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151. Recombinant retroviruses that transduce individual polyoma tumor antigens: effects on growth and differentiation.

Author

Cherington, V, Morgan, B, Spiegelman, B M, and Roberts, T M

Abstract

We have constructed infectious retroviral vectors, derived from Moloney murine leukemia virus, that efficiently transduce the polyoma virus tumor (T) antigens individually. The parental vector we have chosen [pZIP-NeoSV(X)1] expresses a dominant selectable marker for neomycin resistance and is a shuttle vector capable of propagation in both eukaryotic and prokaryotic cells, thus facilitating its use in structure-function studies. To address the relationship between polyoma T-antigen tumorigenesis and the effects of individual T antigens on growth control and differentiation, we used these vectors to introduce and stably express large, middle-sized, or small T antigens into mouse fibroblasts and preadipocytes. All cDNAs introduced into the vector are expressed stably even in the absence of selective pressure. The stable expression of small T antigen is noted particularly because cell lines expressing small T antigen have not been readily available prior to the use of retroviral vectors. Small T antigen-induced increase in saturation density of NIH 3T3 cells can be scored on the basis of the morphology of drug-resistant colonies. Middle-sized T antigen eliminates the growth requirement of NIH 3T3 cells for epidermal growth factor in a defined medium and permits growth in platelet-poor plasma, indicating elimination of the platelet-derived growth factor requirement as well. Large T antigen suppresses mouse preadipocyte (3T3-F442A) differentiation. These vectors and these functional assays of T-antigen activity permit genetic analysis of the relationship between tumorigenesis by T antigens and the alteration of cellular growth and differentiation.

Published
1986
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152. Purification of biologically active simian virus 40 small tumor antigen.

Author

Bikel, I, Roberts, T M, Bladon, M T, Green, R, Amann, E, and Livingston, D M

Abstract

The simian virus 40 small tumor antigen (t antigen) gene has been cloned downstream from a hybrid Escherichia coli trp-lac promoter and a suitable ribosome binding site. A bacterial clone (865i) transformed by such a plasmid (pTR865) expresses this gene and, under optimal conditions, can produce greater than or equal to 5% of its total protein as t antigen. Soluble extracts of such a clone were relatively depleted in t antigen, which was found in the initial pellet fraction. The protein was recovered from this fraction in a significantly purified form by extraction with urea-containing buffer. After gel filtration of such t antigen-enriched solutions, highly purified protein was obtained. When either this fraction (freed of urea) or NaDodSO4 gel-purified 865i t antigen (rendered free of detergent) was injected into untransformed rat cells, dissolution of intracellular actin cable networks was observed.

Published
1983
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156. A partial genomic DNA clone for the alpha subunit of the mouse complement receptor type 3 and cellular adhesion molecule Mac-1.

Author

Sastre, L, Roman, J M, Teplow, D B, Dreyer, W J, Gee, C E, Larson, R S, Roberts, T M, and Springer, T A

Abstract

A genomic clone coding for the alpha subunit of the mouse complement receptor type 3 and the cellular adhesion molecule Mac-1 has been isolated directly from a genomic library using synthetic oligonucleotide probes based on the amino-terminal amino acid sequence of the protein. The identity of the clone has been established by DNA sequencing and in vitro translation of hybrid-selected mRNA. The gene is present in a single copy in the murine genome. The region containing the amino-terminal exon has been sequenced. RNA gel blotting shows that the Mac-1 alpha-subunit mRNA is 6 kilobases in length. Mac-1 alpha-subunit mRNA is present in macrophages but not T lymphoma or L cells. During gamma interferon-stimulated maturation of the mouse premyelocytic cell line M1, Mac-1 alpha-subunit mRNA is induced. This corresponds with the tissue distribution of the Mac-1 alpha subunit, showing expression is regulated at least partially at the message level.

