IdA
stringlengths 6
21
| IdB
stringlengths 6
21
| labels
int64 0
2
| mechanism
stringclasses 40
values | effect
stringclasses 10
values | score
float64 0.1
0.99
⌀ | sentence
stringlengths 10
1.63k
⌀ | signor_id
stringlengths 12
14
|
|---|---|---|---|---|---|---|---|
P35579
|
Q9BRS2
| 0
|
phosphorylation
|
up-regulates activity
| 0.2
|
This study demonstrates that SPC25 acts as a molecular scaffold, mediating SPC25/RIOK1/MYH9 complex formation and triggering the RIOK1‐mediated phosphorylation of MYH9 at Ser1943.Taken together, these results suggested that SPC25 increases MYH9 phosphorylation at Ser1943, enhancing the nuclear accumulation of MYH9 and consequently modulating the transcription of CTNNB1.
|
SIGNOR-278895
|
O14641
|
P30408
| 2
|
binding
|
up-regulates activity
| 0.2
|
TM4SF1 is a partner of DVL2 and positively modulates Wnt/beta-catenin signaling by enhancing DVL2-Axin interaction.
|
SIGNOR-272402
|
P63096
|
P00533
| 0
|
phosphorylation
|
up-regulates activity
| 0.464
|
RTKs directly phosphorylate Gαi on Y154, 155, and Y320.
|
SIGNOR-277227
|
P84243
|
Q15418
| 0
|
phosphorylation
|
down-regulates activity
| 0.2
|
Phosphorylation at ser-11 (h3s10ph) by rps6ka4 and rps6ka5 is important during interphase because it enables the transcription of genes following external stimulation, like mitogens, stress, growth factors or uv irradiation and result in the activation of genes, such as c-fos and c-jun.
|
SIGNOR-70428
|
Q9NXA8
|
P48735
| 1
|
catalytic activity
|
up-regulates activity
| 0.409
|
Here, we report that SIRT5 desuccinylates and deglutarylates isocitrate dehydrogenase 2 (IDH2) and glucose-6-phosphate dehydrogenase (G6PD), respectively, and thus activates both NADPH-producing enzymes.
|
SIGNOR-261212
|
P25098
|
P24941
| 0
|
phosphorylation
|
down-regulates
| 0.2
|
We report that grk2 protein levels are transiently down-regulated during the g2/m transition by a mechanism involving cdk2-mediated phosphorylation of grk2 at serine670, which triggers binding to the prolyl-isomerase pin1 and subsequent degradation.
|
SIGNOR-163279
|
P36507
|
P15056
| 0
|
phosphorylation
|
up-regulates
| 0.75
|
We show that, consequently, b-raf interacts with mek-1 and mek-2 with a better affinity than does c-raf-1, thus strengthening the notion that b-raf is a stronger mek activator than c-raf-l.
|
SIGNOR-42664
|
Q99500
|
P50148
| 2
|
binding
|
up-regulates activity
| 0.517
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-257388
|
P49959
|
Q9NWS0
| 2
|
binding
|
up-regulates activity
| 0.2
|
Here we show that MRE11 directly interacts with PIH1D1, a subunit of heat-shock protein 90 cochaperone R2TP complex, which is required for the assembly of large protein complexes, such as RNA polymerase II, small nucleolar ribonucleoproteins and mammalian target of rapamycin complex 1. The MRE11-PIH1D1 interaction is dependent on casein kinase 2 (CK2) phosphorylation of two acidic sequences within the MRE11 C terminus containing serines 558/561 and 688/689.
|
SIGNOR-265898
|
P11309
|
Q92597
| 1
|
phosphorylation
|
down-regulates activity
| 0.2
|
Collectively, we find that PIM1 expression leads to increased levels of NDRG1 pS330, and PIM1 dependent NDRG1 phosphorylation decreases NDRG1 protein stability.|NDRG1 is phosphorylated by PIM1 at serine 330 (pS330), and the level of NDRG1 pS330 is associated higher grade prostate tumors.
|
SIGNOR-279308
|
O43865
|
Q9NRJ5
| 2
|
binding
|
down-regulates activity
| 0.2
|
Inositol 1,4,5-triphosphate receptor-binding protein released with inositol 1,4,5-triphosphate (IRBIT) associates with components of the mRNA 3' processing machinery in a phosphorylation-dependent manner and inhibits polyadenylation|In addition to CPSF, IRBIT interacted in vitro with poly(A) polymerase (PAP), which is the enzyme recruited by CPSF to elongate the poly(A) tail, and inhibited PAP activity in a phosphorylation-dependent manner.
|
SIGNOR-268331
|
Q8N5V2
|
Q00535
| 0
|
phosphorylation
|
up-regulates activity
| 0.42
|
Importantly, ephexin1, a Rho GEF, is phosphorylated by Cdk5 in vivo .
|
SIGNOR-279021
|
Q9UJD0
|
O15034
| 2
|
binding
|
down-regulates activity
| 0.282
|
SH3 domains of RBPs interact with RIMs. The enhancement of depolarization-induced secretion in PC12 cells by fusion proteins that suppress the associations of RBPs with RIMs and α1 suggests that RBPs may repress RIMs, either directly or through associated proteins.
