Your search keyword '"Brinster RL"' showing total 351 results

151. High expression of cloned immunoglobulin kappa gene in transgenic mice is restricted to B lymphocytes.

Author

Storb U, O'Brien RL, McMullen MD, Gollahon KA, and Brinster RL

Subjects

Animals, Bone Marrow metabolism, Lymphoid Tissue metabolism, Mice, Mice, Mutant Strains, RNA, Messenger metabolism, Spleen metabolism, Thymus Gland metabolism, Transcription, Genetic, Transcriptional Activation, B-Lymphocytes immunology, Gene Expression Regulation, Immunoglobulin Light Chains genetics, Immunoglobulin kappa-Chains genetics

Abstract

Immunoglobulin genes are normally expressed only in cells of the B lymphocyte lineage after a variable (V) and constant (C) gene rearrangement has occurred. To study the control of immunoglobulin gene expression in a defined situation, we have produced transgenic mice by microinjecting a rearranged mouse immunoglobulin kappa gene (designated pB1-14) into fertilized mouse eggs. We present here the analysis of six different kappa-transgenic mouse lines. All the transgenic mice express the microinjected kappa gene in a completely tissue-specific fashion. Transcripts from pB1-14 are found at a high level in the spleen, but are undetectable in nonlymphoid tissues of testis, liver, kidney, heart, muscle, brain and thyroid gland. In lymphoid cell subpopulations, the level of pB1-14 transcripts is correlated with the relative number of B cells; there is no correlation with the proportion of T lymphocytes. We concluded, therefore, that the microinjected kappa gene contains target sequences for B lymphocyte-specific gene activation signals that override the influence of the integration site.

Published

1984

152. Targeted correction of a major histocompatibility class II E alpha gene by DNA microinjected into mouse eggs.

Author

Brinster RL, Braun RE, Lo D, Avarbock MR, Oram F, and Palmiter RD

Subjects

Animals, Base Sequence, Female, Male, Mice, Mice, Inbred Strains, Mice, Transgenic, Microinjections, Molecular Sequence Data, Nucleic Acid Hybridization, Oligonucleotide Probes, Polymorphism, Genetic, Restriction Mapping, Chromosome Deletion, DNA genetics, Genes, MHC Class II, Mutation

Abstract

DNA molecules containing the 5' end of a functional major histocompatibility class II E alpha gene were injected into mouse eggs bearing E alpha genes with 630-base-pair (bp) deletions encompassing the promoter and first exon. The deletion was corrected by homologous recombination in 1 of about 500 transgenic mice that incorporated the injected DNA. The corrected E alpha gene was transmitted to progeny, which were bred to homozygosity. Southern blot analysis, polymerase chain reaction amplification of the DNA spanning the deletion, and sequence analysis revealed that the corrected allele resembles the wild-type E alpha gene. At sites of single-base-pair polymorphisms, there was apparently random conversion to either the donor or recipient sequence. In addition, many point mutations were introduced. mRNAs were produced from the corrected allele in a tissue-specific manner, but their sizes were different from the wild-type allele, and they did not produce detectable E alpha protein. This experiment demonstrates the feasibility of targeting foreign DNA to a gene that is completely inactive in fertilized mouse eggs.

Published

1989

153. A novel MHC class II epitope expressed in thymic medulla but not cortex.

Author

Murphy DB, Lo D, Rath S, Brinster RL, Flavell RA, Slanetz A, and Janeway CA Jr

Subjects

Animals, Antibodies, Monoclonal, B-Lymphocytes immunology, Epithelium immunology, Epitopes analysis, Gene Expression Regulation, Histocompatibility Antigens Class II genetics, Histocytochemistry, Immunoenzyme Techniques, Immunosorbent Techniques, Mice, Mice, Inbred BALB C, Mice, Transgenic, T-Lymphocytes immunology, Tissue Distribution, Histocompatibility Antigens Class II analysis, Thymus Gland immunology

Abstract

The repertoire of receptors expressed by peripheral T cells is the result of two selective events that occur during intrathymic development. Positive selection expands cells able to recognize foreign peptides presented by self MHC molecules, and negative selection eliminates cells reactive to self MHC molecules and associated self peptides. Chimaera studies suggest that, at least in the case of T cells recognizing MHC class II, interaction with thymic cortical epithelial cells is responsible for the former, whereas thymic medullary cells, of bone marrow origin, mediate the latter. This view of thymic development is supported by recent morphometric analyses, showing that autoreactive cells are found in thymic cortex but not medulla. Although numerous studies have shown that MHC class II molecules are expressed in both sites, none provides any explanation for the differential selection of T cells that is observed. Here, we describe a novel MHC class II epitope which is found on cells in thymic medulla but not cortex. The antibody to this epitope reacts with about 10% of class II molecules on B cells and may be recognizing a self peptide-MHC complex. These results provide the first evidence for differential expression of class II epitopes in different tissues and are compatible with the hypothesis that different ligands, rather than different affinity thresholds for the same ligand, are involved in positive and negative selection of the T-cell repertoire.

Published

1989

154. De novo pyrimidine nucleotide synthesis in the preimplantation mouse embryo.

Author

Troike DE and Brinster RL

Subjects

Animals, Aspartate Carbamoyltransferase antagonists & inhibitors, Aspartic Acid analogs & derivatives, Aspartic Acid pharmacology, Blastocyst drug effects, Mice, Morula drug effects, Orotic Acid pharmacology, Phosphonoacetic Acid analogs & derivatives, Phosphonoacetic Acid pharmacology, Uridine pharmacology, Blastocyst metabolism, Pyrimidine Nucleotides biosynthesis

Published

1981

155. Effects of cordycepin on macromolecular synthesis and development in the preimplantation mouse embryo.

Author

Levey IL and Brinster RL

Subjects

Animals, Deoxyadenosines metabolism, Dose-Response Relationship, Drug, Embryo, Mammalian metabolism, Mice, Poly A, RNA, Messenger biosynthesis, RNA, Ribosomal biosynthesis, Uridine metabolism, Deoxyadenosines pharmacology, Embryo, Mammalian drug effects, Protein Biosynthesis, RNA biosynthesis

Published

1977

156. Germ-line transformation of mice.

Author

Palmiter RD and Brinster RL

Subjects

Animals, DNA, Recombinant administration & dosage, Female, Gene Expression Regulation, Immunoglobulins genetics, Microinjections, Mutation, Neoplasms, Experimental genetics, Oncogenes, Organ Specificity, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Genetic Engineering, Mice genetics, Transformation, Genetic

Published

1986

157. Dramatic growth of mice that develop from eggs microinjected with metallothionein-growth hormone fusion genes.

Author

Palmiter RD, Brinster RL, Hammer RE, Trumbauer ME, Rosenfeld MG, Birnberg NC, and Evans RM

Subjects

Animals, Gene Expression Regulation, Growth Hormone blood, Liver physiology, Operon, Genetic Engineering, Growth Hormone genetics, Metalloproteins genetics, Metallothionein genetics, Mice growth & development

Abstract

A DNA fragment containing the promoter of the mouse metallothionein-I gene fused to the structural gene of rat growth hormone was microinjected into the pronuclei of fertilized mouse eggs. Of 21 mice that developed from these eggs, seven carried the fusion gene and six of these grew significantly larger than their littermates. Several of these transgenic mice had extraordinarily high levels of the fusion mRNA in their liver and growth hormone in their serum. This approach has implications for studying the biological effects of growth hormone, as a way to accelerate animal growth, as a model for gigantism, as a means of correcting genetic disease, and as a method of farming valuable gene products.

