桩蛋白Y118位点的磷酸化通过黏着斑激酶和黏附作用,有助于控制Src诱导的非锚定依赖性生长。
Paxillin-Y118 phosphorylation contributes to the control of Src-induced anchorage-independent growth by FAK and adhesion.
作者信息
Sachdev Sanjay, Bu Yahao, Gelman Irwin H
机构信息
Department of Cancer Genetics, Roswell Park Cancer Institute, Elm and Carlton Streets, Buffalo, NY 14263, USA.
出版信息
BMC Cancer. 2009 Jan 12;9:12. doi: 10.1186/1471-2407-9-12.
BACKGROUND
Focal adhesion kinase (FAK) and Src are protein tyrosine kinases that physically and functionally interact to facilitate cancer progression by regulating oncogenic processes such as cell motility, survival, proliferation, invasiveness, and angiogenesis.
METHOD
To understand how FAK affects oncogenesis through the phosphorylation of cellular substrates of Src, we analyzed the phosphorylation profile of a panel of Src substrates in parental and v-Src-expressing FAK+/+ and FAK-/- mouse embryo fibroblasts, under conditions of anchorage-dependent (adherent) and -independent (suspension) growth.
RESULTS
Total Src-induced cellular tyrosine phosphorylation as well as the number of phosphotyrosyl substrates was higher in suspension versus adherent cultures. Although the total level of Src-induced cellular phosphorylation was similar in FAK+/+ and FAK-/- backgrounds, the phosphorylation of some substrates was influenced by FAK depending on adherence state. Specifically, in the absence of FAK, Src induced higher phosphorylation of p190RhoGAP, paxillin (poY118) and Crk irrespective of adhesion state, PKC-delta (poY311), connexin-43 (poY265) and Sam68 only under adherent conditions, and p56Dok-2 (poY351) and p120catenin (poY228) only under suspension conditions. In contrast, FAK enhanced the Src-induced phosphorylation of vinculin (poY100 and poY1065) and p130CAS (poY410) irrespective of adherence state, p56Dok-2 (poY351) and p120catenin (poY228) only under adherent conditions, and connexin-43 (poY265), cortactin (poY421) and paxillin (poY31) only under suspension conditions. The Src-induced phosphorylation of Eps8, PLC-gamma 1 and Shc (poY239/poY240) were not affected by either FAK or adherence status. The enhanced anchorage-independent growth of FAK-/-[v-Src] cells was selectively decreased by expression of paxillin Y118F, but not by WT-paxillin, p120catenin Y228F or ShcY239/240F, identifying for the first time a role for paxillinpoY118 in Src-induced anchorage-independent growth. Knockdown of FAK by siRNA in the human colon cancer lines HT-25 and RKO, resulted in increased paxillinpoY118 levels under suspension conditions as well as increased anchorage-independent growth, supporting the notion that FAK attenuates anchorage-independent growth by suppressing adhesion-dependent phosphorylation of paxillin Y118.
CONCLUSION
These data suggest that phosphorylation of Src substrates is a dynamic process, influenced temporally and spatially by factors such as FAK and adhesion.
背景
粘着斑激酶(FAK)和Src是蛋白质酪氨酸激酶,它们在物理和功能上相互作用,通过调节细胞运动、存活、增殖、侵袭和血管生成等致癌过程促进癌症进展。
方法
为了解FAK如何通过Src细胞底物的磷酸化影响肿瘤发生,我们分析了在锚定依赖性(贴壁)和非依赖性(悬浮)生长条件下,亲本及表达v-Src的FAK+/+和FAK-/-小鼠胚胎成纤维细胞中一组Src底物的磷酸化谱。
结果
与贴壁培养相比,悬浮培养中总Src诱导的细胞酪氨酸磷酸化以及磷酸酪氨酸底物的数量更高。尽管在FAK+/+和FAK-/-背景下,Src诱导的细胞磷酸化总水平相似,但某些底物的磷酸化受FAK影响,具体取决于粘附状态。具体而言,在缺乏FAK的情况下,无论粘附状态如何,Src都会诱导p190RhoGAP、桩蛋白(poY118)和Crk的磷酸化水平升高;仅在贴壁条件下,Src会诱导蛋白激酶Cδ(PKC-δ,poY311)、连接蛋白43(connexin-43,poY265)和Sam68的磷酸化水平升高;仅在悬浮条件下,Src会诱导p56Dok-2(poY351)和p120连环蛋白(poY228)的磷酸化水平升高。相反,无论粘附状态如何,FAK都会增强Src诱导的纽蛋白(poY100和poY1065)和p130CAS(poY410)的磷酸化水平;仅在贴壁条件下,FAK会增强p56Dok-2(poY351)和p120连环蛋白(poY228)的磷酸化水平;仅在悬浮条件下,FAK会增强连接蛋白43(poY265)、皮层肌动蛋白(cortactin,poY421)和桩蛋白(poY31)的磷酸化水平。Src诱导的Eps8、磷脂酶Cγ1(PLC-γ1)和Shc(poY239/poY240)的磷酸化不受FAK或粘附状态的影响。通过表达桩蛋白Y118F可选择性降低FAK-/-[v-Src]细胞增强的非锚定依赖性生长,但表达野生型桩蛋白、p120连环蛋白Y228F或ShcY239/240F则无此作用,这首次确定了桩蛋白poY118在Src诱导的非锚定依赖性生长中的作用。在人结肠癌细胞系HT-25和RKO中,通过小干扰RNA(siRNA)敲低FAK,导致悬浮条件下桩蛋白poY118水平升高以及非锚定依赖性生长增加,这支持了FAK通过抑制桩蛋白Y118的粘附依赖性磷酸化来减弱非锚定依赖性生长的观点。
结论
这些数据表明,Src底物的磷酸化是一个动态过程,在时间和空间上受FAK和粘附等因素的影响。
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