|
SIGNOR-264371
|
Q14566
|
Q13535
| 0
|
phosphorylation
|
up-regulates
| 0.562
|
Together these data strongly support the conclusion that mec1 directly targets the s/tq sites in mcm4 and mcm6, although it is formally possible that mec1 and mrc1 activate a different s/tq-directed kinase to target mcm4 and mcm6.
|
SIGNOR-169450
|
P01303
|
Q15761
| 2
|
binding
|
up-regulates
| 0.74
|
Npy expression significantly increases whereas the gene expression of its receptors npy1r, npy2r, and npy5r initially decreases.
|
SIGNOR-114746
|
Q15031
|
P18848
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.251
|
QRICH1 promotes the expression of translation-related genes. our combined ChIP-seq and RNA-seq analyses identified that QRICH1 and ATF4 were enriched at the promoters of these specific tRNA synthetases, and that ER stress positively regulated their transcription (Fig. 4I). Together, these findings suggest that QRICH1 and ATF4 modulate tRNA metabolic processes to promote secreted protein synthesis during ER stress.
|
SIGNOR-269421
|
P14373
|
P37231
| 1
|
ubiquitination
|
down-regulates quantity by destabilization
| 0.289
|
Mechanically, TRIM27 ubiquitinates and degrades PPARgamma, following induces cleaved Caspase-3 and IL-1beta expression.
|
SIGNOR-278734
|
Q92911
|
P15056
| 0
|
transcriptional regulation
|
down-regulates quantity by repression
| 0.2
|
The BRAFV600E oncogene induces transforming growth factor beta secretion leading to sodium iodide symporter repression and increased malignancy in thyroid cancer. BRAF induces TGFβ secretion leading to NIS repression in a MEK-ERK–independent manner but cooperating with the MEK-ERK pathway to induce strong tumor invasion, two major traits acquired during PTC progression.
|
SIGNOR-251989
|
P19784
|
Q92915
| 1
|
phosphorylation
|
up-regulates activity
| 0.307
|
Bioluminescence-based screening of small molecule modulators of the FGF14:Nav1.6 complex identified 4,5,6,7 -: tetrabromobenzotriazole (TBB), a potent casein kinase 2 (CK2) inhibitor, as a strong suppressor of FGF14:Nav1.6 interaction. Inhibition of CK2 through TBB reduces the interaction of FGF14 with Nav1.6 and Nav1.2 channels. Mass spectrometry confirmed direct phosphorylation of FGF14 by CK2 at S228 and S230, and mutation to alanine at these sites modified FGF14 modulation of Nav1.6-mediated currents.
|
SIGNOR-275741
|
Q9H2K8
|
Q9H2K8
| 2
|
phosphorylation
|
up-regulates activity
| 0.2
|
These data indicate that JIK is indeed the protein kinase present in the immune complex responsible for autophosphorylation and for the phosphorylation of the exogenous substrate. Moreover, our observations suggest that JIK (A181F183) acts as the catalytically inactive mutant of JIK, which is no longer able to potently undergo autophosphorylation and dramatically phosphorylate MBP, as compared with the wild type JIK.
|
SIGNOR-246302
|
Q92913
|
Q15858
| 2
|
binding
|
down-regulates activity
| 0.357
|
Sodium channel fast inactivation is modulated by alpha subunit interaction with a family of cytoplasmic proteins termed fibroblast growth factor homologous factors (FHFs). In this paper, we report that all A-type FHFs exert rapid onset long-term inactivation on Nav1.6 and other sodium channels.
|
SIGNOR-253423
|
P10275
|
P55089
| 1
|
transcriptional regulation
|
down-regulates quantity by repression
| 0.2
|
When cells were treated with DHT alone, AR was upregulated and translocated into the nuclei, which might repress UCN1 expression via a potential androgen-responsive element found in human CRF family promoter|These data suggest that DHT differentially influences UCN1 levels under normal and inflammatory conditions in human umbilical vein endothelial cells, which involves AR-dependent and -independent mechanisms respectively.
|
SIGNOR-253688
|
Q92945
|
P31751
| 0
|
phosphorylation
|
down-regulates
| 0.343
|
AKT phosphorylates the mRNA decay-promoting factor KSRP at a unique serine residue, induces its association with the multifunctional protein 14-3-3, and prevents KSRP interaction with the exoribonucleolytic complex exosome. This impairs KSRPs ability to promote rapid mRNA decay.
|
SIGNOR-151220
|
Q12778
|
P24941
| 0
|
phosphorylation
|
down-regulates
| 0.652
|
Cdk2 specifically phosphorylated foxo1 at serine-249 (ser249) in vitro and in vivo. Phosphorylation of ser249 resulted in cytoplasmic localization and inhibition of foxo1.
|
SIGNOR-150028
|
O15350
|
P06493
| 0
|
phosphorylation
|
down-regulates activity
| 0.556
|
Cyclin-dependent kinases phosphorylate p73 at threonine 86 in a cell cycle-dependent manner and negatively regulate p73.Furthermore, cyclin a/cdk1/2, cyclin b/cdk1/2, and cyclin e/cdk2 complexes can phosphorylate multiple p73 isoforms in vitro at threonine 86.
