Conserved stem-loop structures in the HIV-1 RNA region containing the A3 3' splice site and its cis-regulatory element: possible involvement in RNA splicing

Jacquenet, S.; Ropers, Delphine; Bilodeau, Patricia S.; Damier, Laurence; Mougin, Annie; Stoltzfus, C. Martin; Branlant, Christiane

doi:10.1093/nar/29.2.464

Cited by 71 publications

(84 citation statements)

References 40 publications

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“…Inefficient splicing of the HIV-1 genome is required to preserve a pool of unspliced and singly spliced transcripts, to be transported across the nuclear membrane via the Rev/RRE dependent pathway+ Besides having suboptimal splice sites, exonic and intronic sequences in the tat pre-mRNA function as binding sites for cellular factors of the hnRNP A/B and hnRNP H classes, which leads to further inhibition of splicing (Amendt et al+, 1994(Amendt et al+, , 1995Staffa & Cochrane, 1994, 1995Si et al+, 1997Si et al+, , 1998Caputi et al+, 1999 Our computer predictions and probing results are consistent with the existence of three major stem loop structures, SL1, SL2, and SL3, of which SL1 and SL3 are conserved in M-type HIV-1+ The ISS and the ESS3 are positioned within SL1 and SL3, respectively, whereas the SL2 harbors a GAA repeat at positions 8420-8430, which is part of the degenerate SF2/ASF-dependent enhancer element ESE3 (Mayeda et al+, 1999;Tange & Kjems, 2001)+ This GAA repeat is highly accessible to chemical modifications by DMS/DEP and single-strand specific RNase cleavage (Fig+ 2A, B), consistent with these sequences acting as binding sites for cellular splicing proteins including hnRNP A1 and presumably also SF2/ASF+ In contrast, we found that S3, which is the functionally most hnRNP A1 responsive site of the ISS, was less accessible to enzymatic probing reagents and situated in a helix structure adjacent to an internal bulge+ Intriguingly, this structure is very similar to the recently reported secondary structural context of the ESS2 (Jacquenet et al+, 2001b)+ The functional significance of this structure is supported by the observation that this base-pairing scheme can form in all investigated M-group viruses (Fig+ 3)+ Another similarity between the ISS and the ESS2 is the appearance of a base-paired UAG element immediately upstream, which corresponds to the S2 sequence of the ISS (Jacquenet et al+, 2001b; this report)+ Modulation of hnRNP A1 binding by RNA structure hnRNP A1 has originally been reported to have a general nonspecific RNA-binding activity, although several reports have specified RNA sequences that are bound by hnRNP A1 with 10-1,000-fold increased affinity (Swanson & Dreyfuss, 1988;Buvoli et al+, 1990;Matunis et al+, 1993;Burd & Dreyfuss, 1994;Mayeda et al+, 1994Mayeda et al+, , 1998Chabot et al+, 1997;Blanchette & Chabot, 1999;Caputi et al+, 1999;Del Gatto-Konczak et al+, 1999;…”

Section: Discussionsupporting

confidence: 86%

hnRNP A1 controls HIV-1 mRNA splicing through cooperative binding to intron and exon splicing silencers in the context of a conserved secondary structure

Damgaard

Tange

Kjems

2002

RNA

108

126

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The removal of the second intron in the HIV-1 rev/tat pre-mRNAs, which involves the joining of splice site SD4 to SA7, is inhibited by hnRNP A1 by a mechanism that requires the intronic splicing silencer (ISS) and the exon splicing silencer (ESS3). In this study, we have determined the RNA secondary structure and the hnRNP A1 binding sites within the 39 splice site region by phylogenetic comparison and chemical/enzymatic probing. A biochemical characterization of the RNA/protein complexes demonstrates that hnRNP A1 binds specifically to primarily three sites, the ISS, a novel UAG motif in the exon splicing enhancer (ESE) and the ESS3 element, which are all situated in experimentally supported stem loop structures. A mutational analysis of the ISS region revealed that the core hnRNP A1 binding site directly overlaps with a major branchpoint used in splicing to SA7, thereby providing a direct explanation for the inhibition of U2 snRNP association with the pre-mRNA by hnRNP A1. Binding of hnRNP A1 to the ISS core site is inhibited by RNA structure but strongly stimulated by the exonic silencer, ESS3. Moreover, the ISS also stimulate binding of hnRNP A1 to the exonic splicing regulators ESS3 and the ESE. Our results suggest a model where a network is formed between hnRNP A1 molecules situated at discrete sites in the intron and exon and that these interactions preclude the recognition of essential splicing signals including the branch point.

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Section: Discussionsupporting

confidence: 86%

hnRNP A1 controls HIV-1 mRNA splicing through cooperative binding to intron and exon splicing silencers in the context of a conserved secondary structure

Damgaard

Tange

Kjems

2002

RNA

108

126

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“…Plasmids Used in This Study-pLD-C2, pLD-C3, and pLD-L3-U1 constructs, used for production of the C2, C3, and L3-U1 transcripts, were described previously (11,23,24). To build the plasmid pLD-C1, two DNA fragments were generated by PCR amplifications of plasmid pBRU3 (42) containing the HIV-1 BRU/LAI complete cDNA (GenBank TM accession number K02013).…”

Section: Methodsmentioning

confidence: 99%

“…PCR products were quantified using ImageQuant (Amersham Biosciences). The fractionated cDNAs were identified by reference to previous data on HeLa cells transfected with plasmid ⌬PSP (11,24).…”

