长链非编码RNA SNHG3对人乳腺癌细胞MCF-7增殖、迁移与侵袭的影响 *

目的:探讨长链非编码RNA SNHG3对人乳腺癌细胞MCF-7增殖、迁移与侵袭的影响。方法:构建SNHG3过表达质粒,实验分别设置阴性对照组(pcDNA-3.1+)与SNHG3基因过表达组(pcDNA-3.1+/SNHG3)。将MCF-7细胞转染对照组质粒和SNHG3过表达质粒,采用实时定量PCR 方法检测 SNHG3 mRNA 转录水平,Western blot 检测MMP9及EMT相关蛋白质水平;集落形成实验检测MCF-7细胞增殖能力;划痕愈合实验检测MCF-7细胞横向迁移能力; Transwell 小室实验检测MCF-7细胞纵向迁移能力及侵袭能力。结果:过表达SNHG3后,MCF-7细胞中SNHG3的mRNA水平显著增高(P<0.001);MCF-7细胞的体外增殖能力明显增加(P<0.01),迁移(P<0.01)与侵袭能力(P<0.001)也显著增强,实时定量PCR, Western blot 结果显示SNHG3可激活EMT相关通路。结论:过表达SNHG3可能通过激活EMT通路促进乳腺癌MCF-7细胞的增殖,迁移与侵袭。     

稳定干扰ITGB1抑制人乳腺癌BT549细胞迁移和侵袭

在人乳腺癌细胞系BT549中稳定干扰整合素β1(integrinβ1,ITGB1),研究其对乳腺癌细胞迁移和侵袭的影响。构建靶向干扰ITGB1基因的sh RNA慢病毒,感染BT549细胞,通过筛选成功获得稳定干扰ITGB1蛋白的BT-549细胞系,实验设空白对照组(Blank)、病毒感染阴性对照组(shNC)、ITGB1-shRNA慢病毒感染组(shITGB1);Real-time PCR和Western blotting法检测稳定干扰后ITGB1 mRNA和蛋白的表达情况;Western blotting法检测稳定干扰ITGB1后上皮间质转化(epithelial-mesenchymal transition,EMT)相关标志蛋白(E-cadherin,Vimentin,N-cadherin,Fibronectin)的表达情况;利用划痕试实验和Transwell侵袭试实验分别检测稳定干扰ITGB1后细胞的迁移及侵袭能力。Real-time PCR和Western blotting结果显示,shITGB1组细胞ITGB1 mRNA和蛋白的表达水平显著低于Blank组和shNC组细胞(p0.01,p0.01)。Western blotting结果显示,稳定干扰ITGB1可部分逆转乳腺癌细胞BT549的EMT化;稳定干扰ITGB1后,上皮标志蛋白E-cadherin表达显著上调(p0.01),间质标志蛋白Vimentin(p0.05)、N-cadherin(p0.01)和Fibronectin(p0.01)的表达显著降低。划痕和Transwell侵袭试验实验结果显示,稳定干扰ITGB1后可显著降低乳腺癌细胞的迁移及侵袭能力(p0.05,p0.05)。在乳腺癌BT549细胞中稳定干扰ITGB1后,通过逆转EMT化抑制细胞迁移和侵袭。     

过表达外源ST3Gal I增加MCF-7细胞与胞外基质粘附和侵袭能力

为探讨过表达外源α2,3-唾液酸转移酶（ST3Gal Ⅰ）对乳腺癌MCF-7细胞粘 附和侵袭能力的影响,构建pEGFP-N1-ST3Gal I真核表达载体.采用GenEscortTM Ⅱ包裹后转染MCF-7细胞. MCF-7细胞为3组：未转染组 (M)、转染空质粒组 (P) 和转染ST3Gal I组 (ST3); 荧光显微镜观察融合蛋白EGFP ST3Gal I的表达.采用 半定量RT-PCR、Western印迹法分析转染后MCF-7细胞ST3Gal Ⅰ基因mRNA水平和 蛋白表达水平;流式细胞术分析ST3Gal Ⅰ下游产物细胞表面α2,3-唾液酸含量;采用细胞粘附实验及transwell小室检测转染前后细胞与基质胶Matrigel粘附、迁移和侵袭运动能力的变化.结果表明, 荧光显微镜下P组细胞内绿色荧光呈弥散分 布,而ST3组绿色荧光主要集中在细胞质中,RT-PCR与Western印迹也证实了外源 ST3Gal Ⅰ基因mRNA和蛋白表达均明显增加（P<0.05）,其下游产物细胞表面 α2,3-唾液酸含量明显增加（P<0.05）;与M、P组相比,ST3组表现为粘附、迁移和侵袭能力明显增强（P<0.05）.利用转染技术可明显提高外源ST3Gal Ⅰ在MCF -7细胞表达,明显增加MCF-7细胞与胞外基质（ECM）粘附、迁移和侵袭能力,可形成肿瘤入侵表型,将有望成为治疗乳腺癌转移的新靶点.     