Published

1982

158. Rabbit alpha-globin messenger RNA translation by the mouse ovum.

Author

Ebert KM and Brinster RL

Subjects

Animals, Chemical Precipitation, Electrophoresis, Polyacrylamide Gel, Female, Globins genetics, Mice, Mice, Inbred Strains, Protein Biosynthesis, Rabbits, Zygote metabolism, Globins biosynthesis, RNA, Messenger metabolism, Zygote physiology

Abstract

Fertilized mouse ova were injected with messenger RNA for rabbit globin. The ova were labelled with [3H]leucine and the synthesized rabbit alpha-globin measured by immunoprecipitation. Injection of rabbit globin mRNA from 4.0 to 15.8 pg/ovum resulted in the synthesis of approximately 1200 dpm/ovum of alpha-globin during an 18 h incubation. A concentration of mRNA that was translated below the maximum level of globin synthesis was used to determine translation efficiency. The efficiency of translation was 14.1 molecules of alpha-globin synthesized/cell/h for each molecule of alpha-globin mRNA injected. The radioactivity in alpha-globin was 1% of the total incorporation in acid-precipitable material. Total incorporation of control and injected ova was not significantly different. This study shows that the fertilized mouse ovum can translate an injected foreign message with essentially the same efficiency as that reported for the Xenopus oocyte but substantially lower than the reticulocyte and that the translational capacity of the mouse fertilized ovum for injected mRNA is limited with little if any spare translational ability.

Published

1983

159. A transgenic mouse model of the chronic hepatitis B surface antigen carrier state.

Author

Chisari FV, Pinkert CA, Milich DR, Filippi P, McLachlan A, Palmiter RD, and Brinster RL

Subjects

Animals, Carrier State immunology, Hepatitis B immunology, Hepatitis B virus genetics, Humans, Liver microbiology, Mice, Mice, Inbred C57BL genetics, Nucleic Acid Hybridization, Carrier State genetics, Disease Models, Animal, Genetic Engineering, Hepatitis B genetics, Hepatitis B Surface Antigens genetics

Abstract

In an attempt to establish a model of the healthy carrier state in hepatitis B virus (HBV) infections, transgenic mice expressing HBV genes were produced. Fertilized one-cell eggs were microinjected with subgenomic fragments of HBV DNA containing the coding regions for the HBV surface antigen (HBsAg) and pre-S and X antigens. Either the normal (HBV) or metallothionein promoters were used to obtain expression of the HBV genes. There was no evidence of viral replication or tissue pathology. The integrated HBV DNA sequences were inherited in a normal Mendelian fashion. Three of 16 transgenic mice expressed HBV-encoded gene products to which they were immunologically tolerant. Expression was not tissue specific and may be influenced by the genomic integration site and cellular factors. Both HBsAg and pre-S antigen were detectable within the cytoplasm of hepatocytes and renal tubular epithelial cells. High serum concentrations of HBsAg were detectable and the secreted product appeared authentic as judged by mean density, morphology, mean particle diameter, polypeptide composition, and antigenicity. The absence of tissue pathology in these immunologically tolerant animals supports the hypothesis that cellular injury under these conditions is not a direct consequence of expression of the pre-S or HBs regions of the HBV genome.

Published

1985

160. Expression of Growth Hormone Genes in Transgenic Mice.

Author

Palmiter RD, Hammer RE, and Brinster RL

Abstract

Human or rat growth hormone (GH) genes have been introduced into all cells of a mouse by microinjection of fertilized eggs but they were not expressed under their own promoters. However, substitution of a mouse metallothionein (MT) promoter allowed expression and regulation comparable to that of the endogenous MT genes. These fusion genes have been used to stimulate the growth of both normal mice and dwarf mice that lack sufficient GH. Substitution of a rat elastase-I promoter directed expression of GH exclusively to the acinar cells of the pancreas. Progress has been made towards developing the hGH gene into a vector that is not expressed in vivo unless an enhancer element is inserted. Recombination between overlapping DNA fragments derived from a MThGH gene, each of which is nonfunctional, has been observed when they are coinjected into mouse eggs. In some cases, functional hGH was produced as evidenced by enhanced growth of the mice.

Published

1985

161. Somatic hypermutation of an immunoglobulin transgene in kappa transgenic mice.

Author

O'Brien RL, Brinster RL, and Storb U

Subjects

Animals, DNA genetics, Hybridomas immunology, Immunoglobulin G genetics, Immunoglobulin Heavy Chains genetics, Immunoglobulin M genetics, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Multiple Myeloma immunology, Phosphorylcholine immunology, Transformation, Genetic, Immunoglobulin Variable Region genetics, Immunoglobulin kappa-Chains genetics, Mutation

Abstract

Initial studies of somatically acquired mutations in immunoglobulin V regions from hybridomas and myelomas that are not derived from joining aberrations, suggested a controlled and specific hypermutation process, because spontaneous mutation rates observed for other genes are extremely low. Some evidence for the idea that mutations are introduced during V-gene rearrangement came from the clustering of mutations at the joining sites, from the absence of mutations in unrearranged V genes and from the low level of mutations in only partially (D-J) rearranged nonproductive heavy-chain alleles. Another model in which mutations accumulate with each cell division, rather than being introduced all at once, was supported by the finding that immunoglobulin genes of hybridomas derived from a single mouse frequently had several mutations in common, and so might be derived from the same precursor cell whose daughters then accumulated additional mutations. But the common mutations in some cases could be due to as yet unidentified related germline genes, or could represent the effect of antigen selection for certain amino acids. To try to detect hypermutation in the absence of V-gene rearrangement, we isolated B lymphocytes with endogenous heavy-chain gene mutations from transgenic mice carrying pre-rearranged kappa-transgenes. We found that these kappa-transgenes were also somatically mutated. This and other observations indicated that: ongoing rearrangement is not required for mutation; there are signals for hypermutation in the transgenes; the mutations are found only in the variable region, so the constant region may not be a target; different transgene insertion sites are compatible with hypermutations and more than one transgene is expressed in the same cell.

Published

1987

162. Induction of mouse metallothionein-I mRNA by bacterial endotoxin is independent of metals and glucocorticoid hormones.

Author

Durnam DM, Hoffman JS, Quaife CJ, Benditt EP, Chen HY, Brinster RL, and Palmiter RD

Subjects

Animals, Copper metabolism, Female, Kidney drug effects, Liver drug effects, Mice, Salmonella typhi, Simplexvirus enzymology, Thymidine Kinase genetics, Zinc metabolism, Cadmium pharmacology, Dexamethasone pharmacology, Kidney metabolism, Lipopolysaccharides pharmacology, Liver metabolism, Metallothionein genetics, RNA, Messenger genetics, Transcription, Genetic drug effects, Zinc pharmacology

Abstract

++Induction of metallothionein-I (MT-I) mRNA by bacterial endotoxin (LPS) was examined. A single injection of LPS induced MT-I mRNA accumulation in both liver and kidney comparable to that induced by heavy metals. Maximal message levels were achieved 6 hr after LPS administration, prior to any increase in either hepatic or renal Zn or Cu. Experiments in which LPS was administered to transgenic mice harboring recombinant genes made by fusing the MT-I gene promoter to the herpes simplex virus thymidine kinase structural gene revealed that the response to LPS is independent of glucocorticoid hormones. These experiments begin to define the region of the MT-I gene promoter required for the LPS response.

Published

1984

163. Protein degradation in the mouse blastocyst.

Author

Brinster RL, Brunner S, Joseph X, and Levey IL

Subjects

Actins metabolism, Animals, Egg Proteins analysis, Female, Half-Life, Isoelectric Point, Mice, Molecular Weight, Pregnancy, Protein Biosynthesis, Structure-Activity Relationship, Superovulation, Tubulin metabolism, Blastocyst metabolism, Proteins metabolism

Abstract

The degradation characteristics of 56 individual newly synthesized proteins of the Day 4 mouse blastocyst have been examined employing double isotope labeling of proteins for half-life measurement and two-dimensional electrophoresis for separation of proteins. The half-lives ranged from 1 to approximately 30 h with a mean of 12.4 h. Several proteins appeared to have half-lives greater than 30 h but decay times were insufficient to provide precise information for these proteins. The results suggest there is a tendency for proteins with acidic isoelectric points to be degraded more rapidly than basic proteins, and for high molecular weight proteins to be degraded more rapidly than low molecular weight proteins. Although the regressions of these two parameters on half-life were not significant, the direction and magnitude of the trends were similar to those previously described for liver proteins. Two specific proteins, tubulin and actin, were tentatively identified, and their half-lives determined. Tubulin had a half-life of 9.0 h. The half-lives of the provisionally identified gamma, beta, and alpha forms of actin were 2.2, 8.7, and 5.4 h respectively.

