Eukaryotic Initiation Factor 4GII (eIF4GII), but Not eIF4GI, Cleavage Correlates with Inhibition of Host Cell Protein Synthesis after Human Rhinovirus Infection

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Journal of Virology, April 1999, p. 3467-3472, Vol. 73, No. 4
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Eukaryotic Initiation Factor 4GII (eIF4GII), but Not eIF4GI, Cleavage Correlates with Inhibition of Host Cell Protein Synthesis after Human Rhinovirus Infection

Yuri V. Svitkin, Alessandra Gradi, Hiroaki Imataka, Shigenobu Morino, and Nahum Sonenberg^*

Department of Biochemistry and McGill Cancer Center, McGill University, Montreal, Quebec, Canada H3G 1Y6

Received 17 August 1998/Accepted 22 December 1998

	ABSTRACT

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For many members of the Picornaviridae family, infection of cells results in a shutoff of host protein synthesis. For rhinovirusesand enteroviruses, the shutoff has been explained in part by thecleavage of eukaryotic initiation factor 4GI (eIF4GI), a componentof the cap-binding protein complex eIF4F. The cleavage of eIF4GIis mediated by the virus-specific proteinase 2A^pro and results in inhibition of cap-dependent, but not cap-independent,translation. The inhibition of host protein synthesis after infectionwith human rhinovirus 14 (HRV-14) lags behind the cleavage ofeIF4GI. Recently, we discovered a functional homolog of eIF4GI,termed eIF4GII, and showed that cleavage of eIF4GII coincideswith the shutoff of host cell protein synthesis after poliovirusinfection (Gradi et al., Proc. Natl. Acad. Sci. USA 95:11089-11094,1998). We wished to determine whether eIF4GII cleavage kineticscould also explain the lack of correlation between the kineticsof eIF4GI cleavage and the shutoff of host protein synthesis afterrhinovirus infection. In this study, we examined the correlationbetween human rhinovirus-induced shutoff of host protein synthesisand cleavage of eIF4GI and eIF4GII. In HRV-14-infected HeLa cells,almost no intact eIF4GI could be detected by 4 h postinfection,while only 4% of eIF4GII was cleaved at this time. By 6 h, however,67% of eIF4GII was cleaved, and this cleavage coincided with asignificant (60%) decline of host translation. These results suggestthat cleavage of both eIF4GI and eIF4GII is required for HRV-mediatedinhibition of host cell protein synthesis and that the cleavageof eIF4GII is the rate-limiting step in the shutoff of host cellprotein synthesis after rhinovirusinfection.

	TEXT

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The genome of human rhinoviruses (HRV), similar to that of other picornaviruses, contains a single long open reading framewhich encodes a large polyprotein precursor. The polyprotein isprocessed, partially in the nascent state, by two virus-specificproteases. Protease 2A^pro performs the initial cleavage of the nascent polyprotein thatliberates the capsid protein precursor (P1), while 3C^pro is responsible for the remaining cleavage events (33).

To establish an efficient infection, picornaviruses have evolved mechanisms to inhibit host cell protein synthesis. Translationof the capped cellular mRNAs is blocked at the initiation step,while translation of the uncapped virus mRNA proceeds efficientlyvia a cap-independent mechanism (2, 11). The mechanism ofthis selective inhibition of host protein synthesis varies dependingon the particular virus-host system. In rhinovirus- and enterovirus-infectedcells, a cap-binding protein complex, the eukaryotic initiationfactor 4F (eIF4F), is altered, both structurally and functionally(11). eIF4F is composed of the following three subunits: (i)eIF4E, which specifically recognizes the cap structure (44,45); (ii) eIF4A, which possesses an RNA helicase activity (39,42); and (iii) eIF4G (formerly p220), which serves as a scaffoldto bring together eIF4E, eIF4A, and eIF3, a factor which linkseIF4G to the ribosome (23, 28, 43).