三氧化二砷对人乳腺癌MCF-7细胞的抑制作用及其FOXO1表达的影响

本研究探讨三氧化二砷对人乳腺癌MCF-7细胞的生长及迁移等作用的抑制作用以及对FOXO1的表达的影响。不同浓度三氧化二砷作用人乳腺癌MCF-7细胞后,利用MTT法检测细胞增殖、流式细胞术检测细胞凋亡的变化;通过划痕实验和transwell侵袭实验检测细胞迁移和侵袭能力的变化;通过荧光定量PCR和Western blotting检测FOXO1基因和蛋白水平表达的变化。结果显示不同浓度的三氧化二砷能够抑制细胞生长、迁移及侵袭,诱导细胞发生凋亡,且具有浓度依赖性;并且三氧化二砷可以上调FOXO1基因和蛋白水平的表达。因此三氧化二砷对人乳腺癌MCF-7细胞的抑制作用可能与上调抑癌基因FOXO1表达有关。     

NDRG2 通过影响CD24 调控乳腺癌细胞的粘附能力

目的:阐明NDRG2(N-Myc downstream-regulated gene 2)在乳腺癌细胞中对CD24的调控及其对乳腺癌细胞粘附能力的影响。方法:RT-PCR和Western blot方法检测乳腺癌细胞MCF-7及Bcap-37中NDRG2和CD24的表达;通过腺病毒上调MCF-7细胞中NDRG2的表达,或利用siRNA下调Bcap-37细胞中NDRG2的表达,检测CD24基因和蛋白的变化。粘附实验检测改变NDRG2表达水平后对MCF-7及Bcap-37细胞粘附能力的影响。结果:MCF-7细胞中NDRG2基因和蛋白的表达水平低于Bcap-37细胞,而CD24的表达水平高于Bcap-37细胞;在MCF-7细胞中通过腺病毒载体上调NDRG2可以抑制CD24的表达并抑制其粘附能力,而在Bcap-37细胞中利用siRNA下调NDRG2的表达可以提高CD24的水平及细胞的粘附能力;结论:NDRG2通过影响CD24参与调控乳腺癌细胞的粘附能力。     

MiR-206与ANXA2的3′UTR靶向结合抑制乳腺癌侵袭

膜联蛋白A2（annexin A2,ANXA2）可促进人结直肠癌的侵袭和迁移。然而,ANXA2在乳腺癌中的作用以及调节机制尚缺乏系统的研究。本研究旨在探讨微小RNA-206（microRNA-206,miR-206）如何调节ANXA2基因的表达,进而影响乳腺癌的侵袭。通过基因预测软件TargetScan (TargetScan V5.2)找到与ANXA2的3′UTR区互补结合的miR-206。运用实时定量 PCR（qRT-PCR）检测不同乳腺癌细胞系中miR-206的表达水平,发现低侵袭性乳腺癌MCF-7细胞株miR-206 表达量明显高于高侵袭性乳腺癌细胞株MDA-231、MDA-435和T47D。运用转染技术将 miR-206 质粒及miR-206 抑制剂转入乳腺癌细胞系MDA-231后,qRT-PCR检测转染后各组细胞中miR-206的表达情况,结果显示转染成功。用Western印迹法检测各组细胞中ANXA2的表达情况,结果显示,miR-206负向调控ANXA2蛋白的表达。 qRT-PCR显示,过表达乳腺癌细胞内miR-206 后,ANXA2 mRNA基本没有变化。结果显示,miR-206是在翻译水平上影响ANXA2蛋白的表达。荧光素酶实验显示：miR-206能特异性地与ANXA2 mRNA的3′UTR结合,抑制其荧光素酶活性。Transwell侵袭实验检测各组细胞的侵袭能力。结果显示,过表达miR-206后,乳腺癌细胞体外侵袭能力明显减弱。综上所述,miR-206 通过靶向结合癌基因ANXA2 mRNA的3′UTR区,抑制ANXA2蛋白翻译,从而抑制了乳腺癌细胞的侵袭。因此,miR-206有望成为抑制乳腺癌侵袭与治疗乳腺癌的新靶点和生物学标记物。     