|
SIGNOR-99742
|
P36897
|
P27986
| 2
|
binding
|
up-regulates
| 0.381
|
These studies revealed that PI 3-kinase is associated in vivo with both TGF-_ receptor subtypes and that TGF-_1 stimulation enhances PI 3-kinase activity associated with type I TGF-_ receptor in hASM cells.
|
SIGNOR-227525
|
Q5JTZ9
|
P18848
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.244
|
QRICH1 promotes the expression of translation-related genes. our combined ChIP-seq and RNA-seq analyses identified that QRICH1 and ATF4 were enriched at the promoters of these specific tRNA synthetases, and that ER stress positively regulated their transcription (Fig. 4I). Together, these findings suggest that QRICH1 and ATF4 modulate tRNA metabolic processes to promote secreted protein synthesis during ER stress.
|
SIGNOR-269415
|
Q13976
|
P41220
| 1
|
phosphorylation
|
up-regulates activity
| 0.68
|
Thus, PKGI-alpha binds to, phosphorylates and activates RGS-2, attenuating receptor-mediated vascular contraction.
|
SIGNOR-249241
|
O95837
|
P21452
| 2
|
binding
|
up-regulates activity
| 0.433
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-257131
|
P36873
|
P50750
| 1
|
dephosphorylation
|
up-regulates
| 0.2
|
Pp1 is an activator of cdk9. Pp1 dephosphorylates cdk9 thr186.
|
SIGNOR-173454
|
Q14289
|
P06396
| 1
|
phosphorylation
|
down-regulates activity
| 0.527
|
Our results demonstrate that PYK2 inhibits this EGTA stable gelsolin-actin monomer association.|PYK2 phosphorylates gelsolin at tyrosine residues and regulates gelsolin bioactivity, including decreasing gelsolin binding to actin monomer and increasing gelsolin binding to phosphatidylinositol lipids.
|
SIGNOR-278325
|
P56706
|
Q9NPG1
| 2
|
binding
|
up-regulates
| 0.647
|
Wnt proteins bind to the frizzled receptors and lrp5/6 co-receptors, and through stabilizing the critical mediator betBeta-catenin, initiate a complex signaling cascade that plays an important role in regulating cell proliferation and differentiation.
|
SIGNOR-131978
|
P29353
|
P06213
| 2
|
binding
|
up-regulates
| 0.71
|
The npxy motif around 960-tyr residue of the insulin receptor binds to the n-terminal ptb domain of shc.
|
SIGNOR-84251
|
Q96GD4
|
Q02241
| 1
|
phosphorylation
|
down-regulates quantity
| 0.727
|
Furthermore, reduced turnover of regulatory phosphorylation on another Aurora B substrate MKlp1 was observed, suggesting that PP2A-B56\u03b3 and -\u03b5 play a general role opposing Aurora B at the central spindle.|In anaphase, the KIF4A-targeted pool of B56\u03b3 and -\u03b5 is ideally placed to counteract Aurora B phosphorylations on other central spindle proteins such as MKlp1.
|
SIGNOR-280192
|
P49841
|
P49815
| 1
|
phosphorylation
|
up-regulates activity
| 0.731
|
Gsk3 inhibits the mtor pathway by phosphorylating tsc2 in a manner dependent on ampk-priming phosphorylation.
|
SIGNOR-149380
|
P20309
|
P30679
| 2
|
binding
|
up-regulates activity
| 0.397
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-257224
|
P10912
|
P23467
| 0
|
dephosphorylation
|
down-regulates
| 0.295
|
Inally, mrna tissue distribution of these ptps by rt-pcr analysis and coexpression of the wild-type ptps to test their ability to dephosphorylate ligand-activated ghr suggest ptp-h1 and ptp1b as potential candidates involved in ghr signaling.
|
SIGNOR-104580
|
Q02535
|
Q14938
| 0
|
transcriptional regulation
|
down-regulates quantity
| 0.2
|
By integrating transcriptomic profiling (RNA-seq) of Nfia- and Nfix-deficient GNPs with epigenomic profiling (ChIP-seq against NFIA, NFIB and NFIX, and DNase I hypersensitivity assays), we reveal that these transcription factors share a large set of potential transcriptional targets, suggestive of complementary roles for these NFI family members in promoting neural development
|
SIGNOR-268885
|
Q9H4B4
|
O15350
| 1
|
phosphorylation
|
down-regulates activity
| 0.41
|
In this study, we found that Plk3 inhibits pro-apoptotic activity of p73 through physical interaction and phosphorylation.|Plk3 inhibits pro-apoptotic activity of p73 through physical interaction and phosphorylation.
|
SIGNOR-279647
|
P49768
|
Q14790
| 0
|
cleavage
|
up-regulates activity
| 0.368
|
Remarkably, the caspases acting on PS1 could be subdivided in two groups. One group, containing caspase-8, -6 and -11, cleaved PS1 after residues ENDD329 and to a lesser extent after residues AQRD341. A second group consisting of caspase-3, -7 and -1 acted uniquely on AQRD341. Importantly, these two cleavage sites were also recognized by caspases in the C-terminal PS1 fragment produced by constitutive proteolysis.
