IdA
stringlengths 6
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| IdB
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| mechanism
stringclasses 40
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stringclasses 10
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float64 0.1
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stringlengths 10
1.63k
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14
|
|---|---|---|---|---|---|---|---|
P07949
|
Q12913
| 0
|
dephosphorylation
|
down-regulates activity
| 0.277
|
The receptor-type protein tyrosine phosphatase J antagonizes the biochemical and biological effects of RET-derived oncoproteins.|PTPRJ expression induces dephosphorylation of the RET(C634R) and, probably via an indirect mechanism, RET/PTC1 oncoproteins on two key RET autophosphorylation sites (Tyr1062 and Tyr905). This results in a significant decrease of RET-induced Shc and extracellular signal-regulated kinase 1/2 phosphorylation levels
|
SIGNOR-248701
|
P17252
|
Q01844
| 1
|
phosphorylation
|
down-regulates activity
| 0.331
|
Here we report thatews, a nuclearrna-bindingprooncoprotein, contains an iq domain, is phosphorylated byproteinkinase c, and interacts with calmodulin. Interestingly, pkc phosphorylation of ews inhibits its binding to rna homopolymers, and conversely,rna binding to ews interferes with pkc phosphorylation./ these data indicate that ews contains an iq domain with ser266 acting as the primary site for pkc phosphorylation.
|
SIGNOR-52850
|
Q9UKA1
|
O95863
| 2
|
binding
|
down-regulates quantity by destabilization
| 0.509
|
FBXL5 is located in the nucleus where it interacts with Snail1 promoting its polyubiquitination and affecting Snail1 protein stability and function by impairing DNA binding. Snail1 is ubiquitinated by the SCFFBXL5 complex. Snail1 downregulation by FBXL5 is prevented by Lats2, a protein kinase that phosphorylates Snail1 precluding its nuclear export but not its polyubiquitination. To demonstrate that FBXL5 has a direct activity on Snail1, we carried out polyubiquitination reactions in vitro. For this we purified Snail1 and the SCFFBXL5 complex from Sf9 insect cells infected with different baculoviruses corresponding to Flag-FBXL5, His-Skp1, HA-Cullin1 and Rbx1 (Supplementary Figure S3C).
|
SIGNOR-272135
|
O00159
|
P50570
| 2
|
binding
|
up-regulates
| 0.355
|
Dynamin bind directly to the sh3 domain of myo1e / an intriguing possibility is that binding of dynamin and synaptojanin to myo1e tail may activate motor activity since it has been demonstrated that myo1e atpase activity is autoinhibited by its sh3 domain
|
SIGNOR-152910
|
Q8NHL6
|
P17693
| 2
|
binding
|
up-regulates
| 0.77
|
Hla-g binds a limited repertoire of peptides and interacts with the inhibitory leukocyte ig-like receptors lir-1 and lir-2
|
SIGNOR-134180
|
O00327
|
Q9UBK2
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.519
|
Transcriptional coactivator PGC-1α integrates the mammalian clock and energy metabolism. Here we show that PGC-1alpha (Ppargc1a), a transcriptional coactivator that regulates energy metabolism, is rhythmically expressed in the liver and skeletal muscle of mice. PGC-1alpha stimulates the expression of clock genes, notably Bmal1 (Arntl) and Rev-erbalpha (Nr1d1), through coactivation of the ROR family of orphan nuclear receptors.
|
SIGNOR-268031
|
P35580
|
Q02078
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.317
|
Myocyte enhancer factor-2 and serum response factor binding elements regulate fast Myosin heavy chain transcription in vivo. We show that the upstream promoter region of the gene most abundantly expressed in mouse skeletal muscles, IIb MyHC, retains binding activity and transcriptional activation for three positive transcription factors, the serum response factor, Oct-1, and myocyte enhancer factor-2, whereas the other two genes (IIa and IId/x) have nucleotide substitutions in these sites that reduce binding and transcriptional activation
|
SIGNOR-238763
|
Q96JA1
|
P22681
| 2
|
binding
|
up-regulates
| 0.589
|
We report upregulation of lrig1 transcript and protein upon egf stimulation, and physical association of the encoded protein with the four egfr orthologs of mammals. Upregulation of lrig1 is followed by enhanced ubiquitylation and degradation of egfr. The underlying mechanism involves recruitment of c-cbl, an e3 ubiquitin ligase that simultaneously ubiquitylates egfr and lrig1 and sorts them for degradation.
|
SIGNOR-127298
|
P22681
|
Q96B97
| 2
|
binding
|
up-regulates
| 0.747
|
The cin85 sh3 domains interact with c-cbl, an e3 ubiquitin ligase, via an unconventional pxxxpr ligand sequence, with the highest affinity displayed by the sh3-b domain. Interaction with cin85 recruits c-cbl to the amap1 complex where its ubiquitination activity is necessary for cancer cells to develop an invasive phenotype and to degrade the matrix.
|
SIGNOR-203139
|
P46527
|
O43524
| 0
|
transcriptional regulation
|
up-regulates quantity
| 0.747
|
AFX transcriptionally activates p27kip1, resulting in increased protein levels.
|
SIGNOR-238610
|
Q9UQM7
|
P07101
| 1
|
phosphorylation
|
up-regulates
| 0.256
|
This increase in ser19 phosphorylation was associated with enhanced th activity and was due, in part, to glutamate-receptor-mediated calcium influx and possibly calcium/calmodulin-dependent protein kinase ii (camkii) activation.
