创建涉及胱抑素C的特定遗传结构，以允许标记活动帮助定位研究。传统的荧光显微镜和共聚焦显微镜都将用于定位研究。该项目的具体目的是确定：1 .胱抑素C过表达是否抑制早期肺定植？2. 半胱抑素C是否抑制肿瘤生长，无论是在过表达半胱抑素C的克隆中，还是体内给药半胱抑素C时。3. 体外B16黑色素瘤细胞外源性添加胱抑素C会产生什么影响？4. 基因融合转染黑色素瘤细胞或在表达载体上修饰胱抑素C定位。这些特定的目标将有助于推进我们对半胱氨酸蛋白酶抑制剂作为抗转移剂的作用的认识。这类抑制剂的治疗价值将在这类性质的研究中得到揭示，因为靶酶和抑制剂是明确定义的，而且B16黑色素瘤是最具特征的转移细胞系之一。