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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)
Human
RIN1
was first characterized as a RAS binding protein based on the properties of its carboxyl-terminal domain. We now show that full-length
RIN1
interacts with activated RAS in mammalian cells and defines a minimum region of 434 aa required for efficient RAS binding.
RIN1
interacts with the "effector domain" of RAS and employs some RAS determinants that are common to, and others that are distinct from, those required for the binding of RAF1, a known RAS effector. The same domain of
RIN1
that binds RAS also interacts with 14-3-3 proteins, extending the similarity between
RIN1
and other RAS effectors. When expressed in mammalian cells, the RAS binding domain of
RIN1
can act as a dominant negative signal transduction blocker. The amino-terminal domain of
RIN1
contains a proline-rich sequence similar to consensus Src homology 3 (SH3) binding regions. This
RIN1
sequence shows preferential binding to the
ABL
-SH3 domain in vitro. Moreover, the amino-terminal domain of
RIN1
directly associates with, and is tyrosine phosphorylated by, c-ABL. In addition,
RIN1
encodes a functional SH2 domain that has the potential to activate downstream signals. These data suggest that
RIN1
is able to mediate multiple signals. A differential pattern of expression and alternate splicing indicate several levels of
RIN1
regulation.
...
PMID:Protein binding and signaling properties of RIN1 suggest a unique effector function. 914 71
RIN1
was originally identified by its ability to physically bind to and interfere with activated Ras in yeast. Paradoxically,
RIN1
potentiates the oncogenic activity of the BCR-
ABL
tyrosine kinase in hematopoietic cells and dramatically accelerates BCR-
ABL
-induced leukemias in mice.
RIN1
rescues BCR-
ABL
mutants for transformation in a manner distinguishable from the cell cycle regulators c-Myc and cyclin D1 and the Ras connector Shc. These biological effects require tyrosine phosphorylation of
RIN1
and binding of
RIN1
to the Abl-SH2 and SH3 domains.
RIN1
is tyrosine phosphorylated and is associated with BCR-
ABL
in human and murine leukemic cells.
RIN1
exemplifies a new class of effector molecules dependent on the concerted action of the SH3, SH2, and catalytic domains of a cytoplasmic tyrosine kinase.
...
PMID:Regulation of the oncogenic activity of BCR-ABL by a tightly bound substrate protein RIN1. 920 49
Gene amplification is a common feature of tumors. Overexpression of some amplified genes plays a role in tumor progression. Gene amplification can occur either extrachromosomally as double-minute chromosomes (dmin) or intrachromosomally in the form of homogeneously staining regions (hsrs). Approximately one-half of our oral squamous cell carcinomas (OSCCs) are characterized by amplification of band 11q13, usually as an hsr located entopically (occurring or situated at the normal chromosomal site, as opposed to ectopically). Using chromosomal fluorescence in situ hybridization (FISH), we confirmed the amplification of the cyclin D1 (CCND1/PRAD1) and fibroblast growth factor types 3 and 4 (FGF3/INT2 and FGF4/HSTF1) genes within the 11q13 amplicon in our series of primary OSCCs and derived cell lines. The human
RIN1
gene was isolated as an RAS interaction/interference protein in a genetic selection in yeast and has been described as a putative effector of both the RAS and
ABL
oncogenes. We mapped
RIN1
to 11q13.2. FISH analysis of 10 11q13-amplified OSCC cell lines revealed high-level
RIN1
amplification in two cell lines. Three additional cell lines have what appear to be duplications and/or low-level amplification of
RIN1
, visible in both interphase and metaphase cells. The hybridization pattern of
RIN1
on the metaphase chromosomes is particularly revealing;
RIN1
signals flank the 11q13 hsr, possibly as a result of an inverted duplication. The gene amplification model of Coquelle et al. (1997) predicted that gene amplification occurs by breakage-fusion-bridge (BFB) cycles involving fragile sites. Our data suggest that the pattern of gene amplification at 11q13 in OSCC cell lines is consistent with a BFB model.
RIN1
appears to be a valuable probe for investigating the process of gene amplification in general and, specifically, 11q13 amplification in oral cancer.
...