Published

1979

164. Changes in protein synthesis following fertilization of the mouse ovum.

Author

Chen HY, Brinster RL, and Merz EA

Subjects

Animals, Electrophoresis, Polyacrylamide Gel, Female, Mice, Ovum metabolism, Fertilization, Protein Biosynthesis, Zygote metabolism

Abstract

A quantitative method utilizing double isotope labeling with 3H-methionine and 35S-methionine and two-dimensional polyacrylamide gel electrophoresis was employed to compare synthesis of 95 individual proteins in fertilized and unfertilized mouse ova. It was found that six proteins had significantly (P less than 0.05) increased rates of synthesis while 11 proteins had significantly (P less than 0.05) decreased rates of synthesis following fertilization. The studies indicate that there are changes in the synthetic rates of a much larger number of proteins at the time of fertilization than expected from previous reports.

Published

1980

165. Embryo development.

Author

Brinster RL

Subjects

Animals, Blastocyst, Cats, Cattle, Cell Membrane Permeability, Embryo, Mammalian cytology, Embryo, Mammalian metabolism, Energy Metabolism, Female, Glucose metabolism, Glycogen metabolism, Humans, Lactates metabolism, Mice, Oxygen Consumption, Pregnancy, Protein Biosynthesis, Pyruvates metabolism, RNA biosynthesis, Rabbits, Rats, Sheep, Swine, Embryonic and Fetal Development

Published

1974

166. Promoter and enhancer elements from the rat elastase I gene function independently of each other and of heterologous enhancers.

Author

Ornitz DM, Hammer RE, Davison BL, Brinster RL, and Palmiter RD

Subjects

Animals, Genes, Immunoglobulin, Growth Hormone genetics, Kidney physiology, Liver physiology, Lymphoid Tissue physiology, Metallothionein genetics, Pancreas physiology, Rats, Recombinant Fusion Proteins genetics, Enhancer Elements, Genetic, Gene Expression Regulation, Pancreatic Elastase genetics, Promoter Regions, Genetic

Abstract

An elastase-human growth hormone (hGH) fusion gene containing 205 base pairs of elastase 5' flanking region is expressed exclusively in pancreatic acinar cells of transgenic mice. This paper shows that the promoter region (-72 to +8) and the enhancer (-205 to -73) function independently of each other. The elastase enhancer can activate the heterologous mouse metallothionein gene and the hGH gene promoters; conversely, enhancers from the thymocyte-specific murine leukemia virus MCF13 and the metal regulatory elements from the metallothionein gene can activate the elastase promoter in a variety of cell types. Combinations of immunoglobulin and elastase enhancers with a heterologous promoter and the hGH gene result in expression in all of the tissues predicted by the sum of each enhancer acting alone. Thus these enhancer elements act independently of each other, suggesting that they do not have silencing activity in cells in which they are normally inactive.

Published

1987

167. Metallothionein-human GH fusion genes stimulate growth of mice.

Author

Palmiter RD, Norstedt G, Gelinas RE, Hammer RE, and Brinster RL

Subjects

Animals, Cadmium pharmacology, DNA, Recombinant, Gene Expression Regulation drug effects, Genetic Engineering, Operon, RNA, Messenger genetics, Tissue Distribution, Transcription, Genetic, Zinc pharmacology, Growth Hormone genetics, Metallothionein genetics, Mice growth & development

Abstract

The promoter or regulatory region of the mouse gene for metallothionein-I was fused to the structural gene coding for human growth hormone. These fusion genes were introduced into mice by microinjection of fertilized eggs. Twenty-three (70 percent) of the mice that stably incorporated the fusion genes showed high concentrations of human growth hormone in their serum and grew significantly larger than control mice. Synthesis of human growth hormone was induced further by cadmium or zinc, which normally induce metallothionein gene expression. Transgenic mice that expressed human growth hormone also showed increased concentrations of insulin-like growth factor I in their serum. Histology of their pituitaries suggests dysfunction of the cells that normally synthesize growth hormone. The fusion genes were expressed in all tissues examined, but the ratio of human growth hormone messenger RNA to endogenous metallothionein-I messenger RNA varied among different tissues and different animals, suggesting that expression of the foreign genes is influenced by site of integration and tissue environment.

Published

1983

168. Transgenic mice containing growth hormone fusion genes.

Author

Brinster RL and Palmiter RD

Subjects

Animals, Female, Humans, Hybrid Cells cytology, Male, Mice, Mutation, Pedigree, Transcription, Genetic, Genes, Genes, Regulator, Growth Hormone genetics, Metallothionein genetics, Promoter Regions, Genetic

Abstract

New genes composed of the mouse metallothionein I promoter-regulator and the rat or human growth hormone structural gene have been introduced into mice. A large proportion of mice containing these genes express them, and some animals grow to be up to twice as large as controls. The technique has been used in part to correct the genetic defect that results in the small stature of the mutant little mouse.

Published

1984

169. Synthesis and secretion of ovalbumin by mouse-growing oocytes following microinjection of chick ovalbumin mRNA.

Author

Paynton BV, Ebert KM, and Brinster RL

Subjects

Animals, Chickens, Female, Mice, Microinjections, Molecular Weight, Ovalbumin biosynthesis, Oocytes metabolism, Ovalbumin genetics, Ovum metabolism, Protein Biosynthesis, RNA, Messenger genetics

Abstract

Mouse-growing oocytes were injected with chick ovalbumin mRNA. The oocytes were cultured for 18 h in the presence of [3H]leucine and the labeled ovalbumin was measured by immunoprecipitation. Two types of ovalbumin were precipitated by antibody to ovalbumin; one co-migrated with authentic, glycosylated ovalbumin in an 18% polyacrylamide gel and was estimated to be 45 000 D, whereas the other migrated faster with an apparent MW of 41 500 D. Both types of ovalbumin were also detected in the culture medium. This study demonstrates that mouse-growing oocytes can translate exogenous mRNA coding for a secreted protein and secrete two forms of the product.

Published

1983

170. Differential regulation of metallothionein-thymidine kinase fusion genes in transgenic mice and their offspring.

Author

Palmiter RD, Chen HY, and Brinster RL

Subjects

Animals, Base Sequence, Cadmium pharmacology, DNA metabolism, DNA, Recombinant, Enzyme Induction drug effects, Liver metabolism, Methylation, Mice, Mice, Inbred Strains, Pedigree, Thymidine Kinase metabolism, Gene Expression Regulation, Metalloproteins genetics, Metallothionein genetics, Thymidine Kinase genetics

Abstract

A fusion plasmid, pMK, containing the mouse metallothionein-I promoter/regulatory region joined to the structural gene of herpesvirus thymidine kinase, was introduced into mice by microinjection into fertilized eggs followed by reinsertion of the eggs into foster mothers. Fifteen percent (10 of 69) of the mice developing from this procedure carried pMK sequences. Seven of these mice expressed high levels of viral thymidine kinase in the liver. This enzyme is inducible by heavy metals, as indicated by assay of thymidine kinase activity following sequential partial hepatectomies with or without cadmium treatment. However, glucocorticoid treatment has been ineffective in all transgenic mice tested. The pMK sequences are extensively methylated at a variety of restriction sites, indicating the existence of a de novo methylation enzyme. We have analyzed the inheritance of pMK sequences and their expression in several pedigrees. These fusion genes are inherited as though they were integrated into a single chromosome; however, their expression may be extinguished, diminished or enhanced in the offspring relative to that of the parent. In some animals there is a correlation between changes in DNA methylation and expression of these fusion genes.

Published

1982

171. Growth allometry of the organs in giant transgenic mice.

Author

Shea BT, Hammer RE, and Brinster RL

Subjects

Aging, Animals, Biometry, Body Weight, Female, Heart growth & development, Kidney growth & development, Male, Mice, Organ Size, Organ Specificity, Reference Values, Species Specificity, Mice, Transgenic growth & development

Abstract

We have analyzed the absolute and relative (allometric) growth of a series of internal organs in giant transgenic (MTrGH) and littermate control mice to determine the general and organ-specific effects of the altered hormonal environment on growth in these rodents. Comparison of cross-sectional growth allometries of organ weights and external body dimensions between the two samples was based on analyses of covariance. We report significantly increased growth in all of the organs and measurements examined except for the brain. Coefficients of growth allometry differ significantly from isometric values in a number of cases, and thus, the adult transgenic mice exhibit body proportions different from those of the adult controls. Most of these shape differences reflect general allometric size increase, but the liver and spleen of the transgenics undergo special enlargement or growth. These results indicate that the primary effect of elevated GH and IGF-I levels is increased overall growth, but in the relative proportions set by the intrinsic controls of individual organs and body regions.