A large body of evidence supports the idea that rhinoviruses and enteroviruses inactivate eIF4F by cleavage of the eIF4G subunitin a process mediated by 2A^pro (3, 22, 27). Poliovirus 2A^pro mutants defective in eIF4G cleavage are also defective in inducingthe shutoff of host translation (3, 32). 2A^pro of human rhinovirus 2 (HRV-2) and coxsackievirus B4 cleave eIF4Gdirectly (24, 25). Poliovirus 2A^pro is also capable of directly cleaving eIF4G (7, 17); however,it was concluded that the major eIF4G-specific cleavage activityin poliovirus-infected HeLa cells is not associated with a 2A^pro (8). The C-terminal cleavage product of eIF4G interacts witheIF4A and eIF3 and supports cap-independent translation (6,31, 37). However, it lacks the eIF4E recognition domain andis unable to support cap-dependent translation. In addition, cap-independentviral protein synthesis is stimulated by the C-terminal cleavageproduct of eIF4G of several (6, 31, 47, 48), but notall (5, 41),picornaviruses.

Although eIF4G proteolysis provides an attractive explanation for the shutoff phenomenon, several earlier findings obtainedwith poliovirus are inconsistent with such a model. For example,there is no good temporal correlation between the proteolysisof eIF4G and the shutoff of host translation in poliovirus-infectedHeLa cells (13). While the cleavage of eIF4G occurs rapidly,i.e., within an average of 2 h postinfection, the shutoff is observedat 2.5 h or even later. Moreover, a complete cleavage of eIF4Goccurs in the presence of guanidine-HCl and other inhibitors ofpoliovirus replication, which strongly mitigate the inhibitionof host cell protein synthesis (4, 21, 36). It was suggested,therefore, that complete inhibition of host cell protein synthesisfollowing poliovirus infection requires a second event in additionto the cleavage of eIF4G (4). An alternative interpretationof these data is that eIF4G cleavage is irrelevant to the shutoffof host translation (21). These apparent discrepancies may nowbe explained by recent findings. We have recently identified afunctional homolog of eIF4G, termed eIF4GII (16). eIF4GII is46% identical to the original eIF4G (46), which was renamedeIF4GI. eIF4GII is cleaved both in vivo and in vitro by poliovirus2A^pro (17). However, after poliovirus infection, the cleavage ofeIF4GII is slower than that of eIF4GI and, in contrast to cleavageof eIF4GI, it coincides with the shutoff of host protein synthesis(17).

In human rhinovirus 14 (HRV-14)-infected HeLa cells, as in poliovirus-infected cells, there is a discrepancy between the timecourse of eIF4GI cleavage and the shutoff of host protein synthesis(12). It is possible that this discrepancy can be explainedfor rhinovirus, as was shown for poliovirus, by the slower kineticsof cleavage of eIF4GII. Here, we addressed thispossibility.

HeLa-I cells (Ohio strain) (1) were grown in monolayers in Dulbecco's minimal essential medium (DMEM) containing 10% fetalbovine serum (FBS). HRV-14 was kindly provided by R. Rueckert.Virus stock was generated by passages in HeLa cells at 34°C inDMEM containing 2% FBS. Virus titers were determined in four replicatesin a 50% tissue culture infective dose (TCID₅₀) assay on HeLacells, using 10-fold virus dilutions in 96-well microtiter plates.Virus dilutions were mixed with 10⁴ cells in DMEM containing 2% FBS in a total volume of 0.3 ml.The plates were incubated at 34°C for 4 days. Following incubation,the cytopathic effect was determined, and the titers were estimatedaccording to the method of Reed and Muench (40). For a one-stepinfection, HeLa cells were grown to ~80% confluency in 10-cm petridishes. The cells were infected in serum-free medium at a multiplicityof infection of 50 TCID₅₀ per cell. Following virus adsorptionat room temperature for 30 min, the cells were washed with phosphate-bufferedsaline (PBS) and further incubated in 5 ml of methionine-freeDMEM without serum at 34°C. At the times indicated in the figurelegends, the cells were incubated for 30 min with [³⁵S]methionine (10 µCi/ml; 1 Ci = 37 GBq), washed with PBS, andscraped on ice into 0.2 ml of cold buffer containing 20 mM HEPES-KOH(pH 7.6), 150 mM KCl, 1 mM dithiothreitol, 1 mM EDTA, and a proteaseinhibitor cocktail (Boehringer Mannheim). Cells were lysed bythree cycles of freezing and thawing. Cell debris was pelletedby centrifugation, and protein concentration in the supernatantwas measured by the Bio-Rad assay. The protein concentration wasadjusted to 4 mg/ml by diluting with PBS. Proteins were denaturedwith an equal volume of 2× Laemmli sample buffer and boiled for2 min. Aliquots were analyzed by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) (15% polyacrylamide). The gelswere processed for fluorography with En³Hance (Dupont). Antibodies and the protocol for Western blottinghave been described previously (16, 17). Briefly, 40 µg ofHeLa cell protein extract was subjected to SDS-PAGE (6% acrylamide).The proteins were transferred onto 0.45-µm-pore-size nitrocellulosemembranes (Schleicher & Schuell). The membranes were blocked overnightwith 5% skim milk in PBS at 4°C and probed with the indicatedantibodies for 3 to 4 h at 4°C in 10 mM Tris-HCl (pH 8.0), 150mM NaCl, 0.5% Tween 20, and 5% skim milk. After washing, the blotswere incubated in the same buffer, but without skim milk, withdonkey anti-rabbit immunoglobulin-horseradish peroxidase (Amersham)at a 1:5,000 dilution for 45 min at room temperature. Followingextensive washing, the blots were developed with the RenaissanceECL system (Amersham). The intensities of the bands were quantifiedby using a BioImage densitometer (Milligen/Biosearch).

