The inactive C-terminal cassette of the dual-cassette RNA helicase BRR2 both stimulates and inhibits the activity of the N-terminal helicase unit

Karen Vester; Karine F Santos; Benno Kuropka; Christoph Weise; Markus C Wahl

doi:10.1074/jbc.RA119.010964

The inactive C-terminal cassette of the dual-cassette RNA helicase BRR2 both stimulates and inhibits the activity of the N-terminal helicase unit

J Biol Chem. 2020 Feb 14;295(7):2097-2112. doi: 10.1074/jbc.RA119.010964. Epub 2019 Dec 30.

Authors

Karen Vester¹, Karine F Santos¹, Benno Kuropka², Christoph Weise², Markus C Wahl³

Affiliations

¹ Structural Biochemistry Group, Department of Biochemistry, Freie Universität Berlin, Takustrasse 63, D-14195 Berlin, Germany.
² Protein Biochemistry Group, Department of Biochemistry, Freie Universität Berlin, Thielallee 63, D-14195 Berlin, Germany.
³ Structural Biochemistry Group, Department of Biochemistry, Freie Universität Berlin, Takustrasse 63, D-14195 Berlin, Germany; Macromolecular Crystallography Group, Helmholtz-Zentrum Berlin für Materialien und Energie, Albert-Einstein-Strasse 15, D-12489 Berlin, Germany. Electronic address: markus.wahl@fu-berlin.de.

Abstract

The RNA helicase bad response to refrigeration 2 homolog (BRR2) is required for the activation of the spliceosome before the first catalytic step of RNA splicing. BRR2 represents a distinct subgroup of Ski2-like nucleic acid helicases whose members comprise tandem helicase cassettes. Only the N-terminal cassette of BRR2 is an active ATPase and can unwind substrate RNAs. The C-terminal cassette represents a pseudoenzyme that can stimulate RNA-related activities of the N-terminal cassette. However, the molecular mechanisms by which the C-terminal cassette modulates the activities of the N-terminal unit remain elusive. Here, we show that N- and C-terminal cassettes adopt vastly different relative orientations in a crystal structure of BRR2 in complex with an activating domain of the spliceosomal Prp8 protein at 2.4 Å resolution compared with the crystal structure of BRR2 alone. Likewise, inspection of BRR2 structures within spliceosomal complexes revealed that the cassettes occupy different relative positions and engage in different intercassette contacts during different splicing stages. Engineered disulfide bridges that locked the cassettes in two different relative orientations had opposite effects on the RNA-unwinding activity of the N-terminal cassette, with one configuration enhancing and the other configuration inhibiting RNA unwinding compared with the unconstrained protein. Moreover, we found that differences in relative positioning of the cassettes strongly influence RNA-stimulated ATP hydrolysis by the N-terminal cassette. Our results indicate that the inactive C-terminal cassette of BRR2 can both positively and negatively affect the activity of the N-terminal helicase unit from a distance.

Keywords: ATPase; RNA helicase; RNA splicing; allosteric regulation; dual-cassette Ski2-like helicase; intramolecular regulation; nucleic acid-dependent nucleotide triphosphatase (NTPase); pre-mRNA splicing; protein conformation; small nuclear ribonucleoprotein U5 subunit 200 (SNRNP200); superfamily 2 helicase.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adenosine Triphosphatases / genetics
Catalysis
Crystallography, X-Ray
Humans
Protein Conformation
RNA Splicing / genetics*
RNA-Binding Proteins / chemistry
RNA-Binding Proteins / genetics
RNA-Binding Proteins / ultrastructure*
Ribonucleoproteins, Small Nuclear / chemistry
Ribonucleoproteins, Small Nuclear / genetics
Ribonucleoproteins, Small Nuclear / ultrastructure*
Spliceosomes / genetics*
Spliceosomes / ultrastructure
Substrate Specificity

Substances

PRPF8 protein, human
RNA-Binding Proteins
Ribonucleoproteins, Small Nuclear
SNRNP200 protein, human
Adenosine Triphosphatases

Associated data

PDB/4F91
PDB/4KIT
PDB/6S8Q
PDB/6S8O
PDB/6S9I
PDB/3JCR
PDB/5O9Z
PDB/5Z57
PDB/5YZG
PDB/5XJC
PDB/3JCM
PDB/5GAO
PDB/5NRL
PDB/5GM6
PDB/5LQW
PDB/5LJ5