Published

1987

172. A 12-base-pair DNA motif that is repeated several times in metallothionein gene promoters confers metal regulation to a heterologous gene.

Author

Stuart GW, Searle PF, Chen HY, Brinster RL, and Palmiter RD

Subjects

Animals, Base Composition, Base Sequence, Cell Nucleus metabolism, Chromosome Deletion, DNA Restriction Enzymes, Female, Humans, Male, Mice, Mutation, Oocytes metabolism, Plasmids, Species Specificity, DNA genetics, Genes, Metallothionein genetics, Promoter Regions, Genetic

Abstract

To define DNA sequences involved in mouse metallothionein-I (MT-I) gene promoter function and metal regulation, we fused the 5' flanking sequences of the MT-I gene to the coding sequences of a viral thymidine kinase (TK) gene. A series of 5' deletion, 3' deletion, linker-scanning, and internal deletion mutants of the MT-I promoter was constructed and assayed by microinjection into mouse eggs. The results indicate that at least two related promoter elements can confer some metal regulation independently. Those mutations that had the most severe effect on regulation impinge on a 12-base-pair conserved sequence that is repeated several times within the mouse MT-I and other MT promoters. To test the regulatory function of this sequence, it was synthesized as a pair of complementary oligonucleotides and inserted into the promoter of the TK gene. A single insertion of this sequence conferred limited metal regulation onto the TK promoter, whereas a construct with two separate inserts was regulated as efficiently as the MT-I promoter.

Published

1984

173. Expression of creatine kinase isoenzyme during oogenesis and embryogenesis in the mouse.

Author

Iyengar MR, Iyengar CW, Chen HY, Brinster RL, Bornslaeger E, and Schultz RM

Subjects

Animals, Blastocyst enzymology, Creatine Kinase metabolism, Female, Immunodiffusion, Isoenzymes, Mice, Oocytes enzymology, Ovum enzymology, Pregnancy, Blastocyst physiology, Creatine Kinase genetics, Oogenesis

Abstract

Creatine kinase activity was discovered in the growing mouse oocyte and in the preimplantation embryo. Changes in the enzyme activity during the growth and maturation of the egg and during the development of the embryo up to the blastocyst stage were determined. Close similarity of the protein to the brain-type isoenzyme of creatine kinase was established immunochemically. The kinetic parameters of the brain-type isoenzyme (M. R. Iyengar, C. E. Fluellen, and C. W. L. Iyengar, 1982, J. Muscle Cell Motil. 3, 231-246) and the pattern of development-associated changes in activity suggest a possible role for creatine kinase in maintaining the reported high ATP/ADP ratio (L. Ginsberg and N. Hillman, 1975, J. Reprod. Fertil. 43, 83-90), which is essential for the biosynthetic activities of the embryo.

Published

1983

174. Protein metabolism in preimplanted mouse ova.

Author

Brinster RL, Wiebold JL, and Brunner S

Subjects

Animals, Blastocyst metabolism, Cell Differentiation, Female, Mice, Pregnancy, Embryonic Development, Leucine metabolism, Ovum metabolism, Pregnancy, Animal, Protein Biosynthesis

Published

1976

175. Secretion of protein by the fertilized mouse ovum.

Author

Brinster RL, Chen HY, Trumbauer ME, and Paynton BV

Subjects

Animals, Female, Globins metabolism, Mice, RNA, Messenger metabolism, Albumins metabolism, Egg Proteins metabolism, Ovalbumin metabolism, Zygote metabolism

Published

1981

176. Heart and bone tumors in transgenic mice.

Author

Behringer RR, Peschon JJ, Messing A, Gartside CL, Hauschka SD, Palmiter RD, and Brinster RL

Subjects

Animals, Bone Neoplasms pathology, Gene Expression Regulation, Heart Neoplasms pathology, Male, Mice, RNA Processing, Post-Transcriptional, RNA, Messenger genetics, Simian virus 40 genetics, Antigens, Viral, Tumor genetics, Bone Neoplasms genetics, Heart Neoplasms genetics, Mice, Transgenic genetics, Oncogenes, Protamines physiology, Spermatids physiology

Abstract

Tissue-specific tumorigenesis can be induced in transgenic mice by the directed expression of simian virus 40 (SV40) large tumor (T) antigen. In an attempt to determine the susceptibility of haploid, round spermatids to neoplastic transformation by this oncogene, transgenic mice were generated that harbored a chimeric gene composed of the SV40 T-antigen genes fused to the 5' and 3' flanking sequences of the mouse protamine 1 gene. The transgene was expressed in round spermatids and, surprisingly, in the heart and temporal bone as well. Expression in the heart resulted in rhabdomyosarcomas that always appeared in the right atrium. Bilateral osteosarcomas developed within the petrous portion of the temporal bone. No testicular pathology was observed. T-antigen immunostaining was readily detected in tumor tissue but not in the testis. In addition, SV40 transcripts were processed differently in testis and tumor tissue. Transgenic mouse lines were established that routinely develop these tumors, and they should provide a valuable resource for studies involving cardiac and bone physiology and neoplasia. The atrial tumor cells can be maintained in vitro and some continue to display a cardiac muscle phenotype.

Published

1988

177. Partial correction of murine hereditary growth disorder by germ-line incorporation of a new gene.

Author

Hammer RE, Palmiter RD, and Brinster RL

Subjects

Animals, Female, Genotype, Growth Disorders therapy, Humans, Male, Mice, Pedigree, Rats, Cloning, Molecular, Genes, Growth Disorders genetics, Growth Hormone genetics, Mutation

Abstract

The dwarf little (lit) mouse is a model for the human hereditary disorder, isolated growth hormone (GH) deficiency type I. In these animals, dwarfism results from an autosomal recessively inherited gene mutation. The GH gene is present but production of GH mRNA is deficient, resulting in reduced serum GH and concomitantly decreased serum somatomedin. Growth retardation is evident by 15 days of age and adult animals reach approximately one-half normal size. Mutant mice of both sexes also exhibit a delayed onset of puberty, with males having a high degree of infertility. As administration of GH restores growth, we reasoned that growth failure in the mutant mice might be corrected by providing them with sufficient GH by gene therapy. Here we demonstrate that although the rat and human GH genes alone do not restore growth in transgenic mutants, a metallothionein-rat growth hormone fusion gene (MT-rGH) does. Moreover, the fertility of transgenic mutant males is improved; however, female fertility is impaired.

Published

1984

178. Energy metabolism in primordial germ cells of the mouse.

Author

Brinster RL and Harstad H

Subjects

Alkaline Phosphatase metabolism, Animals, Embryo, Mammalian cytology, Germ Cells enzymology, Glucose metabolism, Isoenzymes, L-Lactate Dehydrogenase metabolism, Mice, Oxidation-Reduction, Pyruvates metabolism, Energy Metabolism, Germ Cells metabolism

Published

1977

179. SV40 T-antigen is a histocompatibility antigen of SV40-transgenic mice.

Author

Wettstein PJ, Jewett L, Faas S, Brinster RL, and Knowles BB

Subjects

Animals, Antibodies, Viral analysis, Antigens, Polyomavirus Transforming genetics, Gene Expression Regulation, Genes, Viral, Graft Rejection, Histocompatibility Antigens genetics, Mice, Mice, Inbred C57BL immunology, Mice, Transgenic genetics, Organ Specificity, Simian virus 40 genetics, Skin Transplantation, T-Lymphocytes, Cytotoxic immunology, Antigens, Polyomavirus Transforming immunology, Histocompatibility Antigens immunology, Mice, Transgenic immunology, Simian virus 40 immunology

