Cytoplasmic cyclin D1 regulates cell invasion and metastasis through the phosphorylation of paxillin

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作者
Noel P. Fusté
Rita Fernández-Hernández
Tània Cemeli
Cristina Mirantes
Neus Pedraza
Marta Rafel
Jordi Torres-Rosell
Neus Colomina
Francisco Ferrezuelo
Xavier Dolcet
Eloi Garí
机构
[1] Cell Cycle Lab,
[2] Institut de Recerca Biomèdica de Lleida (IRBLleida),undefined
[3] and Departament de Ciències Mèdiques Bàsiques; Facultat de Medicina; Universitat de Lleida,undefined
[4] Facultat de Medicina,undefined
[5] Oncopathology Lab,undefined
[6] Institut de Recerca Biomèdica de Lleida (IRBLleida),undefined
[7] and Departament de Ciències Mèdiques Bàsiques; Facultat de Medicina; Universitat de Lleida,undefined
[8] Facultat de Medicina,undefined
[9] Present address: Cell Cycle Group,undefined
[10] Cancer Epigenetics and Biology Program (PEBC),undefined
[11] Institut d’Investigació Biomèdica de Bellvitge (IDIBELL),undefined
[12] Barcelona,undefined
[13] Catalonia,undefined
[14] Spain.,undefined
来源
Nature Communications | / 7卷
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摘要
Cyclin D1 (Ccnd1) together with its binding partner Cdk4 act as a transcriptional regulator to control cell proliferation and migration, and abnormal Ccnd1·Cdk4 expression promotes tumour growth and metastasis. While different nuclear Ccnd1·Cdk4 targets participating in cell proliferation and tissue development have been identified, little is known about how Ccnd1·Cdk4 controls cell adherence and invasion. Here, we show that the focal adhesion component paxillin is a cytoplasmic substrate of Ccnd1·Cdk4. This complex phosphorylates a fraction of paxillin specifically associated to the cell membrane, and promotes Rac1 activation, thereby triggering membrane ruffling and cell invasion in both normal fibroblasts and tumour cells. Our results demonstrate that localization of Ccnd1·Cdk4 to the cytoplasm does not simply act to restrain cell proliferation, but constitutes a functionally relevant mechanism operating under normal and pathological conditions to control cell adhesion, migration and metastasis through activation of a Ccnd1·Cdk4-paxillin-Rac1 axis.
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