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Query: EC:2.7.10.1 (
ERK
)
95,504
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
ALK
-positive anaplastic large-cell lymphoma (ALCL) has been recognized as a distinct type of lymphoma in the heterogeneous group of T/Null-ALCL. While most of the
ALK
-positive ALCL (ALKomas) are characterized by the presence of the NPM-
ALK
fusion protein, the product of the t(2;5)(p23;q35), 10-20% of ALKomas contain variant
ALK
fusions, including ATIC-
ALK
, TFG-
ALK
, CLTC-
ALK
(previously designated CLTCL-
ALK
), TMP3-
ALK
, and MSN-
ALK
. TMP3-
ALK
and TMP4-
ALK
fusions also have been detected in inflammatory myofibroblastic tumors (IMTs), making clear that aberrations of the
ALK
gene are not associated exclusively with the pathogenesis of
ALK
-positive ALCL. Here we report results of molecular studies on two lymphoma cases and one IMT case with variant rearrangements of
ALK
. Our study led to the detection of the CLTC-
ALK
fusion in an ALCL case and to the identification of two novel fusion partners of
ALK
:
ALO17
(
KIAA1618
), a gene with unknown function, which was fused to
ALK
in an ALCL case with a t(2;17)(p23;q25), and CARS, encoding the cysteinyl-tRNA synthetase, which was fused to
ALK
in an IMT case with a t(2;11;2)(p23;p15;q31). These results confirm the recurrent involvement of
ALK
in IMT and further demonstrate the diversity of
ALK
fusion partners, with the ability to homodimerize as a common characteristic.
...
PMID:Identification of novel fusion partners of ALK, the anaplastic lymphoma kinase, in anaplastic large-cell lymphoma and inflammatory myofibroblastic tumor. 1211 24
In anaplastic large cell lymphoma, the
ALK
gene at 2p23 is known to be fused to NPM, TPM3, TPM4, TFG, ATIC, CLTC, MSN, and
ALO17
. All of these translocations result in the expression of chimeric
ALK
transcripts that are translated into fusion proteins with tyrosine kinase activity and oncogenic properties. We report a case showing a restricted cytoplasmic staining pattern of
ALK
and a novel chromosomal abnormality, t(2;22)(p23;q11.2), demonstrated by fluorescence in situ hybridization analysis. The result of 5' RACE analysis showed that the
ALK
gene was fused in-frame to a portion of the non-muscle myosin heavy chain gene, MYH9. Nucleotide sequence of the MYH9-
ALK
chimeric cDNA revealed that the
ALK
breakpoint was different from all those previously reported. It is localized in the same exonic sequence as MSN-
ALK
, but 6 bp downstream, resulting in an in-frame fusion of the two partner proteins. In contrast to the previously reported
ALK
fusion proteins, MYH9-
ALK
may lack a functional oligomerization domain. However, biochemical analysis showed that the new fusion protein is tyrosine phosphorylated in vivo but seems to lack tyrosine kinase activity in vitro. If further investigations confirm this latter result, the in vivo tyrosine phosphorylation of MYH9-
ALK
protein could involve mechanisms different from those described in the other
ALK
hybrid proteins.
...
PMID:Non-muscle myosin heavy chain (MYH9): a new partner fused to ALK in anaplastic large cell lymphoma. 1280 Jan 56
In
ALK
-positive anaplastic large cell lymphomas, positive qualitative PCR for NPM1-
ALK
in peripheral blood and/or bone marrow at diagnosis and during treatment are associated with a higher risk of treatment failure. Real-time quantitative PCR allows identification of very high risk patients. However, this latter technique initially designed for patients with lymphomas carrying the most frequent NPM1-
ALK
translocation necessitates calibration curves, limiting inter-laboratory reproducibility. We designed an
ALK
universal quantitative PCR based on 3'
ALK
transcript amplification to allow the detection of all
ALK
fusion transcripts. We validate the absolute concordance of 3'
ALK
quantitative PCR results with the routine NPM1-
ALK
qualitative and quantitative PCR on 46 samples. The universality of
ALK
fusion transcript detection was also validated on TPM3-,
ALO17
- and ATIC-
ALK
-positive samples, and EML4-
ALK
-positive cell line. Then, we show that digital droplet PCR using 3'
ALK
universal probe gives highly concordant results with 3'
ALK
universal quantitative PCR. A major benefit of digital droplet PCR is a reduced experimental set-up compared with quantitative PCR, without generation of standard curves, leading to a reliable protocol for multilaboratory validation, in multicenter clinical trials essential for this rare pathology. Our
ALK
universal method could be used for the screening of
ALK
fusion transcripts in liquid biopsy of other
ALK
positive tumors, including non-small cell lung carcinomas.
...
PMID:Minimal residual disease monitoring using a 3'ALK universal probe assay in ALK-positive anaplastic large cell lymphoma: ddPCR, an attractive alternative method to real-time quantitative PCR. 3324 76