|
SIGNOR-20912
|
Q96QV6
|
Q14493
| 0
|
translation regulation
|
up-regulates quantity by expression
| 0.2
|
Synthesis of mature histone mRNA requires only a single processing reaction: an endonucleolytic cleavage between a conserved stem-loop and a purine-rich downstream element to form the 3' end. The stem-loop binding protein (SLBP) is required for processing, and following processing, histone mRNA is transported to the cytoplasm, where SLBP participates in translation of the histone mRNA|We used radiolabeled probes generated by PCR targeting the open reading frame (ORF) to detect histones H2A, H2B, H3, H4, and H1 and used 7SK snRNA as a loading control (Fig. 2A). The abundance of histone H2A, H2B, H3, and H4 mRNAs is reduced to 37% to 70% of control levels in the SLBP knockdown cells when compared to the C2 control.
|
SIGNOR-265401
|
P11831
|
Q8IZQ8
| 2
|
binding
|
up-regulates
| 0.797
|
A coactivator of srf, myocd, interacts with srf and activates vsmc expression of contractile genes.
|
SIGNOR-174322
|
Q9Y4E8
|
Q7Z569
| 2
|
deubiquitination
|
up-regulates quantity by stabilization
| 0.267
|
Here we report on a novel interaction between the E3 ligase BRAP (also referred to as IMP), a negative regulator of the MAPK scaffold protein KSR, and two closely related deubiquitylases, USP15 and USP4. USP15 as well as USP4 oppose the autoubiquitylation of BRAP, whereas BRAP promotes the ubiquitylation of USP15.
|
SIGNOR-272030
|
Q9UQM7
|
P35372
| 1
|
phosphorylation
|
down-regulates
| 0.2
|
The decrease in mu-opioid receptor activity after chronic agonist exposure (1 microm [d-ala(2),n-mephe(4),gly-ol(5)]-enkephalin) is largely due to kinase-mediated phosphorylation of intracellular receptor domains. We have recently shown that the substitution of two putative ca(2+)/calmodulin-dependent protein kinase ii (camk ii) phosphorylation sites, s261 and s266, by alanines in the third intracellular loop of the rat mu-opioid receptor (rmor1) confers resistance to camk ii-induced receptor desensitization.
|
SIGNOR-79682
|
P53779
|
P16949
| 1
|
phosphorylation
|
down-regulates
| 0.301
|
Involved in the regulation of the microtubule (mt) filament system by destabilizing microtubules. Prevents assembly and promotes disassembly of microtubules. Here we show that in response to hyperosmotic stress, jnk phosphorylates a key cytoplasmic microtubule regulatory protein, stathmin (stmn), on conserved ser-25 and ser-38 residues. In in vitro biochemical studies, we identified stmn ser-38 as the critical residue required for efficient phosphorylation by jnk and identified a novel kinase interaction domain in stmn required for recognition by jnk. We revealed that jnk was required for microtubule stabilization in response to hyperosmotic stress.
|
SIGNOR-166690
|
Q13315
|
Q96SD1
| 1
|
phosphorylation
|
up-regulates
| 0.619
|
The artemis nuclease is defective in radiosensitive severe combined immunodeficiency patients and is required for the repair of a subset of ionising radiation induced dna double-strand breaks (dsbs) in an atm and dna-pk dependent process. Here, we show that artemis phosphorylation by atm and dna-pk in vitro is primarily attributable to s503, s516 and s645 and demonstrate atm dependent phosphorylation at serine 645 in vivo
|
SIGNOR-148315
|
P07332
|
P07332
| 2
|
phosphorylation
|
up-regulates
| 0.2
|
Substitution of kinase domain tyrosine residues 713 or 811 with phenylalanine resulted in a loss of the 10- and 4-kda phosphopeptides, respectively, identifying these tyrosines as in vitro autophosphorylation sites. Cnbr cleavage analysis of fes isolated from 32po4-labeled 293t cells showed that tyr-713 and tyr-811 are also autophosphorylated in vivo. . Mutagenesis of tyr-713 reduced both autophosphorylation of tyr-811 and transphosphorylation of bcr, a recently identified fes substrate, supporting a major regulatory role for tyr-713.
|
SIGNOR-42655
|
P20339
|
Q96Q42
| 2
|
binding
|
up-regulates activity
| 0.735
|
ALS2 activates Rab5 on macropinosomes. Rab5 is activated and concurrently recruited to macropinosomes during ruffle closure. ALS2 depletion abolishes transient Rab5 activation on macropinosomes, while ALS2 is recruited to macropinosomes simultaneously with Rab5 activation. Thus, we conclude ALS2 activates Rab5 on macropinosomes.
|
SIGNOR-277776
|
O43295
|
P63000
| 1
|
gtpase-activating protein
|
down-regulates activity
| 0.566
|
We therefore developed a screening-compatible live-cell imaging assay, using FRET-based biosensors for the prototype GTPases RHOA, RAC1 and CDC4215,19,20 (Extended Data Fig. 2 and Supplementary Note 1)|We found catalytic activities for 45/75 RhoGEFs and 48/63 RhoGAPs| Our data thus not only reveal extensive promiscuity among regulators, but also that the inactivating RhoGAPs are less selective than the activating RhoGEFs (p-value=0.02)(Supplementary Table 2).
