Expression of normal and transforming H-ras genes in Escherichia coli and purification of their encoded p21 proteins.

Lacal, Juan Carlos; Santos, Eugenio; Notario, Vicente; Barbacid, Mariano; Yamazaki, Shigeko; Kung, Hsiang‐Fu; Seamans, Craig; McAndrew, Stephen J.; Crowl, Robert M.

doi:10.1073/pnas.81.17.5305

Cited by 89 publications

(95 citation statements)

References 49 publications

(35 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…and pEV-vrf-1 containing the bacteriophage X PL promoter were propagated in Escherichia coli DH5 cells previously transformed with the low-copy-number plasmid pRK248cIts that encodes a temperature-sensitive phage X cI repressor (18,19). The construction of the TRK expression plasmids pGM1 and pGM2 is outlined in Fig.…”

Section: Methodsmentioning

confidence: 99%

Identification and biochemical characterization of p70TRK, product of the human TRK oncogene.

Mitra

Martı́n-Zanca²,

Barbacid³

1987

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

Self Cite

View full text Add to dashboard Cite

TRK is a human transforming gene generated in a colon carcinoma by a somatic rearrangement that fused a nonmuscle tropomyosin gene to sequences that shared extensive homology with members of the tyrosine-protein kinase supergene family. These sequences are likely to be derived from a transmembrane receptor gene whose putative ligand binding domain has been replaced by tropomyosin. In the present studies, we have expressed the entire coding sequences of the TRK oncogene as well as its protein kinase-related carboxylterminal domain in Escherichia coli. Antisera raised against these bacteria-synthesized TRK polypeptides has allowed us to identify the gene product of the TRK oncogene as a 70-kDa protein.Immunoprecipitates containing p70TK have an associated protein kinase activity specific for tyrosine residues. Moreover, p79TRK is phosphorylated in vivo in serine (75%), threonine (20%), and tyrosine (5%) residues. Finally, immunofluorescence and cellular fractionation studies indicate that p79TRK is preferentially located in the cytoplasmic fraction.

show abstract

Section: Methodsmentioning

confidence: 99%

Identification and biochemical characterization of p70TRK, product of the human TRK oncogene.

Mitra

Martı́n-Zanca²,

Barbacid³

1987

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

Self Cite

View full text Add to dashboard Cite

show abstract

“…Hybridizations were performed as previously described [7]. ¢t-Fetoprotein [18], albumin [19] and 18S ribosomal [20] lation, whereas v-fos [21], H-ras, [22] and HNF-4 [23] were labeled by random priming reaction. Serial hybridizations with the different probes were performed succesively.…”

Section: Rna Isolation and Northern Blot Analysismentioning

confidence: 99%

Epidermal growth factor, but not hepatocyte growth factor, suppresses the apoptosis induced by transforming growth factor‐beta in fetal hepatocytes in primary culture

et al. 1996

View full text Add to dashboard Cite

We studied whether the TGF-~-induced apoptosis in fetal hepatocyte primary cultures may be modulated by the presence of mitogenic stimuli, such as EGF or HGF. EGF prevented cell death, showing a dose dependence that was identical to that observed for its effect on DNA synthesis stimulation. HGF, in contrast, had no effect, even at high concentrations. EGF blocked apoptosis, since in the presence of this factor cells did not show DNA fragmentation. Moreover, EGF, but not HGF, blocked c-fos induction associated with the apoptotic process induced by TGF-13 in these cells.

show abstract

“…This model postulates that amino acids around position 12 are located in a loop related to the interaction of the phosphate groups of the GTP molecule, between a hydrophobic P-structure (amino acids 5-10) and an amphiphilic a-helix (amino acids [16][17][18][19][20][21][22][23][24][25][26][27][28][29]. Amino acids 59 and 61 would be located in a P-turn which comprises residues 58-61, between a fl-structure (amino acids 50-57) and an or-helix (amino acids 61 -74), possibly implicated in the interaction with Mgz+ ions [18].…”

Section: Circular Dichroic Spectra or Ras P21 Proteins In The Presencmentioning

confidence: 99%

Conformational alterations detected by circular dichroism induced in the normal ras p21 protein by activating point mutations at position 12, 59, or 61

Valencia

Serrano

Caballero

et al. 1988

European Journal of Biochemistry

View full text Add to dashboard Cite

Activation of the oncogenic potential of ras oncogenes occurs by point mutations at codons 12, 13, 59, 61, and 63 of the sequences that codify for its product, a 21-kDa protein designated as p21. This activation has been postulated by computer models as modifiers of the structure of the protein, which may alter its biochemical and biological activities. We have expressed in bacteria the normal ras p21 and five mutated p21 proteins with mutations at positions 12, 59, 61, 12 plus 59, and 12 plus 61. Purification was carried out by solubilization from bacterial pellets in 7 M urea and chromatography through a Sephadex G-100 column to obtain > 95% purified proteins. Circular dichroic (CD) spectra showed that the normal protein and that activated by substitution of Alas' to Thr5' are very similar in their overall structure. By contrast, point mutations affecting either 12 or 61 residues substantially altered the structure of the proteins. When the parameters of Chen et al. [Biochemistry 11, 4120-4131 (1972)l were applied to the CD spectra, both normal and thr5'-mutated ras proteins showed a less organized structure than mutated proteins at position 12 or 61. Since the Thr5' mutant has a more similar transforming activity than other activated proteins, but a GTPase activity similar to that of the normal protein, our results support the hypothesis that there is more than one mechanism of activation of the ras p21 protein.One of these mechanisms involves important structural alterations by point mutations at position 12 or 61 which reduce the GTPase activity of the protein. Another mechanism will be that induced by a substitution of Ala5' to Thr59 which does not substantially alter the protein conformation. A putative alternative mechanism for the activation of this mutant is discussed.The p21 product of the ras oncogene has been related to the production of tumors in man and animals [l -31. Point mutations within the coding sequence of the normal genes at positions 12,13,59,61, or 63 [4-81 alter the biological activity of the protein, inducing a transforming 21-kDa product, p21. However, it is still unknown how such point mutations, which alter the p21 sequence, can affect the normal function of the protein.The rczs p21 proteins have GDP/GTP-binding properties [9, 103, hydrolyze GTP 113-141 and when Thr is at position 59, they show a GTP-dependent, autophosphorylation activity [15]. Point mutations that affect the transforming activity of the protein at position 12, 59, or 61, do not substantially modify its ability to bind GDP or GTP or its location at the plasma membrane [16]. However, point mutations at positions 12 or 61, but not at 59, reduce the GTPase activity of the protein by 5-10-fold 111 -141.Recently, it has been suggested that a reduction of the GTPase activity of the ras p21 protein is not a good estimate of its transforming potential. Proteins with substitution of Ala5' to Thr5' show a GTPase activity comparable to the normal counterpart but are efficient transforming proteins [14]. Moreover, a reduction...

show abstract

Expression of normal and transforming H-ras genes in Escherichia coli and purification of their encoded p21 proteins.

Cited by 89 publications

References 49 publications

Identification and biochemical characterization of p70TRK, product of the human TRK oncogene.

Identification and biochemical characterization of p70TRK, product of the human TRK oncogene.

Epidermal growth factor, but not hepatocyte growth factor, suppresses the apoptosis induced by transforming growth factor‐beta in fetal hepatocytes in primary culture

Conformational alterations detected by circular dichroism induced in the normal ras p21 protein by activating point mutations at position 12, 59, or 61

Contact Info

Product

Resources

About