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分散因子调节EMT6小鼠乳腺肿瘤的转移表型。

Scatter factor modulates the metastatic phenotype of the EMT6 mouse mammary tumor.

作者信息

Rosen E M, Knesel J, Goldberg I D, Jin L, Bhargava M, Joseph A, Zitnik R, Wines J, Kelley M, Rockwell S

机构信息

Department of Therapeutic Radiology, Yale University School of Medicine, New Haven, CT 06510.

出版信息

Int J Cancer. 1994 Jun 1;57(5):706-14. doi: 10.1002/ijc.2910570517.

Abstract

EMT6 is a transplantable mouse mammary tumor cell line that has been utilized widely as a model system to study the effects of various treatments on local tumor growth and pulmonary metastasis. In this study, we examined the cellular mechanisms by which scatter factor (SF), a fibroblast-derived cytokine that stimulates epithelial cell motility, may contribute to tumor-cell dissemination, using the EMT6 model system. In vitro, SF stimulated EMT6 cell motility, invasiveness and cell-surface expression of urokinase (an enzyme required for cell migration through tissue). SF differentially stimulated EMT6 cell adhesion to and migration onto surfaces coated with collagen I and laminin. EMT6 cells treated in vitro with SF and injected i.v. into isogeneic BALB/c-Rw mice showed a small but significant increase (1.7-fold) in lung colony formation as compared with control cells. For EMT6 cells in vitro, SF had no effect on DNA synthesis, cell proliferation, cell size distribution, or in vitro colony-forming ability. Thus, the increase in lung colonization may be due to enhanced ability of SF-treated cells to adhere to subendothelial basement membrane or to invade through tissue. Studies of the tissue distribution of SF in BALB/c-Rw mice demonstrated high levels of active factor in the lung. Thus, the presence of endogenous pulmonary SF may have reduced the degree to which SF treatment stimulated EMT6 lung colonization. Significant SF activity was also found in extracts of EMT6 tumors. Cultured EMT6 cells did not produce SF, but did produce high titers of a soluble low-molecular-weight protein activity that is capable of stimulating SF production in human fibroblasts 3- to 5-fold. EMT6 tumor extracts contained high titers of a similar SF-inducing activity. These observations suggest that SF may contribute to the invasive and metastatic phenotype of EMT6 cells via a paracrine mechanism in which tumor cells induce the production of SF in stromal fibroblasts.

摘要

EMT6是一种可移植的小鼠乳腺肿瘤细胞系,已被广泛用作模型系统,以研究各种治疗对局部肿瘤生长和肺转移的影响。在本研究中,我们使用EMT6模型系统,研究了散射因子(SF)——一种由成纤维细胞衍生的刺激上皮细胞运动的细胞因子——可能促进肿瘤细胞扩散的细胞机制。在体外,SF刺激EMT6细胞的运动性、侵袭性以及尿激酶的细胞表面表达(尿激酶是细胞穿过组织迁移所需的一种酶)。SF对EMT6细胞与包被有I型胶原和层粘连蛋白的表面的黏附及迁移有不同的刺激作用。体外经SF处理并静脉注射到同基因BALB/c-Rw小鼠体内的EMT6细胞,与对照细胞相比,肺集落形成有小幅但显著的增加(1.7倍)。对于体外培养的EMT6细胞,SF对DNA合成、细胞增殖、细胞大小分布或体外集落形成能力没有影响。因此,肺定植增加可能是由于经SF处理的细胞黏附于内皮下基底膜或穿过组织侵袭的能力增强。对BALB/c-Rw小鼠中SF的组织分布研究表明,肺中存在高水平的活性因子。因此,内源性肺SF的存在可能降低了SF处理刺激EMT6肺定植的程度。在EMT6肿瘤提取物中也发现了显著的SF活性。培养的EMT6细胞不产生SF,但确实产生高滴度的可溶性低分子量蛋白活性,该活性能够刺激人成纤维细胞中SF的产生3至5倍。EMT6肿瘤提取物含有高滴度的类似SF诱导活性。这些观察结果表明,SF可能通过旁分泌机制促进EMT6细胞的侵袭和转移表型,其中肿瘤细胞诱导基质成纤维细胞产生SF。

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