PMID:A consistent pattern of RIN1 rearrangements in oral squamous cell carcinoma cell lines supports a breakage-fusion-bridge cycle model for 11q13 amplification. 1082
Cellular transformation by the BCR/ABL oncogene depends on the
ABL
-encoded tyrosine kinase activity. To block BCR/ABL function, we created a unique tyrosine phosphatase by fusing the catalytic domain of SHP1 (SHP1c) to the
ABL
binding domain (ABD) of
RIN1
, an established binding partner and substrate for c-ABL and BCR/ABL. This fusion construct (ABD/SHP1c) binds to BCR/ABL in cells and functions as an active phosphatase. ABD/SHP1c effectively suppressed BCR/ABL function as judged by reductions in transformation of fibroblast cells, growth factor independence of hematopoietic cell lines, and proliferation of primary bone marrow cells. In addition, the leukemogenic properties of BCR/ABL in a murine model system were blocked by coexpression of ABD/SHP1c. Both the "escort" function provided by ABD and the inhibitor function provided by the phosphatase of SHP1c were necessary for effective BCR/ABL interference. Expression of ABD/SHP1c also reversed the transformed phenotype of K562, a human leukemia-derived cell line. These results have direct implications for leukemia therapeutics and suggest an approach to block aberrant signal transduction in other pathologies through the use of appropriately designed escort/inhibitors.
...
PMID:BCR/ABL inhibition by an escort/phosphatase fusion protein. 1102
Multistep carcinogenesis is exemplified by chronic myeloid leukemia with clinical manifestation consisting of a chronic phase and blast crisis. Pathological generation of BCR-
ABL
(breakpoint cluster region-Abelson) results in growth promotion, differentiation, resistance to apoptosis, and defect in DNA repair in targeted blood cells. Domains in BCR and
ABL
sequences work in concert to elicit a variety of leukemogenic signals including Ras, STAT5 (signal transducer and activator of transcription-5), Myc, cyclin D1, P13 (phosphatidylinositol 3-kinase),
RIN1
(Ras interaction/interference), and activation of actin cytoskeleton. However, the mechanism of differentiation of transformed cells is poorly understood. A mutator phenotype of BCR-
ABL
could explain the transformation to blast crisis. The aim of this review is to integrate molecular and biological information on BCR,
ABL
, and BCR-
ABL
and to focus on how signaling from those molecules mirrors the biological phenotypes of chronic myeloid leukemia.
...
PMID:Molecular biology of chronic myeloid leukemia. 1134 96
The human
RIN1
gene was first identified as a cDNA fragment that interfered with RAS-induced phenotypes in the yeast Saccharomyces cerevisiae. Subsequent analysis of full-length
RIN1
clones showed that the protein product of this gene is a downstream effector of RAS and binds with high affinity and specificity to activated HRAS. Two downstream
RIN1
effector pathways have been described. The first involves direct activation of RAB5-mediated endocytosis. The second involves direct activation of
ABL
tyrosine kinase activity. Importantly, each of these distinct
RIN1
functions is enhanced by activated RAS, suggesting that
RIN1
represents a unique class of RAS effector connected to two independent signaling pathways. In this chapter, we summarize our assays and approaches for evaluating the biochemistry and biology of
RIN1
.
...
PMID:The RIN family of Ras effectors. 1675 36
Breast cancer progression is driven by altered gene expression. We show that the
RIN1
gene, which encodes a RAS effector regulating epithelial cell properties, is silenced in breast tumor cell lines compared with cultured human mammary epithelial cells. We also report that
RIN1
is often reduced in human breast tumor cells compared with morphologically normal breast glandular cells. At least two silencing mechanisms seem to be involved. Overexpression of the transcription repressor SNAI1 (Snail) was observed in ZR75-1 cells, and SNAI1 knockdown restored
RIN1
expression. In addition, DNA methylation within the
RIN1
promoter and the first exon in KPL-1 cells suggested that epigenetic modifications may contribute to silencing, and demethylation was shown to restore
RIN1
expression. Reexpression of
RIN1
was shown to inhibit anchorage-independent growth in soft agar. In addition,
RIN1
expression inhibited both the initiation and progression of tumorigenesis for two breast tumor cell lines in a mouse model, consistent with a tumor suppressor function. We also show that
RIN1
acts as a negative regulator of tumor cell invasive growth and that this requires the
ABL
kinase-signaling function of
RIN1
, suggesting a mechanism through which
RIN1
silencing may contribute to breast cancer progression.
...
PMID:RIN1 is a breast tumor suppressor gene. 1808 79
ABL
family tyrosine kinases are tightly regulated by autoinhibition and phosphorylation mechanisms. These kinases maintain an inactive conformation through intramolecular interactions involving SH3 and SH2 domains.
RIN1
, a downstream effector of RAS, binds to the
ABL
SH3 and SH2 domains and stimulates
ABL
tyrosine kinase activity.