HRV-14 infection results in rapid cleavage of eIF4GI between 1 and 2 h after infection (12, 29). However, the shutoffof host protein synthesis lags considerably behind the cleavageof eIF4GI, as significant inhibition of host protein synthesisoccurs only after 3 h of infection (12). To determine whethereIF4GII is more resistant to proteolysis than eIF4GI, we examinedthe integrity of eIF4GII following HRV-14 infection. The stateof eIF4GI and the pattern of protein synthesis in HRV-14-infectedHeLa cells were analyzed in parallel. Samples of mock- or virus-infectedHeLa cells (50 TCID₅₀ per cell) were grown in monolayers in 10-cmpetri dishes and pulse-labeled for 30 min with [³⁵S]methionine at different times after infection. Aliquots of cytoplasmicextracts were processed for SDS-PAGE followed by autoradiographyor Western blotting using polyclonal anti-eIF4GI or anti-eIF4GIIantibody as specified in the figurelegends.

HRV-14 infection resulted in a feeble inhibition of host cell protein synthesis (Fig. 1; for quantitation see Fig. 2C). Thepartial inhibition of host translation (~60% at 5.5 to 6 h postinfection)occurred concomitantly with the synthesis of the bulk of virusproteins. Inhibition of [³⁵S]methionine incorporation into cellular proteins has been assessedby quantification of the amount of radioactivity in an arbitrarilychosen representative cellular polypeptide (p50). Western blotanalysis of infected cell extract revealed that while both eIF4GIand eIF4GII were cleaved during infection, the cleavage kineticsof the two isoforms varied dramatically. Cleavage of eIF4GI wasdetectable at 1.0 to 1.5 h after infection and was almost completeby 4 h (Fig. 2A). The disappearance of the full-size eIF4GI wasaccompanied by accumulation of the characteristic cleavage productsthat have been described for both rhinovirus and poliovirus (12,13). Cleavage of eIF4GII occurred much later than that of eIF4GI(Fig. 2B). Strikingly, only a minute fraction of eIF4GII was cleavedat 4 h postinfection as judged by the first appearance of thecharacteristic cleavage products. Quantification of intact eIF4GIIshowed that about one-third of eIF4GII remained intact even at6 h after infection (Fig. 2C). The low rate of eIF4GII cleavageis consistent with the inefficient inhibition of host mRNA translationafter HRV-14 infection (Fig. 1 and 2C).

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FIG. 1. Protein synthesis in HRV-14-infected cells. HeLa cells were mock infected or infected with HRV-14 (50 TCID₅₀ per cell) and pulse-labeled for 30 min with [³⁵S]methionine at the indicated times after infection. Equal amounts of cytoplasmic protein extract (5 µg) were analyzed by SDS-15% PAGE, and the gel was fluorographed. Arrows indicate virus-specific proteins. The arrowhead indicates an arbitrary cellular protein (p50).

