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53. Distinct mouse DNA sequences enable establishment and persistence of plasmid DNA polymers in mouse cells.

Author

Zastrow G, Koehler U, Müller F, Klavinius A, Wegner M, Wienberg J, Weidle UH, and Grummt F

Subjects
Animals, Base Sequence, DNA Replication, Mice, Nucleic Acid Hybridization, Restriction Mapping, DNA isolation & purification, L Cells analysis, Nucleic Acid Conformation, Plasmids
Abstract

Distinct elements isolated from mouse genomic DNA confer on plasmid DNA the ability to persist at high copy numbers in mouse L fibroblasts (1). Field inversion gel electrophoresis demonstrated that - in contrast to our previous assumption - the persisting plasmid DNA does not exist extrachromosomally but as clusters of tandem repeats integrated into genomic DNA. Digestion with restriction endonucleases that do not cut within the plasmid DNA results in fragments of 50-300 kb in length indicating reiteration of 10-50 plasmid DNA molecules. Restriction with several enzymes that cut once or twice within the plasmid sequences lead to fragment(s) indicative for head-to-tail tandem repeats. In situ hybridization revealed signals for a long homogeneously staining region (HSR) in one or two chromosomes per cell nucleus. Possibilities how these elements could act in the establishment and/or maintenance of the head-to-tail polymers of plasmid DNA in mouse cells are discussed.

Published
1989
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55. Fractionation of L-cell chromatin into DNA, RNA, and protein fractions on Cs2SO4 equilibruim density gradients.

Author

Monahan JJ and Hall RH

Subjects
Animals, Cell Nucleus analysis, Centrifugation, Density Gradient, Cesium, Chromatography, Gel, Citrates, Dimethyl Sulfoxide, Electrophoresis, Electrophoresis, Polyacrylamide Gel, Indicators and Reagents, Methods, Mice, Phosphorus Radioisotopes, Polyethylene Glycols, Polysaccharides, Tritium, Chromatin analysis, DNA isolation & purification, L Cells analysis, Nucleoproteins isolation & purification, RNA isolation & purification
Published
1974
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56. The 5'-termini of heterogeneous nuclear RNA: a comparison among molecules of different sizes and ages.

Author

Schibler U and Perry RP

Subjects
Base Sequence, L Cells analysis, Molecular Weight, Oligoribonucleotides analysis, Ribonucleotides analysis, Cell Nucleus metabolism, RNA metabolism
Abstract

The composition of the 5' polyphosphorylated and capped termini of pulse labeled hnRNA from mouse L cells was analyzed by two-dimensional electrophoresis. Purine tri- and diphosphates: pppG, pppA, ppG and ppA; as well as four varieties of cap structure: m7GpppXm, Xm = Gm, (m6) Am, Cm and Um, were detected. With increasing labeling time the relative proportion of hnRNA molecules with tri- and diphosphorylated 5' ends decreases and the relative proportion of capped hnRNA increases, indicating that caps are metabolically more stable than the polyphosphate termini. About half of the hnRNA molecules that are labeled within 2 hr have capped ends. This finding, together with results of earlier kinetic and structural studies, implies that a relatively high proportion of the labeled hnRNA molecules are mRNA precursors. Large hnRNA molecules exhibit a higher proportion of capped ends and a lower proportion of 5'-triphosphate ends as compared to small hnRNA. Given the lower stability of triphosphate termini relative to caps, this result may mean that capping of some hnRNA molecules can occur before the completion of transcription.

Published
1977
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57. Induction of a new ribonucleotide reductase after infection of mouse L cells with pseudorabies virus.

Author

Lankinen H, Gräslund A, and Thelander L

Subjects
Allosteric Regulation, Animals, Chromatography, Affinity, Electron Spin Resonance Spectroscopy, Hydroxyurea pharmacology, L Cells analysis, Mice, Neutralization Tests, Ribonucleotide Reductases metabolism, Substrate Specificity, Viral Proteins metabolism, Herpesvirus 1, Suid enzymology, Ribonucleotide Reductases isolation & purification, Viral Proteins isolation & purification
Abstract

