Fluorescence Studies on Association of Human Translation Initiation Factor eIF4E with mRNA cap-Analogues

Wieczorek, Z; Niedzwiecka, Anna; Chlebicka, Lidia; Jankowska, Marzena; Kiraga, Katarzyna; Stępiński, Janusz; Dadlez, Michał; Drabent, Regina; Darżynkiewicz, Edward; Stolarski, Ryszard

doi:10.1515/znc-1999-3-420

Cited by 19 publications

(18 citation statements)

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“…This is in contrast to the published data, 12,13) where the binding preference of m 7 GTP over m 7 GpppA/G was observed. The reasons for the discrepancies between these re- sults and ours are not known at present.…”

Section: Resultscontrasting

confidence: 99%

Structural and Thermodynamic Behavior of Eukaryotic Initiation Factor 4E in Supramolecular Formation with 4E-Binding Protein 1 and mRNA Cap Analogue, Studied by Spectroscopic Methods.

Shen

Tomoo

Uchiyama

et al. 2001

CHEMICAL & PHARMACEUTICAL BULLETIN

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Section: Resultscontrasting

confidence: 99%

Structural and Thermodynamic Behavior of Eukaryotic Initiation Factor 4E in Supramolecular Formation with 4E-Binding Protein 1 and mRNA Cap Analogue, Studied by Spectroscopic Methods.

Shen

Tomoo

Uchiyama

et al. 2001

CHEMICAL & PHARMACEUTICAL BULLETIN

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“…From a set of three independent measurements the average K d was found to be 10 (±3) nM for 7MeGTP, which is nearly identical to the value (9.1 nM) previously reported for eIF4E purified by cap-affinity chromatography [25]. The K d value is almost 2-orders of magnitude lower than that reported by others [26,29,30], The fluorescence quenching measurements were also conducted with 7MeGDP, 7MeGMP and 7BnGMP under similar condition and the corresponding K d values were found to be 45 (±10) nM, 10,000(±500) nM and 800 (± 200) nm, respectively. Similar trends in the K d values for 7MeGDP (49 nM) and 7MeGMP (1240 nM) were reported by Stolarski's and co-workers [25] Although a Kd value determined by fluorescence titration has not been reported for 7BnGMP, a nearly 9-fold greater K d value (7,000 nM) was recently determined for 7BnGMP by a novel mass spectroscopic technique [47].…”

Section: Fluorescence Quenching Cap-analog Binding Studiessupporting

confidence: 85%

“…However, extensive dialysis may alter the functional integrity of eIF4E [24,25]. K d values for eIF4E with the cap analogue 7MeGTP have been reported over a broad range from 10 −5 to 10 −8 M −1 [22,23,[25][26][27][28][29][30]. Recently, Stolarski and co-workers have shown that even after repeated dialysis or anion exchange chromatography, 60% of the resulting recombinant eIF4E can still be bound to cap-analogues used for elution [25].…”

Section: Introductionmentioning

confidence: 99%

Expression, purification and characterization of recombinant mouse translation initiation factor eIF4E as a dihydrofolate reductase (DHFR) fusion protein

Ghosh

Cheng

Chou

et al. 2008

Protein Expression and Purification

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One of the earliest steps in translation initiation is recognition of the mRNA cap structure (m7GpppX) by the initiation factor eIF4E. Studies of interactions between purified eIF4E and its binding partners provide important information for understanding mechanisms underlying translational control in normal and cancer cells. Numerous impediments of the available methods used for eIF4E purification led us to develop a novel methodology for obtaining fractions of eIF4E free from undesired byproducts. Herein we report methods for bacterial expression of eIF4E tagged with mutant dihydrofolate reductase (DHFR) followed by isolation and purification of the DHFR-eIF4E protein by using affinity and anion-exchange chromatography. Fluorescence quenching experiments indicated the cap analogue, 7MeGTP, bound to DHFR-eIF4E and eIF4E with a dissociation constant (K d ) of 6±5 and 10±3 nM, respectively. Recombinant eIF4E and DHFR-eIF4E were both shown to significantly enhance in vitro translation in dose dependent manner by 75% at 0.5 uM. Nevertheless increased concentrations of eIF4E and DHFR-eIF4E significantly inhibited translation in a dose dependent manner by a maximum at 2 uM of 60% and 90%, respectively. Thus, we have demonstrated that we have developed an expression system for fully functional recombinant eIF4E. We have also shown that the fusion protein DHFR-eIF4E is functional and thus may be useful for cell based affinity tag studies with fluorescently labeled trimethoprim analogs.

