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Query: EC:2.7.10.2 (
focal adhesion kinase
)
44,029
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
We have recently shown that altered peptide ligands influence differentiation of CD4+ T cells into Th1 and Th2 subsets. In the present study, we have examined the biochemical signals in naive CD4+ T cells after priming with altered peptide ligand (APL) that correlate with differences in cytokine expression. Although we observed zeta-chain phosphorylation in APL-stimulated cells, other signaling events such as
ZAP70
and
Lnk
phosphorylation are not initiated. This altered pattern observed in the early phosphorylation events correlates with a distinct Ca2+ mobilization pattern that characterizes APL-stimulated cells. By changing the calcium signaling environment during T cell priming, we present data indicating that qualitative differences in calcium mobilization are associated with differentiation of naive CD4+ T cells into Th1- and Th2-like effector subsets.
...
PMID:Distinct biochemical signals characterize agonist- and altered peptide ligand-induced differentiation of naive CD4+ T cells into Th1 and Th2 subsets. 955 Mar 76
The APS, SH2-B and
LNK
proteins are adapters that activate and modulate receptor tyrosine kinase and JAK/STAT signaling. We now show that a conserved N-terminal domain mediates APS homodimerization. We determined the crystal structure of the dimerization domain at a resolution of 1.7 A using bromide ion MAD phasing. Each molecule contributes two helices to a compact four-helix bundle having a bisecting-U topology. Its most conspicuous feature is a stack of interdigitated phenylalanine side chains at the domain core. These residues create a new motif we refer to as a 'phenylalanine zipper,' which is critical to dimerization. A newly developed bridging yeast tri-hybrid assay showed that APS dimerizes
JAK2
, insulin receptor and IGF1 receptor kinases using its SH2 and dimerization domains. Dimerization via the phenylalanine zipper domain provides a mechanism for activating and modulating tyrosine kinase activity even in the absence of extracellular ligands.
...
PMID:A phenylalanine zipper mediates APS dimerization. 1537 31
Erythropoietin (Epo), along with its receptor EpoR, is the principal regulator of red cell development. Upon Epo addition, the EpoR signaling through the
Janus kinase 2
(
JAK2
) activates multiple pathways including Stat5, phosphoinositide-3 kinase (PI-3K)/Akt, and p42/44 mitogen-activated protein kinase (MAPK). The
adaptor protein Lnk
is implicated in cytokine receptor signaling. Here, we showed that
Lnk
-deficient mice have elevated numbers of erythroid progenitors, and that splenic erythroid colony-forming unit (CFU-e) progenitors are hypersensitive to Epo.
Lnk
(-/-) mice also exhibit superior recovery after erythropoietic stress. In addition,
Lnk
deficiency resulted in enhanced Epo-induced signaling pathways in splenic erythroid progenitors. Conversely,
Lnk
overexpression inhibits Epo-induced cell growth in 32D/EpoR cells. In primary culture of fetal liver cells,
Lnk
overexpression inhibits Epo-dependent erythroblast differentiation and induces apoptosis.
Lnk
blocks 3 major signaling pathways, Stat5, Akt, and MAPK, induced by Epo in primary erythroblasts. In addition, the
Lnk
Src homology 2 (SH2) domain is essential for its inhibitory function, whereas the conserved tyrosine near the C-terminus and the pleckstrin homology (PH) domain of
Lnk
are not critical. Furthermore, wild-type
Lnk
, but not the
Lnk
SH2 mutant, becomes tyrosine-phosphorylated following Epo administration and inhibits EpoR phosphorylation and
JAK2
activation. Hence,
Lnk
, through its SH2 domain, negatively modulates EpoR signaling by attenuating
JAK2
activation, and regulates Epo-mediated erythropoiesis.
...
PMID:Lnk inhibits erythropoiesis and Epo-dependent JAK2 activation and downstream signaling pathways. 1570 83
The isoforms of SH2-B, APS, and
Lnk
form a family of signaling proteins that have been described as activators, mediators, or inhibitors of cytokine and growth factor signaling. We now show that the three alternatively spliced isoforms of human SH2-B readily homodimerize in yeast two-hybrid and cellular transfections assays, and this is mediated specifically by a unique domain in its amino terminus. Consistent with previous reports, we further show that the SH2 domains of SH2-B and APS bind
JAK2
at Tyr813. These findings suggested a model in which two molecules of SH2-B or APS homodimerize with their SH2 domains bound to two
JAK2
molecules, creating heterotetrameric
JAK2
-(SH2-B)2-
JAK2
or
JAK2
-(APS)2-
JAK2
complexes. We further show that APS and SH2-B isoforms heterodimerize. At lower levels of SH2-B or APS expression, dimerization approximates two
JAK2
molecules to induce transactivation. At higher relative concentrations of SH2-B or APS, kinase activation is blocked. SH2-B or APS homodimerization and SH2-B/APS heterodimerization thus provide direct mechanisms for activating and inhibiting
JAK2
and other kinases from the inside of the cell and for potentiating or attenuating cytokine and growth factor receptor signaling when ligands are present.