|
SIGNOR-261760
|
Q13153
|
P27694
| 1
|
phosphorylation
|
up-regulates activity
| 0.2
|
In this article, we found that Ser-135 and Thr-180 of RPA1 are directly phosphorylated by PAK1 in a DOCK7-Rac1/Cdc42-dependent manner.|We further explored the biological role of PAK1 in replication stress and found that depletion of PAK1 resulted in decreased RPA1 and RPA2 chromatin loading and RPA2 foci formation ( Figure 4I-K ) .
|
SIGNOR-279378
|
P12318
|
P43405
| 0
|
phosphorylation
|
up-regulates activity
| 0.673
|
To identify the FcgammaRII-phosphorylating protein tyrosine kinase (PTK), we used the combination of an in vitro and an in vivo approach. In an in vitro assay using recombinant cytoplasmic tails of the different FcgammaRII isoforms as well as tyrosine exchange mutants, we show that each of the BCR-associated PTKs (Lyn, Blk, Fyn, and Syk) shows different phosphorylation patterns with regard to the different FcgammaR isoforms and pointFyn and Blk definitely phosphorylate Y-282 in the ITAM of Fc_RIIa/c, whereas the non-ITAM tyrosine residue (Y-275) becomes phosphorylated by Syk, as the phosphorylation of double point mutants shows. In addi-tion to these tyrosine residues, Fyn, Blk, and Syk might phosphorylate the most C-terminal tyrosine residue (Y-298) because altering this tyrosine residue together with one of the tyrosine residues clearly shown to be phosphorylated by the respective PTK results in the abrogation of phosphorylation.
|
SIGNOR-247590
|
P47871
|
P63092
| 2
|
binding
|
up-regulates activity
| 0.512
|
Glucagon signals through its receptor on the cell surface (Fig.1). The binding of glucagon to the extracellular loops of the glucagon receptor results in conformational changes of the latter, leading to subsequent activation of the coupled G proteins. At least two classes of G proteins are known to be associated with and involved in the signal transduction of the glucagon receptor, namely Gsα and Gq. The activation of Gsα leads to activation of adenylate cyclase, increase in intracellular cAMP levels, and subsequent activation of protein kinase A (PKA).
|
SIGNOR-267715
|
P15498
|
P00519
| 0
|
phosphorylation
|
up-regulates
| 0.401
|
Thus, the c-terminal tail of vav serves as a direct substrate of bcr-abl in vitro.
|
SIGNOR-114091
|
Q9BY84
|
Q16539
| 1
|
dephosphorylation
|
down-regulates
| 0.805
|
Mkp-7 binds to and inactivates p38 mapk and jnk/sapk, but not erk inhibited by dual specificity phosphatases, such as dusp1, dusp10, and dusp16(uniprot)
|
SIGNOR-108233
|
P02511
|
P04637
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.47
|
Aberrant expression of CRYAB has been shown to be associated with several neurological diseases and malignant neoplasms. To identify transcriptional regulators of CRYAB expression, we examined its promoter for binding sites of transcription factors and identified four potential AP-2 binding sites in addition to a p53 binding site reported previously|Taken together, our results indicate that AP-2_ up-regulates the transcription of the CRYAB gene through stabilizing p53
|
SIGNOR-253638
|
O14929
|
Q16576
| 2
|
binding
|
up-regulates activity
| 0.898
|
AMPK increased HAT1 activity through phosphorylation of HAT1-Ser190 and RBBP7-Ser314| interaction between RBBP7 and HAT1 is required for acetyltransferase activity
|
SIGNOR-264786
|
P45984
|
P41970
| 1
|
phosphorylation
|
down-regulates activity
| 0.323
|
JNK binds to the J box in the middle of the protein, and binding is required for phosphorylation of the adjacent EXport motif. Both the binding and phosphorylation sites (the JEX element) are important for Net export.
|
SIGNOR-250138
|
P54274
|
P68400
| 0
|
phosphorylation
|
up-regulates
| 0.2
|
Regulation of telomeric repeat binding factor 1 binding to telomeres by casein kinase 2-mediated phosphorylation. Mapping of the ck2 target site identified threonine 122 as a substrate in trf1. A threonine to alanine change at this position led to a diminished dna binding due to reduced dimerization of trf1.
|
SIGNOR-178034
|
Q9NRM7
|
P35240
| 2
|
binding
|
up-regulates
| 0.693
|
As expected, the nf2-/- fc-912 cells were defective in lats1/2 phosphorylation (figure s2e-f). Subcellular fractionation revealed a significant increase of endogenous lats1/2 in the cytoplasmic relative to the membrane fraction in the nf2-/- fc-912 schwann cells compared to the nf2+/+ fh-912 schwann cells (figure 2e). This localization defect was rescued by re-expression of nf2
|
SIGNOR-202607
|
Q96JJ3
|
Q8WXX7
| 2
|
binding
|
up-regulates activity
| 0.269
|
Mutations in the Autism susceptibility candidate 2 gene (AUTS2), whose protein is believed to act in neuronal cell nuclei, have been associated with multiple psychiatric illnesses, including autism spectrum disorders, intellectual disability, and schizophrenia. Here we show that cytoplasmic AUTS2 is involved in the regulation of the cytoskeleton and neural development. AUTS2 activates Rac1 to induce lamellipodia but downregulates Cdc42 to suppress filopodia. Our loss-of-function and rescue experiments show that a cytoplasmic AUTS2-Rac1 pathway is involved in cortical neuronal migration and neuritogenesis in the developing brain. These results suggest that FL-AUTS2 can activate Rac1 via interaction with P-Rex1 and the Elmo2/Dock180 complex to regulate actin dynamics in N1E-115 cells.
