Dynamics of the Ras/ERK MAPK Cascade as Monitored by Fluorescent Probes

Fujioka, Aki; Terai, Kenta; Itoh, Reina E.; Aoki, Kazuhiro; Nakamura, Takeshi; Kuroda, Shinya; Nishida, Eisuke; Matsuda, Minoru

doi:10.1074/jbc.m509344200

Cited by 312 publications

(408 citation statements)

References 44 publications

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“…We have not detected any differences in aggregation state between ERK1-WT and ERK1-⌬4, using both FCS and emFRET measurements in live cells. Our experimental conditions were optimal because all ERK1 molecules expressed were tagged with GFP, and the concentration of GFP-ERKs was in the recently determined range of endogenous ERK expression (39). Our results demonstrate that ERK1-⌬4 activation is less efficient than that of WT ERK, possibly due to abnormal formation of the scaffold complex (24,25).…”

Section: Discussionmentioning

confidence: 59%

“…when the nucleus and cytoplasm displayed equal intensity in the resting condition. In this case, the GFP-ERK1 concentration was 0.82 Ϯ 0.4 M in the cytoplasm and 0.77 Ϯ 0.2 M in the nucleus, values still within endogenous expression levels (39).…”

Section: Resultsmentioning

confidence: 99%

“…7B). Furthermore, it has been demonstrated that at peak stimulation only 5% of MEK molecules are active, whereas up to 60% of ERK molecules are active (39). Hence, rapidly inactivated ERK molecules are trapped instantly by the large pool of inactive MEK inside the cytoplasm, and inefficient activation of ERK1-⌬4 would then retard further release from MEK.…”

Section: Discussionmentioning

confidence: 99%

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ERK Nuclear Translocation Is Dimerization-independent but Controlled by the Rate of Phosphorylation

Lidke

Huang

Post

et al. 2010

Journal of Biological Chemistry

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Upon activation, ERKs translocate from the cytoplasm to the nucleus. This process is required for the induction of many cellular responses, yet the molecular mechanisms that regulate ERK nuclear translocation are not fully understood. We have used a mouse embryo fibroblast ERK1-knock-out cell line expressing green fluorescent protein (GFP)-tagged ERK1 to probe the spatiotemporal regulation of ERK1. Real time fluorescence microscopy and fluorescence correlation spectroscopy revealed that ERK1 nuclear accumulation increased upon serum stimulation, but the mobility of the protein in the nucleus and cytoplasm remained unchanged. Dimerization of ERK has been proposed as a requirement for nuclear translocation. However, ERK1-⌬4, the mutant shown consistently to be dimerization-deficient in vitro, accumulated in the nucleus to the same level as wild type (WT), indicating that dimerization of ERK1 is not required for nuclear entry and retention. Consistent with this finding, energy migration Förster resonance energy transfer and fluorescence correlation spectroscopy measurements in living cells did not detect dimerization of GFP-ERK1-WT upon activation. In contrast, the kinetics of nuclear accumulation and phosphorylation of GFP-ERK1-⌬4 were slower than that of GFP-ERK1-WT. These results indicate that the differential shuttling behavior of the mutant is a consequence of delayed phosphorylation of ERK by MEK rather than dimerization. Our data demonstrate for the first time that a delay in cytoplasmic activation of ERK is directly translated into a delay in nuclear translocation.Stimulation of numerous cell surface receptors leads to activation of the Raf/MEK 7 /ERK signaling pathway. In this kinase cascade, Raf phosphorylates only MEK, and MEK phosphorylates only ERK, whereas ERK is able to phosphorylate many substrates in nearly all cell compartments (1). Noncatalytic activation of a few partners by c-Raf is well documented, but the biological outcomes of the ERK pathway are predominantly driven by the kinase activity, as evidenced, for example, by chemical inhibition (reviewed in Ref.2). ERK is primarily located in the cytoplasm of resting cells, although overexpression results in cytoplasmic and nuclear localization (3). It has long been recognized that in the course of physiological signal transduction, ERK accumulates in the nucleus after acute stimulation of the cell (3, 4). Nuclear translocation of ERK is required for cell cycle entry. Thus, retention of ERK in the cytoplasm alters neither ERK kinase activity nor phosphorylation of cytoplasmic substrates, whereas ERK-dependent transcription and cell proliferation are blocked (5). It has been demonstrated that ERK phosphorylates the Phe-Gly nucleoporins Nup50, Nup153, and Nup154, reducing importin-␤-mediated nucleocytoplasmic transport (6). This observation would expand the role of ERK nuclear entry to include the regulation of nucleocytoplasmic transport of certain classes of proteins while crossing the nucleopore.MEK functions as the cytoplasmic anchor for ERK su...