GALNT14对人乳腺癌MCF-7细胞迁移的影响

构建真核表达载体pcDNA 3.1-Flag-T14,重组质粒经酶切分析及测序鉴定后,利用脂质体将重组质粒转染人乳腺癌细胞系MCF-7细胞,经G418筛选并建立稳定转染GALNT14细胞株.应用半定量RT-PCR、Western blot检测稳定细胞株GALNT14 mRNA及蛋白表达水平,细胞划痕修复及穿膜试验检测GALNT14基因对MCF-7迁移能力的影响,同时RT-PCR检测GALNT14对MMP-2,MMP-9,TGF-β1及VEGF等肿瘤浸润转移相关因子表达的影响.结果显示成功构建了真核重组表达载体pcDNA 3.1-Flag-T14,经RT-PCR和Western blot检测显示成功获得了稳定表达GALNT14的MCF-7细胞株;GALNT14能够提高MCF-7细胞株的迁移能力,且能增加侵袭转移相关因子MMP-2,MMP-9,TGF-β1及VEGF的表达.结论:GALNT14可明显促进MCF-7细胞的迁移,可能在肿瘤侵袭转移中起重要作用.     

过表达外源FUT8增加乳腺癌细胞的迁移和侵袭能力

核心岩藻糖的修饰被认为是对糖蛋白进行转录后加工和功能调控的一种重要方式, 与肿瘤的发生发展密切相关, 但其在乳腺癌恶性转化过程中所发挥的生物学功能尚不明确. 本文构建了α1,6-岩藻糖基移转酶（FUT8）基因真核表达载体,将其转染人乳腺癌细胞Bcap-37, 实时PCR及Western印迹检测FUT8 mRNA和蛋白质表达, 通过细胞划痕实验和Transwell小室观察FUT8过表达对细胞体外迁移、侵袭能力的影响, 免疫共沉淀和Western印迹检测肿瘤细胞整合素、基质金属蛋白酶（matrix metalloproteinases, MMPs）家族相关蛋白质表达水平变化. 结果显示,外源FUT8基因在mRNA水平和蛋白质水平的表达均显著增加, FUT8过表达组细胞迁移和侵袭能力明显增强;上调FUT8基因表达可使Bcap-37细胞中核心岩藻糖基化的整合素-α3β1、MMP-2和MMP-9在蛋白质水平呈不同程度升高. 上述研究表明,FUT8可通过核心岩藻糖化修饰正性调控整合素-α3β1的功能, 诱导MMP-2、MMP-9的表达, 促进乳腺癌细胞的迁移和侵袭.     

HIF-2α/Notch3通路介导CoCl_2诱导的乳腺癌MCF-7细胞迁移和侵袭

本研究旨在探究HIF-2α和Notch3在CoCl_2诱导的乳腺癌MCF-7细胞迁移和侵袭中的作用。使用CoCl_2于体外建立化学性低氧模型;采用sh RNA技术沉默MCF-7细胞中HIF-2α和Notch3基因;采用RT-PCR法检测MCF-7细胞中HIF-2α、Notch3和Hey1的m RNA水平;采用Western blot方法检测MCF-7细胞中HIF-2α、Notch3、Hey1、Snail和E-cadherin蛋白的表达水平;采用划痕实验和Transwell实验分别检测CoCl_2诱导的MCF-7细胞迁移和侵袭。结果显示,CoCl_2处理可使MCF细胞中HIF-2α、Notch3、Hey1和Snail蛋白表达水平升高(P0.05),E-cadherin蛋白表达水平下降(P0.05),促进MCF-7细胞迁移和侵袭(P0.05);沉默HIF-2α基因表达可抑制CoCl_2诱导的Notch3和Hey1的m RNA和蛋白表达(P0.05);抑制Notch3基因表达后,CoCl_2诱导的MCF-7细胞迁移和侵袭以及CoCl_2对Snail和E-cadherin蛋白表达的调节随之受到抑制(P0.05)。以上结果表明,在CoCl_2化学性低氧环境下,HIF-2α可通过强化Notch3信号通路,进而导致Snail蛋白水平升高和E-cadherin蛋白水平下降,最终提高乳腺癌MCF-7细胞的迁移和侵袭能力。     