Abstract

Although the extensive family of non-H-2 histocompatibility (H) antigens provides a formidable barrier to transplantation, the origin of their encoding genes are unknown. Recent studies have demonstrated both the linkage between H genes and retroviral sequences and the ability of integrated Moloney-murine leukemia virus to encode what is operationally defined as a non-H-2 H antigen. The experiments described in this communication reveal that skin grafts from an SV40 T-antigen transgenic C57BL/6 mouse strain are rejected by coisogenic C57BL/6 recipients with a median survival time of 49 days, which is comparable to those of many previously defined non-H-2 H antigens. The specificity of this response for SV40 T-antigen was demonstrated by the identification of SV40 T-antigen-specific cytolytic T lymphocytes and antibodies in multiply-grafted recipients. Although these cytolytic T lymphocytes could detect SV40 T-antigen on syngeneic SV40-transformed fibroblasts, they neither could be stimulated by splenic lymphocytes from T-antigen transgenics nor could they lyse lymphoblast targets from T-antigen transgenics. These observations suggest a limited tissue distribution of SV40 T-antigen in these transgenics. These results confirm the role of viral genes in the determination of non-H-2 histocompatibility antigens by the strict criteria that such antigens stimulate (1) tissue graft rejection and (2) generation of cytolytic T lymphocytes. Furthermore, they suggest that the SV40 enhancer and promoter region can target expression of SV-40 T-antigen to skin cells of transgenic animals.

Published

1988

180. Metallothionein-vasopressin fusion gene expression in transgenic mice. Nephrogenic diabetes insipidus and brain transcripts localized to magnocellular neurons.

Author

Habener JF, Cwikel BJ, Hermann H, Hammer RE, Palmiter RD, and Brinster RL

Subjects

Animals, Arginine Vasopressin blood, Arginine Vasopressin metabolism, DNA, Recombinant, Immunohistochemistry, Intestinal Mucosa metabolism, Kidney metabolism, Liver metabolism, Male, Mice, Mice, Transgenic, Neurophysins blood, Neurophysins metabolism, Nucleic Acid Hybridization, Pancreas metabolism, Protein Processing, Post-Translational, RNA, Messenger genetics, Rats, Transcription, Genetic, Arginine Vasopressin genetics, Brain metabolism, Diabetes Insipidus metabolism, Gene Expression genetics, Metallothionein genetics, Neurophysins genetics, Oxytocin, Protein Precursors genetics, Recombinant Fusion Proteins genetics

Abstract

Arginine vasopressin (AVP) is a potent neuroactive and vasoactive nonapeptide encoded in and processed from a precursor, preproarginine vasopressin-neuro-physin II (preproAVP-NPII). To study the physiologic consequences of a genetic model of chronic hypervasopressinemia transgenic mice were produced by introduction of a mouse metallothionein-rat-ppAVP-NPII fusion gene into the germ line of mice. Three stable transgenic pedigrees were analyzed through several generations. Levels of immunoreactive AVP and neurophysin (NP) in sera, livers, kidneys, intestines, pancreas, and brains were markedly elevated. Chromatographic analyses showed sera levels of approximately 500 pg/ml (normal 0-20 pg/ml) of authentic AVP non-apeptide and serum osmolalities were elevated, 315.4 +/- 1.4 mosm/liter (control, 307.3 +/- 1.1), consistent with a state of mild nephrogenic diabetes insipidus. Brain levels of immunoreactive AVP in transgenic mice were 3-4-fold elevated 145 +/- 15 ng/g versus 31 +/- 7 (controls). Although immunoreactive AVP in livers and intestines, and to some extent kidneys, consisted predominantly of unprocessed precursors, in brain and pancreas greater than 90% of AVP consisted of processed bioactive nonapeptide, as determined by chromatography and measurements of cAMP-generation in LLC-PK1 cells. Immunocytochemistry localized immunoreactive AVP to the exocrine pancreas and to the magnacellular neurons (SON and PVN) of the hypothalamus. Expression of the fusion gene in the hypothalamus was further demonstrated by Northern analyses of fusion gene specific transcripts and in situ histohybridization. Although the fusion gene contained only 35 base pairs of 5'-flanking DNA of the ppAVP-NPII gene, a tentative neuronal cell-specific expression element, -17GCCCAG-CC-10 resides in this sequence and may confer neuron-specific expression to the fusion gene.

Published

1989

181. Regulation of metallothionein--thymidine kinase fusion plasmids injected into mouse eggs.

Author

Brinster RL, Chen HY, Warren R, Sarthy A, and Palmiter RD

Subjects

Animals, Cadmium pharmacology, Chromosome Deletion, Female, Mice, Operon, Ovum physiology, Plasmids, Simplexvirus genetics, Thymidine Kinase genetics, Gene Expression Regulation drug effects, Metalloproteins genetics, Metallothionein genetics

Abstract

A plasmid was constructed with the promoter/regulatory region of the mouse metallothionein-I gene fused to the structural gene of herpesvirus thymidine kinase. When mouse eggs were microinjected with this plasmid and incubated with cadmium (a natural inducer of metallothionein gene transcription) thymidine kinase activity increased approximately 10-fold compared with control eggs not exposed to cadmium. Analysis of a set of deletion mutants revealed that the minimum sequence required for cadmium regulation lies within 90 nucleotides of the transcription start site.

Published

1982

182. The rat elastase I regulatory element is an enhancer that directs correct cell specificity and developmental onset of expression in transgenic mice.

Author

Hammer RE, Swift GH, Ornitz DM, Quaife CJ, Palmiter RD, Brinster RL, and MacDonald RJ

Subjects

Animals, Base Composition, Base Sequence, Growth Hormone genetics, Humans, Hybridization, Genetic, Mice, Mice, Inbred Strains, Nucleic Acid Hybridization, Enhancer Elements, Genetic, Genes, Genes, Regulator, Pancreatic Elastase genetics, Transcription, Genetic

Abstract

A total of 134 base pairs of the 5' flanking sequence of the elastase I gene is sufficient and necessary to direct expression of the passive human growth hormone gene (hGH) to the exocrine pancreas. We demonstrate that this elastase I regulatory region contains a transcriptional enhancer which directs acinar cell-specific expression in transgenic animals. The elastase I enhancer specifies correct expression of the linked hGH gene in an orientation- and position-independent manner and can activate a heterologous promoter. The enhancer also directs the appropriate temporal activation of the hGH gene in the developing pancreas. Transcription is initiated correctly for the elastase I or hGH promoter, and the transcripts are correctly processed regardless of the enhancer position within or outside the fusion gene. The elastase I enhancer generates coincident DNase I-hypersensitive sites in pancreatic chromatin when moved 3 kilobases upstream or within the first intron of the hGH gene and when associated with the hGH promoter.

Published

1987

183. Tolerance to class II MHC in transgenic mice.

Author

Lo D, Burkly LC, Flavell RA, Palmiter RD, and Brinster RL

Subjects

Animals, Clonal Deletion, Mice, Mice, Transgenic, Thymus Gland immunology, Genes, MHC Class II immunology, Histocompatibility Antigens Class II immunology, Self Tolerance, T-Lymphocytes immunology

Abstract

Transgenic mice offer new possibilities in experimental techniques for understanding the familiar questions of T cell development and the selection of the T cell repertoire. As a powerful method to manipulate gene expression in the whole animal, precisely defined in vivo models can be developed. In our own studies, we have used transgenic mice with targeted expression of I-E and new monoclonal antibodies defining T cell receptors specific for class II I-E molecules. In the thymus, our results suggest that thymic epithelium has significant tolerance inducing capability, but the mechanism may be different from the clonal deletion induced by bone marrow derived cells. In the periphery, our results suggest that tolerance to tissue restricted antigens is not induced by clonal deletion. Instead, clonal paralysis may be an important mechanism for both inducing and maintaining peripheral tolerance.