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FIG. 2. (A and B) eIF4GI and eIF4GII cleavage. Proteins (40 µg) of the samples indicated in the legend for Fig. 1 were separated by SDS-6% PAGE, blotted onto nitrocellulose paper, and treated with polyclonal antibodies against eIF4GI (A) or eIF4GII (B) (16, 17). Positions of molecular mass standards are shown. (C) Quantitative analysis of the results shown in Fig. 1 and 2. The intensity of the p50 cellular protein band (Fig. 1) was determined by using a Bas 2000 phosphorimager and is presented as a percentage of the signal in p50 of mock-infected extracts (there was no significant change in the labeling of p50 in mock-infected cells at different times). The amount of intact eIF4GI and eIF4GII present in each lane is presented as a percentage of that of uncleaved eIF4Gs in mock-infected cells (no change was observed in the amount of eIF4Gs in mock-infected cells upon incubation). The intensities of the bands were determined with a BioImage densitometer (Milligan Bioresearch). p.i., postinfection.

Our results show a coincidence between the cleavage of eIF4GII and the inhibition of host protein synthesis in HRV-14-infectedcells. eIF4GI is cleaved before eIF4GII, and its cleavage is mostprobably required for the inhibition of host protein synthesis.Thus, the decrease in translation during HRV-14 infection correlateswith eIF4GII cleavage, because this is the last event to occur.Several factors could account for the differential cleavage ofeIF4GI and eIF4GII by HRV-14, as is the case for poliovirus infection(17). First, eIF4GII might be a poorer substrate for HRV-142A^pro than eIF4GI. Second, the fraction of eIF4GI and eIF4GII in thecell that is associated with eIF4E might be different. The susceptibilityof eIF4GI and eIF4GII to HRV-2 2A^pro proteolysis is dramatically increased when these factors arebound to eIF4E (16, 18, 30). It would, therefore, be importantto determine what fraction of eIF4GI and eIF4GII is present asa complex with eIF4E. It is also possible that eIF4GI-eIF4E andeIF4GII-eIF4E complexes differ in their sensitivities to cleavageby 2A^pro.

An important issue in addressing the correlation between eIF4GII cleavage and the inhibition of host translation concernsthe relative abundance of eIF4GI and eIF4GII in cells. We determinedthe concentration of eIF4GI and eIF4GII in HeLa cell extractsby quantitative Western immunoblotting (35) using a range ofeIF4GI and eIF4GII concentrations. Purified recombinant eIF4GIand eIF4GII proteins expressed by the baculovirus system (16)were used as standards. The eIF4Gs possess an Xpress epitope (Invitrogen)within their N-terminal portions. The concentrations of the eIF4Gisoforms were estimated after SDS-PAGE and Coomassie blue staining.The intensities of the recombinant eIF4GI and eIF4GII bands werecompared to those of bovine serum albumin over a range of concentrations.Using these estimations as well as the results of Western blotanalysis with an Anti-Xpress antibody (Invitrogen) the concentrationsof eIF4GI and eIF4GII protein standards were determined and normalized.For eIF4GI quantification, 40 µg of HeLa cell S10 fraction wasanalyzed together with known amounts of eIF4GI (Fig. 3A). Notethat the cytoplasmic eIF4GI migrates as several bands, possiblydue to posttranslational modification or proteolytic cleavage.Also, the recombinant eIF4GI migrates somewhat faster than thenative forms, presumably because it possesses a 156-amino-acid(aa) truncation at the N-terminal portion while containing anextra sequence of 46 aa from the pBlueBacHis2 C baculovirus vector(Invitrogen) (16, 20). The ECL signal of the HeLa S10 correspondedto that elicited by 34 ng of eIF4GI. We calculated that eIF4GIconstitutes about 0.085% of HeLa S10 and eIF4GII constitutes 0.018%(Fig. 3B). Similar to eIF4GI, endogenous eIF4GII migrates as severalforms and does so more slowly than recombinant eIF4GII, whichlacks 158 aa but contains 46 aa derived from the vector (16).Quantification of eIF4GI and eIF4GII in two other batches of HeLaS10 resulted in similar values. The mean content of eIF4GI inthe HeLa S10 fraction is 0.08 ± 0.005% and the content of eIF4GIIis 0.019 ± 0.002%. Assuming similar molecular weights for eIF4GIand eIF4GII, the molar ratio of eIF4GI to eIF4GII is 4.2. Thus,eIF4GII constitutes about 20% of the total amount of eIF4G inHeLa-I cells. Although eIF4GII is less abundant than eIF4GI, itsamount in the cell is sufficient to maintain host cell proteinsynthesis at late times of HRV-14 infection, when eIF4GI is cleaved.Thus, eIF4GI is not rate limiting for translation. Indeed, itis believed that the availability of eIF4E, rather than eIF4GI,limits translation in eukaryotic cells. First, with the exceptionof one report (38), eIF4E was found to be present in most cellsat a lower molar concentration than eIF4GI (10, 15, 19).Second, eIF4E may undergo functional inactivation through sequesteringinto complexes with repressor proteins, the 4E-BPs (26, 34).

