Structural evidence for consecutive Hel308-like modules in the spliceosomal ATPase Brr2

Zhang, Lingdi; Xu, Tao; Maeder, Corina; Bud, Laura-Oana; Shanks, James; Nix, Jay C.; Guthrie, Christine; Pleiss, Jeffrey A.; Zhao, Rui

doi:10.1038/nsmb.1625

Cited by 87 publications

(162 citation statements)

References 62 publications

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“…The S1087L RP33 exchange in human Brr2 reduces RNA affinity as well as ATPase and helicase activities 51 and RP33-like N1104L and R1107L exchanges in yeast Brr2 are associated with reduced ATPdependent U4/U6 unwinding in tri-snRNP preparations. 60 Mutation of a Brr2 element equivalent to the Hel308 separator loop resulted in reduction or loss of cell viability, 41,52 in line with a similar duplex disruption mechanism as in Hel308. However, in a yeast U4/U6 U5 tri-snRNP structure, 12 Brr2 is loaded on the U4/U6 di-snRNA with the putative separator loop distant from the U4/U6 duplex portion to be unwound and instead with an edge of the RecA2 domain abutting the end of this duplex region (Fig.…”

Section: Multiple Layers Of Helicase-associated Domains In Brr2mentioning

confidence: 89%

“…In contrast, in DEAH/RHA helicases an element equivalent to the separator loop (termed "5 0 HP") has been suggested to mainly control access to the single-stranded RNA binding site. 58,59 Comparative modeling 41,51,52 and a recent electron cryomicroscopic (cryo-EM) structure of a yeast U4/U6 U5 trisnRNP 12 showed that Brr2 engages its U4/U6 di-snRNA substrate in a similar manner as Hel308. A single-stranded region of the U4 snRNA is threaded through the central tunnel of the NC between the RNA-binding motifs of the RecA and HB domains, with 3 0 -portions of the RNA extending toward the CC (Fig.…”

Section: Multiple Layers Of Helicase-associated Domains In Brr2mentioning

confidence: 99%

“…This idea is in line with previous proposals of Brr2 functioning as a landing pad for multiple other helicases, which might sequentially interact in similar fashion with the C-terminal cassette. 40,41,52,63,64 Based on the observations that a temperature-sensitive yeast Brr2 variant (E909K), encoded by the slt22-1 allele, is synthetically lethal with mutations in U2 or U6 snRNAs that affect the stability or conformation of U2/U6 helix II, and that the ATPase activity of this variant is no longer stimulated by a U2/ U6 duplex, it was proposed that Brr2 might proofread U2/U6 interactions. 45 Furthermore, different cross-linking profiles of wt Brr2 and a variant exhibiting a residue exchange (G858R) in the NC 5 0 HP/separator loop with U6 snRNA 46 together with the latter variant exhibiting a second step defect and showing synthetic lethality with step 2 mutations in Slu7, Prp18 and Prp16 46,49 suggest that Brr2 participates in a transient opening of the catalytic core between the 2 steps of splicing, which is characterized by the intermittent disruption of U6-5SS and U2-U6 interactions.…”

Section: Brr2 Regulation During Splicingmentioning

confidence: 99%

“…2A,B). 41,52 Only the N-terminal helicase cassette (NC) is active in nucleotide hydrolysis and RNA unwinding, 51 and the enzymatic activity of the NC alone is required for splicing in vivo. 27 The C-terminal cassette (CC) is still able to bind ATP, 51 but it contains noncanonical residues in the ATP binding and hydrolysis motifs, which abrogate the ATPase activity.…”

Section: Brr2 Exhibits a Unique Structurementioning

confidence: 99%

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Functions and regulation of the Brr2 RNA helicase during splicing