过表达P185可抑制EMT并促进胃癌细胞侵袭和迁移

为探究过表达P185基因对胃癌SGC7901细胞侵袭、迁移的影响以及可能作用机制,本研究通过脂质体将携带P185基因的过表达pcDNA3.1-P185质粒,转染至胃癌SGC7901细胞中;本研究采用qRT-PCR和免疫印迹试验(Western blotting)检测P185 mRNA的转录水平和蛋白水平,Western blotting检测钙黏蛋白E(E-cadherin)、波形蛋白(Vimentin)、基质金属蛋白酶-2 (matrix metalloprotease, MMP-2)表达;以Transwell小室法检测细胞的侵袭、迁移能力的变化。研究结果表明:胃癌细胞转染过表达pcDNA3.1-P185质粒能显著上调P185 mRNA和蛋白质的表达(p0.05);SGC7901细胞转染重组质粒pcDNA3.1-P185后,细胞的侵袭、迁移能力较对照组显著增强(p0.05),细胞中E-cadherin蛋白水平显著下调(p0.05),Vimentin、MMP-2蛋白水平显著增加(p0.05)。本研究显示P185可能通过抑制EMT,促进细胞外基质的降解、促进胃癌细胞的侵袭、迁移。     

Dynamic interplay between breast cancer cells and normal endothelium mediates the expression of matrix macromolecules,proteasome activity and functional properties of endothelial cells

Background

Breast cancer–endothelium interactions provide regulatory signals facilitating tumor progression. The endothelial cells have so far been mainly viewed in the context of tumor perfusion and relatively little is known regarding the effects of such paracrine interactions on the expression of extracellular matrix (ECM), proteasome activity and properties of endothelial cells.

Methods

To address the effects of breast cancer cell (BCC) lines MDA-MB-231 and MCF-7 on the endothelial cells, two cell culture models were utilized; one involves endothelial cell culture in the presence of BCCs-derived conditioned media (CM) and the other co-culture of both cell populations in a Transwell system. Real-time PCR was utilized to evaluate gene expression, an immunofluorescence assay for proteasome activity, and functional assays (migration, adhesion and invasion) and immunofluorescence microscopy for cell integrity and properties.

Results

BCC-CM decreases the cell migration of HUVEC. Adhesion and invasion of BCCs are favored by HUVEC and HUVEC-CM. HA levels and the expression of CD44 and HA synthase-2 by HUVEC are substantially upregulated in both cell culture approaches. Adhesion molecules, ICAM-1 and VCAM-1, are also highly upregulated, whereas MT1-MMP and MMP-2 expressions are significantly downregulated in both culture systems. Notably, the expression and activity of the proteasome β5 subunit are increased, especially by the action of MDA-MB-231-CM on HUVEC.

Conclusions and general significance

BCCs significantly alter the expression of matrix macromolecules, proteasome activity and functional properties of endothelial cells. Deep understanding of such paracrine interactions will help to design novel drugs targeting breast cancer at the ECM level. This article is part of a Special Issue entitled Matrix-mediated cell behaviour and properties.     

PTH-related protein enhances MCF-7 breast cancer cell adhesion, migration, and invasion via an intracrine pathway

Breast cancer is the most common carcinoma that metastasizes to the bone. Parathyroid hormone-related protein (PTHrP), a known stimulator of osteoclastic bone resorption, is a major mediator of the osteolytic process in breast cancer. PTHrP overexpression increases mitogenesis and decreases apoptosis in the human breast cancer cell line MCF-7. In this study, MCF-7 cells were used as a model system to study the effects of PTHrP on breast cancer cell adhesion, migration, and invasion. Clones of MCF-7 cells were established that overexpress wild-type PTHrP or PTHrP mutated in the nuclear localization sequence (NLS). Wild-type PTHrP-overexpressing cells showed significantly higher laminin adhesion and migration, and Matrigel invasion than empty vector-transfectants or cells overexpressing NLS-mutated PTHrP. Wild-type PTHrP also increased the cell surface expression of the pro-invasive integrins alpha6 and beta4; deletion of the NLS negated these effects. Exogenous PTHrP (1-34), (67-86), (107-139), and (140-173) had no effect on integrin expression, or on cell adhesion, migration, and invasion. These results indicate that PTHrP exerts its effects on cell adhesion, migration, invasion, and integrin expression via an intracrine pathway. PTHrP may play a role in breast cancer metastasis by upregulating proinvasive integrin expression, and controlling PTHrP production in breast cancer may provide therapeutic benefit.     

