Sir William Dunn School of Pathology, University of Oxford, South Parks Road, Oxford OX1 3RE, UK
Correspondence
George G. Brownlee
George.Brownlee{at}path.ox.ac.uk
![]() |
ABSTRACT |
---|
![]() ![]() ![]() |
---|
Published online ahead of print on 10 February 2005 as DOI 10.1099/vir.0.80755-0.
Introduction
It is well known that cap structures at the 5' end of mRNA (Fig. 1) are required for efficient translation of mRNA on the ribosome and to protect mRNA from degradation by cellular 5' exonucleases. Cap-binding proteins have evolved to bind to this cap structure. In turn, these cap-binding proteins are associated with other binding proteins that regulate binding of the mRNA and the cap-binding proteins themselves. Details of how cap structures are recognized at the molecular level are now available from extensive structural and functional data on different cap-binding proteins derived from unrelated cellular or viral origins.
|
Some viruses, e.g. retroviruses, utilize the host cellular capping mechanism (Coffin, 1990). Most viruses, however, have evolved their own, virus-specific, capping mechanism. They can be divided into two main groups. The first group includes viruses such as poxviruses, coronaviruses, flaviviruses and reoviruses that replicate in the cytoplasm of cells. A well-studied example of such viruses is vaccinia virus, a double-stranded DNA poxvirus (Moss, 2001
). Thus VP39 the vaccinia viral protein 39 recognizes its own capped mRNAs. After binding to the cap structure, the enzyme acts as a 2'-O-methyltransferase transferring a methyl group to the 2' carbon atom of the ribose moiety of the first residue of the cap structure (see Fig. 2
and Condit & Niles, 2002
; Moss, 2001
; Smith et al., 2002
). Baculoviruses, like flaviviruses, also appear to have evolved cap-dependent 2'-O-methyltransferases, (Wu & Guarino, 2003
) but the mechanism of cap binding by the flavivirus 2'-O-methyltransferase domain may differ from that of VP39 (Egloff et al., 2002
). The second group includes negative-strand RNA viruses replicating either in the nucleus, like orthomyxoviruses (e.g. influenza virus) or in the cytoplasm, like bunyaviruses. These viruses have not evolved capping enzymes as such. Instead they have evolved a mechanism to snatch the cap structure from host cell mRNAs (Fodor & Brownlee, 2002
; Lamb & Krug, 2001
). The viral polymerase binds to cellular capped mRNA in infected cells. An endonuclease activity associated with the polymerase then cleaves the capped oligonucleotides, which subsequently act as primers to initiate viral transcription. Fig. 3
illustrates this mechanism for the influenza virus life cycle (Fodor & Brownlee, 2002
; Lamb & Krug, 2001
; Portela et al., 1999
).
|
|
Structural studies on VP39, eIF4E and CBC suggest a common aromatic sandwich motif binds cap structures
How do cap-binding proteins discriminate between capped RNAs and non-capped ones? This is of paramount importance to the functions of the specific cap-binding proteins. In 1997, the NMR or crystal structures of complexes between short-cap analogues and two evolutionary unrelated cap-binding proteins were solved. These were the complexes between eIF4E and m7GDP (Marcotrigiano et al., 1997; Matsuo et al., 1997
), and between VP39 and m7GDP (Hodel et al., 1997
). Because a similar aromatic cap-binding pocket was present in both proteins, this suggested that convergent evolution of the cap-binding pocket had occurred (reviewed by Quiocho et al., 2000
). The structural description of cap binding was later improved by crystallization of both proteins with longer cap analogues (m7GpppA in the case of eIF4E, a capped hexamer in the case of VP39) (Hodel et al., 1998
; Tomoo et al., 2003
). More recently, the crystal structure of the complex between the cap analogue m7GpppG and CBC has revealed a similar aromatic cap-binding pocket, adding support to the convergent evolution hypothesis (Calero et al., 2002
; Mazza et al., 2002
). Specific binding of purine residues is common to another major class of enzymes the nucleotidyltransferases (e.g. DNA and RNA ligases, RNA capping enzymes). Interestingly, they also recognize the purine residues of ATP or GTP by the formation of a hydrophobic sandwich between a conserved aromatic and a conserved aliphatic residue (Shuman & Lima, 2004
).
Here, we will summarize the main features of the interactions described between these different cap-binding proteins and the cap structure. The reader is referred to the detailed structural papers above for a fuller and more complete description of the interactions involved since not all interactions of eIF4E, CBC and VP39 with the cap are mentioned below.
Although the overall structure of the three cap-binding proteins eIF4E, CBC and VP39 differ widely due to their evolutionary unrelated origin, the cap-binding pockets are essentially very similar, although there are some differences in the detail (Fig. 4). In addition to the two aromatic amino acids, the pocket comprises an acidic area to accommodate the positively charged
-ring system of the m7G, and a basic area to accommodate the triphosphate moiety of the cap structure. Overall five main features may be identified that contribute to the specific recognition of the m7GpppN of the cap in the three proteins.
|
Second the delocalized positive charge of the m7G purine ring, due to the methylation of N7, it is generally believed, allows both salt bridges and hydrogen bonds to form between N1 and/or N2 of m7G and the carboxylate groups of Glu or Asp residues in an acidic cavity. This cavity contains at least one critical acidic amino acid E103 in eIF4E, D116 in CBC and E233 in VP39 (Fig. 4). Mutations of these critical acidic residues to Ala decrease affinity as well as specificity (Hodel et al., 1997
; Mazza et al., 2002
; Morino et al., 1996
). There are conflicting results in the literature of the VP39 phenotype resulting from the mutation of E233 to Gln, which lead to different interpretations of the importance of salt bridges in stabilizing cap binding (Hsu et al., 2000
; Hu et al., 1999
; Quiocho et al., 2000
). Additional contacts are made between O6, N1 and N2 of m7G (see Figs 1 and 4
) and other amino acids. Thus, W102 is involved in these additional contacts in the case of eIF4E, although this residue is also involved in the aromatic stacking with m7G see above. D114, R112 and W115 are involved in these additional contacts in the case of CBC. D182 and water molecules (not shown) make contacts with m7G in the case of VP39.