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FIG. 3. Quantification of eIF4GI and eIF4GII in HeLa S10 cell extracts. (A) HeLa cell protein (40 µg) was analyzed side by side with known amounts of recombinant eIF4GI by SDS-8% PAGE and Western immunoblotting using anti-eIF4GI antibodies (insert). The signals of the eIF4GI standards were used to generate a calibration curve. The dashed line indicates the signal of the HeLa cell S10 fraction. (B) HeLa cell protein (80 µg) was analyzed together with known amounts of recombinant eIF4GII as described above, with anti-eIF4GII antibodies (insert). The signals of the eIF4GII standards were used to generate a calibration curve. The dashed line indicates the signal of the HeLa cell S10 fraction.

Taken together, our results show that after poliovirus (17) and HRV-14 infections (this report), cleavage of eIF4GII lagsbehind that of eIF4GI. Interestingly, this pattern might not begeneral for all picornavirus infections, as our preliminary datado not reveal such a difference after aphthovirus infection (45b).It is possible that aphthovirus L protease does not discriminatebetween eIF4GI and eIF4GII cleavage sites in a manner similarto poliovirus and HRV-14 2A^pro proteases. Finally, it should be noted that although the cleavageof eIF4G might be the sole cause of the inhibition of host translationafter rhinovirus infection, the contributions of other mechanisms,such as 4E-BP1 dephosphorylation (14) or changes in ionic conditionsto favor virus versus host mRNA translation (9), cannot beexcluded. We, however, were unable to detect any 4E-BP1 dephosphorylationin the course of HRV-14 or HRV-16 infections (45a).

	ACKNOWLEDGMENTS

We thank R. Rueckert for HRV-14 and F. G. Hayden, E. Arruda, and C. E. Crump for HeLa-I (Ohio)cells.

This work was supported by grants from the Medical Research Council of Canada to N.S. N.S. is a Medical Research Council DistinguishedScientist and a Howard Hughes Medical School InternationalScholar.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry, McIntyre Medical Sciences Building, McGill University,3655 Drummond St., Montreal, Quebec, Canada H3G 1Y6. Phone: (514)398-7274. Fax: (514) 398-1287. E-mail: sonenberg{at}medcor.mcgill.ca.

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35. Pause, A., N. Méthot, Y. V. Svitkin, W. C. Merrick, and N. Sonenberg. 1994. Dominant negative mutants of mammalian translation initiation factor eIF-4A define a critical role for eIF-4F in cap-dependent and cap-independent initiation of translation. EMBO J. 13:1205-1215[Medline].

36. Pérez, L., and L. Carrasco. 1992. Lack of direct correlation between p220 cleavage and the shut-off of host translation after poliovirus infection. Virology 189:178-186[Medline].

37. Pestova, T. V., I. N. Shatsky, and C. U. T. Hellen. 1996. Functional dissection of eukaryotic initiation factor 4F: the 4A subunit and the central domain of the 4G subunit are sufficient to mediate internal entry of 43S preinitiation complexes. Mol. Cell. Biol. 16:6870-6878[Abstract].

38. Rau, M., T. Ohlmann, S. J. Morley, and V. M. Pain. 1996. A reevaluation of the cap-binding protein, eIF4E, as a rate-limiting factor for initiation of translation in reticulocyte lysate. J. Biol. Chem. 271:8983-8990[Abstract/Free Full Text].

39. Ray, B. K., T. G. Lawson, J. C. Kramer, M. H. Cladaras, J. A. Grifo, R. D. Abramson, W. C. Merrick, and R. E. Thach. 1985. ATP-dependent unwinding of messenger RNA structure by eukaryotic initiation factors. J. Biol. Chem. 260:7651-7658[Abstract/Free Full Text].