Published
1986
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157. Tyrosine phosphorylations in vivo associated with v-fms transformation

Author

Morrison, D K, Browning, P J, White, M F, and Roberts, T M

Abstract

The role of tyrosine-specific phosphorylation in v-fms-mediated transformation was examined by immunoblotting techniques together with a high-affinity antibody that is specific for phosphotyrosine. This antiphosphotyrosine antibody detected phosphorylated tyrosine residues on the gp140v-fms molecule, but not gP180v-fms or gp120v-fms, in v-fms-transformed cells. This antibody also identified a number of cellular proteins that were either newly phosphorylated on tyrosine residues or showed enhanced phosphorylation on tyrosine residues as a result of v-fms transformation. However, the substrates of the v-fms-induced tyrosine kinase activity were not the characterized pp60v-src substrates. The phosphorylation of some of these cellular proteins and of the gp140fms molecule was found to correlate with the ability of v-fms/c-fms hybrids to transform cells. In addition, immunoblotting with the phosphotyrosine antibody allowed a comparison to be made of the substrates phosphorylated on tyrosine residues in various transformed cell lines. This study indicates that the pattern of tyrosine phosphorylation in v-fms-transformed cells is strikingly similar to that in v-sis-transformed cells.

Published
1988
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158. Large-scale production of polyoma middle T antigen by using genetically engineered tumors

Author

Kaplan, D R, Bockus, B, Roberts, T M, Bolen, J, Israel, M, and Schaffhausen, B S

Abstract

A recombinant plasmid containing a metallothionein promoter-polyoma middle T cDNA fusion was constructed and used to transfect NIH 3T3 cells. Transformed cells expressing middle T were injected into nude mice. Within 3 weeks, each mouse produced tumors containing middle T equivalent to that in 250 to 1,000 100-mm dishes of polyomavirus-infected cells. This middle T, partially purified by immunoaffinity chromatography, retained activity as measured by its ability to be phosphorylated in vitro. The combined approach of fusing strong promoters to genes of interest and utilizing nude mice to grow large quantities of cells expressing the gene provides a quick, inexpensive alternative to other expression systems.

Published
1985
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159. The cellular proteins which can associate specifically with polyomavirus middle T antigen in human 293 cells include the major human 70-kilodalton heat shock proteins

Author

Pallas, D C, Morgan, W, and Roberts, T M

Abstract

We compared the proteins which associate with middle T antigen (MT) of polyomavirus in human cells infected with Ad5(pymT), a recombinant adenovirus which directs the overexpression of MT, with the MT-associated proteins (MTAPs) previously identified in murine fibroblasts expressing MT. MTAPs of 27, 29, 36, and 63 kilodaltons (kDa) appeared to be fairly well conserved between the two species, as judged by comigration on two-dimensional gels. Several 61-kDa MTAP species detected in MT immunoprecipitates from both cell sources also comigrated on these gels. However, no protein comigrating precisely with the murine 85-kDa MTAP could be detected in the human cells. Furthermore, two proteins of 72 and 74 kDa associated with wild-type MT in the infected human cells but not in murine fibroblasts expressing MT. It had been previously reported for murine cells that the 70-kDa heat shock protein associates with a particular mutant MT but not with wild-type MT (G. Walter, A. Carbone, and W.J. Welch, J. Virol. 61:405-410, 1987). By the criteria of comigration on two-dimensional gels, tryptic peptide mapping, and immunoblotting, we showed that the 72- and 74-kDa proteins that associate with wild-type MT in human cells are the major human 70-kDa heat shock proteins.

Published
1989
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160. Cellular proteins that associate with the middle and small T antigens of polyomavirus

Author

Pallas, D C, Cherington, V, Morgan, W, DeAnda, J, Kaplan, D, Schaffhausen, B, and Roberts, T M

Abstract

We have used two-dimensional gel electrophoresis to analyze in more detail the cellular proteins which associate with the middle and small tumor antigens (MT and ST, respectively) of polyomavirus. Proteins with molecular masses of 27, 29, 36, 51, 61, 63, and 85 kilodaltons (kDa) that specifically coimmunoprecipitated with MT were identified on these gels. The 36-, 51-, 61-, 63-, and 85-kDa proteins are probably the same as the proteins of similar sizes previously reported by a number of groups, whereas the 27- and 29-kDa proteins represent proteins that are heretofore undescribed. The 27- and 29-kDa proteins were abundant cellular proteins, whereas the others were minor cellular constituents. The association of each of these proteins with MT was sensitive to one or more mutations in MT that rendered it transformation defective. The association of the 85-kDa protein was the most sensitive indicator of the transformation competence of MT mutants. In addition, the 85-kDa protein was the only associated protein whose association with MT changed consistently in parallel with MT-associated phosphatidylinositol kinase activity. Furthermore, the fraction of the 85-kDa protein which was found associated with the MT complex contained 15 to 20% of its phosphate content on tyrosine. The 36- and 63-kDa proteins complexed with both polyomavirus MT and ST and comigrated on two-dimensional gels with two simian virus 40 ST-associated proteins originally described by Rundell and coworkers (K. Rundell, E. O. Major, and M. Lampert, J. Virol. 37:1090-1093, 1981). None of the other MT-associated proteins associated significantly with ST.