Third the triphosphate moiety is bound in a cavity by residues forming salt bridges with the oxygen atoms of the phosphate groups (Fig. 4). R157, K162 and water molecules (not shown) form a binding cavity in the case of eIF4E. In CBC, R135, R127, Y20, Q133 and V134 are involved, while in VP39, R177, E207 and S205 form the cavity.
Fourth the N7-methyl group of the guanine is stabilized by van der Waals or weak polar interactions with W166 in the case of eIF4E and Y204 in the case of VP39. In CBC, however, no interaction with the N7-methyl group has yet been reported in the crystal structure.
Finally, interactions with base 1 of the cap structure (see Fig. 1) also contribute to binding, although non-specifically, to accommodate any base at that position. Base 1 is stacked with Y138 in CBC (not shown in Fig. 4
), or is stabilized by hydrogen bonds and electrostatic interactions with residues T205, S207 and K206 in eIF4E (not shown in Fig. 4
). No structural data, however, have been described detailing the interaction of cap-binding proteins with the 2'-O-methyl groups present of bases 1 and 2 in cap 1 and cap 2 structures (see Fig. 1
).
Functional studies on the mechanism of cap recognition
Further biophysical and functional studies have proved controversial. Initially binding of m7GTP to eIF4E was studied by stopped flow dynamics and fluorometric titration (Blachut-Okrasinska et al., 2000; Niedzwiecka et al., 2002
). A two-step binding mechanism was proposed, the binding of the triphosphate moiety being the primary anchor of the cap structure, enabling the subsequent specific interactions with m7G. In contrast, Hu et al. (2003)
proposed a simple one-step binding mechanism for VP39, suggesting that the binding to the triphosphate was not contributing to the fast rate of association. Binding depended, it was suggested, almost entirely on interactions of m7G with the two aromatic residues in a cation-
sandwich. From the results of the pH-dependence of the association rate constant, Hu et al. (2003)
further proposed that the keto tautomer of the cap structure (the keto form is represented in Fig. 1
) rather than the enol form is bound.
Interestingly, Hsu and co-workers (Hsu et al., 2000) conducted mutational studies on both VP39 and eIF4E, showing that different combinations of aromatic residues in the aromatic sandwich could support high affinity for cap structures, providing that at least one Tyr or one Trp was present. These results agreed with those obtained later by Mazza and co-workers (Mazza et al., 2001
, 2002
) on CBC. Thus, there is a specific interaction between the cap and the aromatic side chains of either Tyr or Trp which would not be possible, or somewhat weaker with Phe. It was suggested that the second stacking residue may only provide a flat complementary surface for lower affinity van der Waals interactions with the cap and may thus accommodate any aromatic amino acid. Further studies on different cap-binding proteins are needed to confirm this hypothesis (Hsu et al., 2000
). Interestingly, single or double Trp substitutions of the Tyr or Phe residues of the aromatic sandwich in VP39 increased affinity for cap structures, but not for bona fides substrates containing RNA downstream of the cap (Hu et al., 2002
). Another protein, 4EHP, with homology to eIF4E, has been described. It has an aromatic sandwich formed from Trp and Tyr but its function is unknown (Rom et al., 1998
).
The specificity of the different cap-binding proteins for caps and cap analogues
The specificity of the different cap-binding proteins for cap structures has been addressed by studies of their affinity for a broad set of capped or uncapped substrates, using a variety of approaches. A preliminary comparison of the data obtained by different authors (see below) seems to suggest some differences in the binding mechanisms by the different cap-binding proteins. All three proteins studied (eIF4E, CBC and VP39) had different affinities for m7GTP. CBC had the strongest affinity, in the range of 10 nM (Wilson et al., 1999), while eIF4E had an affinity of about 260280 nM (Niedzwiecka et al., 2002
; Scheper et al., 2002
). VP39 had a lower affinity in the micromolar range (Hu et al., 1999
). Interestingly the different affinities correlate with the number of hydrogen bonds made by the three proteins with m7GTP, CBC making more hydrogen bonds than eIF4E, and eIF4E more than VP39. Adding 1 nt residue to the cap analogue used in these studies affected the three proteins in different ways. Thus, the affinity of eIF4E for m7GTP or m7GpppG was not significantly increased (Carberry et al., 1989
, 1991
). Similarly, no significant difference in affinity was detected between VP39 and m7GDP or m7GpppG (Hu et al., 1999
). CBC, on the other hand, had a 100-times higher affinity for m7GpppG than for m7GTP (Izaurralde et al., 1992
). In the crystal structure it was observed that the second G of the m7GpppG is stacked on Y138 of CBP20. It has recently been confirmed by fluorescence studies that this stacking interaction with the first base of the transcribed RNA enhances the affinity for pyrimidines but not for purines. However, this stacking does not fully account for the extra affinity of m7GpppG compared with m7GTP (S. Cusack, E. Darzynkiewicz and R. Stolarski, personal communication). The relative affinity of longer oligonucleotides (>20 mer) has also been studied. While VP39 had an almost 100-fold increased affinity (Lockless et al., 1998
), the affinity of both eIF4E and CBC increased but to a lesser extent (<6-fold) (Goss et al., 1990
; Mazza et al., 2002
; Wilson & Cerione, 2000
). The significance of the 2'-O-methylation of base 1 and base 2 in cap binding has, however, not been addressed, in either structural or functional studies.