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“…U1 snRNA, which harbors a trimethylated cap in the cytoplasm, did not detectably coimmunoprecipitate with eIF4E (Fig. 6D), as was evident from several observations: (1) Cellular U snRNPs appear to be largely free of sequestering CBPs, based on their quantitative IP using anti-trimethyl G (Bringmann et al 1983); (2) eIF4E binds trimethylated caps 10-fold less efficiently than it binds monomethylated caps (Wieczorek et al 1999); and (3) snurportin binds the trimethylated cap of cytoplasmic U snRNAs (Will and Lü hrmann 2001) so as to mediate together with IMPb snRNA import into nuclei to function in pre-mRNA splicing (Rollenhagen and Pante 2006;Cook et al 2007).…”

Section: Resultsmentioning

confidence: 68%

Remodeling of the pioneer translation initiation complex involves translation and the karyopherin importin β

Sato¹,

Maquat²

2009

Genes Dev.

133

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Mammalian mRNAs lose and acquire proteins throughout their life span while undergoing processing, transport, translation, and decay. How translation affects messenger RNA (mRNA)-protein interactions is largely unknown. The pioneer round of translation uses newly synthesized mRNA that is bound by cap-binding protein 80 (CBP80)-CBP20 (also known as the cap-binding complex [CBC]) at the cap, poly(A)-binding protein N1 (PABPN1) and PABPC1 at the poly(A) tail, and, provided biogenesis involves pre-mRNA splicing, exon junction complexes (EJCs) at exon-exon junctions. Subsequent rounds of translation engage mRNA that is bound by eukaryotic translation initiation factor 4E (eIF4E) at the cap and PABPC1 at the poly(A) tail, but that lacks detectable EJCs and PABPN1. Using the level of intracellular iron to regulate the translation of specific mRNAs, we show that translation promotes not only removal of EJC constituents, including the eIF4AIII anchor, but also replacement of PABPN1 by PABPC1. Remarkably, translation does not affect replacement of CBC by eIF4E. Instead, replacement of CBC by eIF4E is promoted by importin b (IMPb): Inhibiting the binding of IMPb to the complex of CBC-IMPa at an mRNA cap using the IMPa IBB (IMPb-binding) domain or a RAN variant increases the amount of CBC-bound mRNA and decreases the amount of eIF4E-bound mRNA. Our studies uncover a previously unappreciated role for IMPb and a novel paradigm for how newly synthesized messenger ribonucleoproteins (mRNPs) are matured.[Keywords: Iron response element; EJC; CBP80-CBP20; PABP; IMPa; IMPb; RAN] Supplemental material is available at http://www.genesdev.org.

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Fluorescence Studies on Association of Human Translation Initiation Factor eIF4E with mRNA cap-Analogues

Cited by 19 publications

References 0 publications

Structural and Thermodynamic Behavior of Eukaryotic Initiation Factor 4E in Supramolecular Formation with 4E-Binding Protein 1 and mRNA Cap Analogue, Studied by Spectroscopic Methods.

Structural and Thermodynamic Behavior of Eukaryotic Initiation Factor 4E in Supramolecular Formation with 4E-Binding Protein 1 and mRNA Cap Analogue, Studied by Spectroscopic Methods.

Expression, purification and characterization of recombinant mouse translation initiation factor eIF4E as a dihydrofolate reductase (DHFR) fusion protein

Remodeling of the pioneer translation initiation complex involves translation and the karyopherin importin β

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