|
SIGNOR-266819
|
P05549
|
P02511
| 1
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.259
|
Aberrant expression of CRYAB has been shown to be associated with several neurological diseases and malignant neoplasms. To identify transcriptional regulators of CRYAB expression, we examined its promoter for binding sites of transcription factors and identified four potential AP-2 binding sites in addition to a p53 binding site reported previously|Taken together, our results indicate that AP-2_ up-regulates the transcription of the CRYAB gene through stabilizing p53
|
SIGNOR-253636
|
O14757
|
P04637
| 1
|
phosphorylation
|
up-regulates activity
| 0.78
|
Phosphorylation by chk1 of at least three of these sites, Ser366, Ser378, and Thr387, was induced by DNA damage.
|
SIGNOR-217861
|
Q9BVG3
|
Q9BVG3
| 2
|
polyubiquitination
|
down-regulates quantity by destabilization
| 0.2
|
A ubiquitination assay performed in HEK293T cells further confirmed the E3 ubiquitin ligase activity and self-ubiquitination activity of TRIM62 and the requirement of the RING finger domain. Importantly, the treatment of HEK293T cells with a proteasome inhibitor stabilized poly-ubiquitinated TRIM62, indicating that self-ubiquitination promoted the proteasomal degradation of TRIM62.
|
SIGNOR-272102
|
Q9GZQ4
|
P08754
| 2
|
binding
|
up-regulates activity
| 0.435
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-256874
|
P49841
|
P36956
| 1
|
phosphorylation
|
down-regulates quantity by destabilization
| 0.485
|
Importantly, we demonstrate that the mature form of endogenous SREBP1 is phosphorylated on Ser-434. Glycogen synthase kinase-3 phosphorylates Ser-434, and the phosphorylation of this residue is attenuated in response to insulin signaling. Interestingly, phosphorylation of Ser-434 promotes the glycogen synthase kinase-3-dependent phosphorylation of Thr-426 and Ser-430 and destabilizes SREBP1.
|
SIGNOR-236667
|
Q9UPQ7
|
P62837
| 2
|
binding
|
up-regulates activity
| 0.385
|
Our initial tests of various E2s showed that the RING domain of PDZRN3 exhibits ubiquitin ligase activity in the presence of E1 and the UbcH5 family of E2 enzymes (Fig. 3 A). Consistent with this finding, GST pull-down assays showed that PDZRN3 directly interacts with the UbcH5B ubiquitin conjugating enzyme (Fig. 3 B).
|
SIGNOR-271663
|
Q13976
|
Q9UH03
| 1
|
phosphorylation
|
up-regulates activity
| 0.2
|
Mutation of Ser-91 to Ala in recombinant Sept3 also abolished PKG phosphorylation, confirming that Ser-91 is the major site in vitro. Therefore Sept3 is phosphorylated on Ser-91 in nerve terminals and its phosphorylation may contribute to the regulation of its subcellular localization in neurons.
|
SIGNOR-263183
|
P15927
|
Q8N2W9
| 0
|
phosphorylation
|
up-regulates
| 0.2
|
Pias1 and pias4 promote brca1 accumulation and sumoylation, rpa phosphorylation, and dsb repair furthermore, phosphorylation of the 34 kda subunit of rpa on ser-4 and ser-8 (ps4/ps8) in response to ir or camptothecin treatment was diminished by pias4 depletion, while pias1 depletion impaired ir-induced but not camptothecin-induced rpa phosphorylation
|
SIGNOR-162164
|
Q96QU1
|
Q8TDI8
| 2
|
binding
|
up-regulates activity
| 0.45
|
Although several studies show that the tip links, composed of PCDH15 and CDH23, are required for normal mechanotransduction, it is unclear how they are coupled to the transduction machinery. Likewise, it has been demonstrated that the transmembrane channel-like proteins TMC1 and TMC2 are required for mechanosensitive responses in hair cells, but how they interact with other components of the mechanotransduction complex is not known. Here, we show that TMC1 and TMC2 can interact with PCDH15, thereby establishing a critical connection between the tip link and these putative components of the mechanotransduction channel in hair cells.
|
SIGNOR-262582
|
Q9Y6R4
|
P45985
| 1
|
phosphorylation
|
up-regulates activity
| 0.568
|
When truncated mapkkk4 (deltamapkkk4) was overexpressed in hek293 cells, it was constitutively activeco-expressed map kinase kinase (mkk)-1, mkk-4, mkk-3 and mkk-6 were activated in vivo by deltamapkkk4. All of the above mkks purified from escherichia coli were phosphorylated and activated by deltamapkkk4 immunoprecipitates in vitro.
|
SIGNOR-62369
|
P20020
|
P17612
| 0
|
phosphorylation
|
up-regulates activity
| 0.451
|
The ATPase is phosphorylated only at this site by the cAMP-dependent protein kinase, and the phosphorylation is inhibited by calmodulin. The effect of the phosphorylation is to decrease the Km for Ca2+ of the purified ATPase from about 10 microM to about 1.4 microM and to increase the Vmax of ATP hydrolysis about 2-fold.