The relative contribution of the different chemical groups of the m7GTP analogue was tested by binding studies of different derivatives. The important contribution of the triphosphate moiety for binding to eIF4E, but not to VP39, has been shown by comparing the binding of m7GTP, m7GDP, m7GMP or m7G (Cai et al., 1999; Hooker et al., 2003
; Hu et al., 1999
; Niedzwiecka et al., 2002
). The study of other methylated analogues in which guanine was substituted with adenine, cytidine (Hu et al., 1999
) or other analogues (Cai et al., 1999
; Hooker et al., 2003
) showed that different bases, e.g. adenine derivatives, but not acyclic nucleosides, could replace guanine. Both eIF4E and CBC were able to bind guanine substituted by ethyl or benzyl groups at N7 (Cai et al., 1999
; Carberry et al., 1990
; Darzynkiewicz & Lonnberg, 1989
; Izaurralde et al., 1992
; Niedzwiecka et al., 2002
). The crystal structures of eIF4E and CBC are consistent with these results, as there is sufficient space to accommodate these longer side chains at N7 (Calero et al., 2002
; Marcotrigiano et al., 1997
; Matsuo et al., 1997
; Mazza et al., 2002
). The binding cavity for N7-methyl, however, is smaller in the case of VP39, suggesting that VP39 would not bind longer side chains at N7, but this remains to be tested (Hodel et al., 1997
). Taken together, these different cap analogues have helped establish further details of the specificity of cap-binding proteins for the m7G moiety of the cap structure. Nevertheless, further quantitative data with different analogues of m7GTP are still needed to accurately compare the properties of the different cap-binding proteins.
Cap binding by the PB2 subunit of influenza RNA polymerase, a fourth example of an aromatic sandwich?
Another viral cap-binding protein the influenza RNA-dependant RNA polymerase has been the subject of extensive studies. This polymerase is a heterotrimer, approximately 250 kDa, composed of three subunits, PB1, PB2 and PA. Influenza RNA-dependant RNA polymerase is unable to cap its own mRNAs. Instead it has evolved a specific cap-snatching mechanism that allows it to bypass this step (Fig. 3). Cap snatching can be divided into three steps. First, the polymerase binds the virion RNA promoter, formed by circularization of the 5' and 3' ends of each of the eight influenza RNA segments, thought to exist in a local secondary structure called a corkscrew (Flick et al., 1996
; Leahy et al., 2001
). The polymerase is likely to undergo a conformational change on binding of the virion RNA promoter (Cianci et al., 1995
; Li et al., 1998
). Second, the cap structure of host mRNAs is specifically recognized by the PB2 subunit, but only in the context of the trimeric holoenzyme (Blaas et al., 1982
; Bouloy et al., 1979
; Ulmanen et al., 1981
). Third, the bound host mRNA is cleaved 917 nt from the cap structure by an endonuclease activity of the polymerase complex (Plotch et al., 1981
), an activity requiring all three subunits of the RNA polymerase (Fodor et al., 2002
; Li et al., 2001
; Shi et al., 1995
, 1996
).
The specificity of cap binding by the PB2 subunit of the influenza RNA polymerase has been studied extensively. The RNA polymerase is essentially inactive in transcription, but not in replication (Vreede et al., 2004), in the absence of a cap structure (Bouloy et al., 1979
). Omission of the N7-methyl group of the guanine induces a 520-fold loss in binding, depending on the substrate (Bouloy et al., 1980
; Hooker et al., 2003
). This decrease in binding affinity is less, however, than observed for eIF4E, CBC or VP39, which are typically >100-fold (see above). Thus, the contribution of aromatic stacking interactions to cap binding in the case of PB2 is probably less than in eIF4E, CBC or VP39. Influenza RNA polymerase is the only cap-binding complex for which the contribution of 2'-O-methyl group in cap binding has been shown to be critical, since deletion of this group led to >10-fold decrease in cap binding (Bouloy et al., 1980
; Brownlee et al., 1995
). The length of the capped RNAs is also crucial for cap binding. m7GpppG is a poor binder (Ulmanen et al., 1981
), and 4 nt seem to be the minimal length for efficient binding (Chung et al., 1994
). Binding efficiency is increased further if 1215 nt-long capped oligonucleotides were used (Chung et al., 1994
; Fechter et al., 2003
). Hooker et al. (2003)
compared the affinity of influenza polymerase and eIF4E for different cap analogues. Based on a comparison of the binding of acycloguanosine and guanosine to PB2 and to eIF4E, they argued that ribose was perhaps less significant for the specificity of binding for PB2 than for eIF4E. This work allowed the design of the first influenza inhibitor (Fig. 5
) that has been described in the literature that is specific for cap binding (Hooker et al., 2003
).
|
Several studies have attempted to define the region of PB2 involved in cap binding. (i) Honda et al. (1999) studied the 32P-labelled, V8 protease peptides of PB2 derived by UV cross-linking of the influenza ribonucleoprotein complex to a m7G32ppp-labelled capped oligonucleotide. They concluded that residues 242282 and a second region 538577, were involved. (ii) Li et al. (2001)
extended this approach by UV cross-linking a 4 thioU-containing, 32P-labelled, capped oligonucleotide. A peptide, SVLVNTYQWIIRNW (residues 544557) was identified after V8 protease digestion. Mutation of W552 to Ala reduced cap binding to 25 % of wild-type levels. Given the proximity of the 4 thioU residue (at residue 2 of the oligonucleotide) to the labelled cap structure, it was proposed that the isolated peptide must be close to the aromatic sandwich. The authors concluded that one or other of the nearby aromatic residues, i.e. W537, Y550, W557 or W564, form the aromatic sandwich with the cap structure, similar to eIF4E or VP39. However, they excluded position W552 as being directly involved in the aromatic sandwich, because the observed 25 % activity of the A552 mutant in cap binding is inconsistent with direct binding. No direct evidence for the involvement of W537, Y550, W557 or W564 was possible because Ala mutants at these positions in PB2 failed to assemble into a functional complex. (iii) Fechter et al. (2003)
adopted a systematic mutation approach of all evolutionary conserved aromatic residues of PB2 identified in an alignment between influenza A, B, C and Thogotovirus. Twenty-seven aromatic residues were mutated either to an Ala or to a conservative amino acid (W, Y or F) on the assumption that aromatics directly involved in cap binding would retain cap-binding activity if a conservative mutation were introduced, but would loose binding if an Ala mutation was present. F363 and F404, it was proposed, were directly involved in cap binding in an aromatic sandwich.