下调CENP-E对乳腺癌MCF-7细胞的影响

目的:探讨有丝分裂检查点蛋白着丝粒蛋白-E(CENP-E)基因在肿瘤发生发展中的作用。方法:利用shRNA下调CENP-E基因的表达,分别用巢式PCR和Western blot检测CENP-E mRNA和蛋白的表达;MTT检测CENP-E下调后MCF-7细胞的增殖变化;流式细胞术检测CENP-E下调后对MCF-7细胞凋亡的影响;Transwell试验检测MCF-7细胞的迁移和侵袭能力变化;间接免疫荧光检测细胞内CENP-E蛋白和有丝分裂情况。结果:shRNA能有效抑制CENP-E mRNA和蛋白的表达。MTT结果显示CENP-E下调后MCF-7细胞的增殖能力减弱(P<0.05);流式细胞术显示下调CENP-E后能促进MCF-7细胞的凋亡;间接荧光结果显示CENP-E干扰后MCF-7细胞内CENP-E蛋白减少并伴有核分裂异常;Transwell试验显示CENP-E干扰组细胞的迁移和侵袭能力增强(P<0.05)。结论:下调部分CENP-E的表达能抑制MCF-7细胞的增殖,促进MCF-7细胞的凋亡,增强MCF-7细胞的迁移和侵袭能力。     

miR-449a对人乳腺癌细胞MCF-7增殖及迁移能力的影响

目的：通过敲低微小RNA （microRNA,miRNA）-449a的方法研究miR-449a对人乳腺癌细胞MCF-7的增殖和迁移能力的影响。方法：采用miRNA芯片在乳腺癌细胞MCF-7和人正常乳腺细胞MCF-10A筛选具有表达差异的miRNA;化学合成法制备miR-449a的抑制剂（inhibitor）,转染后经real-time PCR验证表达的变化;细胞增殖CCK-8实验对转染后细胞增殖能力进行检测;划痕实验检测细胞转移能力,transwell小室实验检测细胞侵袭的改变;蛋白免疫印迹法（Western blot）实验对MCF-7细胞增殖和迁移相关的β-catenin和E-cadherin蛋白进行检测;通过生物信息学软件预测miR-449a潜在靶基因为Notch 1,荧光素酶实验检测Notch 1是miR-449a的靶基因。结果：分别收集MCF-7和MCF-10A细胞,芯片结果显示miR-449a在MCF-7细胞的表达水平显著高于MCF-10A;本研究将细胞分为未处理组（Mock组）,阴性对照组（negative control组,NC组）和处理组,通过收集不同组MCF-7细胞进行试验,CCK-8结果显示miR-449a下调后MCF-7细胞增殖能力显著降低;划痕实验结果显示miR-449a表达降低导致MCF-7细胞转移能力降低;transwell实验结果显示MCF-7细胞侵袭受到抑制;Western blot结果发现miR-449a敲低后β-catenin表达降低,E-cadherin表达增加;荧光素酶试验结果显示,miR-449a能够显著降低Notch 1-3'-UTR质粒的荧光素活性（P<0.01）。结论：在乳腺癌细胞MCF-7中敲低miR-449a能够显著抑制癌细胞增殖和迁移,而这一变化可能通过降低Notch 1蛋白表达实现的。     

Biological Properties of Melanoma and Endothelial Cells after Plasmid AMEP Gene Electrotransfer Depend on Integrin Quantity on Cells

The data on the biological responsiveness of melanoma and endothelial cells that are targeted by Antiangiogenic MEtargidin Peptide (AMEP) are limited; therefore, the antiproliferative, antimetastatic and antiangiogenic effects of AMEP were investigated in murine melanoma and human endothelial cells after plasmid AMEP gene electrotransfer into the cells in vitro. Plasmid AMEP, a plasmid coding for the disintegrin domain of metargidin targeting specific integrins, had cytotoxic and antiproliferative effects on murine melanoma and human endothelial cells. Among the metastatic properties of cells, migration, invasion and adhesion were investigated. Plasmid AMEP strongly affected the migration of murine melanoma and human endothelial cell lines and also affected the invasion of highly metastatic murine melanoma B16F10 and human endothelial cell lines. There was no effect on cell adhesion on Matrigel^TM or fibronectin in all cell lines. The antiangiogenic effect was shown with tube formation assay, where human microvascular endothelial cell line (HMEC-1) proved to be more sensitive to plasmid AMEP gene electrotransfer than the human umbilical vein endothelial cell line (HUVEC). The study indicates that antiproliferative and antimetastatic biological responses to gene electrotransfer of plasmid AMEP in murine melanoma cells were dependent on the integrin quantity on melanoma cells and not on the expression level of AMEP. The strong antiangiogenic effect expressed in human endothelial cell lines was only partly dependent on the quantity of integrins and seemed to be plasmid AMEP dose dependent.     