|
SIGNOR-262694
|
P21333
|
Q08209
| 0
|
dephosphorylation
|
down-regulates
| 0.259
|
We report that a purified c-terminal recombinant region of filamin is a suitable substrate for calcineurin in vitro. Furthermore, 1 microm cyclosporin a (csa), a specific calcineurin inhibitor, reduced the dephosphorylation of the recombinant fragment in 293ft cells
|
SIGNOR-143979
|
P23946
|
P14138
| 1
|
cleavage
|
up-regulates activity
| 0.374
|
Chymase from human mast cells selectively cleaved big endothelins (ETs) at the Tyr31-Gly32 bond and produced novel trachea-constricting 31-amino acid-length endothelins, ETs(1-31), without any further degradation products.
|
SIGNOR-256355
|
P14174
|
P25025
| 2
|
binding
|
up-regulates activity
| 0.382
|
We identify the chemokine receptors CXCR2 and CXCR4 as functional receptors for MIF [] By activating both CXCR2 and CXCR4, MIF displays chemokine-like functions and acts as a major regulator of inflammatory cell recruitment and atherogenesis.
|
SIGNOR-252061
|
P08559
|
Q13131
| 0
|
phosphorylation
|
up-regulates activity
| 0.2
|
AMPKα phosphorylates PDHA subunit on Ser295 and Ser314 to activate PDH complex
|
SIGNOR-276837
|
O95166
|
O75385
| 2
|
binding
|
up-regulates
| 0.637
|
N-terminal proline/serine rich (ps) domain of ulk1 (amino acid 287-416) is required for ulk1-gate-16 and ulk1-gabarap protein interactions
|
SIGNOR-85614
|
Q92585
|
P49336
| 2
|
binding
|
up-regulates
| 0.597
|
Mastermind recruits cycc:cdk8 to phosphorylate the notch icd and coordinate activation with turnover
|
SIGNOR-130715
|
Q05397
|
P16591
| 0
|
phosphorylation
|
up-regulates activity
| 0.251
|
The Fer mediated phosphorylation of specific tyrosine residues of FAK was abolished by cotransfection of shRNA against Fer (i.e., shFer), but not by control shRNA, indicating that the phosphorylation of Tyr577, 861, or 925 of FAK in suspended cells was indeed caused by Fer.
|
SIGNOR-279409
|
Q5T1M5
|
P60709
| 2
|
binding
|
up-regulates activity
| 0.2
|
However, we did detect WAFL binding to bothWIP and actin by immunoprecipitation (Fig. 4). In conclusion, we propose a model whereby WAFL associates toendocytic vesicles by its coiled-coil domain and is involved in actin-based movement of early endosomes via WIP and binding to actin.
|
SIGNOR-260595
|
P24941
|
P07948
| 0
|
phosphorylation
|
down-regulates activity
| 0.353
|
We also show that Lyn phosphorylates Tyr15 of Cdk2 and that incubation of Lyn with Cdk2 results in inhibition of Cdk2 activity.
|
SIGNOR-279204
|
P32238
|
O95837
| 2
|
binding
|
up-regulates activity
| 0.459
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-257361
|
O60566
|
Q8NG31
| 2
|
binding
|
up-regulates
| 0.2
|
Association of the amino and middle domain of blinkin with the tpr domains in the amino termini of bubr1 and bub1 is essential for bubr1 and bub1 to execute their distinct mitotic functions
|
SIGNOR-158894
|
P35968
|
P23467
| 0
|
dephosphorylation
|
down-regulates activity
| 0.454
|
VE-PTP/VEGFR2 complex formation resumes with time, leading to dephosphorylation and deactivation of VEGFR2 (right). B) In VE-PTP-deficient cells, such as after siRNA treatment, VEGFR2 activation (middle) is exaggerated, leading to increased phosphorylation at the Y951 and Y1175 phosphorylation sites
|
SIGNOR-248441
|
Q8WWA0
|
P02788
| 2
|
binding
|
up-regulates activity
| 0.362
|
Intelectin 1 (IntL) is known as a lectin expressed in intestinal epithelia and also as a receptor for an iron-binding protein, lactoferrin (LF).
|
SIGNOR-272500
|
P47211
|
P09471
| 2
|
binding
|
up-regulates activity
| 0.25
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-256966
|
P10636-2
|
P17252
| 0
|
phosphorylation
|
down-regulates activity
| 0.265
|
We have studied the relationship between the phosphorylation oftau by several kinases (MARK, PKA, MAPK, GSK3) and its assembly into PHFs. By contrast, MARK and PKA phosphorylate several sites within the repeats (notably theKXGS motifs including Ser262, Ser324, and Ser356, plus Ser320); in addition PKA phosphorylates somesites in the flanking domains, notably Ser214. This type of phosphorylation strongly reduces tau’s affinityfor microtubules, and at the same time inhibits tau’s assembly into PHFs.
|
SIGNOR-275441
|
P63096
|
O00254
| 2
|
binding
|
up-regulates activity
| 0.2
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-257033
|
Q92560
|
Q14145
| 2
|
binding
|
up-regulates quantity by stabilization
| 0.2
|
BAP1 directly binds to and deubiquitinates KEAP1. BAP1 stabilizes KEAP1 by binding to the BTB domain.