The contradictory results (above) suggest there are design flaws in the different approaches. Although it may be argued that cross-linking is a more direct approach than the mutagenesis approach, the length of the oligonucleotide probe used (14 nt), the distance of the 4 thioU residue from the cap [which could be 1015 Å (11·5 nm)] and the unknown folding of PB2 could result in the labelling of a peptide distant from the aromatic pocket. Equally, the mutagenesis approach may fail because some conservative mutations may interfere in cap binding and some Ala mutations may interfere with the formation of a functional polymerase complex. A potential criticism of the emphasis placed on aromatic residues, W537, Y550, W557 or W564 by Li et al. (2001) arises since these residues are not completely conserved as aromatics between influenza A, B, C and Thogotovirus. It seems likely that once recognition of cap structures by PB2 had evolved in a progenitor influenza virus, this feature would have been retained by natural selection in the subsequent evolution of influenza viruses. There remain other discrepancies. First, Fechter et al. (2003)
failed to confirm the reduced cap-binding efficiency of the Y550A mutant (Li et al., 2001
). Second, Honda et al. (1999)
reported two regions of PB2 involved in cap binding whereas Li et al. (2001)
, reported one. Presumably differences in the conditions of UV cross-linking and/or the V8 protease digestion conditions are responsible.
Interestingly, mutagenesis data on eIF4E shows that a cap-binding pocket formed from two Phe residues has a lower affinity for caps than one formed from two Trp residues (Hsu et al., 2000). This result is consistent with the suggestion that two Phe residues comprise the cap-binding pocket in influenza RNA polymerase (Fechter et al., 2003
) and recent data (Hooker et al., 2003
), which imply that the influenza RNA polymerase is about 100-fold less potent at binding cap analogues than eIF4E.
Structural studies are obviously needed to confirm that influenza RNA polymerase binds capped RNAs through an aromatic sandwich, to detail further its cap-binding mechanism and to resolve the discrepancies highlighted above. In particular, the nature of the acidic residues predicted to interact with the m7G ring, and the basic residues predicted to be involved in binding the triphosphate linkage of the cap structure remain unknown. Such studies could improve our knowledge of the detailed mechanism of cap binding, and potentially provide new targets for the generation of novel specific antivirals against influenza viruses.
Regulation of cap-binding proteins
Relatively little is known about the intracellular regulation of cap-binding proteins with the exception of eIF4E, which has been extensively studied (Clemens, 2001; Kimball, 2001
; McKendrick et al., 1999
; Proud, 2002
; Raught & Gingras, 1999
; Sonenberg & Gingras, 1998
; reviewed by von der Haar et al., 2004
). eIF4E together with eIF4G (scaffold) and eIF4A (helicase) form a large translation initiation complex, known as eIF4F (Fig. 6
). It is thought that eIF4E interacts with mRNA cap structures only as part of the eIF4F complex (Haghighat & Sonenberg, 1997
). Interaction of eIF4G with eIF4E induces a conformational change, enhancing the affinity for capped RNAs (Gross et al., 2003
; Haghighat & Sonenberg, 1997
; Ptushkina et al., 1998
; von der Haar et al., 2000
). Different proteins can compete with eIF4G for eIF4E binding, and thus inhibit the formation of the active eIF4F initiation complex. Inhibition occurs with eIF4E-binding proteins (4E-BP) (Haghighat & Sonenberg, 1997
; Lawrence et al., 1997
; Lin et al., 1994
; Pause et al., 1994
; von der Haar et al., 2000
) or an eIF4E-transporter (Dostie et al., 2000
). Marcotrigiano et al. (1999)
defined a short amino acid motif in eIF4G that is involved in interaction with eIF4E. Interestingly this motif was also present in 4E-BP suggesting that molecular mimicry is involved in controlling initiation of translation. The negative regulation of translation mediated by 4E-BP can be reversed by phosphorylation in response to extracellular stimuli (Kimball, 2001
; Lin et al., 1994
; Pause et al., 1994
). Other translation stimulatory proteins, like the poly(A)-binding protein (PABP) (Fig. 6
), increase mRNA affinity for eIF4E by binding to the active eIF4F complex, (Borman et al., 2000
; Le et al., 1997
; Wei et al., 1998
). Finally, affinity of eIF4E for caps is partially inhibited by phosphorylation of S209 of eIF4E (Flynn & Proud, 1995
; Joshi et al., 1995
), correlating with the stage in the cell cycle (reviewed by Kleijn et al., 1998
; Proud, 2002
). Phosphorylation decreases affinity of eIF4E for mRNAs, possible because of electrostatic repulsion between the negatively charged phosphate group attached to S209 and the triphosphate group of the cap structure (Zuberek et al., 2003
). This may allow recycling of the eIF4F complex at the level of the ribosome (Scheper & Proud, 2002
; Scheper et al., 2002
).
|
Up to now, no regulatory pathways affecting the well studied viral cap-binding proteins (the vaccinia virus, VP39, and the PB2 subunit of influenza RNA polymerase) have been described. However, both viral proteins exist as complexes with other viral proteins or nucleic acids, VP39 with VP55 in the case of vaccinia virus, and PB2 in association with PB1 and PA and viral RNA, in the case of influenza virus. These associated proteins and nucleic acids are essential cofactors for cap-binding activity in the case of influenza virus. Thus, the PB1 and PA subunits of influenza RNA polymerase along with viral RNA may be regarded as playing a similar scaffold role for cap binding, as eIF4G does for eIF4E or CBP80 does for CBP20.