RIN1
binding to the
ABL2
kinase resulted in a large decrease in Km and a small increase in Vmax toward an
ABL
consensus substrate peptide. The enzyme efficiency (k(cat)/Km) was increased more than 5-fold by
RIN1
. In addition,
RIN1
strongly enhanced
ABL
-mediated phosphorylation of CRK, PSTPIP1, and DOK1, all established
ABL
substrates but with unique protein structures and distinct target sequences. Importantly
RIN1
-mediated stimulation of
ABL
kinase activity was independent of activation by
SRC
-mediated phosphorylation.
RIN1
increased the kinase activity of both
ABL1
and
ABL2
, and this occurred in the presence or absence of
ABL
regulatory domains outside the SH3-SH2-tyrosine kinase domain core. We further demonstrate that a catalytic site mutation associated with broad drug resistance, ABL1T315I, remains responsive to stimulation by
RIN1
. These findings are consistent with an allosteric kinase activation mechanism by which
RIN1
binding promotes a more accessible
ABL
catalytic site through relief of autoinhibition. Direct disruption of
RIN1
binding may therefore be a useful strategy to suppress the activity of normal and oncogenic
ABL
, including inhibitor-resistant mutants that confound current therapeutic strategies. Stimulation through derepression may be applicable to many other tyrosine kinases autoinhibited by coupled SH3 and SH2 domains.
...
PMID:Enhancement of ABL kinase catalytic efficiency by a direct binding regulator is independent of other regulatory mechanisms. 1879 34
ABL
gene translocations create constitutively active tyrosine kinases that are causative in chronic myeloid leukemia, acute lymphocytic leukemia and other hematopoietic malignancies. Consistent retention of
ABL
SH3/SH2 autoinhibitory domains, however, suggests that these leukemogenic tyrosine kinase fusion proteins remain subject to regulation. We resolve this paradox, demonstrating that BCR-ABL1 kinase activity is regulated by
RIN1
, an
ABL
SH3/SH2 binding protein. BCR-ABL1 activity was increased by
RIN1
overexpression and decreased by
RIN1
silencing. Moreover, Rin1(-/-) bone marrow cells were not transformed by BCR-ABL1, ETV6-
ABL1
or BCR-ABL1(T315I), a patient-derived drug-resistant mutant, as judged by growth factor independence. Rescue by ectopic
RIN1
verified a cell autonomous mechanism of collaboration with BCR-ABL1 during transformation. Sensitivity to the
ABL
kinase inhibitor imatinib was increased by
RIN1
silencing, consistent with
RIN1
stabilization of an activated BCR-ABL1 conformation having reduced drug affinity. The dependence on activation by
RIN1
to unleash full catalytic and cell transformation potential reveals a previously unknown vulnerability that could be exploited for treatment of leukemic cases driven by
ABL
translocations. The findings suggest that
RIN1
targeting could be efficacious for imatinib-resistant disease and might complement
ABL
kinase inhibitors in first-line therapy.
...
PMID:ABL fusion oncogene transformation and inhibitor sensitivity are mediated by the cellular regulator RIN1. 2110 29
Stimulation of epidermal growth factor receptor (EGFR) initiates RAS signaling simultaneously with EGFR internalization. Endocytosed EGFR is then either recycled or degraded. EGFR fate is determined in part by the RAS effector
RIN1
, a guanine nucleotide exchange factor (GEF) for RAB5 GTPases. EGFR degradation was slowed by
RIN1
silencing, enhanced by
RIN1
overexpression and accelerated by
RIN1
localization to the plasma membrane.
RIN1
also directly activates
ABL
tyrosine kinases, which regulate actin remodeling, a function not previously connected to endocytosis. We report that
RIN1
-RAB5 signaling favors EGFR downregulation over EGFR recycling, whereas
RIN1
-
ABL
signaling stabilizes EGFR and inhibits macropinocytosis.
RIN1
(QM), a mutant that blocks
ABL
activation, caused EGF-stimulated membrane ruffling, actin remodeling, dextran uptake and EGFR degradation. An
ABL
kinase inhibitor phenocopied these effects in cells overexpressing
RIN1
. EGFR activation also promotes
RIN1
interaction with BIN1, a membrane bending protein. These findings suggest that
RIN1
orchestrates RAB5 activation,
ABL
kinase activation and BIN1 recruitment to determine EGFR fate.
...
PMID:RIN1 orchestrates the activation of RAB5 GTPases and ABL tyrosine kinases to determine the fate of EGFR. 2297 91
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