Section: Methodsmentioning

confidence: 99%

“…(ii) Their branch point sequences are not canonical, and in some cases, a residue other than an adenosine is used as the branch site (22,23). (iii) Their accessibility is limited by their sequestering in stable secondary structures (24). (iv) Several cis-inhibitory elements have been identified that down-regulate the A2, A3, and A7 sites by binding of hnRNP A1 or hnRNP H proteins (11,12,14,16,18,19,21).…”

mentioning

confidence: 99%

“…The present knowledge in this field can be summarized as follows: (i) deep studies, which were performed both in vitro and in vivo, demonstrated the action of proteins ASF/SF2 and SC35 at acceptor site A7 (17,19,20,39,40); (ii) an in vitro study performed with S100 extract showed that, among the SR proteins SC35, SRp40, SRp55, and SRp70, only protein SC35 is able to activate site A3 in S100 extract (41). For a complete study of the effects of individual SR proteins on the entire set of HIV-1 splicing sites in cellular conditions, we cotransfected HeLa cells with a construct that produces a truncated HIV-1 RNA containing all the splicing sites (13,24), and a plasmid that overexpresses one of the SC35, SRp40, ASF/SF2, and 9G8 SR proteins. In these ex vivo experiments, very different HIV-1 RNA splicing patterns were obtained with different overexpressed SR protein.…”

mentioning

confidence: 99%

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Differential Effects of the SR Proteins 9G8, SC35, ASF/SF2, and SRp40 on the Utilization of the A1 to A5 Splicing Sites of HIV-1 RNA

Ropers¹,

Ayadi²,

Gattoni

et al. 2004

Journal of Biological Chemistry

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Splicing is a crucial step for human immunodeficiency virus, type 1 (HIV-1) multiplication; eight acceptor sites are used in competition to produce the vif, vpu, vpr, nef, env, tat, and rev mRNAs. The effects of SR proteins have only been investigated on a limited number of HIV-1 splicing sites by using small HIV-1 RNA pieces. To understand how SR proteins influence the use of HIV-1 splicing sites, we tested the effects of overproduction of individual SR proteins in HeLa cells on the splicing pattern of an HIV-1 RNA that contained all the splicing sites. The steady state levels of the HIV-1 mRNAs produced were quantified by reverse transcriptase-PCR. For interpretation of the data, transcripts containing one or several of the HIV-1 acceptor sites were spliced in vitro in the presence or the absence of one of the tested SR proteins. Both in vivo and in vitro, acceptor sites A2 and A3 were found to be strongly and specifically regulated by SR proteins. ASF/SF2 strongly activates site A2 and to a lesser extent site A1. As a result, upon ASF/SF2 overexpression, the vpr mRNA steady state level is specifically increased. SC35 and SRp40, but not 9G8, strongly activate site A3, and their overexpression ex vivo induces a dramatic accumulation of the tat mRNA, to the detriment of most of the other viral mRNAs. Here we showed by Western blot analysis that the Nef protein synthesis is strongly decreased by overexpression of SC35, SRp40, and ASF/SF2. Finally, activation by ASF/ SF2 and 9G8 was found to be independent of the RS domain. This is the first investigation of the effects of variations of individual SR protein concentrations that is performed ex vivo on an RNA containing a complex set of splicing sites.Splicing plays a key role for production of the HIV-1 1 retroviral proteins. By using the integrated proviral genome as the template, RNA polymerase II of the infected cell produces long primary transcripts that are all identical. Some of these transcripts are transported to the cytoplasm in an intact form to serve as genomes for new virions or as messenger RNAs for the production of the Gag-Pol protein precursor. The other transcripts undergo alternative splicing to produce mRNAs for the auxiliary and regulatory proteins and the Env precursor protein. Production of mRNAs encoding HIV-1 proteins depends on the alternative utilization of four 5Ј-splice sites D1 to D4 (1) and eight 3Ј-splice sites (A1, A2, A3, A4a, -b, -c, A5, and A7) (1). An additional 3Ј-splice site (A6) was only found in one HIV-1 strain (2). Donor sites D1, D2, and D3 can be coupled to any of the A1 to A5 acceptor sites, whereas donor site D4 is exclusively coupled to site A7 and to site A6 when this site is present (1, 2). The combination of these various sites gives rise to at least 35 different mRNAs (1). Although the relative efficiencies of the HIV-1 donor sites seem to depend mainly upon their complementarity to the U1 snRNA 5Ј-terminal sequence (3, 4), efficiencies of HIV-1 acceptor sites depend upon the presence of cis-regulatory elements (5...

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Study of RNA–Protein Interactions and RNA Structure in Ribonucleoprotein Particles

Marchand¹,

Mougin²,

Mreau³

et al. 2005

Handbook of RNA Biochemistry

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Conserved stem-loop structures in the HIV-1 RNA region containing the A3 3' splice site and its cis-regulatory element: possible involvement in RNA splicing

Cited by 71 publications

References 40 publications

hnRNP A1 controls HIV-1 mRNA splicing through cooperative binding to intron and exon splicing silencers in the context of a conserved secondary structure

hnRNP A1 controls HIV-1 mRNA splicing through cooperative binding to intron and exon splicing silencers in the context of a conserved secondary structure

Differential Effects of the SR Proteins 9G8, SC35, ASF/SF2, and SRp40 on the Utilization of the A1 to A5 Splicing Sites of HIV-1 RNA

Study of RNA–Protein Interactions and RNA Structure in Ribonucleoprotein Particles

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