Toward a Comprehensive Characterization of a Human Cancer Cell Phosphoproteome

Zhou, Houjiang; Palma, Serena Di; Preisinger, Christian; Peng, Mao; Polat, Ayşe Nur; Heck, Albert J. R.; Mohammed, Shabaz

doi:10.1021/pr300630k

Cited by 363 publications

(288 citation statements)

References 65 publications

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“…Multiple large-scale proteomic analyses have indicated that Cdc7 is phosphorylated at Ser16, Ser302, and Thr503 in prometaphase, [26][27][28] which is consistent with our prediction (Fig 1E.). To further confirm it, we determined the extent of hyper-phosphorylation in vivo by two-dimensional PAGE with mycFLAGtagged Cdc7 WT and Cdc7 £5A expressed in HEK293T cells.…”

Section: Cdc7 Is Phosphorylated During Prometaphase In a Cdk1-dependesupporting

confidence: 92%

“…This may be due to Cdc7 autophosphorylation 14 or phosphorylation by other kinases such as polo-like kinase (Plk), as large scale proteomics studies indicated that Plk phosphorylates Cdc7 at Serine 27 and 277 in prometaphase. 26,28,[30][31][32][33] In any event, our data demonstrate that Cdc7 is phosphorylated at multiple sites in a mitotic Cdkdependent manner around prometaphase.…”

Section: Cdc7 Is Phosphorylated During Prometaphase In a Cdk1-dependementioning

confidence: 61%

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Cdk1-mediated phosphorylation of Cdc7 suppresses DNA re-replication

et al. 2016

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To maintain genetic stability, the entire mammalian genome must replicate only once per cell cycle. This is largely achieved by strictly regulating the stepwise formation of the pre-replication complex (pre-RC), followed by the activation of individual origins of DNA replication by Cdc7/Dbf4 kinase. However, the mechanism how Cdc7 itself is regulated in the context of cell cycle progression is poorly understood. Here we report that Cdc7 is phosphorylated by a Cdk1-dependent manner during prometaphase on multiple sites, resulting in its dissociation from origins. In contrast, Dbf4 is not removed from origins in prometaphase, nor is it degraded as cells exit mitosis. Our data thus demonstrates that constitutive phosphorylation of Cdc7 at Cdk1 recognition sites, but not the regulation of Dbf4, prevents the initiation of DNA replication in normally cycling cells and under conditions that promote re-replication in G2/M. As cells exit mitosis, PP1a associates with and dephosphorylates Cdc7. Together, our data support a model where Cdc7 (de)phosphorylation is the molecular switch for the activation and inactivation of DNA replication in mitosis, directly connecting Cdc7 and PP1a/Cdk1 to the regulation of once-per-cell cycle DNA replication in mammalian cells.

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Section: Cdc7 Is Phosphorylated During Prometaphase In a Cdk1-dependesupporting

confidence: 92%

Section: Cdc7 Is Phosphorylated During Prometaphase In a Cdk1-dependementioning

confidence: 61%

Cdk1-mediated phosphorylation of Cdc7 suppresses DNA re-replication

et al. 2016

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“…All peptides will bind to a cation exchanger at low pH condition, and bound peptides are predominantly separated by a stepwise elution with increasing ionic strength and/or increasing pH value. 28 Through the above process, the peptides obtained from complex biological sample are divided to 6~12 fractions. Phosphoprotein (or phosphpeptides) bound to SCX matrix are eluted in the early fractions, and peptides except for phosphorylated counterparts are eluted gradually on high salt or pH conditions.…”

Section: Strong Cation Exchange (Scx )mentioning

confidence: 99%

“…HILIC has been reported frequently in recent years in phosphoproteomic studies, because highly hydrophilic solutes as phosphorylated ones in comparison with common peptides are retained on the column for the longest time. [28][29][30] In HILIC, hydrophilic components acquired from biological specimens are typically bound onto HILIC column matrix when used with below 10 % aqueous. To isolate the phosphopeptides from ordinary ones, all peptides are fractionated by predominantly increasing the aqueous mobile phase up to 40% (Figure 2-B).…”

Section: Hydrophilic Interaction Chromatography (Hilic)mentioning

confidence: 99%

“…A variety of enrichment and fractionation methods in phosphoproteomics have been reported including the enrichment with immobilized metal affinity chromatography (IMAC) 6,[14][15][16] and metal oxide affinity chromatography (MOAC) as well as titanium dioxide (TiO 2 ), [17][18][19][20][21][22][23][24][25] and fractionation with strong cation exchange (SCX), 26,27 hydrophilic interaction chromatography (HILIC), [28][29][30] and electrostatic repulsion-hydrophilic interaction chromatography (ERLIC). [31][32][33] More recently, the two sequential steps of preparation methods are commonly used in large scale phosphoproteomics.…”

Section: Introductionmentioning

confidence: 99%

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Enrichment Strategies for Identification and Characterization of Phosphoproteome

Lee¹,

Kang²,

Ji³

2015

Mass Spectrometry Letters

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Phosphorylation upon protein is well known to a key regulator that implicates in modulating many cellular processes like growth, migration, and differentiation. Up to date, grafting of multidimensional separation techniques onto advanced mass spectrometry (MS) has emerged as a promising tool for figuring out the biological functions of phosphorylation in a cell. However, advanced MS-based phosphoproteomics is still challenging, due to its intrinsic issues, i.e., low stoichiometry, less susceptibility in positive ion mode, and low abundance in biological sample. To overcome these bottlenecks, diverse techniques (e.g., SCX, HILIC, ERLIC, IMAC, TiO 2 , etc.) are continuously developed for on-/off-line enrichment of phosphorylated protein (or peptide) from biological samples, thereby helping qualitative/quantitative determination of phosphorylated protein and its phosphorylated sites. In this review, we introduce to the overall views of enrichment tools that are universally used to selectively isolate targeted phosphorylated protein (or peptide) from ordinary ones before MS-based phospoproteomic analysis.

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Generation of phospho‐ubiquitin variants by orthogonal translation reveals codon skipping

et al. 2016

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Edited by Michael IbbaThe activity of the Parkinson's disease-linked E3 ligase parkin is stimulated by phosphorylation at ubiquitin Ser65 (pUb S65 ). The role of other ubiquitin phospho-sites and their kinases are unknown. We produced pUb variants (pS7, pS12, pS20, pS57, pS65) by genetically encoding phosphoserine with the UAG codon. In release factor-deficient Escherichia coli (DRF1), intended to enhance UAG read-through, we discovered ubiquitin variants lacking the UAG-encoded residue, demonstrating previously undocumented +3 frame shifting. We successfully purified each pUb variant from mistranslated products. While pUb S20 failed to stimulate parkin, parkin was partially active with pUb S12 . We observed significant ubiquitination when pUb S65 was the sole substrate.

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Toward a Comprehensive Characterization of a Human Cancer Cell Phosphoproteome

Cited by 363 publications

References 65 publications

Cdk1-mediated phosphorylation of Cdc7 suppresses DNA re-replication

Cdk1-mediated phosphorylation of Cdc7 suppresses DNA re-replication

Enrichment Strategies for Identification and Characterization of Phosphoproteome

Generation of phospho‐ubiquitin variants by orthogonal translation reveals codon skipping

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