Pregled bibliografske jedinice broj: 90061
The accuracy of seryl-tRNA synthesis
The accuracy of seryl-tRNA synthesis // 1st Croatian Congress on Molecular Life Sciences with international participation / Dumić, Jerka (ur.).
Zagreb: Farmaceutsko-biokemijski fakultet Sveučilišta u Zagrebu, 2002. str. - (pozvano predavanje, domaća recenzija, sažetak, znanstveni)
CROSBI ID: 90061 Za ispravke kontaktirajte CROSBI podršku putem web obrasca
Naslov
The accuracy of seryl-tRNA synthesis
Autori
Weygand-Đurašević, Ivana
Vrsta, podvrsta i kategorija rada
Sažeci sa skupova, sažetak, znanstveni
Izvornik
1st Croatian Congress on Molecular Life Sciences with international participation
/ Dumić, Jerka - Zagreb : Farmaceutsko-biokemijski fakultet Sveučilišta u Zagrebu, 2002
Skup
1st Croatian Congress on Molecular Life Sciences with international participation
Mjesto i datum
Opatija, Hrvatska, 09.06.2002. - 13.06.2002
Vrsta sudjelovanja
Pozvano predavanje
Vrsta recenzije
Domaća recenzija
Ključne riječi
biosinteza proteina ; točnost translacije ; aminoacil-tRNA-sintetaze
(protein biosynthesis ; accuracy of translation ; aminoacyl-tRNA synthetases)
Sažetak
The high level of translational fidelity is ensured by various types of quality control mechanisms, which are adapted to prevent or correct naturally occurring mistakes. Accurate aminoacyl-tRNA synthesis is mostly dependent on the specificity of the aminoacyl-tRNA synthetases, i.e. their ability to choose between competing structurally similar substrates. Our studies have revealed that accurate seryl-tRNA synthesis in yeast and plants is accomplished via tRNA-assisted optimization of amino acid binding to the enzyme active site. Based on our recent kinetic data, a mechanism is proposed by which transient protein:RNA complex activates the cognate amino acid more efficiently and more specifically than the apoenzyme alone. This may proceed via a tRNA-induced conformational change in the enzyme’ s active site. As shown by the truncation of tRNA at the 3’ -end, terminal adenosine is not important in effecting the rearrangement of the serine binding site. The influence of 3’ -truncated tRNASer on the activation of serine by mutated SerRS variants is much less pronounced. These mutants also misactivate structurally similar threonine, indicating that amino acid substitutions in the active site interfere with the ability of the synthetase to discriminate against noncognate substrates. Less significant misactivation of threonine was also observed by wild type SerRS. However, the formation of erroneous threonyl-adenylate is reduced in the presence of tRNASerCC. Thus, the sequence-specific tRNA:SerRS interactions enhance the accuracy of amino acid recognition. Different quality control mechanism in tRNA serylation may be accomplished by the complex formation between SerRS and a nonsynthetase protein. The interaction between yeast SeRS and peroxin Pex21p has been identified in yeast, by using the two-hybrid screen. This was confirmed by an in vitro binding assay with truncated Pex21p fused to glutathione-S-transferase. Experiments revealing potential relevance of this unusual interaction in enhancing the specificity of substrate recognition are in progress.
Izvorni jezik
Engleski
Znanstvena područja
Biologija
POVEZANOST RADA
Ustanove:
Prirodoslovno-matematički fakultet, Zagreb
Profili:
Ivana Weygand Đurašević
(autor)