|
SIGNOR-260518
|
Q5SQI0
|
P68366
| 1
|
acetylation
|
up-regulates quantity by stabilization
| 0.262
|
Alpha-Tubulin acetyltransferase (alphaTAT1) is the major α-tubulin lysine-40 (K40) acetyltransferase in mammals, nematodes, and protozoa, and its activity plays a conserved role in several microtubule-based processes.|The tubulin subunits of microtubules are acetylated, and lysine-40 (K40) of the alpha-tubulin subunit has been identified as an important conserved site of microtubule acetylation (6–8). This modification is considered a hallmark of stable, long-lived microtubules
|
SIGNOR-272249
|
P0DPH7
|
Q5SQI0
| 0
|
acetylation
|
up-regulates quantity by stabilization
| 0.242
|
Alpha-Tubulin acetyltransferase (alphaTAT1) is the major α-tubulin lysine-40 (K40) acetyltransferase in mammals, nematodes, and protozoa, and its activity plays a conserved role in several microtubule-based processes.|The tubulin subunits of microtubules are acetylated, and lysine-40 (K40) of the alpha-tubulin subunit has been identified as an important conserved site of microtubule acetylation (6–8). This modification is considered a hallmark of stable, long-lived microtubules
|
SIGNOR-272244
|
Q93009
|
P68400
| 0
|
phosphorylation
|
up-regulates quantity by stabilization
| 0.372
|
We find that stabilization of Mdm2, and correspondingly p53 downregulation in unstressed cells, is accomplished by a specific isoform of USP7 (USP7S), which is phosphorylated at serine 18 by the protein kinase CK2. Phosphorylation stabilizes USP7S and thus contributes to Mdm2 stabilization and downregulation of p53.
|
SIGNOR-276530
|
P05026
|
O76024
| 2
|
binding
|
up-regulates quantity
| 0.397
|
Sodium-potassium ATPase 1 Subunit Is a Molecular Partner of Wolframin, an Endoplasmic Reticulum Protein Involved in ER Stress|We conclude that the interaction may be important for Na+/K+ ATPase beta1 subunit maturation
|
SIGNOR-260999
|
Q6W2J9
|
Q13547
| 2
|
binding
|
up-regulates activity
| 0.377
|
BCoR can interact w Because HDACs appear to be involved in repression by an increasing number of transcriptional repressors, we tested whether BCoR can associate with HDACs. BCoR can interact with HDAC1, HDAC3, and HDAC-B/5 more strongly than with HDAC-A/4, HDAC-C, HDAC-D, and HDAC-E.
|
SIGNOR-252236
|
P43403
|
Q9UJU6
| 1
|
phosphorylation
|
up-regulates
| 0.64
|
We found an interaction between the tyrosine kinase zap-70 and hip-55, which was induced by tcr stimulation. Zap-70 phosphorylated hip-55 at tyr-334 and tyr-344, which were shown to be the tyrosine phosphorylation sites of hip-55 in stimulated t cells.Our results demonstrate for the first time that hip-55 is an important adaptor protein for the jnk kinase cascade in tcr signaling.
|
SIGNOR-118695
|
P08754
|
P21918
| 2
|
binding
|
up-regulates activity
| 0.282
|
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-257156
|
Q05209
|
P04626
| 1
|
dephosphorylation
|
down-regulates activity
| 0.619
|
In MDA-MB-231 cells, a human triple negative breast cancer cell line, phosphorylation of PTPN12 on Ser 19 was increased in response to cyclin dependent kinase 2 (CDK2), and this impaired PTPN12 's ability to dephosphorylate HER2 on Y1196.|PTPN12 negatively regulates Her2, by dephosphorylation on Tyr 1196 on Her2.
|
SIGNOR-277038
|
P00519
|
Q9HAZ1
| 0
|
phosphorylation
|
down-regulates
| 0.272
|
Here, we identify clk1, clk4, mst1, mst2 and ttk (also known as mps1) as novel thr735 kinases in vitro / phosphorylation of thr735 in c-abl is critical for binding to 14-3-3
|
SIGNOR-181052
|
P42658
|
Q9UBC3
| 0
|
transcriptional regulation
|
down-regulates quantity by repression
| 0.327
|
Dnmt3b was responsible for transcriptional silencing of Dpp6 gene as depletion of Dnmt3b resulted in increased mRNA and protein expression of Dpp6.
|
SIGNOR-268963
|
P14780
|
P10915
| 1
|
cleavage
|
down-regulates quantity by destabilization
| 0.341
|
Matrix metalloproteinases cleave at two distinct sites on human cartilage link protein. Sequencing studies of modified link protein components revealed that stromelysins-1 and -2, gelatinases A and B and collagenase cleaved specifically between His16 and Ile17, and matrilysin, stromelysin-2 and gelatinase A cleaved between Leu25 and Leu26. Based on previously determined in situ cleavage sites it is evident that matrix metalloproteinases are not solely responsible for the accumulation of link protein degradation products in adult human cartilage, indicating that additional proteolytic agents are involved in the normal catabolism of human cartilage matrix.
|
SIGNOR-256328
|
Q04206
|
P17612
| 0
|
phosphorylation
|
up-regulates
| 0.516
|
The transcriptional activity of nf-kappa b is stimulated upon phosphorylation of its p65 subunit on serine 276 by protein kinase a (pka).
|
SIGNOR-58972
|
Q93009
|
Q8TB45
| 1
|
deubiquitination
|
up-regulates quantity by stabilization
| 0.2
|
Screening the DEPTOR interactome identified that the association of USP-7 deubiquitinase with DEPTOR was dependent upon S235 phosphorylation. Inhibition of USP-7 activity resulted in DEPTOR polyubiquitination and degradation. A scansite search suggested that ERK1 may be responsible for S235 phosphorylation, which was confirmed through the use of inhibitors, ERK1 knockdown, and an in vitro kinase assay.
|
SIGNOR-277588
|
P06748
|
Q13315
| 0
|
phosphorylation
|
up-regulates activity
| 0.352
|
In addition to Serine 125, ATM may also phosphorylate other sites on NPM.