|
SIGNOR-268924
|
Q96A54
|
P25098
| 0
|
phosphorylation
|
down-regulates activity
| 0.2
|
AdipoR1 is Directly Phosphorylated by GRK2.|In summary, our study demonstrates for the first time that cardiometabolic-regulatory, anti-inflammatory, and cardioprotective functions of APN are significantly impaired by GRK2 mediated AdipoR1 phosphorylative desensitization during a critical period of post-MI HF development.
|
SIGNOR-279463
|
Q13315
|
Q7LG56
| 1
|
phosphorylation
|
up-regulates
| 0.512
|
Atm-mediated serine 72 phosphorylation stabilizes ribonucleotide reductase small subunit p53r2 protein against mdm2 to dna damage
|
SIGNOR-182423
|
Q96PU5
|
Q15796
| 1
|
ubiquitination
|
down-regulates activity
| 0.781
|
Through its ww domain, nedd4l specifically recognizes a tgf-beta-induced phosphothr-protyr motif in the linker region, resulting in smad2/3 polyubiquitination and degradation
|
SIGNOR-217622
|
Q9Y5H9
|
Q9Y5G6
| 2
|
binding
|
up-regulates activity
| 0.2
|
The clustered protocadherins comprise the largest subfamily of the cadherin superfamily and are predominantly expressed in the nervous system. Pcdh-alpha proteins interact with beta1-integrin to promote cell adhesion. They also form oligomers with Pcdh-gamma proteins at the same membrane sites.
|
SIGNOR-265687
|
Q86Y07
|
Q9UHP3
| 1
|
phosphorylation
|
down-regulates activity
| 0.294
|
Here, we report that USP25 is a novel TRiC interacting protein that is also phosphorylated by VRK2. USP25 catalyzed deubiquitination of the TRiC protein and stabilized the chaperonin, thereby reducing accumulation of misfolded polyglutamine protein aggregates. Notably, USP25 deubiquitinating activity was suppressed when VRK2 phosphorylated the Thr(680), Thr(727), and Ser(745) residues.
|
SIGNOR-273579
|
P17252
|
P09211
| 1
|
phosphorylation
|
up-regulates activity
| 0.2
|
Peptide phosphorylation analyses and both phosphorylation and enzyme kinetic studies with GSTP1 proteins mutated at candidate amino acid residues established Ser-42 and Ser-184 as putative phospho-acceptor residues for both kinases in the GSTP1 protein. Together, these findings show PKA- and PKC-dependent phosphorylation as a significant post-translational mechanism of regulation of GSTP1 function. Together, these results further support S42 and S184 as major phosphor-acceptor residues for PKA and PKC and suggest that the increased activity of the phospho-GSTP1 was not simply a consequence of the negative charge introduced in the GSTP1 protein by the phosphate group.All eight PKC isoforms, PKC-α, PKC-βI, PKC-βII, PKC-ε, PKC-γ, PKC-η, and PKC-ζ phosphorylated the GSTP1 protein efficiently
|
SIGNOR-276024
|
Q9NPG1
|
P56704
| 2
|
binding
|
up-regulates activity
| 0.64
|
Here we focus on the role of Wnts, their putative receptors Frizzled and the soluble antagonist Frzb1 in regulating mammalian myogenesis. Although it is becoming evident that the signaling downstream of Frizzled receptors is much more complex than anticipated, it is conceivable that it may lead to transcriptional activation of Myf5 and MyoD and to initiation of myogenesis.
|
SIGNOR-73039
|
P68400
|
Q13698
| 1
|
phosphorylation
|
up-regulates activity
| 0.2
|
To identify the regulatory sites of phosphorylation under physiologically relevant conditions, Ca(V)1.1 channels were purified from skeletal muscle and sites of phosphorylation on the α1 subunit were identified by mass spectrometry. Two phosphorylation sites were identified in the proximal C-terminal domain, serine 1575 (S1575) and threonine 1579 (T1579), which are conserved in cardiac Ca(V)1.2 channels (S1700 and T1704, respectively). In vitro phosphorylation revealed that Ca(V)1.1-S1575 is a substrate for both cAMP-dependent protein kinase and calcium/calmodulin-dependent protein kinase II, whereas Ca(V)1.1-T1579 is a substrate for casein kinase 2.
|
SIGNOR-263114
|
Q13043
|
Q06830
| 1
|
phosphorylation
|
down-regulates activity
| 0.2
|
Mst1 inactivates Prdx1 by phosphorylating it at Thr-90 and Thr-183, leading to accumulation of hydrogen peroxide in cells.Prdx1 is phosphorylated by Mst1 predominantly at Thr-18, Thr-90, and Thr-183.
