Transcriptional and posttranscriptional regulation of the adaptor/scaffold protein gene ITSN1

Transcriptional and posttranscriptional regulation of the adaptor/scaffold protein gene ITSN1

ITSN1 adaptor/scaffold protein takes part in a variety of physiological and pathological cellular processes. It has a complex expression regulation and many protein partners. Aim. Characterization of the ITSN1 functioning and expression control is important for understanding its role in cell. Method...

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Datum:2016
Hauptverfasser: Kropyvko, S.V., Gubar, O.S., Gryaznova, T.A., Morderer, D.Ye., Gerasymchuk, D.O., Syvak, L.A., Grabovoy, A.N., Rynditch, A.V.
Format: Artikel
Sprache:English
Veröffentlicht: Інститут молекулярної біології і генетики НАН України 2016
Schriftenreihe:Вiopolymers and Cell
Schlagworte:
Genomics, Transcriptomics and Proteomics
Online Zugang:https://nasplib.isofts.kiev.ua/handle/123456789/152823
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Назва журналу:Digital Library of Periodicals of National Academy of Sciences of Ukraine
Zitieren:Transcriptional and posttranscriptional regulation of the adaptor/scaffold protein gene ITSN1 / S.V. Kropyvko, O.S. Gubar, T.A. Gryaznova, D.Ye. Morderer, D.O. Gerasymchuk, L.A. Syvak, A.N. Grabovoy, A.V. Rynditch // Вiopolymers and Cell. — 2016. — Т. 32, № 3. — С. 203-221. — Бібліогр.: 76 назв. — англ.

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Digital Library of Periodicals of National Academy of Sciences of Ukraine
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Zusammenfassung:ITSN1 adaptor/scaffold protein takes part in a variety of physiological and pathological cellular processes. It has a complex expression regulation and many protein partners. Aim. Characterization of the ITSN1 functioning and expression control is important for understanding its role in cell. Methods. Bioinformatic analysis, semi-quantitative expression analysis by RT-PCR, immunoprecipitation. Results. We have described and analyzed the ITSN1 promoter regions, detected ITSN1 alternatively spliced isoforms at mRNA and protein levels in different cancer specimens. By means of different bioinformatic servers, we have identified the sites for miRNA binding and analyzed the sites for serine, threonine and tyrosine phosphorylation of the ITSN1 protein. Conclusions. We have obtained new data on the ITSN1 expression in pathology. We have also shown the possibility of ITSN1 expression regulation by miRNA and phosphorylation of serine, threonine and tyrosine.

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