|
SIGNOR-280182
|
Q9H211
|
P45983
| 0
|
phosphorylation
|
up-regulates quantity by stabilization
| 0.368
|
We discovered that human Cdt1, an essential origin licensing protein whose activity must be restricted to G(1) phase, is a substrate of the stress-activated mitogen-activated protein (MAP) kinases p38 and c-Jun N-terminal kinase (JNK). These MAP kinases phosphorylate Cdt1 both during unperturbed G(2) phase and during an acute stress response. Phosphorylation renders Cdt1 resistant to ubiquitin-mediated degradation during S phase and after DNA damage by blocking Cdt1 binding to the Cul4 adaptor, Cdt2.
|
SIGNOR-276361
|
Q14493
|
Q93079
| 1
|
translation regulation
|
up-regulates quantity by expression
| 0.2
|
Synthesis of mature histone mRNA requires only a single processing reaction: an endonucleolytic cleavage between a conserved stem-loop and a purine-rich downstream element to form the 3' end. The stem-loop binding protein (SLBP) is required for processing, and following processing, histone mRNA is transported to the cytoplasm, where SLBP participates in translation of the histone mRNA|We used radiolabeled probes generated by PCR targeting the open reading frame (ORF) to detect histones H2A, H2B, H3, H4, and H1 and used 7SK snRNA as a loading control (Fig. 2A). The abundance of histone H2A, H2B, H3, and H4 mRNAs is reduced to 37% to 70% of control levels in the SLBP knockdown cells when compared to the C2 control.
|
SIGNOR-265391
|
P00533
|
P35070
| 2
|
binding
|
up-regulates
| 0.747
|
Betacellulin is synthesized primarily as a transmembrane precursor, which is then processed to mature molecule by proteolytic events;ten growth factors and their erbb specificities are depicted: egf, amphiregulin((ar), and tgfalfa bind erbb-1, betacellulin, heparin binding egf-like growth factor, and epiregulin bing both erbb-1 and erbb-4.
|
SIGNOR-121953
|
P11678
|
P11678
| 2
|
post translational modification
|
up-regulates activity
| 0.2
|
Human eosinophils are bone marrow-derived, non-dividing granulocytes of the innate immune system, which store the highly cationic proteins eosinophil peroxidase (EPO), major basic protein (MBP), eosinophil-derived neurotoxin (EDN), and eosinophil cationic protein (ECP) in secondary granules. we demonstrated that Tyr nitration of the eosinophil granule proteins is exclusively mediated by EPO, in the presence of functional NADPH oxidase and minute amounts of NOx. EPO appears to nitrate itself via an autocatalytic mechanism.
|
SIGNOR-261706
|
P31269
|
O14744
| 0
|
methylation
|
up-regulates activity
| 0.462
|
Hoxa9 methylation by prmt5 is essential for endothelial cell expression of leukocyte adhesion molecules. / prmt5 is a critical coactivator component in a newly defined, hoxa9-containing transcription complex./ Hoxa9 is methylated on arg140 by prmt5.
|
SIGNOR-195526
|
P22362
|
P51685
| 2
|
binding
|
up-regulates
| 0.726
|
Ccl1 activates the mapk pathway in ccr8-transfected cho cells.
|
SIGNOR-99401
|
P35558
|
Q53ET0
| 0
|
transcriptional regulation
|
up-regulates quantity
| 0.386
|
These results reveal that CRTC2 plays an essential role in the regulation of hepatic gluconeogenesis through coordinated regulation of the glucocorticoid/GR- and glucagon/CREB-signaling pathways on the key genes G6P and PEPCK.
|
SIGNOR-256106
|
P84022
|
O43541
| 2
|
binding
|
down-regulates activity
| 0.497
|
Smad6 and smad7, can prevent tgfb signaling by interacting either with the receptor or with smad2 and smad3
|
SIGNOR-64071
|
P04637
|
P40692
| 1
|
transcriptional regulation
|
up-regulates quantity
| 0.61
|
.... numerous potentially novel targets, including the DNA mismatch repair genes MLH1 and PMS2. Both of these genes were determined to be responsive to DNA damage and p53 activation in normal human fibroblasts, and have p53-response elements within their first intron.
|
SIGNOR-257605
|
Q86X55
|
P23759
| 1
|
methylation
|
up-regulates
| 0.421
|
Carm1 specifically methylates Pax7 at multiple arginine residues in the N terminus of Pax7
|
SIGNOR-255898
|
Q9Y618
|
Q9UQM7
| 0
|
phosphorylation
|
down-regulates
| 0.2
|
We demonstrated that camkii directly bound and phosphorylated smrt at ser-1407, thereby facilitating smrt translocation from the nucleus to the cytoplasm and proteasome-dependent degradation.
|
SIGNOR-191773
|
P78527
|
P52945
| 1
|
phosphorylation
|
down-regulates quantity by destabilization
| 0.307
|
The interaction of PDX-1 with Ku subunits and its phosphorylation on threonine 11 by the DNA-PK appear to be implicated in its degradation by the proteosome.
|
SIGNOR-225542
|
P21757
|
Q86VS8
| 2
|
binding
|
down-regulates
| 0.333
|
We have identified a microtubule-binding protein, hook3, as a novel interacting partner of sr-a. / by transfecting small interfering rna targeting hook3, total and surface expression, receptor-mediated ligand uptake and protein stability of sr-a were significantly promoted, whereas the protein synthesis and maturation were not altered. We propose for the first time that hook3 may participate in the turnover of the endocytosed scavenger receptor
|
SIGNOR-152314
|
Q9BR01
|
P27361
| 0
|
phosphorylation
|
down-regulates
| 0.2
|
The phosphorylation of sult4a1 allows interaction with pin1, which then promotes degradation of the sulfotransferase.