|
SIGNOR-276486
|
Q9UIQ6
|
P01178-PRO_0000020495
| 1
|
cleavage
|
down-regulates quantity by destabilization
| 0.2
|
It has been shown that the steady state of the mature OT form can be controlled by an oxytocinase (P-LAP) that is produced in periphery and centrally by the OT-magnocellular neurons. Noticeably, P-LAP is also expressed in parvocellular OT neurons and in other brain structures| The OT intermediate forms are produced from E16.5 (see above) but the mature amidated OT form is detected only from birth. The released mature form is then degraded by an oxytocinase (PLAP)
|
SIGNOR-268552
|
O43353
|
Q9HC29
| 2
|
binding
|
up-regulates activity
| 0.765
|
The function of NOD2 could be to recruit RICK at the plasma membrane to form an active complex able to activate part of the NF-κB pathway. NOD2 induces a membrane recruitment of RICK that is dependent on a CARD-CARD interaction.
|
SIGNOR-252402
|
O15350
|
P0C2W1
| 2
|
binding
|
down-regulates quantity by destabilization
| 0.597
|
The F-box protein FBXO45 promotes the proteasome-dependent degradation of p73.Importantly, SCFFBXO45 ubiquitylates p73 both in vivo and in vitro. Expression of Cul1 dominant negative mutant, but not Cul2, Cul3, Cul4 and Cul5 dominant negative mutants, increased p73 levels (Figure 1c) to an extent similar to that observed in the ts41 cell line at not permissive temperature, suggesting that a Cul1-associated activity is required for p73 protein stability.
|
SIGNOR-271876
|
Q15750
|
O43318
| 2
|
binding
|
up-regulates activity
| 0.929
|
The yeast two-hybrid system has now revealed two human proteins, termed tab1 and tab2 (for tak1 binding protein), that interact with tak1. Overproduction of tab1 enhanced activity of the plasminogen activator inhibitor 1 gene promoter, which is regulated by tgf-beta, and increased the kinase activity of tak1. Tab1 activates the kinase activity of tak1 by directly binding to its catalytic domain. Tab1 overexpression increase the kinase activity of tak1 in mammalian cells.
|
SIGNOR-153031
|
O43921
|
Q9UF33
| 2
|
binding
|
up-regulates
| 0.75
|
Ephrin-a ligands (named ephrin-a1_ephrin-a5) are anchored in the plasma membrane through a gpi-linkage, and each can bind any of the epha subclass of receptors (epha1_epha8)
|
SIGNOR-65419
|
Q9NWZ3
|
Q9NWZ3
| 2
|
phosphorylation
|
up-regulates activity
| 0.2
|
We show irak4 autophosphorylation occurs by an intermolecular reaction and that autophosphorylation is required for full catalytic activity of the kinase. Phosphorylation of any two of the residues thr-342, thr-345, and ser-346 is required for full activity
|
SIGNOR-204657
|
Q02750
|
O15530
| 0
|
phosphorylation
|
up-regulates activity
| 0.27
|
In vitro kinase assay revealed that the direct targets of pdk1 in the mapk pathway were the upstream mapk kinases mek1 and mek2. The identified pdk1 phosphorylation sites in mek1 and mek2 are ser222 and ser226, respectively, and are known to be essential for full activation
|
SIGNOR-236633
|
P63167
|
Q15139
| 0
|
phosphorylation
|
down-regulates activity
| 0.2
|
We now provide evidence that PKD phosphorylates an additional site in DLC1, namely serine 807 within the GAP domain, adding another layer of complexity to PKD-mediated negative regulation of the DLC1 tumor suppressor protein.|We previously reported that PKD inhibits DLC1 cellular function through phosphorylation of serines 327 and 431 [10].
|
SIGNOR-279265
|
P38405
|
Q9UNW8
| 2
|
binding
|
up-regulates activity
| 0.2
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-256945
|
P30679
|
O43613
| 2
|
binding
|
up-regulates activity
| 0.449
|
Here we systematically quantified ligand-induced interactions between 148 GPCRs and all 11 unique G alpha subunit C-termini. For each receptor, we probed chimeric G alpha subunit activation via a transforming growth factor-alpha (TGF alpha) shedding response in HEK293 cells lacking endogenous Gq/11- and G12/13- signaling. | We defined positive coupling if any member of the subfamily scored LogRAi ≥ -1 and negative coupling if all of the members scored LogRAi < -1 (Figure 3A-B). ROC analysis gives AUC = 0.78 (Figure S4A) when considering high-confidence known coupling data and suggested a threshold of LogRAi ≥ -1.0 for defining true couplings. | The score associated to this interaction has a LogRAi ≥ -1.0.
|
SIGNOR-257354
|
P31749
|
Q07352
| 1
|
phosphorylation
|
down-regulates
| 0.657
|
Here we report that protein kinase b (pkb/akt) stabilizes are transcripts by phosphorylating brf1 at serine 92 (s92). Recombinant brf1 promoted in vitro decay of are-containing mrna (are-mrna), yet phosphorylation by pkb impaired this activity.
|
SIGNOR-130376
|
P67775
|
O14757
| 1
|
dephosphorylation
|
down-regulates activity
| 0.496
|
Phosphorylation of Chk1 by ATR is antagonized by a Chk1-regulated protein phosphatase 2A circuit|In response to genotoxic stress, Chk1 is phosphorylated on serines 317 (S317) and 345 (S345) by the ataxia-telangiectasia-related (ATR) protein kinase. Phosphorylation of Chk1 on these C-terminal serine residues is used as an indicator of Chk1 activation in vivo.
|
SIGNOR-248615
|
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