Published
1988
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161. Recombinant retroviruses that transduce middle T antigen cDNAs derived from polyomavirus mutants: separation of focus formation and soft-agar growth in transformation assays and correlations with kinase activities in vitro

Author

Morgan, W C, Kaplan, D R, Pallas, D C, and Roberts, T M

Abstract

To study correlations between cellular transformation and the biochemical properties of polyomavirus middle T antigen, middle T cDNAs have been derived from the polyomavirus mutants dl1015, dl23, and NG59b and have been introduced into rodent fibroblast cell lines by using a retrovirus vector. It was found that all three mutants are completely defective in inducing growth in soft agar but possess a range of activities in assays of focus formation on cell monolayers. Furthermore, when assays of middle T antigen-associated kinase activities were performed in vitro, a correlation between the level of associated phosphatidylinositol kinase activity and the ability of mutant middle T antigens to induce focus formation was observed. However, the association of this activity with middle T antigen does not appear to be sufficient to bring about full transformation, since the middle T antigen derived from dl1015 is completely defective for soft-agar growth but is associated with a level of phosphatidylinositol kinase activity which is comparable to that of the wild type. Therefore, some other unidentified middle T antigen function may also be required for full transformation.

Published
1988
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162. Characterization of middle T antigen expressed by using an adenovirus expression system

Author

Schaffhausen, B S, Bockus, B J, Berkner, K L, Kaplan, D, and Roberts, T M

Abstract

The adenovirus Ad5(pymT) has been used to express middle T antigen at very high levels in 293 cells. The middle T antigen produced was localized to membranes and was modified in the same way as that expressed in polyoma virus-infected mouse cells. It was phosphorylated in vivo on serine residues and in vitro on tyrosine residues. The in vivo phosphorylations occurred between residues 223 and 275. The middle T antigen encoded by A d5(pymT) was phosphorylated in vitro in a complex with human pp60c-src. Interestingly, the extreme overexpression of middle T antigen did not cause a parallel increase in the amount of complex; most of the pp60c-src remained unassociated. Immunoaffinity purification resulted in approximately 100 micrograms of middle T antigen from a 100-mm tissue culture dish. Several cell proteins copurified with the Ad5(pymT)-derived middle T antigen. Two of these, the 74- and 63-kilodalton species, are of particular interest because they were also purified from mouse tumors expressing middle T antigen.

Published
1987
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163. Abundant expression of polyomavirus middle T antigen and dihydrofolate reductase in an adenovirus recombinant

Author

Berkner, K L, Schaffhausen, B S, Roberts, T M, and Sharp, P A

Abstract

A modular gene with a cDNA encoding the polyomavirus middle T antigen positioned behind the adenovirus type 2 major late promoter and tripartite leader was substituted for the E1a region in an adenovirus vector. Permissive human cells infected with this recombinant produce middle T protein at levels as high as those of the most abundant late adenoviral proteins, e.g., hexon or fiber. This level represents at least a 40-fold increase over that observed in a polyomavirus lytic infection of murine cells. Partial proteolytic mapping showed that this protein has the same primary structure as middle T protein produced in polyomavirus-infected murine cells. The adenovirus recombinant-generated middle T protein exhibited in vitro kinase activity, although at an approximately 10-fold-lower specific activity than that of middle T protein from polyomavirus-infected murine cells. Comparison of the expression levels of this middle T antigen-containing adenovirus vector with a similar construction encoding dihydrofolate reductase suggested that the translation efficiency of the inserted gene was dependent upon the proximity of its initiation codon to the tripartite leader. We tested this possibility by comparing three dihydrofolate reductase recombinants among which the spacing between the initiation codon and tripartite leader varied from 188 to 36 nucleotides. The efficiency of expression of dihydrofolate reductase protein dramatically increased as this spacing was reduced.

