Cryo-EM Visualization of a Viral Internal Ribosome Entry Site Bound to Human Ribosomes

Spahn, C.M.T.; Jan, Eric; Mulder, Anke M.; Grassucci, Robert A.; Sarnow, Peter; Frank, Joachim

doi:10.1016/j.cell.2004.08.001

Cited by 240 publications

(369 citation statements)

References 50 publications

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“…Thus, within the 7.3-Å cryo-EM reconstruction of the CrPV IGR IRES-80S ribosome complex, domain 3 occupies the 40S subunit A site (Fig. 4A), also in agreement with earlier low-resolution cryo-EM observations (43). This observation suggests that initiation begins with domain 3 bound to the small subunit A site, followed by translocation to the P site, followed by the steps discussed above.…”

Section: Discussionsupporting

confidence: 77%

“…stem (Fig. 3A), orienting the distal end of domain 3 toward the E site, where domains 1 and 2 are observed in cryo-EM reconstructions of complexes containing complete IGR IRES RNAs bound to 80S ribosomes (23,43). This orientation, similar to that of a P/E hybrid state tRNA (46), would potentially allow an A site tRNA to enter the A/P hybrid state without steric clash (Fig.…”

Section: Discussionmentioning

confidence: 96%

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Crystal structures of complexes containing domains from two viral internal ribosome entry site (IRES) RNAs bound to the 70S ribosome

Zhu

Коростелев²,

Costantino³

et al. 2011

Proc. Natl. Acad. Sci. U.S.A.

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Internal ribosome entry site (IRES) RNAs are elements of viral or cellular mRNAs that bypass steps of canonical eukaryotic capdependent translation initiation. Understanding of the structural basis of IRES mechanisms is limited, partially due to a lack of highresolution structures of IRES RNAs bound to their cellular targets. Prompted by the universal phylogenetic conservation of the ribosomal P site, we solved the crystal structures of proposed P site binding domains from two intergenic region IRES RNAs bound to bacterial 70S ribosomes. The structures show that these IRES domains nearly perfectly mimic a tRNA•mRNA interaction. However, there are clear differences in the global shape and position of this IRES domain in the intersubunit space compared to those of tRNA, supporting a mechanism for IRES action that invokes hybrid state mimicry to drive a noncanonical mode of translocation. These structures suggest how relatively small structured RNAs can manipulate complex biological machines.ribosome structure | RNA structure | tRNA mimicry

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Section: Discussionsupporting

confidence: 77%

Section: Discussionmentioning

confidence: 96%

Crystal structures of complexes containing domains from two viral internal ribosome entry site (IRES) RNAs bound to the 70S ribosome

Zhu

Коростелев²,

Costantino³

et al. 2011

Proc. Natl. Acad. Sci. U.S.A.

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“…Although uncommon, there are examples of transcripts with specific requirement for large subunit proteins during translation initiation. For example, during initiation on the CrPV IRES, the RNA must associate with rpL1 for subunit joining of the 60S to the 40S and correct ribosome positioning (43,44). Furthermore, by studying mice with a short tail phenotype, rpL38 was found to be required for 80S formation on Homeobox mRNAs and thus correct tissue patterning during development (45).…”

Section: Discussionmentioning

confidence: 99%

A ribosome-specialized translation initiation pathway is required for cap-dependent translation of vesicular stomatitis virus mRNAs

Lee

Burdeinick-Kerr

Whelan

2012

Proc. Natl. Acad. Sci. U.S.A.

