Direct molecular fishing in molecular partners investigation in protein–protein and protein–peptide interactions


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Resumo

An original experimental method of direct molecular fishing has been developed for identification of potential partners of protein–protein and protein–peptide interactions. It is based on combination of surface plasmon resonance technology (SPR), size exclusion and affinity chromatography and mass spectrometric identification of proteins (LC-MS/MS). Previously, we demonstrated applicability of this method for protein interactomics using experimental model system, as well as in the pilot study in the frame of the Human Proteome Project (HPP). In the present paper, this method was successfully applied to identify possible molecular partners of 7 target proteins encoded by genes of 18 chromosome (also in the frame of the HPP). Fishing on the affinity sorbents with immobilized target proteins as ligands was carried out using total lysate of human liver tissue as well as pooled sets of fractions (individual for each bait-protein) obtained by means of a combination of size exclusion chromatography and SPR analysis for the presence of potential prey-proteins in each fraction. As a result we obtained lists of possible molecular partners of all 7 proteins and performed a comparative evaluation of direct fishing specificity for these target proteins. Direct molecular fishing was also successfully used for search of potential protein partners interacting with different isoforms of amyloid-beta peptide, playing a key role in the development of Alzheimer’s disease. The synthetic peptides that are analogues of the metal-binding domain isoforms of beta-amyloid were used as molecular baits and the fishing was performed in various fractions of immortalized human neural cells. As a result, 13 potential partner proteins were identified in the cytosol fraction of the cells by fishing on amyloid-beta peptide (1-16).

Sobre autores

A. Ivanov

Institute of Biomedical Chemistry

Autor responsável pela correspondência
Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

P. Ershov

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

A. Molnar

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

Yu. Mezentsev

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

L. Kaluzhskiy

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

E. Yablokov

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

A. Florinskaya

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

O. Gnedenko

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

A. Medvedev

Institute of Biomedical Chemistry

Email: asi@icnet.ru
Rússia, Pogodinskaya ul. 10-8, Moscow, 119121

S. Kozin

Engelhardt Institute of Molecular Biology

Email: asi@icnet.ru
Rússia, ul. Vavilova 32, Moscow, 119991

V. Mitkevich

Engelhardt Institute of Molecular Biology

Email: asi@icnet.ru
Rússia, ul. Vavilova 32, Moscow, 119991

A. Makarov

Engelhardt Institute of Molecular Biology

Email: asi@icnet.ru
Rússia, ul. Vavilova 32, Moscow, 119991

A. Gilep

Institute of Bioorganic Chemistry

Email: asi@icnet.ru
Belarus, ul. akad. Kuprevicha 5/2, Minsk, 220141

A. Luschik

Institute of Bioorganic Chemistry

Email: asi@icnet.ru
Belarus, ul. akad. Kuprevicha 5/2, Minsk, 220141

I. Gaidukevich

Institute of Bioorganic Chemistry

Email: asi@icnet.ru
Belarus, ul. akad. Kuprevicha 5/2, Minsk, 220141

S. Usanov

Institute of Bioorganic Chemistry

Email: asi@icnet.ru
Belarus, ul. akad. Kuprevicha 5/2, Minsk, 220141


Declaração de direitos autorais © Pleiades Publishing, Ltd., 2016

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