2016

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Pre-mRNA splicing entails the stepwise assembly of an inactive spliceosome, its catalytic activation, splicing catalysis and spliceosome disassembly. Transitions in this reaction cycle are accompanied by compositional and conformational rearrangements of the underlying RNA-protein interaction networks, which are driven and controlled by 8 conserved superfamily 2 RNA helicases. The Ski2-like helicase, Brr2, provides the key remodeling activity during spliceosome activation and is additionally implicated in the catalytic and disassembly phases of splicing, indicating that Brr2 needs to be tightly regulated during splicing. Recent structural and functional analyses have begun to unravel how Brr2 regulation is established via multiple layers of intra-and inter-molecular mechanisms. Brr2 has an unusual structure, including a long N-terminal region and a catalytically inactive C-terminal helicase cassette, which can auto-inhibit and auto-activate the enzyme, respectively. Both elements are essential, also serve as protein-protein interaction devices and the N-terminal region is required for stable Brr2 association with the tri-snRNP, tri-snRNP stability and retention of U5 and U6 snRNAs during spliceosome activation in vivo. Furthermore, a C-terminal region of the Prp8 protein, comprising consecutive RNase H-like and Jab1/MPN-like domains, can both up-and downregulate Brr2 activity. Biochemical studies revealed an intricate cross-talk among the various cis-and transregulatory mechanisms. Comparison of isolated Brr2 to electron cryo-microscopic structures of yeast and human U4/U6 U5 tri-snRNPs and spliceosomes indicates how some of the regulatory elements exert their functions during splicing. The various modulatory mechanisms acting on Brr2 might be exploited to enhance splicing fidelity and to regulate alternative splicing. KEYWORDSPre-mRNA splicing; regulation of pre-mRNA splicing; remodeling of RNAprotein complexes; RNA helicase structure, function and regulation; spliceosome catalytic activation

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Section: Multiple Layers Of Helicase-associated Domains In Brr2mentioning

confidence: 89%

Section: Multiple Layers Of Helicase-associated Domains In Brr2mentioning

confidence: 99%

Section: Brr2 Regulation During Splicingmentioning

confidence: 99%

Section: Brr2 Exhibits a Unique Structurementioning

confidence: 99%

See 2 more Smart Citations

Functions and regulation of the Brr2 RNA helicase during splicing

2016

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“…Further, the Prp8-CTR facilitates the binding of the Brr2/Prp8-CTR complex to U4/U6 in yeast. 41 In this current study, we have identified a potentially pathogenic mutation, p.R1779H, which is located between the second helicase CTR and sec-63 domains. It is the first candidate mutation found in the hel308-II module for RP.…”

Section: Discussionmentioning

confidence: 99%

Contribution of SNRNP200 sequence variations to retinitis pigmentosa

Zhang

Lai

Chiang

et al. 2013

Eye

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Purpose Mutations in the SNRNP200 gene have been reported to cause autosomal dominant retinitis pigmentosa (adRP). In this study, we evaluate the mutation profile of SNRNP200 in a cohort of southern Chinese RP patients. Methods Twenty adRP patients from 11 families and 165 index patients with non-syndromic RP with mixed inheritance patterns were screened for mutations in the mutation hotspots of SNRNP200. These included exons 12-16, 22-32, and 38-45, which covered the two helicase ATP-binding domains in DEAD-box and two sec-63 domains. The targeted regions were amplified by polymerase chain reaction and analyzed by direct DNA sequencing, followed by in silico analyses. Results Totally 26 variants were identified, 18 of which were novel.

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Next generation sequencing of pooled samples reveals new SNRNP200 mutations associated with retinitis pigmentosa

et al. 2011

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ABSTRACT:The gene SNRNP200 is composed of 45 exons and encodes a protein essential for premRNA splicing, the 200 kDa helicase hBrr2. Two mutations in SNRNP200 have recently been associated with autosomal dominant retinitis pigmentosa (adRP), a retinal degenerative disease, in two families from China. In this work we analyzed the entire 35-Kb SNRNP200 genomic region in a cohort of 96 unrelated North American patients with adRP. To complete this large-scale sequencing project, we performed ultra high-throughput sequencing of pooled, untagged PCR products. We then validated the detected DNA changes by Sanger sequencing of individual samples from this cohort and from an additional one of 95 patients. One of the two previously known mutations (p.S1087L) was identified in 3 patients, while 4 new missense changes (p.R681C, p.R681H, p.V683L, p.Y689C) affecting highly conserved codons were identified in 6 unrelated individuals, indicating that the prevalence of SNRNP200-associated adRP is relatively high. We also took advantage of this research to evaluate the pool-and-sequence method, especially with respect to the generation of false positive and negative results. We conclude that, although this strategy can be adopted for rapid discovery of new disease-associated variants, it still requires extensive validation to be used in routine DNA screenings.

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Structural evidence for consecutive Hel308-like modules in the spliceosomal ATPase Brr2

Cited by 87 publications

References 62 publications

Functions and regulation of the Brr2 RNA helicase during splicing

Functions and regulation of the Brr2 RNA helicase during splicing

Contribution of SNRNP200 sequence variations to retinitis pigmentosa

Next generation sequencing of pooled samples reveals new SNRNP200 mutations associated with retinitis pigmentosa

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