|
SIGNOR-168248
|
P78527
|
P78527
| 2
|
phosphorylation
|
up-regulates activity
| 0.2
|
We have identified seven in vitro autophosphorylation sites in DNA-PKcs. Six of these sites (Thr2609, Ser2612, Thr2620, Ser2624, Thr2638 and Thr2647) are clustered in a region of 38 amino acids in the central region of the protein. Five of these sites (Thr2609, Ser2612, Thr2638, Thr2647 and Ser3205) are conserved between six vertebrate species. Moreover, we show that DNA-PKcs is phosphorylated in vivo at Thr2609, Ser2612, Thr2638 and Thr2647 in okadaic acid-treated human cells. | Thus phosphorylation of DNA-PKcs at one or more of the autophosphorylation sites identified in this study is likely to be required for DNA-PKcs function.
|
SIGNOR-249157
|
O14727
|
P99999
| 2
|
binding
|
up-regulates activity
| 0.792
|
During apoptosis, Apaf-1 binds to cytochrome c and in the presence of ATP/dATP forms an apoptosome, leading to the recruitment and activation of the initiator caspase, caspase-9.
|
SIGNOR-135384
|
P31271
|
O15550
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.285
|
Evidence for direct involvement of UTX in regulation of HOX gene activity was demonstrated through UTX knockdown experiments in HEK293T cells in which loss of UTX induced transcriptional repression of HOXA and HOXC clusters.
|
SIGNOR-260022
|
P52333
|
P17706
| 0
|
dephosphorylation
|
down-regulates activity
| 0.697
|
Upon ligand binding, IL-2R , IL-6R or LeptinR , IFN-_R , IFN-_R and PRLR or growth hormone (GH) receptor associated JAKs become activated. These JAKs mediate phosphorylation of specific tyrosine residues and recruit STATs. Activated STATs are released from the receptor and translocate to the nucleus. PTP1B dephosphorylates JAK2, TYK2 and STAT5 . The 45-kDa form of TC-PTP was shown to dephosphorylate JAK1 and JAK3 as well as STAT1, STAT3 and STAT5.
|
SIGNOR-133078
|
O75306
|
P06493
| 0
|
phosphorylation
|
up-regulates activity
| 0.2
|
Here, we show that a fraction of cyclin B1/Cdk1 proteins localizes to the matrix of mitochondria and phosphorylates a cluster of mitochondrial proteins, including the complex I (CI) subunits in the respiratory chain. Cyclin B1/Cdk1-mediated CI phosphorylation enhances CI activity, whereas deficiency of such phosphorylation in each of the relevant CI subunits results in impairment of CI function.|These results were confirmed by generating phosphorylation defective forms of the five CI subunits through substitutions of S/T residues with Alanine (A) on either Cdk1 optimal or minimal consensus motifs (T383 on NDUFV1, S105 on NDUFV3, S364 on NDUFS2, S55/S29/T5 on NDUFB6, and T142/T120 on NDUFA12). The mutation of Cdk1 consensus motifs severely diminished their phosphorylation
|
SIGNOR-275592
|
P31749
|
Q8TDN4
| 1
|
phosphorylation
|
down-regulates activity
| 0.34
|
Here, we report that Cables1 levels are controlled by a phosphorylation and 14-3-3-dependent mechanism. Mutagenic analyses identified two residues, T44 and T150, that are specifically critical for 14-3-3 binding and that serve as substrates for phosphorylation by the cell survival kinase Akt, which by binding directly to Cables1 recruits 14-3-3 to the complex.Ectopic expression of activated Akt (AKT1) prevented Cables1-induced apoptosis.
|
SIGNOR-276756
|
P41180
|
Q9NV58
| 0
|
ubiquitination
|
down-regulates quantity by destabilization
| 0.381
|
Coexpression with dorfin decreased the amount of total CaR protein and increased CaR ubiquitination, whereas a dominant negative fragment of dorfin had opposite effects. dorfin-mediated proteasomal degradation of immature CaR occurs from the endoplasmic reticulum. Because endogenous CaR in Madin-Darby canine kidney cells is also subject to degradation from the endoplasmic reticulum, dorfin-mediated ubiquitination may contribute to a general mechanism for CaR quality control during biosynthesis.
|
SIGNOR-271456
|
P42345
|
Q96F24
| 1
|
phosphorylation
|
up-regulates activity
| 0.2
|
Human NRBF2 is phosphorylated by MTORC1 at S113 and S120. Upon nutrient starvation or MTORC1 inhibition, NRBF2 phosphorylation is diminished. Phosphorylated NRBF2 preferentially interacts with PIK3C3/PIK3R4. Suppression of NRBF2 phosphorylation by MTORC1 inhibition alters its binding preference from PIK3C3/PIK3R4 to ATG14/BECN1, leading to increased autophagic PtdIns3K complex assembly, as well as enhancement of ULK1 protein complex association.
|
SIGNOR-265875
|
Q9UM73
|
P31939
| 1
|
phosphorylation
|
up-regulates activity
| 0.377
|
ATIC and VASP phosphorylation is dependent on NPM-ALK kinase activity. ATIC activity is enhanced in the presence of NPM-ALK in vitro.The ATIC activity is enhanced by NPM-ALK in HEK-293T-Rex cells.
|
SIGNOR-276171
|
P00519
|
O14818
| 1
|
phosphorylation
|
up-regulates quantity by stabilization
| 0.397
|
PSMA7 degradation is suppressed by c-Abl-mediated tyrosine phosphorylation at Y106
|
SIGNOR-260937
|
P08047
|
P15172
| 0
|
transcriptional regulation
|
down-regulates quantity by repression
| 0.373
|
These data suggest a regulatory model in which MyoD activation during myogenesis causes the down-regulation of Sp1, which contributes to the repression of GLUT1 gene transcription and, therefore, leads to the reduction in GLUT1 expression and glucose transport.