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Section: Discussionmentioning

confidence: 59%

Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

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ERK Nuclear Translocation Is Dimerization-independent but Controlled by the Rate of Phosphorylation

Lidke

Huang

Post

et al. 2010

Journal of Biological Chemistry

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“…Each kinetic simulation model reported previously recapitulates the stimulus-induced ERK activation fairly well. Nevertheless, the parameters used therein are sometimes astonishingly different from each other (14). One apparent reason for this discrepancy is that these studies often use different algorithms to fit the parameters to the experimental data (15)(16)(17).…”

mentioning

confidence: 97%

“…To collect and evaluate the parameters in living cells, we previously adopted fluorescent protein technologies and developed a kinetic simulation model based on the experimentally validated parameters (14). This simulation model contained only four signaling molecules, Ras, Raf, MEK, and ERK, but still successfully reproduced the essential features of the Ras-ERK MAPK pathway and demonstrated the usefulness of the parameters collected in living cells.…”

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confidence: 99%

Multiple Decisive Phosphorylation Sites for the Negative Feedback Regulation of SOS1 via ERK*

Kamioka

Yasuda²,

Fujita

et al. 2010

Journal of Biological Chemistry

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EGF-induced activation of ERK has been extensively studied by both experimental and theoretical approaches. Here, we used a simulation model based mostly on experimentally determined parameters to study the ERK-mediated negative feedback regulation of the Ras guanine nucleotide exchange factor, son of sevenless (SOS). Because SOS1 is phosphorylated at multiple serine residues upon stimulation, we evaluated the role of the multiplicity by building two simulation models, which we termed the decisive and cooperative phosphorylation models. The two models were constrained by the duration of Ras activation and basal phosphorylation level of SOS1. Possible solutions were found only in the decisive model wherein at least three, and probably more than four, phosphorylation sites decisively suppress the SOS activity. Thus, the combination of experimental approaches and the model analysis has suggested an unexpected role of multiple phosphorylations of SOS1 in the negative regulation.

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In Vivo Imaging of Signal Transduction Cascades with Probes Based on Förster Resonance Energy Transfer (FRET)

Nakamura

2009

CP Cell Biology

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Genetically encoded FRET probes enable us to visualize a variety of signaling events such as protein phosphorylation and G‐protein activation in living cells. This unit focuses on FRET probes wherein both the donor and acceptor are fluorescence proteins and incorporated into a single molecule, i.e., a unimolecular probe. Advantages of these probes lie in their easy loading into cells, simple acquisition of FRET images, and clear evaluation of data. We have developed FRET probes for Ras‐superfamily GTPases, designated Ras and interacting protein chimeric unit (Raichu) probes. We hereby describe strategies to develop Raichu‐type FRET probes, procedures for their characterization, and acquisition and processing of images. Although improvements upon FRET probes are still based on trial‐and‐error, we provide practical tips for their optimization and briefly discuss the theory and applications of unimolecular FRET probes. Curr. Protoc. Cell Biol. 45:14.10.1‐14.10.12. © 2009 by John Wiley & Sons, Inc.

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Dynamics of the Ras/ERK MAPK Cascade as Monitored by Fluorescent Probes

Cited by 312 publications

References 44 publications

ERK Nuclear Translocation Is Dimerization-independent but Controlled by the Rate of Phosphorylation

ERK Nuclear Translocation Is Dimerization-independent but Controlled by the Rate of Phosphorylation

Multiple Decisive Phosphorylation Sites for the Negative Feedback Regulation of SOS1 via ERK*

In Vivo Imaging of Signal Transduction Cascades with Probes Based on Förster Resonance Energy Transfer (FRET)

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