CD44v4 is a major E-selectin ligand that mediates breast cancer cell transendothelial migration

Background

Endothelial E-selectin has been shown to play a pivotal role in mediating cell–cell interactions between breast cancer cells and endothelial monolayers during tumor cell metastasis. However, the counterreceptor for E-selectin and its role in mediating breast cancer cell transendothelial migration remain unknown.

Methodology/Principal Findings

By assessing migration of various breast cancer cells across TNF-α pre-activated human umbilical vein endothelial cells (HUVECs), we found that breast cancer cells migrated across HUVEC monolayers differentially and that transmigration was E-selectin dependent. Cell surface labeling with the E-selectin extracellular domain/Fc chimera (exE-selectin/Fc) showed that the transmigration capacity of breast cancer cells was correlated to both the expression level and localization pattern of E-selectin binding protein(s) on the tumor cell surface. The exE-selectin/Fc strongly bound to metastatic MDA-MB-231, MDA-MB-435 and MDA-MB-468 cells, but not non-metastatic MCF-7 and T47D cells. Binding of exE-selectin/Fc was abolished by removal of tumor cell surface sialyl lewis x (sLe^x) moieties. Employing an exE-selectin/Fc affinity column, we further purified the counterreceptor of E-selectin from metastatic breast cancer cells. The N-terminal protein sequence and cDNA sequence identified this E-selectin ligand as a ∼170 kD human CD44 variant 4 (CD44v4). Purified CD44v4 showed a high affinity for E-selectin via sLe^x moieties and, as expected, MDA-MB-231 cell adhesion to and migration across HUVEC monolayers were significantly reduced by down-regulation of tumor cell CD44v4 via CD44v4-specific siRNA.

Conclusions/Significance

We demonstrated, for the first time, that breast cancer cell CD44v4 is a major E-selectin ligand in facilitating tumor cell migration across endothelial monolayers. This finding offers new insights into the molecular basis of E-selectin–dependent adhesive interactions that mediate breast cancer cell transendothelial metastasis.     

Distinct mechanisms mediate the initial and sustained phases of cell migration in epidermal growth factor receptor-overexpressing cells

Elevated levels of epidermal growth factor receptor (EGFR) are predictive of increased invasion and metastasis in many human cancers. In the present study, we have shown that two distinct pathways regulate cell migration in EGFR-overexpressing invasive cells such as MDA 468 breast cancer cells: mitogen-activated protein kinase (MAPK or ERK 1 and 2) pathways play a major role in early stages to cell migration; and protein kinase C delta isoforms (PKC-delta) play a significant role in later stages of sustained cell migration. Inhibition of MAPK activity with MAP kinase kinase (MEK) inhibitor PD98059 blocks early stages of cell migration (up to 4 h); however, cells revert back to enhanced cell migration after 4 h. While inhibition of PKC-delta activity with rottlerin or dominant-negative PKC-delta expression blocks sustained cell migration after 4 h and up to 12 h, the combination of MAPK and PKC inhibitors completely blocked transforming growth factor alpha (TGF-alpha)-induced cell migration in EGFR-overexpressing breast cancer cells. However, inhibition of MAPK activity completely blocked cell migration in low EGFR-expressing non-invasive breast cancer cells such as MCF-7 cells. Forced overexpression of EGFR in MCF-7 cells (EGFR/MCF-7 cells) resulted in cell migration patterns seen in MDA 468 cells, that is, MAPK pathways play a major role in early stages to cell migration, and PKC-delta plays a major role in later stages of sustained cell migration. The above data demonstrate that EGFR-overexpressing invasive cells have the ability to compensate the loss of MAPK-mediated signaling through activation of PKC-delta signaling for cell migration, which plays a major role in invasion and metastasis. In addition, data suggest that inhibition of MAPK and PKC-delta signaling pathways should abrogate cell migration and invasion in EGFR-overexpressing human breast cancer cells.