|
SIGNOR-241765
|
O15169
|
P49674
| 0
|
phosphorylation
|
up-regulates
| 0.747
|
We conclude that a major role of axin in the wnt is to provide the kinase activity that initiates the betBeta-catenin phosphorylation cascade at s45. This process is mediated by cki, the alfa, delta, or ? Isoform, all detected in association with axin by lc/ms.
|
SIGNOR-87444
|
Q99607
|
Q13315
| 0
|
phosphorylation
|
down-regulates activity
| 0.349
|
Elf4 is phosphorylated by Atm after gamma irradiation, leading to its degradation.|Thus, Atm promotes Elf4 protein degradation after gamma irradiation via phosphorylation at these sites.
|
SIGNOR-278466
|
P02452
|
P03956
| 0
|
cleavage
|
down-regulates quantity by destabilization
| 0.378
|
In vitro, MMP1 initiates degradation of native fibrillar collagens, crucial components of vertebrate extracellular matrix (ECM), by cleaving the peptide bond between Gly775–Ile776 or Gly775–Lys776 in native type I, II or III collagen molecules3,4.
|
SIGNOR-272336
|
P10909
|
Q86TM6
| 0
|
polyubiquitination
|
down-regulates quantity by destabilization
| 0.32
|
We also report that the ER-associated ubiquitin ligase Hrd1/synoviolin can interact with, and ubiquitinate clusterin. The fact that cleaved endogenous clusterin appears, under certain conditions, to be subject to polyubiquitination (Figure 2C) and proteasomal degradation (1, 2) strongly suggests that it passed through the secretory pathway before reaching the cytosol.
|
SIGNOR-272629
|
P49591
|
P18848
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.2
|
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-269424
|
Q8TCS8
|
P78527
| 0
|
phosphorylation
|
up-regulates activity
| 0.2
|
We also demonstrated that DNAPK phosphorylates PNPase at Ser-776, which is critical for its ribonuclease activity.
|
SIGNOR-263182
|
P78543
|
P17482
| 2
|
binding
|
up-regulates activity
| 0.685
|
The leukemia-associated protein Btg1 and the p53-regulated protein Btg2 interact with the homeoprotein Hoxb9 and enhance its transcriptional activation.
|
SIGNOR-220987
|
Q15796
|
P27361
| 0
|
phosphorylation
|
down-regulates
| 0.748
|
These results suggest that oncogenic ras, acting through mek1 and erk kinases, induces the phosphorylation of smad2 and smad3
|
SIGNOR-66778
|
Q86WV6
|
Q969V5
| 0
|
ubiquitination
|
up-regulates activity
| 0.2
|
Identification of MUL1 as an essential activator of dsDNA mediated STING dependent pathway.|We further report that the mitochondrial E3 ubiquitin protein ligase 1 (MUL1, also known as GIDE/MAPL/MULAN/RNF218) ubiquitinates STING on K224 via K63-linked polyubiquitination, which facilitates optimal STING trafficking and the transcription of host defense genes.
|
SIGNOR-278634
|
Q9GZX7
|
Q9UKB1
| 2
|
binding
|
down-regulates quantity by destabilization
| 0.2
|
Further analysis indicated that CUL7 mediated AID ubiquitination by forming a complex with FBXW11. In a CUL7 fl/fl CD19 cre+ mouse model, we demonstrated that CUL7 knockout significantly enhanced AID protein levels in B cells in the germinal center and increased both the IgG1 and IgA class switching. Collectively, our results reveal a subtle regulation mechanism for tightly controlling AID protein levels. F-box proteins are components of SCF ubiquitin-ligase complexes that contain Skp1, CUL1, or CUL7, and an F-box protein
|
SIGNOR-272024
|
P19174
|
P17948
| 2
|
binding
|
up-regulates
| 0.679
|
We conclude that both flt-1 and kdr have the potential to signal through plc gamma via phosphotyrosine residues located in juxta-membrane and carboxyl tail regions
|
SIGNOR-53743
|
Q9HAU4
|
Q13887
| 1
|
ubiquitination
|
down-regulates quantity by destabilization
| 0.37
|
Consistent with these observations, another study documented that Smurf2 specifically destabilizes KLF5, that the degradation of KLF5 by Smurf2 is disrupted by the proteasome inhibitor MG132, and that Smurf2 ubiquitinates KLF5 .
|
SIGNOR-278781
|
P05129
|
Q16625
| 1
|
phosphorylation
|
up-regulates activity
| 0.307
|
Protein kinase C regulates the phosphorylation and cellular localization of occludin. Ser(338) of occludin was identified as an in vitro protein kinase C phosphorylation site using peptide mass fingerprint analysis and electrospray ionization tandem mass spectroscopy. Both the phosphorylation of occludin and its incorporation into tight junctions induced by calcium switch were markedly inhibited by the PKC inhibitor GF-109203X.
|
SIGNOR-249107
|
Q71DI3
|
Q14493
| 0
|
translation regulation
|
up-regulates quantity by expression
| 0.2
|
Synthesis of mature histone mRNA requires only a single processing reaction: an endonucleolytic cleavage between a conserved stem-loop and a purine-rich downstream element to form the 3' end. The stem-loop binding protein (SLBP) is required for processing, and following processing, histone mRNA is transported to the cytoplasm, where SLBP participates in translation of the histone mRNA|We used radiolabeled probes generated by PCR targeting the open reading frame (ORF) to detect histones H2A, H2B, H3, H4, and H1 and used 7SK snRNA as a loading control (Fig. 2A). The abundance of histone H2A, H2B, H3, and H4 mRNAs is reduced to 37% to 70% of control levels in the SLBP knockdown cells when compared to the C2 control.