Other regulatory pathways probably remain to be discovered. For example, it is known that capped mRNAs, initially bound by CBC in the nucleus, must be subsequently bound to eIF4F in the cytoplasm. Few details are known about this process, which could be controlled by undiscovered proteins (Lewis & Izaurralde, 1997). Another puzzle is how viral cap-snatching proteins, such as the influenza virus polymerase, compete effectively with cellular cap-binding complexes for mRNAs. This may be a significant problem considering the fact that the affinity of the influenza virus cap binding for mRNAs is much lower than that of cellular cap-binding proteins (Hooker et al., 2003
; Niedzwiecka et al., 2002
; Scheper et al., 2002
; Wilson et al., 1999
).
Concluding remarks
Many cap-binding proteins, other than CBC, eIF4E and VP39 or the PB2 subunit of the influenza virus RNA polymerase, must have evolved in viruses that replicate in the cytoplasm, e.g coronaviruses, flaviviruses and reoviruses. These viruses need to have their own capping enzymes and probably O-methylases if they are to effectively take-over the host-cell translation machinery, unless they have evolved specialist IRES sequences or other mechanisms that bypass the need for caps. We predict that an aromatic sandwich motif will be found in newly discovered O-methylases, such as has recently been described in the SARS coronavirus. Nevertheless, there is a need to experimentally verify such predictions by studying the 3-dimensional structure of these cap-recognizing proteins in the future and comparing their structure with the structures already known for eIF4E, CBP and VP39. Only armed with this knowledge will it be possible to fully assess the subtleties that have evolved in cap-binding proteins. Moreover, such information allows the rational design of a new class of antiviral agents that targets viral cap-binding proteins whilst avoiding cap-binding proteins, such as eIF4E and CBP, needed for normal cellular function.
![]() |
ACKNOWLEDGEMENTS |
---|
![]() |
REFERENCES |
---|
![]() ![]() ![]() |
---|
Blachut-Okrasinska, E., Bojarska, E., Niedzwiecka, A., Chlebicka, L., Darzynkiewicz, E., Stolarski, R., Stepinski, J. & Antosiewicz, J. M. (2000). Stopped-flow and Brownian dynamics studies of electrostatic effects in the kinetics of binding of 7-methyl-GpppG to the protein eIF4E. Eur Biophys J 29, 487498.[CrossRef][Medline]
Borman, A. M., Michel, Y. M. & Kean, K. M. (2000). Biochemical characterisation of cap-poly(A) synergy in rabbit reticulocyte lysates: the eIF4G-PABP interaction increases the functional affinity of eIF4E for the capped mRNA 5'-end. Nucleic Acids Res 28, 40684075.
Bouloy, M., Morgan, M. A., Shatkin, A. J. & Krug, R. M. (1979). Cap and internal nucleotides of reovirus mRNA primers are incorporated into influenza viral complementary RNA during transcription in vitro. J Virol 32, 895904.[Medline]
Bouloy, M., Plotch, S. J. & Krug, R. M. (1980). Both the 7-methyl and the 2'-O-methyl groups in the cap of mRNA strongly influence its ability to act as primer for influenza virus RNA transcription. Proc Natl Acad Sci U S A 77, 39523956.[Abstract]
Brownlee, G. G., Fodor, E., Pritlove, D. C., Gould, K. G. & Dalluge, J. J. (1995). Solid phase synthesis of 5'-diphosphorylated oligoribonucleotides and their conversion to capped m7Gppp-oligoribonucleotides for use as primers for influenza A virus RNA polymerase in vitro. Nucleic Acids Res 23, 26412647.[Abstract]
Cai, A., Jankowska-Anyszka, M., Centers, A., Chlebicka, L., Stepinski, J., Stolarski, R., Darzynkiewicz, E. & Rhoads, R. E. (1999). Quantitative assessment of mRNA cap analogues as inhibitors of in vitro translation. Biochemistry 38, 85388547.[CrossRef][Medline]
Calero, G., Wilson, K. F., Ly, T., Rios-Steiner, J. L., Clardy, J. C. & Cerione, R. A. (2002). Structural basis of m7GpppG binding to the nuclear cap-binding protein complex. Nat Struct Biol 9, 912917.[CrossRef][Medline]
Carberry, S. E., Rhoads, R. E. & Goss, D. J. (1989). A spectroscopic study of the binding of m7GTP and m7GpppG to human protein synthesis initiation factor 4E. Biochemistry 28, 80788083.[CrossRef][Medline]
Carberry, S. E., Darzynkiewicz, E., Stepinski, J., Tahara, S. M., Rhoads, R. E. & Goss, D. J. (1990). A spectroscopic study of the binding of N-7-substituted cap analogues to human protein synthesis initiation factor 4E. Biochemistry 29, 33373341.[CrossRef][Medline]
Carberry, S. E., Darzynkiewicz, E. & Goss, D. J. (1991). A comparison of the binding of methylated cap analogues to wheat germ protein synthesis initiation factors 4F and (iso)4F. Biochemistry 30, 16241627.[CrossRef][Medline]
Chung, T. D., Cianci, C., Hagen, M., Terry, B., Matthews, J. T., Krystal, M. & Colonno, R. J. (1994). Biochemical studies on capped RNA primers identify a class of oligonucleotide inhibitors of the influenza virus RNA polymerase. Proc Natl Acad Sci U S A 91, 23722376.
Cianci, C., Tiley, L. & Krystal, M. (1995). Differential activation of the influenza virus polymerase via template RNA-binding. J Virol 69, 39953999.[Abstract]
Clemens, M. J. (2001). Translational regulation in cell stress and apoptosis. Roles of the eIF4E binding proteins. J Cell Mol Med 5, 221239.[Medline]
Coffin, J. M. (1990). Retroviridae and their replication. In Fields Virology, pp. 14371500. Edited by P. M. Howley. Philadelphia: Lippincott Williams & Wilkins.
