Molecular cloning and regulated expression of the human c-myc gene in Escherichia coli and Saccharomyces cerevisiae: comparison of the protein products.

Miyamoto, Chikako; Chizzonite, R; Crowl, Robert M.; Rupprecht, Kevin; Kramer, R. Arjen; Schaber, Michael D.; Kumar, Gaurav; Poonian, Mohindar S.; Ju, G

doi:10.1073/pnas.82.21.7232

Cited by 44 publications

(20 citation statements)

References 40 publications

(49 reference statements)

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“…Cell-free mRNA decay reaction mixtures were incubated for various times (see Materials and Methods), after which RNA was purified, electrophoresed, transferred, and hybridized to a full-length c-myc cDNA probe (60 variable lengths (see below). Poly(A) was a major source of the heterogeneity, because discrete bands were observed when the RNA was treated with oligo(dT) and RNase H before electrophoresis (lane 8, P1 and P2).…”

Section: Resultsmentioning

confidence: 99%

Poly(A) shortening and degradation of the 3' A+U-rich sequences of human c-myc mRNA in a cell-free system.

Brewer¹,

Ross²

1988

Mol. Cell. Biol.

314

243

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The early steps in the degradation of human c-myc mRNA were investigated, using a previously described cell-free mRNA decay system. The first detectable step was poly(A) shortening, which generated a pool of oligoadenylated mRNA molecules. In contrast, the poly(A) of a stable mRNA, gamma globin, was not excised, even after prolonged incubation. The second step, degradation of oligoadenylated c-myc mRNA, generated decay products whose 3' termini were located within the A+U-rich portion of the 3' untranslated region. These products disappeared soon after they were formed, consistent with rapid degradation of the 3' region. In contrast, the 5' region, corresponding approximately to c-myc exon 1, was stable in vitro. The data indicate a sequential degradation pathway in which 3' region cleavages occur only after most or all of the poly(A) is removed. To account for rapid deadenylation, we suggest that the c-myc poly(A)-poly(A)-binding protein complex is readily dissociated, generating a protein-depleted poly(A) tract that is no longer resistant to nucleases.

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Section: Resultsmentioning

confidence: 99%

Poly(A) shortening and degradation of the 3' A+U-rich sequences of human c-myc mRNA in a cell-free system.

Brewer¹,

Ross²

1988

Mol. Cell. Biol.

314

243

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“…RNase protection mapping with RNases P1 and Ti, deoxyoligonucleotidedirected RNase H cleavage assays (H mapping), and blotting of c-myc mRNA were performed as previously described (6). The c-myc probes for these assays were derived from cDNA clone pMl-ll, kindly provided by Grace Ju and colleagues (42). In some P1-plus-Ti RNase-mapping experiments, the protected fragments were electrophoresed in a polyacrylamide minigel (7 by 9 cm; Bio-Rad Laboratories, Richmond, Calif.).…”

Section: Methodsmentioning

confidence: 99%

Regulation of c-myc mRNA stability in vitro by a labile destabilizer with an essential nucleic acid component.

Brewer¹,

Ross²

1989

Mol. Cell. Biol.

156

124

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The turnover rates of some mRNAs vary by an order of magnitude or more when cells change their growth pattern or differentiate. To identify regulatory factors that might be responsible for this variability, we investigated how cytosolic fractions affect mRNA decay in an in vitro system. A 130,000 x g supernatant (S130) from the cytosol of exponentially growing erythroleukemia cells contains a destabilizer that accelerates the decay of polysome-bound c-myc mRNA by eightfold or more compared with reactions lacking S130. The destabilizer is deficient in or absent from the S130 of cycloheximide-treated cells, indicating that it is labile or is repressed when translation is blocked. It is not a generic RNase, because it does not affect the turnover of 8-globin, -y-globin, or histone mRNA and does not destabilize a major portion of polysomal polyadenylated mRNA. The destabilizer accelerates the turnover of the c-myc mRNA 3' region, as well as subsequent 3'-to-5' degradation of the mRNA body. It is inactivated in vitro by mild heating and by micrococcal nuclease, suggesting that it contains a nucleic acid component. c-myb mRNA is also destabilized in S130-supplemented in vitro reactions. These results imply that the stability of some mRNAs is regulated by cytosolic factors that are not associated with polysomes. mRNA levels can be regulated by changing not only gene transcription rates but also mRNA turnover rates, and the half-lives of some mRNAs can vary by an order of magnitude or more (reviewed in references 55, 56, and 63). Such variations apparently make up part of the normal pleiotropic respbnse to cell proliferation and differentiation factors and usually involve only a subset of mRNAs.The apparent rationale for regulating mRNA stability is to provide alternate posttranscriptional pathways for controlling the levels of subsets of mRNAs. For example, mRNAs like c-myc mRNA, whose products are thought to influence cell replication, are usually relatively unstable, with halflives of -1 h (2, 13). As a result of their intrinsic instability, even modest changes in their turnover rates affect their steady-state levels over a relatively short time. This sort of short-term regulation might ensure that the quantities of these mRNAs per cell are maintained within a very limited range. The necessity for such precise regulation is consistent with the finding that inappropriate expression of these and other mRNAs and their protein products can interfere with cell replication and differentiation (1,7,12,30,31,39,47). mRNAs whose decay rates seem to be regulated include those expressed from proto-oncogenes (13,15,20,35,41,72); genes related to cell division, including the histones (reviewed in reference 36); acute-phase response and inflammatory response genes (3, 19); interferon genes (80); heat shock protein genes (65, 71); and developmentally regulated gehes (16,62,73).Since the turnover rates of so many mRNAs vary, it is important to identify and characterize putative stabilityregulating factors. We and others have develop...