Published
1987
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164. Polyomavirus small t antigen: overproduction in bacteria, purification, and utilization for monoclonal and polyclonal antibody production

Author

Pallas, D C, Schley, C, Mahoney, M, Harlow, E, Schaffhausen, B S, and Roberts, T M

Abstract

Polyomavirus small t antigen was purified from genetically engineered Escherichia coli and used as the immunogen for the production of polyclonal and monoclonal antibodies. A new series of plasmids for increased expression of polyomavirus T antigens or a T antigen-beta-galactosidase fusion protein was constructed by replacing sequences coding for the ribosome-binding site of previously published plasmids with a chemically synthesized sequence that has a higher degree of complementarity to the 3' end of the 16S rRNA. Cells expressing the fusion protein from the plasmid with the synthetic sequence contained 5- to 10-fold more fusion protein after a 3-h induction than did control cells. Pulse-labeling of cells bearing the new plasmids revealed that the T antigens were synthesized at high levels after induction: 10% of total synthesis for small t; 15% for Py-1387T middle T, a truncated mutant of middle T; and probably 1 to 5% for middle T. Small t and Py-1387T middle T, but not wild-type middle T, were seen as minor bands in total cell protein analyzed on sodium dodecyl sulfate-polyacrylamide gels stained with Coomassie blue. A simple, rapid procedure for purification of bacterial small t from the pellet of sonicated bacteria yielded 1 to 2 mg of small t per liter of bacterial culture at 80 to 90% homogeneity. High-titer polyclonal rabbit antisera raised against purified small t recognized all three T antigens and were suitable for immunoaffinity purification of middle T. Mouse monoclonal antibodies raised against bacterial small t were of four classes, immunoprecipitating either all three polyomavirus T antigens, small t and middle T only, primarily small t, or middle T and large T in preference to small t. One of the latter monoclonal antibodies also immunoprecipitated large T but not small t of simian virus 40, suggesting that the site recognized by this antibody may be functionally important. None of the monoclonal antibodies yielded an immunoprecipitate active in phosphorylating middle T in vitro.

Published
1986
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165. Polyoma virus major capsid protein, VP1. Purification after high level expression in Escherichia coli.

Author

Leavitt, A D, Roberts, T M, and Garcea, R L

Abstract

We have expression-cloned in Escherichia coli the major polyoma virus capsid protein, VP1. Under the inducible control of the hybrid tac promoter, VP1 constituted between 2 and 3% of the total host cell protein. The expressed VP1 was purified to near homogeneity with initial yields to 10%. Optimal expression was temperature-dependent, and significant intracellular degradation could be demonstrated. The final product was obtained as one predominant isoelectric focusing species, without the pattern of post-translational modification seen in virus-infected eukaryotic cells. The purified VP1 from E. coli will be useful as a substrate for the purification of VP1 modification enzymes and in the study of inter-VP1 oligomerization.

Published
1985
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166. Monoclonal antibodies that recognize a polypeptide antigenic determinant shared by multiple Caenorhabditis elegans sperm-specific proteins.

Author

Ward, S, Roberts, T M, Strome, S, Pavalko, F M, and Hogan, E

Abstract

Four monoclonal antibodies that are directed against antigens present in sperm and absent from other worm tissues were characterized. Antibody TR20 is directed against the major sperm proteins, a family of small, abundant, cytoplasmic proteins that have been previously described (Klass, M. R., and D. Hirsh, 1981, Dev. Biol., 84:299-312; Burke, D. J., and S. Ward, 1983, J. Mol. Biol., 171:1-29). Three other antibodies, SP56, SP150, and TR11, are all directed against the same set of minor sperm polypeptides that range in size from 29 to 215 kD. More than eight different sperm polypeptides are antigenic by both immunotransfer and immunoprecipitation assays. The three antibodies are different immunoglobulin subclasses, yet they compete with each other for antigen binding so they are directed against the same antigenic determinant on the multiple sperm proteins. This antigenic determinant is sensitive to any of six different proteases, is insensitive to periodate oxidation or N-glycanase digestion, and is detectable on a polypeptide synthesized in vitro. Therefore, the antigenic determinant resides in the polypeptide chain. However, peptide fragments of the proteins are not antigenic, thus the determinant is likely to be dependent on polypeptide conformation. The antigenic determinant shared by these proteins could represent a common structural feature of importance to the localization or cellular specificity of these proteins.