Published

1989

184. Transgenic mice harboring SV40 T-antigen genes develop characteristic brain tumors.

Author

Brinster RL, Chen HY, Messing A, van Dyke T, Levine AJ, and Palmiter RD

Subjects

Animals, Antigens, Polyomavirus Transforming, Base Sequence, Brain Neoplasms genetics, Crosses, Genetic, DNA Restriction Enzymes, Female, Male, Mice, Nucleic Acid Hybridization, Pedigree, Plasmids, RNA, Messenger genetics, Brain Neoplasms microbiology, Genes, Genes, Viral, Oncogenes, Simian virus 40 genetics, Viral Proteins genetics

Abstract

A high percentage of transgenic mice developing from eggs microinjected with plasmids containing the SV40 early region genes and a metallothionein fusion gene develop tumors within the choroid plexus. A line of mice has been established in which nearly every affected animal succumbs to this brain tumor. Thymic hypertrophy and kidney pathology are also observed in some mice. SV40 T-antigen mRNA and protein are readily detected in affected tissues; however, SV40 T-antigen gene expression is barely detectable in unaffected tissues or in susceptible tissues prior to overt pathology, suggesting that tumorigenesis depends upon activation of the SV40 genes. Comparison of DNA from tumor tissue (or cell lines derived from tumors) with DNA from unaffected tissues reveals structural rearrangements as well as changes in DNA methylation of the foreign DNA. The SV40 genes are frequently amplified in tumor tissue, which further indicates that their expression is intimately involved in tumorigenesis in transgenic mice.

Published

1984

185. Transgenic mice express the human phenylethanolamine N-methyltransferase gene in adrenal medulla and retina.

Author

Baetge EE, Behringer RR, Messing A, Brinster RL, and Palmiter RD

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cloning, Molecular, DNA Restriction Enzymes, Humans, Mice, Mice, Transgenic, Molecular Sequence Data, Nucleic Acid Hybridization, Adrenal Medulla enzymology, Genes, Phenylethanolamine N-Methyltransferase genetics, Retina enzymology

Abstract

The human gene for phenylethanolamine N-methyltransferase (hPNMT), responsible for the conversion of norepinephrine to epinephrine, has been cloned and the complete nucleotide sequence has been determined. The structural gene consists of three exons and two introns spanning approximately equal to 2100 base pairs. Transgenic mice containing the hPNMT gene with either 2 or 8 kilobases of 5'-flanking sequence were produced and resulted in expression of hPNMT mRNA in the adrenal gland and eye. A chimeric gene consisting of 2 kilobases of the hPNMT 5'-flanking region fused to the simian virus 40 early region also resulted in tumor (T) antigen mRNA expression in adrenal glands and eyes; furthermore, immunocytochemistry showed that tumor antigen was localized in nuclei of adrenal medullary cells and cells of the inner nuclear cell layer of the retina, prominent sites of epinephrine synthesis. These results indicate that the enhancer(s) for appropriate expression of the hPNMT gene in these cell types is in the 2-kilobase 5'-flanking region of the human gene.

Published

1988

186. Erythroid-specific expression of human beta-globin genes in transgenic mice.

Author

Townes TM, Lingrel JB, Chen HY, Brinster RL, and Palmiter RD

Subjects

Animals, Base Sequence, DNA genetics, DNA Restriction Enzymes, Humans, Mice, Mice, Inbred Strains, Microinjections, Nucleic Acid Hybridization, Protein Biosynthesis, RNA, Messenger genetics, Reticulocytes metabolism, Genes, Globins genetics, Transcription, Genetic

Abstract

Transgenic mice carrying human beta-globin genes were produced by microinjecting linear DNA molecules containing cloned beta-globin genes with up to 4300 bp of 5'-flanking sequence and 1700 bp of 3'-flanking sequence. Most (15 of 20) of these transgenic mice expressed the human beta-globin genes in blood cells and the level of expression in some mice was comparable with that obtained from endogenous beta-globin genes. Human beta-globin gene expression appeared to be restricted to cells of the erythroid lineage and was first detected between 11 and 14 days of development, in parallel with mouse beta-globin. Constructs with as little as 48 bp of 5'-flanking sequence also appeared to be expressed appropriately. The mRNA transcripts had correct 5' ends and directed human beta-globin synthesis in reticulocyte lysates. Human beta-globin protein was detectable in mature erythrocytes from progeny of one of these mice. The frequency and extent of expression was severely depressed when the procaryotic vector DNA was not removed prior to microinjection.

Published

1985

187. Expression of a metallothionein-vasopressin fusion gene in transgenic mice produces hypervasopressinemia and manifestations of nephrogenic diabetes insipidus.

Author

Habener JF, Cwikel B, Hermann H, Hammer RE, Palmiter RD, and Brinster RL

Subjects

Animals, Arginine Vasopressin blood, Blood, Male, Mice, Mice, Transgenic, Osmolar Concentration, Protein Processing, Post-Translational, Vasopressins genetics, Arginine Vasopressin genetics, DNA, Recombinant, Diabetes Insipidus genetics, Gene Expression, Metallothionein genetics, Neurophysins genetics, Oxytocin, Protein Precursors genetics, Vasopressins blood

Published

1988

188. Translation and stability of ovalbumin messenger RNA injected into growing oocytes and fertilized ova of mice.

Author

Ebert KM, Paynton BV, McKnight GS, and Brinster RL

Subjects

Animals, Cells, Cultured, Chickens, Conalbumin biosynthesis, Female, Leucine metabolism, Mice, Oocytes growth & development, RNA, Messenger genetics, Oocytes metabolism, Ovalbumin biosynthesis, Protein Biosynthesis, RNA, Messenger metabolism, Zygote metabolism

Abstract

Growing mouse oocytes and fertilized ova were injected with chicken ovalbumin messenger RNA (mRNAov) and chicken conalbumin mRNA (mRNAcon) and cultured in vitro. Estimation of mRNAov and mRNAcon stability by hybridization of cDNAov and cDNAcon to extracted mRNA from injected oocytes and fertilized ova indicated a half-life of 147 and 366 h in the oocyte and 5 and 3 h in the fertilized ovum respectively. Stability of mRNAov was similar in the fertilized and unfertilized ovum. Oocytes injected with chicken ovalbumin mRNA were also labelled with [3H]leucine and ovalbumin synthesis was measured by immunoprecipitation. The amount of ovalbumin synthesized during the initial 7 h was less than during the period of 18-25 or 66-73 h postinjection. The greatest percentage of ovalbumin to total protein synthesis occurred between 66-73 h. Oocytes secreted 12% of the synthesized ovalbumin during each of the 7 h periods (0-7, 18-25 and 66-73 h) indicating a stable mechanism for secretion throughout the culture period. These studies demonstrate: a dramatic difference in stability of injected mRNA between the growing oocyte and the unfertilized or fertilized ovum, and a gradual increase in the translation of injected mRNA by the growing oocyte during in vitro culture.

Published

1984

189. Dramatic pituitary hyperplasia in transgenic mice expressing a human growth hormone-releasing factor gene.

Author

Mayo KE, Hammer RE, Swanson LW, Brinster RL, Rosenfeld MG, and Evans RM

Subjects

Animals, Cloning, Molecular, Gene Expression Regulation drug effects, Growth Hormone-Releasing Hormone pharmacology, Hyperplasia, Mice, Pituitary Gland drug effects, Pituitary Gland growth & development, Growth Hormone-Releasing Hormone genetics, Mice, Transgenic genetics, Pituitary Gland pathology

Abstract

A transgenic animal model system was used to analyze the mitogenic effects of GRF on its target cell, the pituitary somatotroph. We have previously established a strain of mice that express a mouse metallothionein-I/human GRF (hGRF) fusion gene, and that grow to be abnormally large due to GH hypersecretion. We show here that chronic GRF production in these mice leads to the development of enormous pituitary glands. The increase in pituitary size appears to be largely the result of a selective proliferation (hyperplasia) of somatotrophs, the GH-producing cells. This observation provides direct evidence that a neuropeptide may act as a specific trophic factor for its target cell. In addition to this effect on pituitary development, we find that the pituitary is a major site of expression of mouse metallothionein-I/hGRF mRNA, and of hGRF peptide. This tissue specificity was unexpected in that neither component of the fusion gene is highly expressed in the normal pituitary. It suggests that pituitary somatotrophs might produce and respond to GRF in an essentially autocrine fashion in these transgenic animals.