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“…In E. coli, strains deficient in EcLon were used to direct overproduction of several heterologous gene products (Buell et al 1985;Miyamoto et al 1985;Brodin et al 1986;Walker et al 1990;Alexander et al 1992;Singh et al 1992;Hutter and Singh 1998;Philibert and Martineau 2004). In some cases, the production was observed only in Eclon mutants, not in wild type strains.…”

Section: Physiological Characterization Of Ttlon Mutantsmentioning

confidence: 99%

“…Physiologically, they are known to contribute to protein quality control in the cells, as well as regulating many cellular processes, by determining the fates of short-lived proteins (Goldberg 1992;Gottesman and Maurizi 1992;Gottesman 1996;Wicker et al 1999). The Lon protease was also reported to degrade heterologous gene-products in E. coli (Buell et al 1985;Miyamoto et al 1985;Brodin et al 1986;Walker et al 1990;Alexander et al 1992;Singh et al 1992;Hutter and Singh 1998;Philibert and Martineau 2004).…”

Section: Introductionmentioning

confidence: 99%

Characterization of three putative Lon proteases of Thermus thermophilus HB27 and use of their defective mutants as hosts for production of heterologous proteins

2007

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In the genome of a thermophilic bacterium, Thermus thermophilus HB27, three genes, TTC0418, TTC0746 and TTC1975, were annotated as ATP-dependent protease La (Lon). Sequence comparisons indicated that TTC0418 and TTC0746 showed significant similarities to bacterial LonA-type proteases, such as Escherichia coli Lon protease, especially in regions corresponding to domains for ATP-binding and hydrolysis, and for proteolysis, but TTC1975 exhibited a similarity only at the C-terminal proteolytic domain. The enzymatic analyses, using purified recombinant proteins produced by E. coli, revealed that TTC0418 and TTC0746 exhibited peptidase and protease activities against two synthetic peptides and casein, respectively, in an ATP-dependent manner; and at the same time, both the enzymes had significant ATPase activities in the presence of substrates.On the other hand, TTC1975 possessed a protease activity against casein, but addition of ATP did not enhance this activity. Moreover, a T. thermophilus mutant deficient in both TTC0418 and TTC0746 showed a similar growth characteristic to an E. coli lon mutant, i.e., a long growth lag after a nutritional downshift. These results indicate that TTC0418 and TTC0746 are actually members of bacterial LonA-type proteases with different substrate specificities, whereas TTC1975should not be classified as a Lon protease. Finally, the effects of mutations deficient in these proteases were assessed on production of several heterologous gene products from Pyrococcus horikoshii and Geobacillus stearothermophilus. It was shown that TTC0746 mutation was more effective in improving production than the other two mutations, especially for production of P. horikoshii α-mannosidase and G. stearothermophilus α-amylase, indicating that the TTC0746 mutant of T. thermophilus HB27 may be useful for production of heterologous proteins from thermophiles and hyperthermophiles.

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Molecular cloning and regulated expression of the human c-myc gene in Escherichia coli and Saccharomyces cerevisiae: comparison of the protein products.

Cited by 44 publications

References 40 publications

Poly(A) shortening and degradation of the 3' A+U-rich sequences of human c-myc mRNA in a cell-free system.

Poly(A) shortening and degradation of the 3' A+U-rich sequences of human c-myc mRNA in a cell-free system.

Regulation of c-myc mRNA stability in vitro by a labile destabilizer with an essential nucleic acid component.

Characterization of three putative Lon proteases of Thermus thermophilus HB27 and use of their defective mutants as hosts for production of heterologous proteins

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