ERef Bayreuth

Literature by the same author

at Google Scholar

Bibliografische Daten exportieren

Mechanistic insights into recruitment and regulation of the RNA helicase UPF1 in replication-dependent histone mRNA decay

Title data

Machado de Amorim, Alexandrina ; Xue, Guangpu ; He, Wenxia ; Dittmers, Theresa ; Lewandowski, Sarah ; Perez-Borrajero, Cecilia ; Bethmann, Juliane ; Mateva, Nevena ; Krage, Clemens ; Nandana, Vidhyadhar ; Loll, Bernhard ; Hilal, Tarek ; Hennig, Janosch ; Urlaub, Henning ; Marzluff, William F. ; Chakrabarti, Sutapa:
Mechanistic insights into recruitment and regulation of the RNA helicase UPF1 in replication-dependent histone mRNA decay.
In: Nature Communications. Vol. 17 (2026) Issue 1 . - 155.
ISSN 2041-1723
DOI: https://doi.org/10.1038/s41467-025-67991-z

Project information

Project title:	Project's official title Project's id SPP 1935: Deciphering the mRNP code: RNA-bound determinants of post-transcriptional gene regulation 273941853
Project financing:	Deutsche Forschungsgemeinschaft

Abstract in another language

Metazoan histone mRNAs are a unique class of mRNAs that lack the poly(A) tail present in all other eukaryotic transcripts. Instead, they end in a conserved stem-loop (SL) structure, necessitating a decay mechanism that is distinct from deadenylation-initiated degradation. Here, combining structural and functional approaches, we elucidate molecular mechanisms of initiation of histone mRNA decay. At the end of S-phase, the RNA helicase UPF1, the exoribonuclease 3'hExo and stem-loop binding protein SLBP all contribute to histone mRNA degradation, although how they are mechanistically coupled remained unknown. The cryoEM structure of an UPF1:SL RNA complex, presented here, shows that binding of UPF1 partially melts the RNA stem in the absence of ATP, harnessing the free energy derived from RNA-binding to unwind RNA. This melting event primes the SL-RNA for decay by 3'hExo. Using biochemical and cellular analyses, we demonstrate that SLBP directly engages the UPF1 helicase core to attenuate its unwinding activity and prevent premature degradation. Activation of UPF1 at a later stage promotes SL-RNA decay. We provide direct evidence that UPF1, SLBP and 3'hExo form a degradosome-like assembly that functionally couples SL unwinding and degradation, highlighting a dynamic and intricate network of UPF1-centric interactions that orchestrates timely histone mRNA decay.

Further data

Item Type:	Article in a journal
Refereed:	Yes
Institutions of the University:	Faculties Faculties > Faculty of Biology, Chemistry and Earth Sciences Faculties > Faculty of Biology, Chemistry and Earth Sciences > Department of Chemistry Faculties > Faculty of Biology, Chemistry and Earth Sciences > Department of Chemistry > Chair Biochemistry IV - Biophysical Chemistry Faculties > Faculty of Biology, Chemistry and Earth Sciences > Department of Chemistry > Chair Biochemistry IV - Biophysical Chemistry > Chair Biochemistry IV - Biophysical Chemistry - Univ.-Prof. Dr. Janosch Hennig Research Institutions > Central research institutes > Nordbayerisches Zentrum für NMR-Spektroskopie - NMR-Zentrum Research Institutions Research Institutions > Central research institutes
Result of work at the UBT:	Yes
DDC Subjects:	500 Science > 500 Natural sciences 500 Science > 540 Chemistry 500 Science > 570 Life sciences, biology
Date Deposited:	09 Jan 2026 08:59
Last Modified:	09 Jan 2026 08:59
URI:	https://eref.uni-bayreuth.de/id/eprint/95562