Published
1986
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167. Membrane and cytoplasmic proteins are transported in the same organelle complex during nematode spermatogenesis.

Author

Roberts, T M, Pavalko, F M, and Ward, S

Abstract

During the development of pseudopodial spermatozoa of the nematode, Caenorhabditis elegans, protein synthesis stops before differentiation is completed. Colloidal gold conjugates of monoclonal antibody SP56, which binds to the surface of spermatozoa, and TR20, which recognizes the major sperm cytoplasmic protein (MSP), were used to label thin sections of testes embedded in Lowicryl K4M in order to follow polypeptides from their synthesis early in spermatogenesis to their segregation to specific compartments of the mature cell. Both antigens are synthesized in primary spermatocytes and are assembled into a unique double organelle, the fibrous body-membranous organelle (FB-MO) complex. However, the antigens are localized in different regions of this FB-MO complex. As described in detail, the assembly of proteins into the FB-MO complex allows both membrane and cytoplasmic components to be concentrated in the spermatids after meiosis. Then, the stepwise disassembly of this transient structure ensures delivery of each component to its final destination in the mature spermatozoan: MSP filaments in the fibrous body depolymerize, releasing MSP into the cytoplasm and the membranous organelles fuse with the plasma membrane, delivering SP56 antigen to the surface.

Published
1986
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168. Shear and Normal Stresses in Adhesive Joints

Author

Roberts, T. M.

Abstract

A two‐stage analytical procedure for determining the distribution of shear and normal stresses in a variety of adhesive joints, subjected to bending and axial forces, is described. The analytical procedure is based on previous assumptions that the adhesive layer is relatively flexible and can be idealized as a medium possessing only shear and normal stiffnesses, The solutions are validated by comparison with existing two‐dimensional finite element solutions for single and double lap joints. Solutions are also presented for a variety of adhesive joints subjected to axial forces and bending. The nonlinear interaction between eccentric axial forces and bending of adhesive joints is also discussed and quantified.

Published
1989

169. Lck unique domain influences Lck specificity and biological function.

Author

Carrera, A C, Paradis, H, Borlado, L R, Roberts, T M, and Martinez, C

Abstract

Src-family tyrosine kinases share structural and amino acid sequence homology, particularly in the catalytic domain as well as in the SH2 and SH3 domains of the regulatory region. However, each src-family member also contains a unique domain which is specific to and characteristic of each individual tyrosine kinase. These unique or specific domains may contribute to the functional specificity of each src-family kinase. To address this possibility, we analyzed the kinase activities and substrate specificities of the lymphoid src-kinase, pp56lck, and a mutant of pp56lck lacking its specific domain. Our data show that both the wild type enzyme and the specific domain-deleted mutant displayed similar affinities for ATP and the non-physiological substrate denatured enolase. However, the specific domain-deleted mutant failed to phosphorylate a number of physiological substrates of pp56lck. In addition, the ability of pp56lck to mediate induction of the interleukin-2 promoter was strongly impaired upon deletion of its specific domain. Thus, the unique domain is not required for the intrinsic kinase activity of pp56lck, however, it influences substrate preference and contributes to the unique physiological function of this src-family tyrosine kinase.

Published
1995

170. Direct association of Grb2 with the p85 subunit of phosphatidylinositol 3-kinase.

Author

Wang, J, Auger, K R, Jarvis, L, Shi, Y, and Roberts, T M

Abstract

Phosphatidylinositol 3-kinase (PI 3-kinase) has been shown to play a key role in growth factor signaling pathways, although its signaling mechanism has not been fully elucidated. Using the yeast interaction trap system, we have identified Grb2 as a PI 3-kinase interacting protein. Our experiments demonstrate that p85, the regulatory subunit of PI 3-kinase, interacts with Grb2 in vivo, and this interaction is independent of growth factor stimulation. The direct association between Grb2 and p85 was reconstituted in vitro with glutathione S-transferase fusion proteins. Domain analyses and peptide competition indicate that the association is mediated by the SH3 domains of Grb2 and the proline-rich motifs of p85 and that only one SH3 domain is required for minimal binding. The interaction does not displace the catalytic subunit of PI 3-kinase but is exclusive of Sos. Signaling through PI 3-kinase, therefore, may involve the ubiquitous adapter Grb2, which serves as a convergence point for multiple pathways.