Condit, R. C. & Niles, E. G. (2002). Regulation of viral transcription elongation and termination during vaccinia virus infection. Biochim Biophys Acta 1577, 325336.[Medline]
Darzynkiewicz, E. & Lonnberg, H. (1989). Base stacking of simple mRNA cap analogues. Association of 7,9-dimethylguanine, 7-methylguanosine and 7-methylguanosine 5'-monophosphate with indole and purine derivatives in aqueous solution. Biophys Chem 33, 289293.[CrossRef][Medline]
Dostie, J., Ferraiuolo, M., Pause, A., Adam, S. A. & Sonenberg, N. (2000). A novel shuttling protein, 4E-T, mediates the nuclear import of the mRNA 5' cap-binding protein, eIF4E. EMBO J 19, 31423156.
Egloff, M. P., Benarroch, D., Selisko, B., Romette, J. L. & Canard, B. (2002). An RNA cap (nucleoside-2'-O-)-methyltransferase in the flavivirus RNA polymerase NS5: crystal structure and functional characterization. EMBO J 21, 27572768.
Fechter, P., Mingay, L., Sharps, J., Chambers, A., Fodor, E. & Brownlee, G. G. (2003). Two aromatic residues in the PB2 subunit of influenza A RNA polymerase are crucial for cap binding. J Biol Chem 278, 2038120388.
Flick, R., Neumann, G., Hoffmann, E., Neumeier, E. & Hobom, G. (1996). Promoter elements in the influenza vRNA terminal structure. RNA 2, 10461057.[Abstract]
Flynn, A. & Proud, C. G. (1995). Serine 209, not serine 53, is the major site of phosphorylation in initiation factor eIF-4E in serum-treated Chinese hamster ovary cells. J Biol Chem 270, 2168421688.
Fodor, E. & Brownlee, G. G. (2002). Influenza virus replication. In Influenza, pp. 129. Edited by C. W. Potter. Oxford: Elsevier.
Fodor, E., Crow, M., Mingay, L. J., Deng, T., Sharps, J. & Brownlee, G. G. (2002). A single amino acid mutation in the PA subunit of the influenza virus RNA polymerase inhibits endonucleolytic cleavage of capped RNAs. J Virol 76, 89899001.
Gingras, A. C., Raught, B. & Sonenberg, N. (1999). eIF4 initiation factors: effectors of mRNA recruitment to ribosomes and regulators of translation. Annu Rev Biochem 68, 913963.[CrossRef][Medline]
Goss, D. J., Carberry, S. E., Dever, T. E., Merrick, W. C. & Rhoads, R. E. (1990). Fluorescence study of the binding of m7GpppG and rabbit globin mRNA to protein synthesis initiation factors 4A, 4E, and 4F. Biochemistry 29, 50085012.[CrossRef][Medline]
Gross, J. D., Moerke, N. J., von der Haar, T., Lugovskoy, A. A., Sachs, A. B., McCarthy, J. E. & Wagner, G. (2003). Ribosome loading onto the mRNA cap is driven by conformational coupling between eIF4G and eIF4E. Cell 115, 739750.[CrossRef][Medline]
Haghighat, A. & Sonenberg, N. (1997). eIF4G dramatically enhances the binding of eIF4E to the mRNA 5'-cap structure. J Biol Chem 272, 2167721680.
Hodel, A. E., Gershon, P. D., Shi, X. N., Wang, S. M. & Quiocho, F. A. (1997). Specific protein recognition of an mRNA cap through its alkylated base. Nat Struct Biol 4, 350354.[CrossRef][Medline]
Hodel, A. E., Gershon, P. D. & Quiocho, F. A. (1998). Structural basis for sequence-nonspecific recognition of 5'-capped mRNA by a cap-modifying enzyme. Mol Cell 1, 443447.[CrossRef][Medline]
Honda, A., Mizumoto, K. & Ishihama, A. (1999). Two separate sequences of PB2 subunit constitute the RNA cap-binding site of influenza virus RNA polymerase. Genes Cells 4, 475485.
Hooker, L., Sully, R., Handa, B., Ono, N., Koyano, H. & Klumpp, K. (2003). Quantitative analysis of influenza virus RNP interaction with RNA cap structures and comparison to human cap binding protein eIF4E. Biochemistry 42, 62346240.[CrossRef][Medline]
Hsu, P. C., Hodel, M. R., Thomas, J. W., Taylor, L. J., Hagedorn, C. H. & Hodel, A. E. (2000). Structural requirements for the specific recognition of an m7G mRNA cap. Biochemistry 39, 1373013736.[CrossRef][Medline]
Hu, G., Gershon, P. D., Hodel, A. E. & Quiocho, F. A. (1999). mRNA cap recognition: dominant role of enhanced stacking interactions between methylated bases and protein aromatic side chains. Proc Natl Acad Sci U S A 96, 71497154.
Hu, G., Oguro, A., Li, C., Gershon, P. D. & Quiocho, F. A. (2002). The "cap-binding slot" of an mRNA cap-binding protein: quantitative effects of aromatic side chain choice in the double-stacking sandwich with cap. Biochemistry 41, 76777687.[CrossRef][Medline]
Hu, G., Tsai, A. L. & Quiocho, F. A. (2003). Insertion of an N7-methylguanine mRNA cap between two coplanar aromatic residues of a cap-binding protein is fast and selective for a positively charged cap. J Biol Chem 278, 5151551520.
Ishida, T. & Inoue, M. (1981). An X-ray evidence for the charge-transfer interaction between adenine and indole rings: crystal structure of 1,9-dimethyladenine-indole-3-acetic acid trihydrate complex. Biochem Biophys Res Commun 99, 149154.[CrossRef][Medline]
Ishida, T., Doi, M. & Inoue, M. (1988). A selective recognition mode of a nucleic acid base by an aromatic amino acid: L-phenylalanine-7-methylguanosine 5'-monophosphate stacking interaction. Nucleic Acids Res 16, 61756190.[Abstract]
Izaurralde, E., Stepinski, J., Darzynkiewicz, E. & Mattaj, I. W. (1992). A cap binding protein that may mediate nuclear export of RNA polymerase II-transcribed RNAs. J Cell Biol 118, 12871295.[Abstract]
Joshi, B., Cai, A. L., Keiper, B. D. & 7 other authors (1995). Phosphorylation of eukaryotic protein synthesis initiation factor 4E at Ser-209. J Biol Chem 270, 1459714603.