...
PMID:Kinase activation through dimerization by human SH2-B. 1576 67
In addition to its role in megakaryocyte production, signaling initiated by thrombopoietin (TPO) activation of its receptor, myeloproliferative leukemia virus protooncogene (c-Mpl, or Mpl), controls HSC homeostasis and self-renewal. Under steady-state conditions, mice lacking the inhibitory
adaptor protein Lnk
harbor an expanded HSC pool with enhanced self-renewal. We found that HSCs from
Lnk
-/- mice have an increased quiescent fraction, decelerated cell cycle kinetics, and enhanced resistance to repeat treatments with cytoablative 5-fluorouracil in vivo compared with WT HSCs. We further provide genetic evidence demonstrating that
Lnk
controls HSC quiescence and self-renewal, predominantly through Mpl. Consistent with this observation,
Lnk
-/- HSCs displayed potentiated activation of
JAK2
specifically in response to TPO. Biochemical experiments revealed that
Lnk
directly binds to phosphorylated tyrosine residues in
JAK2
following TPO stimulation. Of note, the
JAK2
V617F mutant, found at high frequencies in myeloproliferative diseases, retains the ability to bind
Lnk
. Therefore, we identified
Lnk
as a physiological negative regulator of
JAK2
in stem cells and TPO/Mpl/
JAK2
/
Lnk
as a major regulatory pathway in controlling stem cell self-renewal and quiescence.
...
PMID:Lnk controls mouse hematopoietic stem cell self-renewal and quiescence through direct interactions with JAK2. 1861 18
The
JAK2
mutation JAK2V617F is found frequently in patients with myeloproliferative disorders (MPD) and transforms hematopoietic cells to cytokine-independent proliferation when expressed with specific cytokine receptors. The Src homology 2 (SH2) and pleckstrin homology (PH) domain-containing
adaptor protein Lnk
(SH2B3) is a negative regulator of hematopoietic cytokine signaling. Here, we show that
Lnk
is a potent inhibitor of JAK2V617F constitutive activity.
Lnk
down-regulates JAK2V617F-mediated signaling and transformation in hematopoietic Ba/F3-erythropoietin receptor cells. Furthermore, in CFU assays,
Lnk
-deficient murine bone marrow cells are significantly more sensitive to transformation by JAK2V617F than wild-type (WT) cells.
Lnk
, through its SH2 and PH domains, interacts with WT and mutant
JAK2
and is phosphorylated by constitutively activated JAK2V617F. Finally, we found that
Lnk
levels are high in CD34(+) hematopoietic progenitors from MPD patients and that
Lnk
expression is induced following
JAK2
activation. Our data suggest that JAK2V617F is susceptible to endogenous negative-feedback regulation, providing new insights into the molecular pathogenesis of MPD.
...
PMID:Lnk inhibits myeloproliferative disorder-associated JAK2 mutant, JAK2V617F. 1929 2
Dysregulated Janus kinase-signal transducer and activator of transcription (JAK-STAT) signaling due to activation of tyrosine kinases is a common feature of myeloid malignancies. Here we report the first human disease-related mutations in the adaptor protein
LNK
, a negative regulator of JAK-STAT signaling, in 2 patients with
JAK2
V617F-negative myeloproliferative neoplasms (MPNs). One patient exhibited a 5 base-pair deletion and missense mutation leading to a premature stop codon and loss of the pleckstrin homology (PH) and Src homology 2 (SH2) domains. A second patient had a missense mutation (E208Q) in the PH domain. BaF3-MPL cells transduced with these
LNK
mutants displayed augmented and sustained thrombopoietin-dependent growth and signaling. Primary samples from MPN patients bearing
LNK
mutations exhibited aberrant JAK-STAT activation, and cytokine-responsive CD34(+) early progenitors were abnormally abundant in both patients. These findings indicate that JAK-STAT activation due to loss of
LNK
negative feedback regulation is a novel mechanism of MPN pathogenesis.
...