Published
1995

171. Association of Polyomavirus middle tumor antigen with phospholipase C-gamma 1.

Author

Su, W, Liu, W, Schaffhausen, B S, and Roberts, T M

Abstract

Middle tumor antigen (MT) is the primary transforming protein of murine Polyomavirus. MT transforms by associating with and modulating the activities of cellular proteins involved in control of cell proliferation. MT binds to and is phosphorylated by cellular tyrosine kinases. The phosphorylated tyrosines become docking sites for SH2 (Src homology 2) domain-containing molecules. Tyrosine 322 of MT is known to be phosphorylated but has no known binding protein. We have found that phospholipase C-gamma 1 (PLC-gamma 1), a SH2 domain-containing protein, coimmunoprecipitates with MT. Tyrosine phosphorylation of PLC-gamma 1 is elevated in cells expressing MT, suggesting activation of this enzyme by MT. A Tyr-322-->Phe mutation in MT renders it defective in MT-PLC-gamma 1 interaction and in transformation. From the correlation between transformation and MT-PLC-gamma 1 interaction, we suggest that PLC-gamma 1 may play a role in transformation.

Published
1995

172. Natural Frequencies of Thin‐Walled Bars of Open Cross Section

Author

Roberts, T. M.

Abstract

The natural vibration frequencies of thin‐walled bars of open cross section are studied, with particular emphasis on the influence of asymmetry and destabilizing forces on the interaction between various modes. It is concluded that interactive vibrations are induced by both asymmetry and destabilizing forces. The validity of the solutions obtained is confirmed by the fact that the lowest natural frequencies reduce to zero when the applied forces are equal to the static critical forces for instability in the corresponding modes.

Published
1987

173. A unique cytoskeleton associated with crawling in the amoeboid sperm of the nematode, Ascaris suum.

Author

Sepsenwol, S, Ris, H, and Roberts, T M

Abstract

Nematode sperm extend pseudopods and pull themselves over substrates. They lack an axoneme or the actin and myosins of other types of motile cells, but their pseudopods contain abundant major sperm protein (MSP), a family of 14-kD polypeptides found exclusively in male gametes. Using high voltage electron microscopy, a unique cytoskeleton was discovered in the pseudopod of in vitro-activated, crawling sperm of the pig intestinal nematode Ascaris suum. It consists of 5-10-nm fuzzy fibers organized into 150-250-nm-thick fiber complexes, which connect to each of the moving pseudopodial membrane projections, villipodia, which in turn make contact with the substrate. Individual fibers in a complex splay out radially from its axis in all directions. The centripetal ends intercalate with fibers from other complexes or terminate in a thickened layer just beneath the pseudopod membrane. Monoclonal antibodies directed against MSP heavily label the fiber complexes as well as individual pseudopodial filaments throughout their length. This represents the first evidence that MSP may be the major filament protein in the Ascaris sperm cytoskeleton. The large fiber complexes can be seen clearly in the pseudopods of live, crawling sperm by computer-enhanced video, differential-interference contrast microscopy, forming with the villipodia at the leading edge of the sperm pseudopod. Even before the pseudopod attaches, the entire cytoskeleton and villipodia move continuously rearwards in unison toward the cell body. During crawling, complexes and villipodia in the pseudopod recede at the same speed as the spermatozoon moves forward, both disappearing at the pseudopod-cell body junction. Sections at this region of high membrane turnover reveal a band of densely packed smooth vesicles with round and tubular profiles, some of which are associated with the pseudopod plasma membrane. The exceptional anatomy, biochemistry, and phenomenology of Ascaris sperm locomotion permit direct study of the involvement of the cytoskeleton in amoeboid motility.

Published
1989
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174. Isolation of ras GTP-binding mutants using an in situ colony-binding assay.