|
SIGNOR-265414
|
P24928
|
Q92576
| 2
|
binding
|
down-regulates activity
| 0.46
|
PHF3 interacts with RNA polymerase II through the SPOC domain. PHF3 negatively regulates mRNA levels. Here, we identify PHD-finger protein 3 (PHF3) as a regulator of transcription and mRNA stability that docks onto Pol II CTD through its SPOC domain. Our data suggest that PHF3 acts as a prominent effector of neuronal gene regulation by bridging transcription with mRNA decay. PHF3 SPOC preferentially binds RNA Pol II CTD phosphorylated on Serine-2
|
SIGNOR-266965
|
Q9UQC2
|
P31749
| 0
|
phosphorylation
|
down-regulates
| 0.699
|
Pkb constitutively associates with gab2, phosphorylates gab2 on a consensus phosphorylation site, ser159, in vitro and inhibits gab2 tyrosine phosphorylation.
|
SIGNOR-252468
|
P16104
|
Q9UIG0
| 0
|
phosphorylation
|
up-regulates
| 0.2
|
We show that wstf phosphorylates tyr 142 of h2a.x, and that wstf activity has an important role in regulating several events that are critical for the dna damage response
|
SIGNOR-182831
|
Q01851
|
Q99578
| 2
|
binding
|
up-regulates activity
| 0.525
|
we describe the evidence for a functional interaction between Brn-3a and Rin and demonstrate the role of Rin in modulating the activation of the Brn-3a regulated egr-1 promoter by the N-terminal domain of Brn-3a.
|
SIGNOR-224546
|
P35452
|
O15525
| 2
|
binding
|
down-regulates activity
| 0.376
|
Hoxd12 and MHox, that interact with v-/c-Maf, using the phage display method. The Hox proteins also could associate with the other Maf protein family members, MafB, MafK, MafF, and MafG, but not with Jun and Fos. The Hox proteins negatively regulated the DNA binding, transactivation and cell-transforming abilities of Maf.
|
SIGNOR-221958
|
Q8IYM1
|
Q14141
| 2
|
binding
|
down-regulates
| 0.2
|
Sept12 interacts with sept6 and this interaction alters the filament structure of sept6 in hela cells.
|
SIGNOR-159537
|
P41968
|
P63092
| 2
|
binding
|
up-regulates activity
| 0.547
|
The melanocortin (MC) receptor family consists of five Gs-coupled receptors that control various physiological functions in response to four distinct agonists, adrenocorticotropic hormone (ACTH, also known as corticotrophin) and alpha, beta, and gamma melanocyte-stimulating hormone (MSH), which are derived from the proopiomelanocortin precursor protein, and two inverse agonists, agouti and agouti-related proteins
|
SIGNOR-268702
|
P30793
|
P04792
| 2
|
binding
|
up-regulates quantity by stabilization
| 0.2
|
GTP cyclohydrolase I (GCH), an oligomeric protein composed of 10 identical subunits, is required for the synthesis of neurotransmitters; mutations in GCH are associated with dopa-responsive dystonia (DRD) and hyperphenylalaninemia. Mutated GCH proteins are unstable and prone to dominant-negative effect. We show herein that expression of the GCH mutant GCH-201E or the splicing variant GCH-II caused intracellular inclusion bodies. When Hsp27 was expressed together with the GCH mutants, Hsp27 expression decreased the formation of inclusion bodies by GCH (as assessed by immunofluorescence) and decreased the amount of insoluble GCH mutant proteins (as assessed by Western blot). we demonstrated that Hsp27 increases the expression of the wild-type GCH protein, causes the appearance of the soluble GCH-II protein, and decreases the quantities of insoluble mutated GCH protein. Therefore, it is likely that Hsp27 improves the folding of mutated GCH proteins, so they can stay in free cytosolic compartment.
|
SIGNOR-252222
|
P51668
|
Q9HAU4
| 0
|
ubiquitination
|
up-regulates activity
| 0.702
|
Our data further show that SMURF2 monoubiquitinates UBCH5 at lysine 144 to form an active complex required for efficient degradation of a RAS family E3, beta transducing repeat containing protein 1 (beta-TrCP1).
|
SIGNOR-278718
|
P02745
|
Q07021
| 2
|
binding
|
down-regulates activity
| 0.384
|
Previous studies have shown that gC1qR inhibits aggregated IgG-mediated complement activation by binding to the gC1q site on C1q, thereby preventing IgG from binding to the gh’s (28), suggesting that the binding sites for gC1qR and IgG on C1q may be identical or at least overlapping.
|
SIGNOR-263402
|
Q13127
|
Q9UKL0
| 2
|
binding
|
up-regulates activity
| 0.769
|
We show here that CoREST, a newly identified human protein, functions as a corepressor for REST. A single zinc finger motif in REST is required for CoREST interaction. Together, REST and CoREST mediate repression of the type II sodium channel promoter in nonneural cells, and the REST/CoREST complex may mediate long-term repression essential to maintenance of cell identity.
|
SIGNOR-220618
|
P05067
|
P11802
| 0
|
phosphorylation
|
down-regulates quantity by destabilization
| 0.258
|
These include a significant increase in APP phosphorylation at Thr 668 by cdk2, cdk4, and cdk5, which increases its beta-amyloid production and APP proteolysis by the activated caspases during cell cycle ( xref ; xref ; xref ; xref ).