40. Reed, L. J., and H. Muench. 1938. A simple method of estimating fifty per cent endpoints. Am. J. Hyg. 27:493-497.

41. Roberts, L. O., R. A. Seamons, and G. J. Belsham. 1998. Recognition of picornavirus internal ribosome entry sites within cells: influence of cellular and viral proteins. RNA 4:520-529[Abstract].

42. Rozen, F., I. Edery, K. Meerovitch, T. E. Dever, W. C. Merrick, and N. Sonenberg. 1990. Bidirectional RNA helicase activity of eucaryotic translation initiation factors 4A and 4F. Mol. Cell. Biol. 10:1134-1144[Abstract/Free Full Text].

43. Sachs, A. B., P. Sarnow, and M. W. Hentze. 1997. Starting at the beginning, middle, and end: translation initiation in eukaryotes. Cell 89:831-838[Medline].

44. Sonenberg, N. 1996. mRNA 5' cap-binding protein eIF4E and control of cell growth, p. 245-269. In J. W. B. Hershey, M. B. Mathews, and N. Sonenberg (ed.), Translational control. Cold Spring Harbor Laboratory Press, Plainview, N.Y.

45. Sonenberg, N., M. A. Morgan, W. C. Merrick, and A. J. Shatkin. 1978. A polypeptide in eukaryotic initiation factors that crosslinks specifically to the 5'-terminal cap in mRNA. Proc. Natl. Acad. Sci. USA 75:4843-4847[Abstract/Free Full Text].

45a. Svitkin, Y. V., and A. Gradi. Unpublished observations.

45b. Svitkin, Y. V., A. Gradi, and G. Belsham. Unpublished observations.

46. Yan, R., W. Rychlik, D. Etchison, and R. E. Rhoads. 1992. Amino acid sequence of the human protein synthesis initiation factor eIF-4 $gamma$ . J. Biol. Chem. 267:23226-23231[Abstract/Free Full Text].

47. Ziegler, E., A. M. Borman, F. G. Deliat, H. D. Liebig, D. Jugovic, K. M. Kean, T. Skern, and E. Kuechler. 1995. Picornavirus 2A proteinase-mediated stimulation of internal initiation of translation is dependent on enzymatic activity and the cleavage products of cellular proteins. Virology 213:549-557[Medline].

48. Ziegler, E., A. M. Borman, R. Kirchweger, T. Skern, and K. M. Kean. 1995. Foot-and-mouth disease virus Lb proteinase can stimulate rhinovirus and enterovirus IRES-driven translation and cleave several proteins of cellular and viral origin. J. Virol. 69:3465-3474[Abstract].

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41.	Roberts, L. O., R. A. Seamons, and G. J. Belsham. 1998. Recognition of picornavirus internal ribosome entry sites within cells: influence of cellular and viral proteins. RNA 4:520-529[Abstract].
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44.	Sonenberg, N. 1996. mRNA 5' cap-binding protein eIF4E and control of cell growth, p. 245-269. In J. W. B. Hershey, M. B. Mathews, and N. Sonenberg (ed.), Translational control. Cold Spring Harbor Laboratory Press, Plainview, N.Y.
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45a.	Svitkin, Y. V., and A. Gradi. Unpublished observations.
45b.	Svitkin, Y. V., A. Gradi, and G. Belsham. Unpublished observations.
46.	Yan, R., W. Rychlik, D. Etchison, and R. E. Rhoads. 1992. Amino acid sequence of the human protein synthesis initiation factor eIF-4 $gamma$ . J. Biol. Chem. 267:23226-23231[Abstract/Free Full Text].
47.	Ziegler, E., A. M. Borman, F. G. Deliat, H. D. Liebig, D. Jugovic, K. M. Kean, T. Skern, and E. Kuechler. 1995. Picornavirus 2A proteinase-mediated stimulation of internal initiation of translation is dependent on enzymatic activity and the cleavage products of cellular proteins. Virology 213:549-557[Medline].
48.	Ziegler, E., A. M. Borman, R. Kirchweger, T. Skern, and K. M. Kean. 1995. Foot-and-mouth disease virus Lb proteinase can stimulate rhinovirus and enterovirus IRES-driven translation and cleave several proteins of cellular and viral origin. J. Virol. 69:3465-3474[Abstract].