Kimball, S. R. (2001). Regulation of translation initiation by amino acids in eukaryotic cells. Prog Mol Subcell Biol 26, 155184.[Medline]
Kleijn, M., Scheper, G. C., Voorma, H. O. & Thomas, A. A. (1998). Regulation of translation initiation factors by signal transduction. Eur J Biochem 253, 531544.[Abstract]
Lamb, R. A. & Krug, R. M. (2001). Orthomyxoviridae: the viruses and their replication. In Fields Virology, 4th edn, pp. 14871579. Edited by P. M. Howley. Philadelphia: Lippincott Williams & Wilkins.
Lawrence, J. C. Jr, Fadden, P., Haystead, T. A. & Lin, T. A. (1997). PHAS proteins as mediators of the actions of insulin, growth factors and cAMP on protein synthesis and cell proliferation. Adv Enzyme Regul 37, 239267.[CrossRef][Medline]
Le, H., Tanguay, R. L., Balasta, M. L., Wei, C. C., Browning, K. S., Metz, A. M., Goss, D. J. & Gallie, D. R. (1997). The translation initiation factors eIFiso-4G and eIF-4B interact with the poly(A)-binding protein and increase its RNA binding activity. J Biol Chem 272, 1624716255.
Leahy, M. B., Dobbyn, H. C. & Brownlee, G. G. (2001). Hairpin loop structure in the 3' arm of the influenza A virus virion RNA promoter is required for endonuclease activity. J Virology 75, 70427049.
Lewis, J. D. & Izaurralde, E. (1997). The role of cap structure in RNA processing and nuclear export. Eur J Biochem 247, 461469.[Abstract]
Li, M. L., Ramirez, B. C. & Krug, R. M. (1998). RNA-dependent activation of primer RNA production by influenza virus polymerase: different regions of the same protein subunit constitute the two required RNA-binding sites. EMBO J 17, 58445852.
Li, M. L., Rao, P. & Krug, R. M. (2001). The active sites of the influenza cap-dependent endonuclease are on different polymerase subunits. EMBO J 20, 20782086.
Lin, T. A., Kong, X., Haystead, T. A., Pause, A., Belsham, G., Sonenberg, N. & Lawrence, J. C., Jr (1994). PHAS-I as a link between mitogen-activated protein kinase and translation initiation. Science 266, 653656.[Medline]
Lockless, S. W., Cheng, H. T., Hodel, A. E., Quiocho, F. A. & Gershon, P. D. (1998). Recognition of capped RNA substrates by VP39, the vaccinia virus-encoded mRNA cap-specific 2'-O-methyltransferase. Biochemistry 37, 85648574.[CrossRef][Medline]
Marcotrigiano, J., Gingras, A. C., Sonenberg, N. & Burley, S. K. (1997). Cocrystal structure of the messenger RNA 5' cap-binding protein (eIF4E) bound to 7-methyl-GDP. Cell 89, 951961.[CrossRef][Medline]
Marcotrigiano, J., Gingras, A. C., Sonenberg, N. & Burley, S. K. (1999). Cap-dependent translation initiation in eukaryotes is regulated by a molecular mimic of eIF4G. Mol Cell 3, 707716.[CrossRef][Medline]
Matsuo, H., Li, H. J., McGuire, A. M., Fletcher, C. M., Gingras, A. C., Sonenberg, N. & Wagner, G. (1997). Structure of translation factor eIF4E bound to m7GDP and interaction with 4E-binding protein. Nat Struct Biol 4, 717724.[CrossRef][Medline]
Mazza, C., Ohno, M., Segref, A., Mattaj, I. W. & Cusack, S. (2001). Crystal structure of the human nuclear cap binding complex. Mol Cell 8, 383396.[CrossRef][Medline]
Mazza, C., Segref, A., Mattaj, I. W. & Cusack, S. (2002). Large-scale induced fit recognition of an m7GpppG cap analogue by the human nuclear cap-binding complex. EMBO J 21, 55485557.
McKendrick, L., Pain, V. M. & Morley, S. J. (1999). Translation initiation factor 4E. Int J Biochem Cell Biol 31, 3135.[CrossRef][Medline]
Morino, S., Hazama, H., Ozaki, M., Teraoka, Y., Shibata, S., Doi, M., Ueda, H., Ishida, T. & Uesugi, S. (1996). Analysis of the mRNA cap-binding ability of human eukaryotic initiation factor-4E by use of recombinant wild-type and mutant forms. Eur J Biochem 239, 597601.[Abstract]
Moss, B. (2001). Poxviridae: the viruses and their replication. In Fields Virology, 4th edn, vol. 2, pp. 28492883. Edited by D. M Knipe & P. M. Howley. Philadelphia: Lippincott Williams & Wilkins.
Niedzwiecka, A., Marcotrigiano, J., Stepinski, J. & 9 other authors (2002). Biophysical studies of eIF4E cap-binding protein: recognition of mRNA 5' cap structure and synthetic fragments of eIF4G and 4E-BP1 proteins. J Mol Biol 319, 615635.[CrossRef][Medline]
Pause, A., Belsham, G. J., Gingras, A. C., Donze, O., Lin, T. A., Lawrence, J. C., Jr & Sonenberg, N. (1994). Insulin-dependent stimulation of protein synthesis by phosphorylation of a regulator of 5'-cap function. Nature 371, 762767.[CrossRef][Medline]
Plotch, S. J., Bouloy, M., Ulmanen, I. & Krug, R. M. (1981). A unique cap(m7GpppXm)-dependent influenza virion endonuclease cleaves capped RNAs to generate the primers that initiate viral RNA transcription. Cell 23, 847858.[CrossRef][Medline]
Portela, A., Zurcher, T., Nieto, A. & Ortín, J. (1999). Replication of orthomyxoviruses. Adv Virus Res 54, 319348.[Medline]
Proud, C. G. (2002). Regulation of mammalian translation factors by nutrients. Eur J Biochem 269, 53385349.