143

138

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Initiation is the primary target of translational control for all organisms. Regulation of eukaryotic translation is traditionally thought to occur through initiation factors and RNA structures. Here, we characterize a transcript-specific translation initiation mechanism that is mediated by the ribosome. By studying vesicular stomatitis virus (VSV), we identify the large ribosomal subunit protein rpL40 as requisite for VSV cap-dependent translation but not bulk cellular or internal ribosome entry site-driven translation. This requirement is conserved among members of the order Mononegavirales, including measles virus and rabies virus. Polysome analyses and in vitro reconstitution of initiation demonstrate that rpL40 is required for 80S formation on VSV mRNAs through a cis-regulatory element. Using deep sequencing, we further uncover a subset of cellular transcripts that are selectively sensitive to rpL40 depletion, suggesting VSV may have usurped an endogenous translation pathway. Together, these findings demonstrate that the ribosome acts as a translational regulator outside of its catalytic role during protein synthesis.ribosome code | rhabdovirus | alternative translation | uba52 | paramyxovirus T ranslation initiation in eukaryotes proceeds generally by a cap-dependent scanning mechanism. The rate-limiting step in this process is recognition of the 5′ m 7 GpppN mRNA cap structure by eukaryotic translation initiation factor 4E (eIF4E) (1). The cap-binding complex recruits the small 40S subunit in complex with initiation factors, which then scans along the mRNA until it reaches the initiation codon AUG. Start codon recognition causes the release of the initiation factors, and the large 60S subunit joins, forming an elongation competent 80S complex (2, 3).The study of viral gene expression has uncovered several exceptions to this general mechanism of translation initiation. Poliovirus mRNA contains an ∼750-nt highly structured 5′ UTR that directly recruits the ribosome to an internal RNA site independently of the cap-recognition complex (4). Such internal ribosome entry sites (IRESs) are present in many RNA viruses, and those used by members of the Dicistroviridae family, including Plautia stali intestine virus and cricket paralysis virus, remarkably do not require any initiation factors or the initiating methionine tRNA (5-7). Investigation of the mechanism by which capped but nonpolyadenylated viral mRNAs are translated has also demonstrated that structures or viral proteins can negate the need for poly(A) binding protein during mRNA translation (8, 9). Such studies on translation initiation in viruses have invariably led to subsequent identification of cellular RNAs that are translated by similar mechanisms (10, 11).Replication of negative-strand RNA viruses in the order Mononegavirales induces profound host shutoff, and inhibition of cellular translation effectively suppresses the host immune response and antiviral immunity (12). However, the mechanistic basis of selective viral translation by these viruses...

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“…On the other hand, structural studies performed on the HCV IRES and the IGR of members of the family Dicistroviridae have shown the capacity of these IRES elements to be accommodated in the interface of the ribosomal subunits (Spahn et al, 2001;Boehringer et al, 2005;Schuler et al, 2006;Pfingsten et al, 2006). Although the IGR and the HCV IRES elements exhibit different structural organization (Kieft et al, 2002;Rijnbrand et al, 2004;Jan & Sarnow, 2002;Nishiyama et al, 2003) and their binding sites in the ribosomal subunit are different, similar conformational changes are induced in the 40S ribosomal subunit (Spahn et al, 2004). This finding opens the possibility that IRES elements could share the property of having a universal structural IRES motif (USIM) that could mediate its direct interaction with the 40S subunit.…”

Section: Relevance Of Rna Structure For Ires Functionmentioning

confidence: 99%

“…In marked difference to any other IRES described to date, the IGRs of dicistroviruses assemble initiation complexes in the absence of any eIFs (Table 1) (Spahn et al, 2004;Wilson et al, 2000a). This RNA sequence establishes direct contacts with ribosomal proteins (Schuler et al, 2006).…”

Section: Hepatitis C and Dicistrovirus Ires-driven Protein Synthesismentioning

confidence: 99%

New insights into internal ribosome entry site elements relevant for viral gene expression

Martínez‐Salas

Pacheco

Serrano

et al. 2008

Journal of General Virology

119

105

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A distinctive feature of positive-strand RNA viruses is the presence of high-order structural elements at the untranslated regions (UTR) of the genome that are essential for viral RNA replication. The RNA of all members of the family Picornaviridae initiate translation internally, via an internal ribosome entry site (IRES) element present in the 59 UTR. IRES elements consist of cis-acting RNA structures that usually require specific RNA-binding proteins for translational machinery recruitment. This specialized mechanism of translation initiation is shared with other viral RNAs, e.g. from hepatitis C virus and pestivirus, and represents an alternative to the cap-dependent mechanism. In cells infected with many picornaviruses, proteolysis or changes in phosphorylation of key host factors induces shut off of cellular protein synthesis. This event occurs simultaneously with the synthesis of viral gene products since IRES activity is resistant to the modifications of the host factors. Viral gene expression and RNA replication in positive-strand viruses is further stimulated by viral RNA circularization, involving direct RNA-RNA contacts between the 59 and 39 ends as well as RNA-binding protein bridges. In this review, we discuss novel insights into the mechanisms that control picornavirus gene expression and compare them to those operating in other positive-strand RNA viruses.

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Cryo-EM Visualization of a Viral Internal Ribosome Entry Site Bound to Human Ribosomes

Cited by 240 publications

References 50 publications

Crystal structures of complexes containing domains from two viral internal ribosome entry site (IRES) RNAs bound to the 70S ribosome

Crystal structures of complexes containing domains from two viral internal ribosome entry site (IRES) RNAs bound to the 70S ribosome

A ribosome-specialized translation initiation pathway is required for cap-dependent translation of vesicular stomatitis virus mRNAs

New insights into internal ribosome entry site elements relevant for viral gene expression

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