Published

1988

190. Transgenic progeny inherit tissue-specific expression of rat elastase I genes.

Author

MacDonald RJ, Hammer RE, Swift GH, Davis BP, and Brinster RL

Subjects

Animals, Gene Expression Regulation, Isoelectric Point, Mice, Molecular Weight, Rats, Tissue Distribution, Transcription, Genetic, Transfection, Pancreas physiology, Pancreatic Elastase genetics

Abstract

Six different lines of transgenic mice bearing rat elastase I genes stably inherit both the high-level pancreatic expression and low-level nonpancreatic expression characteristic of each original founding mouse. The high pancreatic expression of the introduced rat genes is transcriptionally determined. In response to high rat elastase I mRNA content in the pancreas, rat elastase I protein is synthesized and secreted at high levels. The stable inheritance of expression of the foreign rat elastase I genes in transgenic mice allows the development of animal lines that synthesize and secrete high levels of foreign protein by the pancreas.

Published

1986

191. Expression of human HPRT in the central nervous system of transgenic mice.

Author

Stout JT, Chen HY, Brennand J, Caskey CT, and Brinster RL

Subjects

Animals, Brain enzymology, Cadmium pharmacology, DNA Restriction Enzymes, Female, Humans, Kidney enzymology, Liver enzymology, Lung enzymology, Mice, Myocardium enzymology, Organ Specificity, Plasmids, Pseudopregnancy, Species Specificity, Spleen enzymology, Genes drug effects, Hypoxanthine Phosphoribosyltransferase genetics

Abstract

Severe deficiency of hypoxanthine phosphoribosyltransferase (HPRT) in man results in the Lesch-Nyhan syndrome, an X-linked neurological disorder characterized by mental retardation, choreoathetosis and a compulsive tendency towards self-mutilation. Although the HPRT gene is normally constitutively expressed in all tissues at low levels, expression is elevated approximately fourfold in several regions of the central nervous system, particularly in the basal ganglia. The relationships between HPRT deficiency, tissue-specific alterations of nucleotide metabolism and the neuropathology of the Lesch-Nyhan syndrome remain unclear. Here we have microinjected recombinant molecules containing human HPRT (hHPRT) complementary DNA, the mouse metallothionein-I (MT-I) promoter and the 3'-untranslated portion of the human growth hormone (hGH) gene into mouse embryos to produce transgenic animals that express hHPRT on induction by cadmium. The hHPRT cDNA in these experiments contained 88 base pairs (bp) of 5'-untranslated and 190 bp of 3'-untranslated sequences, and the full-length coding sequence. We studied the in vivo expression of this MT-hHPRT fusion gene and observed preferential hHPRT expression in tissues of the central nervous system (CNS). This study suggests that sequences within the hHPRT transcript (cDNA) influence CNS expression via increased synthesis or stability of messenger RNA.

Published

1985

192. Pre-B cells in kappa-transgenic mice.

Author

Storb U, Denis KA, Brinster RL, and Witte ON

Subjects

Abelson murine leukemia virus, Alleles, Animals, B-Lymphocytes, Bone Marrow Cells, Cell Line, Cell Transformation, Viral, DNA analysis, Genetic Engineering, Immunoglobulin mu-Chains genetics, Mice, Phenotype, RNA, Messenger biosynthesis, Transcription, Genetic, Gene Expression Regulation, Hematopoietic Stem Cells metabolism, Immunoglobulin Light Chains genetics, Immunoglobulin kappa-Chains genetics

Abstract

Recent experiments have shown that the microinjected kappa-chain gene of transgenic mice is expressed in a tissue-specific fashion only in B lymphocytes. The next step was to determine whether, within the B-lymphocyte lineage, the kappa-chain gene was expressed in a normal developmental fashion. Normally, only mu heavy(H)-chain genes, and not kappa-chain genes, are expressed in pre-B cells. To obtain cloned cell lines derived from early cells of the B-cell lineage, we transformed bone marrow cells from kappa-transgenic mice with Abelson murine leukaemia virus (A-MuLV) and tested the resultant cell lines for the retention of the kappa transgene and its expression in RNA and protein. We found that cells with the pre-B phenotype exist in kappa-transgenic mice. We further observed that in A-MuLV-transformed cell lines from a kappa-transgenic mouse with a high copy number of the transgene, the proportion of cell lines expressing kappa (transgenic kappa) was higher than in cell lines from normal or low copy number transgenic mice.

Published

1985

193. Elevation of 1,2-diacylglycerol in ras-transformed neonatal liver and pancreas of transgenic mice.

Author

Wilkison WO, Sandgren EP, Palmiter RD, Brinster RL, and Bell RM

Subjects

Animals, Animals, Newborn, Gene Expression Regulation, Hyperplasia metabolism, Liver pathology, Mice, Mice, Transgenic, Diglycerides metabolism, Genes, ras, Glycerides metabolism, Liver metabolism, Pancreas metabolism, Transformation, Genetic

Abstract

Expression of the activated Harvey-ras (H-ras) oncogene in cultured cells is associated with an elevated steady-state concentration of 1,2-diacylglycerol (DG), an intracellular second messenger capable of promoting cell division. To explore the biochemistry of ras expression in vivo, we measured DG in ras-transformed neonatal liver and pancreas of transgenic mice. DG was elevated over 2-fold in these tissues compared to controls, but was not elevated in transgenic neonatal liver expressing normal H-ras, the nuclear oncogene myc, or the Simian Virus 40 T-antigens. DG was also not elevated in ras-induced lung adenomas in transgenic mice. These findings demonstrate an association between activated ras expression and DG concentration in neonatal tissue, but suggest that marked elevation of DG is not necessary for the development of ras-induced tumors in lung.

Published

1989

194. High plasma levels of immunoreactive somatostatin in transgenic mice expressing a metallothionein-somatostatin fusion gene.

Author

Low MJ, Goodman RH, Brinster RL, Palmiter RD, Hammer RE, and Habener JF

Subjects

Animals, Cloning, Molecular, Genes, Mice, Plasmids, Radioimmunoassay, Somatostatin genetics, Gene Expression Regulation, Metallothionein genetics, Somatostatin blood

Abstract

To test the hypothesis that processing of pre-prosomatostatin (pre-proSS) can be accomplished by cells that do not normally synthesize the precursor, we have introduced the rat pre-proSS gene under control of the mouse metallothionein promoter into the germ line of mice. Four of the 11 resultant transgenic mice had markedly elevated plasma levels of somatostatin-like immunoreactivity (SLI); however, their growth was identical to control littermates. Liver contained 263 +/- 89 pg of SLI/mg of protein and kidney had 152 +/- 19 pg/mg. Gel filtration chromatography of tissue extracts resolved one major 6000-dalton peak of SLI and three minor peaks of 8500, 3000, and 1600 daltons. The latter two corresponded in elution position to synthetic somatostatin-28 (S-28) and somatostatin-14 (S-14). Almost all of the plasma SLI corresponded in size to the 6000-dalton peptide. These findings indicate that a metallothionein-somatostatin fusion gene was successfully integrated into the mouse genome and was expressed in tissues that do not normally synthesize pre-proSS. Pre-proSS was processed to S-28 and S-14 but atypical processing to a 6000-dalton peptide also occurred.

Published

1984

195. Clonal anergy of I-E-tolerant T cells in transgenic mice with pancreatic expression of MHC class II I-E.

Author

Burkly LC, Lo D, Kanagawa O, Brinster RL, and Flavell RA

Subjects

Animals, Antibodies, Monoclonal immunology, Crosses, Genetic, Histocompatibility Antigens Class II immunology, Lymph Nodes immunology, Lymphocyte Activation, Mice, Mice, Inbred C57BL, Mice, Inbred Strains, Mice, Transgenic, Receptors, Antigen, T-Cell immunology, Genes, MHC Class II, Histocompatibility Antigens Class II genetics, Islets of Langerhans immunology, T-Lymphocytes immunology

Published

1989

196. Expression of insulin-like growth factor I in transgenic mice with elevated levels of growth hormone is correlated with growth.