Author

Feig, L A, Pan, B T, Roberts, T M, and Cooper, G M

Abstract

We have developed a strategy to isolate mutant ras genes encoding proteins defective in GTP binding. Random in vitro mutagenesis of a v-Harvey (Ha)-ras expression vector was followed by an in situ GTP-binding assay on lysed bacterial colonies. Single amino acid substitutions at ras codon 83, 119, or 144 decreased the affinity of p21 for GTP by a factor of 25-100 primarily as a consequence of increased rates of dissociation of GTP from p21. Nevertheless, these mutant genes induced transformation of NIH 3T3 cells with efficiencies comparable to wild-type v-Ha-ras. In transformed cells, mutant p21s were phosphorylated to a degree similar to that of wild-type v-Ha-ras p21, suggesting that a decrease in affinity by a factor of 100 did not prevent the mutant ras protein from binding GTP in vivo. These results are discussed with respect to the role of GTP in the regulation of p21 function.

Published
1986
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175. Synthesis of simian virus 40 t antigen in Escherichia coli.

Author

Roberts, T M, Bikel, I, Yocum, R R, Livingston, D M, and Ptashne, M

Abstract

Plasmids are constructed by using recombination in vitro according to Roberts, T.M., Kacich, R. & Ptashne, M. (1979) Proc. Natl. Acad. Sci. USA 76, 760-764 in which the t antigen gene of simian virus 40 is fused to a promoter of the Escherichia coli lac operon. In the fusions, transcription commences at the lac promoter, and, in some of the fusions, translation begins at the ATG initiator codon of the t gene. This translation is directed most efficiently by those plasmids in which the lac sequences abut the t gene such that a hybrid ribosome binding is encoded. In this case, the Shine-Dalgarno sequence is of lac origin but the ATG derives from the t gene. translation from this initiator codon is greatly decreased if the lac sequences are separated from the ATG by 17 base pairs and is abolished if the AT of this triplet is deleted. Cells bearing the productive fusions synthesize a 20,000-dalton protein with t antigenic determinants. This protein has an isoelectric point(s) indistinguishable from that of t antigen isolated from simian virus 40-transformed cells. Moreover, a partial sequence of the amino-terminal region of the bacterial product is that predicted for authentic t antigen. We conclude that these bacteria are for authentic t antigen. We conclude that these bacteria are producing a protein, the sequence of which is identical to that of authentic t antigen unfused to other polypeptides.

Published
1979
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176. Differentiation of myeloid cells is accompanied by increased levels of pp60c-src protein and kinase activity.

Author

Gee, C E, Griffin, J, Sastre, L, Miller, L J, Springer, T A, Piwnica-Worms, H, and Roberts, T M

Abstract

We have detected a significant increase in the levels of pp60c-src kinase activity associated with the differentiation of myeloid cell lines HL-60 and U-937. The induction of pp60c-src kinase activity becomes apparent approximately 14 hr after the addition of phorbol 12-myristate 13-acetate and increases 20-fold by 72 hr. The enhanced kinase activity can be accounted for by elevated levels of c-src protein in the differentiated cells. When nonleukemic bone marrow cells were examined, myeloid progenitor cells exhibited a low level of pp60c-src kinase activity. As these cells are allowed to differentiate in culture, the resulting adherent monocytes are as high in pp60c-src kinase activity as HL-60 cells induced to differentiate into monocytes. A strong correlation is found between the levels of pp60c-src kinase activity and the degree of monocytic differentiation of the cells from patients with acute myeloid leukemia. Our findings suggest that the activation of pp60c-src kinase activity is a normal physiological event associated with myeloid differentiation.

Published
1986
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177. Plants and Soils as Indicators of Metals in the Air

Author

GOODMAN, GORDON T. and ROBERTS, T. M.

Abstract

Simple techniques have been used to monitor the non-ferrous metal content of the air in South-West Wales. Metal concentrations downwind of the Swansea urban-industrial complex are found to be significantly greater than the normal background.

Published
1971
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178. Metacarpal and Finger Fractures

Author

Roberts, T. M. F.

