Comparative analysis of proteins associated with 26S and 20S proteasomes isolated from rabbit brain and liver

Abstract

We have isolated fractions of 26S and 20S proteasomes were from the rabbit liver and the brain. According to mass spectrometric (MS) analysis, the 26S proteasome fractions from these organs contained catalytic and regulatory subunits characteristic of the proteasome core and regulatory subunits. The 20S fractions of brain and liver proteasomes contained only catalytic proteasome subunits. In addition to proteasome subunits, the isolated fractions contained components of the ubiquitin-proteasome system, ubiquitinated proteins, enzymes that play an important role in metabolic processes, cytoskeletal components, signaling, regulatory, and protective proteins, as well as proteins regulating gene expression, cell division, and differentiation. The abundance of a number of proteasome-associated proteins was comparable or exceeded the abundance of intrinsic proteasome components. About a third of the proteins common to all studied fractions (26S and 20S of brain and liver proteasomes) belong to the group of multifunctional proteins. Selective biosensor validation confirmed the affinity binding of proteins (aldolase, phosphoglycerate kinase) identified during MS analysis to the brain 20S proteasome. Comparison of the subproteomes of the 26S and 20S brain proteasomes showed that removal of components of the regulatory (19S) subparticles caused almost two-fold increase in the total number of individual proteins associated with the core part of the proteasome (20S). In the liver, the number of proteins associated with the core part of the proteasome remained basically unchanged after the removal of the components of the regulatory (19S) subparticles. This indicates that in the brain and, possibly, in other organs, proteins of the regulatory (19S) subunit play an important role in the formation of the proteasome interactome.Iz pecheni i mozga krolika vydeleny fraktsii 26S i 20S proteasom. Po dannym mass-spektrometricheskogo (MS) analiza, fraktsii 26S proteasom iz étikh organov soderzhali kataliticheskie i reguliatornye sub"edinitsy, kharakternye dlia korovoĭ chasti proteasom i dlia reguliatornykh subchastits. Fraktsii 20S proteasom mozga i pecheni soderzhali tol'ko kataliticheskie sub"edinitsy proteasom. Pomimo sub"edinits proteasom, v poluchennykh fraktsiiakh obnaruzheny komponenty ubikvitin-proteasomnoĭ sistemy, ubikvitinirovannye belki, fermenty, igraiushchie vazhnuiu rol' v metabolicheskikh protsessakh, komponenty tsitoskeleta, signal'nye, reguliatornye i zashchitnye belki, a takzhe belki reguliatsii ékspressii genov, kletochnogo deleniia i differentsirovki. Predstavlennost' riada assotsiirovannykh s proteasomami belkov byla sopostavima ili prevyshala predstavlennost' sobstvennykh komponentov proteasom. Okolo treti belkov, obshchikh dlia vsekh issledovannykh fraktsiĭ (26S i 20S proteasom mozga i pecheni), otnosiatsia k gruppe mul'tifunktsional'nykh belkov. Vyborochnaia biosensornaia validatsiia podtverdila affinnoe sviazyvanie identifitsirovannykh v khode MS analiza belkov (al'dolaza, fosfoglitseratkinaza) s 20S proteasomoĭ mozga. Sopostavlenie subproteomov 26S i 20S proteasom mozga pokazalo, chto pri udalenii komponentov reguliatornykh (19S) subchastits kolichestvo individual'nykh belkov, assotsiirovannykh s korovoĭ chast'iu proteasomy (20S), prakticheski udvaivalos'. V pecheni kolichestvo belkov, assotsiirovannykh s korovoĭ chast'iu proteasomy, posle udaleniia komponentov reguliatornykh subchastits prakticheski ne izmenialos'. Éto svidetel'stvuet o tom, chto v mozge i, vozmozhno, v drugikh organakh belki reguliatornoĭ (19S) subchastitsy igraiut vazhnuiu rol' v formirovanii proteasomnogo interaktoma.