Ptushkina, M., von der Haar, T., Vasilescu, S., Frank, R., Birkenhager, R. & McCarthy, J. E. (1998). Cooperative modulation by eIF4G of eIF4E-binding to the mRNA 5' cap in yeast involves a site partially shared by p20. EMBO J 17, 47984808.
Quiocho, F. A., Hu, G. & Gershon, P. D. (2000). Structural basis of mRNA cap recognition by proteins. Curr Opin Struct Biol 10, 7886.[CrossRef][Medline]
Raught, B. & Gingras, A. C. (1999). eIF4E activity is regulated at multiple levels. Int J Biochem Cell Biol 31, 4357.[CrossRef][Medline]
Rom, E., Kim, H. C., Gingras, A. C., Marcotrigiano, J., Favre, D., Olsen, H., Burley, S. K. & Sonenberg, N. (1998). Cloning and characterization of 4EHP, a novel mammalian eIF4E-related cap-binding protein. J Biol Chem 273, 1310413109.
Scheper, G. C. & Proud, C. G. (2002). Does phosphorylation of the cap-binding protein eIF4E play a role in translation initiation? Eur J Biochem 269, 53505359.
Scheper, G. C., van Kollenburg, B., Hu, J., Luo, Y., Goss, D. J. & Proud, C. G. (2002). Phosphorylation of eukaryotic initiation factor 4E markedly reduces its affinity for capped mRNA. J Biol Chem 277, 33033309.
Shi, L. C., Summers, D. F., Peng, Q. H. & Galarza, J. M. (1995). Influenza-A virus-RNA polymerase subunit PB2 is the endonuclease which cleaves host cell messenger RNA and functions only as the trimeric enzyme. Virology 208, 3847.[CrossRef][Medline]
Shi, L., Galarza, J. M. & Summers, D. F. (1996). Recombinant-baculovirus-expressed PB2 subunit of the influenza A virus RNA polymerase binds cap groups as an isolated subunit. Virus Res 42, 19.[CrossRef][Medline]
Shuman, S. & Lima, C. D. (2004). The polynucleotide ligase and RNA capping enzyme superfamily of covalent nucleotidyltransferases. Curr Opin Struct Biol 14, 757764.[CrossRef][Medline]
Smith, G. L., Vanderplasschen, A. & Law, M. (2002). The formation and function of extracellular enveloped vaccinia virus. J Gen Virol 83, 29152931.
Sonenberg, N. & Gingras, A. C. (1998). The mRNA 5' cap-binding protein eIF4E and control of cell growth. Curr Opin Cell Biol 10, 268275.[CrossRef][Medline]
Stolarski, R., Sitek, A., Stepinski, J., Jankowska, M., Oksman, P., Temeriusz, A., Darzynkiewicz, E., Lonnberg, H. & Shugar, D. (1996). 1H-NMR studies on association of mRNA cap-analogues with tryptophan-containing peptides. Biochim Biophys Acta 1293, 97105.[Medline]
Tomoo, K., Shen, X., Okabe, K. & 9 other authors (2003). Structural features of human initiation factor 4E, studied by X-ray crystal analyses and molecular dynamics simulations. J Mol Biol 328, 365383.[CrossRef][Medline]
Ueda, H., Iyo, H., Doi, M., Inoue, M. & Ishida, T. (1991). Cooperative stacking and hydrogen bond pairing interactions of fragment peptide in cap binding protein with mRNA cap structure. Biochim Biophys Acta 1075, 181186.[Medline]
Ulmanen, I., Broni, B. A. & Krug, R. M. (1981). Role of two of the influenza virus core P proteins in recognizing cap 1 structures (m7GpppNm) on RNAs and in initiating viral RNA transcription. Proc Natl Acad Sci U S A 78, 73557359.[Abstract]
von der Haar, T., Ball, P. D. & McCarthy, J. E. (2000). Stabilization of eukaryotic initiation factor 4E binding to the mRNA 5'-cap by domains of eIF4G. J Biol Chem 275, 3055130555.
von der Haar, T., Gross, J. D., Wagner, G. & McCarthy, J. E. (2004). The mRNA cap-binding protein eIF4E in post-transcriptional gene expression. Nat Struct Mol Biol 11, 503511.[CrossRef][Medline]
Vreede, F. T., Jung, T. E. & Brownlee, G. G. (2004). Model suggesting that replication of influenza virus is regulated by stabilization of replicative intermediates. J Virol 78, 95689572.
Wei, C. C., Balasta, M. L., Ren, J. & Goss, D. J. (1998). Wheat germ poly(A) binding protein enhances the binding affinity of eukaryotic initiation factor 4F and (iso)4F for cap analogues. Biochemistry 37, 19101916.[CrossRef][Medline]
Wilson, F. K. & Cerione, R. A. (2000). Signal transduction and post-transcriptional gene expression. Biol Chem 381, 357365.[CrossRef][Medline]
Wilson, K. F., Fortes, P., Singh, U. S., Ohno, M., Mattaj, I. W. & Cerione, R. A. (1999). The nuclear cap-binding complex is a novel target of growth factor receptor-coupled signal transduction. J Biol Chem 274, 41664173.
Wu, X. & Guarino, L. A. (2003). Autographica californica nucleopolyhedrovirus orf69 encodes an RNA cap (nucleoside-2'-O)methyltransferase. J Virol 77, 34303440.
Zuberek, J., Wyslouch-Cieszynska, A., Niedzwiecka, A. & 9 other authors (2003). Phosphorylation of eIF4E attenuates its interaction with mRNA 5' cap analogs by electrostatic repulsion: intein-mediated protein ligation strategy to obtain phosphorylated protein. RNA 9, 5261.