Subjects
body regions, Features
Abstract

If loss of hand function is to be avoided, metacarpal and finger fractures must be treated early, correctly, and for sufficient time. Maintaining the hand in a correct position of function during the healing process is vital. Immobilization should be for as short a period as possible, but as complete as possible. Patients tend to remove splints, making casts more advisable. Methods of anesthesia, reduction and fixation are described for metacarpal, thumb metacarpal, proximal, middle and distal phalangeal fractures.

Published
1982

192. Book reviews

Author

Wheelock, V., primary, Wathern, P., additional, Hughes, J. A., additional, Vaughan, Michalina, additional, McNeilly, T., additional, Jolliffe, I. P., additional, Mortimer, A. M., additional, Turner, B. D., additional, Mills, G., additional, Browne, R. C., additional, Edwards, H., additional, James, G. V., additional, Davies, T. D., additional, Thomas, M. Pugh, additional, Roberts, T. M., additional, Pigott, C. D., additional, and Hughes, R., additional

Published
1978
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197. Patents and literature

Author

Long, M. E., primary, Lee, C. K., additional, Griffith, W. L., additional, Compere, A. L., additional, Holleman, J. W., additional, Simonson, L. G., additional, Lamberts, B. L., additional, Fenton, D. M., additional, Goldstein, J., additional, Dawson, E. C., additional, Roman, J. D. H., additional, Weemen, B. K. Van, additional, Matsumura, E., additional, lshikawa, H., additional, Misaki, H., additional, Griffiths, M. W., additional, Muir, D. D., additional, Phillips, J. D., additional, Gauhl, H., additional, Schawohl, G., additional, Seidel, H., additional, Beaucamp, K., additional, Johal, S., additional, Norman, B. E., additional, Terada, O., additional, Aisaka, K., additional, Teague, J. R., additional, Huebner, A. L., additional, Hershberger, D. F., additional, Sternberg, M. M., additional, Shimizu, J., additional, Suzuki, K., additional, Nakajima, Y., additional, Higgins, I. J., additional, Spence, K. D., additional, Andrews, R. E., additional, Peel, E., additional, Dalton, C. C., additional, Litchfield, J. H., additional, Lawhon, W. T., additional, Nakajima, H., additional, Nagata, K., additional, Kageyma, M., additional, Suga, T., additional, Suzuki, T., additional, Motosugi, K., additional, Sozzi, T., additional, Schrenk, A., additional, Buhler, M., additional, Rosenberg, R. A., additional, Gong, C. S., additional, Chen, L. F., additional, Tsao, G. T., additional, Kurane, R., additional, Takahara, Y., additional, Carduck, F. J., additional, Kloetzer, D., additional, Veldman, G., additional, Tolbert, W. R., additional, Hitt, M. M., additional, Feder, J., additional, Kimes, R. C., additional, Hartmeier, W., additional, Senior, P. J., additional, Wright, L. F., additional, Alderson, B., additional, Yukawa, H., additional, Nara, T., additional, Takayama, Y., additional, Hayes, F. W., additional, Weisrock, W. P., additional, Updike, M. H., additional, Calton, G. J., additional, Cox, R. G., additional, Steer, D. C., additional, Lawford, G. R., additional, Lewis, P. N., additional, Whistler, R. L., additional, Nakazawa, H., additional, Yamane, I., additional, Akutsu, E., additional, Heady, R. E., additional, Assai, Y., additional, Shimada, M., additional, Soda, K., additional, Powell, K. A., additional, Collinson, B. A., additional, Muller, W. C., additional, Miller, F. D., additional, Iizuka, H., additional, Nakamura, Y., additional, Hung, P. P., additional, Lee, S. G., additional, Ptashne, M., additional, Lauer, G. D., additional, Roberts, T. M., additional, Backman, K. C., additional, Reusser, F., additional, Manis, J. J., additional, Highlander, K., additional, Silhavy, T. J., additional, Shuman, H. A., additional, Beckwith, J., additional, Schwartz, M., additional, Sugano, H., additional, Kleid, D. G., additional, Yansura, D. G., additional, Heyneken, H. L., additional, and Miozzari, G. F., additional

Published
1983
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198. Book reviews

Author

Preining, Othmar, primary, Ormrod, D. P., additional, Golueke, Clarence G., additional, Siegel, B. Z., additional, Siegel, S. M., additional, and Roberts, T. M., additional

Published
1989
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