PMID:Novel mutations in the inhibitory adaptor protein LNK drive JAK-STAT signaling in patients with myeloproliferative neoplasms. 2070 65
Hematopoietic stem and progenitor cell (HSPC) expansion is regulated by intrinsic signaling pathways activated by cytokines. The intracellular kinase
JAK2
plays an essential role in cytokine signaling, and activating mutations in
JAK2
are found in a number of hematologic malignancies. We previously demonstrated that lymphocyte adaptor protein (
Lnk
, also known as Sh2b3) binds
JAK2
and attenuates its activity, thereby limiting HSPC expansion. Here we show that loss of
Lnk
accelerates and exacerbates oncogenic
JAK2
-induced myeloproliferative diseases (MPDs) in mice. Specifically,
Lnk
deficiency enhanced cytokine-independent JAK/STAT signaling and augmented the ability of oncogenic
JAK2
to expand myeloid progenitors in vitro and in vivo. An activated form of
JAK2
, unable to bind
Lnk
, caused greater myeloid expansion than activated
JAK2
alone and accelerated myelofibrosis, indicating that
Lnk
directly inhibits oncogenic
JAK2
in constraining MPD development. In addition,
Lnk
deficiency cooperated with the BCR/ABL oncogene, the product of which does not directly interact with or depend on
JAK2
or
Lnk
, in chronic myeloid leukemia (CML) development, suggesting that
Lnk
also acts through endogenous pathways to constrain HSPCs. Consistent with this idea, aged
Lnk
-/- mice spontaneously developed a CML-like MPD. Taken together, our data establish
Lnk
as a bona fide suppressor of MPD in mice and raise the possibility that
Lnk
dysfunction contributes to the development of hematologic malignancies in humans.
...
PMID:Lnk constrains myeloproliferative diseases in mice. 2045 46
Activating mutations in signaling molecules, such as
JAK2
-V617F, have been associated with myeloproliferative neoplasms (MPNs). Mice lacking the inhibitory
adaptor protein Lnk
display deregulation of thrombopoietin/thrombopoietin receptor signaling pathways and exhibit similar myeloproliferative characteristics to those found in MPN patients, suggesting a role for
Lnk
in the molecular pathogenesis of these diseases. Here, we showed that
LNK
levels are up-regulated and correlate with an increase in the
JAK2
-V617F mutant allele burden in MPN patients. Using megakaryocytic cells, we demonstrated that
Lnk
expression is regulated by the TPO-signaling pathway, thus indicating an important negative control loop in these cells. Analysis of platelets derived from MPN patients and megakaryocytic cell lines showed that
Lnk
can interact with
JAK2
-WT and V617F through its SH2 domain, but also through an unrevealed
JAK2
-binding site within its N-terminal region. In addition, the presence of the V617F mutation causes a tighter association with
Lnk
. Finally, we found that the expression level of the
Lnk
protein can modulate
JAK2
-V617F-dependent cell proliferation and that its different domains contribute to the inhibition of multilineage and megakaryocytic progenitor cell growth in vitro. Together, our results indicate that changes in
Lnk
expression and
JAK2
-V617F-binding regulate
JAK2
-mediated signals in MPNs.
...
PMID:Expression level and differential JAK2-V617F-binding of the adaptor protein Lnk regulates JAK2-mediated signals in myeloproliferative neoplasms. 2087 Aug 99
Dysregulated signaling is a hallmark of chronic myeloproliferative neoplasms (MPNs), as evidenced by the identification of the activating
JAK2
V617F somatic mutation in almost all patients with polycythemia vera (PV) and 50-60% of essential thrombocythemia and primary myelofibrosis patients. These disorders are clinically distinct, raising the question of how a single mutation can result in such phenotypic diversity. Mouse models have demonstrated that the level of
JAK2
V617F expression can modulate the phenotype, and clinical studies of
JAK2
V617F allele burden have reported similar findings. It has also been hypothesized that one or more pre-
JAK2
V617F events may modify the MPN phenotype. However, the molecular basis of
JAK2
V617F-negative essential thrombocythemia and primary myelofibrosis remains largely unexplained. Mutations in the TET2 gene have been identified in both
JAK2
V617F-positive and -negative MPNs and other myeloid neoplasms, but their functional and clinical significance have yet to be clarified. In addition, recent reports have identified a specific germline haplotype that increases the predisposition to MPNs. The role of inhibitory pathways (e.g., SOCS and
LNK
) in regulating JAK-STAT signaling in MPNs is being increasingly recognized. The implications of these findings and their clinical relevance are the focus of this article.
...
PMID:JAK2 V617F and beyond: role of genetics and aberrant signaling in the pathogenesis of myeloproliferative neoplasms. 2108 83
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