Author

Mathews LS, Hammer RE, Brinster RL, and Palmiter RD

Subjects

Aging, Animals, Cloning, Molecular, Genes, Metallothionein genetics, Mice, Promoter Regions, Genetic, RNA, Messenger genetics, Reference Values, Transcription, Genetic, Growth Hormone genetics, Insulin-Like Growth Factor I genetics, Liver growth & development, Mice, Transgenic growth & development, Pituitary Gland growth & development, Somatomedins genetics

Abstract

To study the role of insulin-like growth factor I (IGF-I) in mediating the growth-promoting function of GH, IGF-I expression was assayed in transgenic mice carrying either GH or GRF fusion genes. These mice exhibit enhanced growth as a result of high level ectopic expression of GH and have 2-fold elevation of both hepatic IGF-I mRNA levels and circulating IGF-I levels. Hepatic IGF-I mRNA levels are low at birth regardless of GH levels; they increase approximately 10-fold during postnatal development and become GH inducible 2 weeks after birth. The ontogeny of circulating IGF-I is similar. Accelerated growth in transgenic mice with GH fusion genes commences 3 weeks after birth despite high circulating GH levels at least as early as birth. In addition, endogenous mouse GH-secreting somatotroph cells in the pituitary are present in normal numbers at 3 weeks, but are undetectable 4 weeks after birth. Because the time at which IGF-I expression becomes GH responsive slightly precedes both the initiation of accelerated growth and the time when endogenous GH disappears, we conclude that IGF-I is directly involved in mediating the GH signal and that delayed induction of IGF-I gene expression is responsible, at least in part, for the delayed onset of other GH-responsive events.

Published

1988

197. Expression from the transferrin gene promoter in transgenic mice.

Author

Idzerda RL, Behringer RR, Theisen M, Huggenvik JI, McKnight GS, and Brinster RL

Subjects

Animals, Base Sequence, Cloning, Molecular, Genes, Growth Hormone genetics, Liver metabolism, Mice, Mice, Transgenic, Molecular Sequence Data, Organ Specificity genetics, Restriction Mapping, Transcription, Genetic, Gene Expression Regulation, Promoter Regions, Genetic, Transferrin genetics

Abstract

Transferrin is an iron-binding protein that is expressed as a major product in liver and secreted into the plasma. To study the tissue-specific regulatory regions of this gene, the genomic mouse transferrin (mTf) gene was cloned and characterized by partial sequence analysis and S1 nuclease mapping of the transcriptional start site. Fusion genes containing the transferrin gene promoter and 5'-flanking sequences were ligated to the human growth hormone (hGH) gene and used to produce transgenic mice. A deletion construct containing the -581 to +50 region of the transferrin gene was sufficient to direct a high level of liver-specific expression resembling endogenous transferrin gene expression. Deletion to -139 base pairs of 5'-flanking sequence gave a construct which retained liver specificity, but the magnitude of expression decreased severalfold. These results demonstrate the presence of a liver-specific transcriptional element between -139 and +50 and suggest the presence of a distal element between -581 and -139 that can further increase expression. Surprisingly, fusion constructs containing -3 kilobase pairs (kb) of 5'-flanking sequence gave higher levels of mRNA in nonhepatic tissues than did either the -581 or -139 construct. Further studies indicated that the high levels of circulating hGH in these transgenic mice specifically induced the endogenous transferrin and albumin genes in liver and also stimulated the normally low levels of expression of the endogenous transferrin gene in brain, heart, kidney, and muscle. A mutated hGH gene that does not produce active growth hormone was fused to the -3- to +50-kb transferrin sequences to produce the -3-kb mTf-hGX construct. A liver-specific pattern of expression was observed in transgenic mice harboring the -3-kb mTf-hGX construct, and this mutated transgene was shown to be induced four- to sevenfold by either bovine or human growth hormone. These results demonstrate the presence of a growth hormone-responsive element between -3 and +50 kb in the 5'-flanking region of the mTf gene promoter.

Published

1989

198. Translation of globin messenger RNA by the mouse ovum.

Author

Brinster RL, Chen HY, Trumbauer ME, and Avarbock MR

Subjects

Animals, Female, Macromolecular Substances, Mice, Microinjections, Rabbits, Species Specificity, Zygote metabolism, Globins genetics, Ovum metabolism, Protein Biosynthesis, RNA, Messenger genetics

Abstract

It has been demonstrated that the Xenopus oocyte can translate rabbit haemoglobin messenger RNA (mRNA) following microinjection of the message into the cell. The Xenopus oocyte has since been shown to be capable of translating a variety of messenger RNAs from different species. This system has proved useful in un-erstanding the mechanism of message translation and has also provided information about the translation capability of the Xenopus oocyte. Several other cell types, including HeLa cells and fibroblasts, can also translate exogenous message injected into the cell. However, there have been no reports of injection of mRNA into oocytes or fertilised one-cell ova of mammalian species. Nevertheless, the latter system could be of considerable use in studying the processing of exogenous messages in a mammalian system undergoing development, as well as providing insight into the way the early embryo processes injected messages and the protein products of such messages. We report here the results of injecting message into the fertilised one-cell mouse ovum and show that both mouse and rabbit globin mRNA are translated in this system.

Published

1980

199. Ig lambda-producing B cells do not show feedback inhibition of gene rearrangement.

Author

Gollahon KA, Hagman J, Brinster RL, and Storb U

Subjects

Animals, Feedback, Fluorescent Antibody Technique, Hybridomas analysis, Hybridomas metabolism, Immunoglobulin kappa-Chains biosynthesis, Immunoglobulin kappa-Chains genetics, Immunoglobulin kappa-Chains isolation & purification, Immunoglobulin lambda-Chains genetics, Immunoglobulin lambda-Chains isolation & purification, Mice, Mice, Inbred AKR, Mice, Inbred BALB C, Mice, Transgenic, B-Lymphocytes metabolism, Gene Rearrangement, B-Lymphocyte, Light Chain, Genes, Immunoglobulin, Immunoglobulin lambda-Chains biosynthesis

Abstract

In order to study the regulation of expression of Ig lambda genes we have analyzed lambda-producing hybridomas derived from transgenic mice which harbor a functionally rearranged kappa transgene. We also analyzed lambda-producing hybridomas from nontransgenic mice. Surprisingly, all but one of the transgenic lambda-hybridomas co-produce kappa L chains. Also, in contrast to transgenic kappa-hybridomas, most lambda-hybridomas have rearranged endogenous kappa genes despite the presence of transgenic kappa-chains and endogenous H chains. Analysis of spleen cells and hybridomas from nontransgenic mice shows that about 20% of lambda-producing B cells in the spleen co-produce kappa, and a similar proportion of lambda-hybridomas from normal spleens produce both kappa- and lambda-chains. The data argue strongly against the strictly sequential expression of kappa and lambda genes. We present a new model for the regulation of kappa and lambda gene expression, whose key feature is the distinction between a kappa cell lineage in which Ig gene rearrangement is susceptible to feedback by a complete antibody molecule at the pre-B cell stage, and a kappa lambda B cell lineage which does not show feedback inhibition during B cell development.

Published

1988

200. Tissue-specific expression of the rat pancreatic elastase I gene in transgenic mice.

Author

Swift GH, Hammer RE, MacDonald RJ, and Brinster RL

Subjects

Animals, Base Composition, Base Sequence, Female, Mice, Nucleic Acid Hybridization, Organ Specificity, Ovum enzymology, Plasmids, RNA, Messenger genetics, Rats, Cloning, Molecular, Genes, Pancreas enzymology, Pancreatic Elastase genetics, Transcription, Genetic

Abstract

The gene for rat pancreatic elastase I is selectively expressed to high levels in the rat exocrine pancreas. When the cloned rat elastase I gene with 7 kb upstream and 5 kb downstream flanking sequences was introduced into mice by microinjection into fertilized eggs, the gene was expressed in a pancreas-specific manner. In four of five transgenic mice, the level of rat elastase I mRNA in the pancreas was equal to or greater than the normal rat level (10,000 mRNAs per cell) and correlated with the number of integrated gene copies. In nonpancreatic tissues the levels were at least 10(3)-fold lower, except for expression in the liver of one mouse. Thus transfer of a 23 kb genomic DNA segment containing the rat elastase I gene to a foreign chromosomal location in the mouse can give rise to qualitatively and quantitatively normal expression.

Published

1984