|
SIGNOR-280214
|
Q92945
|
Q16539
| 0
|
phosphorylation
|
down-regulates activity
| 0.572
|
KSRP, an important factor for AU-rich element (ARE)-directed mRNA decay, undergoes p38-dependent phosphorylation during muscle differentiation. KSRP phosphorylated by p38 displays compromised binding to ARE-containing transcripts and fails to promote their rapid decay, although it retains the ability to interact with the mRNA degradation machinery
|
SIGNOR-235856
|
P38405
|
P24530
| 2
|
binding
|
up-regulates activity
| 0.267
|
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-256924
|
P08603
|
P05156
| 2
|
binding
|
up-regulates activity
| 0.92
|
FH also serves as cofactor for the serine protease factor I (FI) that cleaves C3b into iC3b, unable to form C3 convertase (Fig 1B).
|
SIGNOR-263490
|
Q14344
|
Q15077
| 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-257398
|
P06493
|
Q2NKX8
| 1
|
phosphorylation
|
up-regulates
| 0.579
|
Following phosphorylation of pich on the cdk1 site t1063, plk1 is recruited to pich and controls its localization. Starting in prometaphase, pich accumulates at kinetochores and inner centromeres.
|
SIGNOR-152133
|
P46527
|
Q00535
| 0
|
phosphorylation
|
down-regulates activity
| 0.643
|
CDK5 knockdown in HEY cells significantly prolonged the half-life of TP53 and p27 Kip1 proteins (XREF_FIG).|During neural stem cell differentiation, CDK5 can phosphorylate p27 at Thr187 and at Ser10, promoting neurite outgrowth as neurons differentiate .
|
SIGNOR-279681
|
Q14872
|
O95835
| 0
|
phosphorylation
|
down-regulates activity
| 0.2
|
The Hippo pathway kinases LATS1 and LATS2 attenuate cellular responses to heavy metals through phosphorylating MTF1|the Hippo pathway kinase LATS phosphorylates and inhibits MTF1|LATS phosphorylates MTF1 at S152 and disrupts its association with the promoters of heavy metal response genes, resulting in the loss of heavy metal response gene expression
|
SIGNOR-275473
|
P16112
|
Q9UNA0
| 0
|
cleavage
|
down-regulates quantity by destabilization
| 0.765
|
Aggrecan Degradation in Human Cartilage Evidence for both Matrix Metalloproteinase and Aggrecanase Activity in Normal, Osteoarthritic, and Rheumatoid Joints|Stromelysin-1 (MMP-3), as well as other MMPs, cleave aggrecan in the interglobular domain between Asn341 and Phe342 to generate a G1 fragment with the COOH terminus VDIPEN341 (11–13). This fragment has been isolated and identified by NH2-terminal sequence analysis from human OA cartilage (11). A second proteolytic activity identified as “aggrecanase” also cleaves aggrecan in the interglobular domain, but between Glu373 and Ala374 (19–24), generating a G1 fragment with a COOH terminus of NITEGE374
|
SIGNOR-266985
|
P18031
|
P35568
| 1
|
dephosphorylation
|
down-regulates
| 0.779
|
Tyrosine dephosphorylation and deactivation of insulin receptor substrate-1 by protein-tyrosine phosphatase 1B. Possible facilitation by the formation of a ternary complex with the Grb2 adaptor protein.
|
SIGNOR-74852
|
O75182
|
P04637
| 2
|
binding
|
down-regulates activity
| 0.497
|
The present study shows that under bleomycin-induced stress, expression of Sin3B gets up-regulated and it gets recruited by p53 at its target promoters. Knockdown of Sin3B leads to impaired negative regulation of p53 target genes and thus exemplifies Sin3B as a critical player in down-regulation of p53 subset target genes.
|
SIGNOR-266776
|
O43768
|
Q66LE6
| 2
|
binding
|
down-regulates activity
| 0.769
|
We identified cyclic adenosine monophosphateregulated phosphoprotein 19 (Arpp19) and -Endosulfine as two substrates of Gwl that, when phosphorylated by this kinase, associate with and inhibit PP2A, thus promoting mitotic entry.
|
SIGNOR-243735
|
Q14004
|
Q13541
| 1
|
phosphorylation
|
up-regulates activity
| 0.2
|
CDK13 directly phosphorylates 4E-BP1 at Thr46 and eIF4B at Ser422; genetically or pharmacologically inhibiting CDK13 disrupts mRNA translation.
|
SIGNOR-273113
|
P04637
|
P10415
| 2
|
binding
|
down-regulates activity
| 0.749
|
Mechanistic insights into the mitochondrial function of wtp53 came when it was realized that mitochondrially translocated p53 interacts directly with members of the Bcl-2 family, which are central in governing the induction of mitochondrial outer membrane permeabilization. In response to stress, wtp53 interacts with and neutralizes the anti-apoptotic members Bcl-xL and Bcl-2. This interaction stimulates MOMP and subsequent apoptosis
|
SIGNOR-99712
|
O43541
|
P31273
| 2
|
binding
|
up-regulates activity
| 0.529
|
Smad6 interacts with hox transcription factors as part of the negative feedback circuit in the bmp signaling pathway
|
SIGNOR-75823
|
Q16620
|
P35398
| 0
|
transcriptional regulation
|
up-regulates quantity by expression
| 0.266
|
Some genes which are directly regulated by RORA such as NLGN1 and NTRK2 have been shown to be associated with increased susceptibility to ASD (Correia et al. 2010; Ylisaukko-oja et al. 2005).
|
SIGNOR-265137
|
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