The mammalian ribonucleotide reductase consists of two nonidentical subunits, protein M1 and M2. M1 binds nucleoside triphosphate allosteric effectors, whereas M2 contains a tyrosine free radical essential for activity. The activity of ribonucleotide reductase increased 10-fold in extracts of mouse L cells 6 h after infection with pseudorabies virus. The new activity was not influenced by antibodies against subunit M1 of calf thymus ribonucleotide reductase, whereas the reductase activity in uninfected cells was completely neutralized. Furthermore, packed infected cells (but not mock-infected cells) showed an electron paramagnetic resonance spectrum of the tyrosine free radical of subunit M2 of the cellular ribonucleotide reductase. These data given conclusive evidence that on infection, herpesvirus induces a new or modified ribonucleotide reductase. The virus-induced enzyme showed the same sensitivity to inhibition by hydroxyurea as the cellular reductase. The allosteric regulation of the virus enzyme was completely different from the regulation of the cellular reductase. Thus, CDP reduction catalyzed by the virus enzyme showed no requirement for ATP as a positive effector, and no feedback inhibition was observed by dTTP or dATP. The virus reductase did not even bind to a dATP-Sepharose column which bound the cellular enzyme with high affinity.

Published
1982
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58. HLA-JY328: mapping studies and expression of a polymorphic HLA class I gene.

Author

Duceman BW, Ness D, Rende R, Chorney MJ, Srivastava R, Greenspan DS, Pan J, Weissman SM, and Grumet FC

Subjects
Animals, Antigens, Surface analysis, B-Lymphocytes analysis, B-Lymphocytes immunology, DNA analysis, DNA genetics, DNA Restriction Enzymes, Genetic Markers, HLA-B27 Antigen, Humans, L Cells analysis, Mice, Polymorphism, Genetic, Sequence Homology, Nucleic Acid, HLA Antigens genetics, Major Histocompatibility Complex
Abstract

The JY328 clone was identified in a human genomic library using cDNA corresponding to mRNA for HLA-B7 as a probe. The L/328 cell line was established by cotransformation of mouse Ltk- cells with the herpes thymidine kinase gene and clone JY328. On Northern blots, RNA from L/328 strongly hybridized to an HLA class I probe, and an antigen was recognized by an anti-HLA class I framework antibody on the cell surface. A DNA probe corresponding to a segment of intron 7 was developed by comparing the nucleotide sequence of clone JY328 with that of other HLA class I-type genes. Using the radiolabeled probe to screen Southern blots of DNA from families with siblings exhibiting intra-HLA recombinations, a restriction fragment length polymorphism was revealed--a 1.4 kb BstE II band not present in all individuals. A corresponding fragment was apparent in the base sequence of clone JY328. The occurrence of this band on Southern blots established that JY328 maps distinct from and centromeric to the HLA-C locus and near to the HLA-B locus. Antibody absorption studies and cytotoxicity tests indicated that the JY328 gene product was not an HLA-B antigen but that it did specifically absorb CW7-specific antibody. In sum, these results suggest a novel, polymorphic HLA class I gene which expresses a product serologically similar to HLA-Cw7 but which does not map within the corresponding locus.

Published
1986
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59. Genetic engineering of an H-2Dd/Q10b chimeric histocompatibility antigen: purification of soluble protein from transformant cell supernatants.

Author

Margulies DH, Ramsey AL, Boyd LF, and McCluskey J

Subjects
Animals, Antibodies, Monoclonal immunology, Epitopes immunology, H-2 Antigens immunology, H-2 Antigens isolation & purification, Histocompatibility Antigen H-2D, L Cells analysis, Mice, Recombinant Proteins isolation & purification, Transformation, Genetic, H-2 Antigens genetics, Recombinant Proteins genetics
Abstract

We have constructed a recombinant class I gene in which 5' sequences of H-2Dd are linked to the 3' half of a Qa subregion gene, Q10b. This hybrid gene would be expected to direct the synthesis of a protein containing the N and C1 domains of H-2Dd covalently linked to the C2 domain of the secreted, nonpolymorphic, Q10b antigen. Following DNA-mediated gene transfer into mouse L cells, transformants were analyzed by radiolabeling and immunoprecipitation. These cells secreted a molecule reactive with anti-H-2Dd monoclonal antibodies that identify epitopes on the N and C1 domains as well as with an anti-Q10 carboxyl-terminal peptide antiserum. The H-2Dd-derived antigen is associated with beta 2-microglobulin and is readily purified in milligram amounts from culture supernatants by immunoaffinity chromatography.

Published
1986
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60. The polysomal proteins of L cells. Discrimination between the structural ribosomal proteins, the exchangeable ribosomal proteins and the non-ribosomal proteins by two-dimensional dodecylsulfate electrophoresis and autoradiography.

Author

Cazillis M and Houssais JF

Subjects
Dactinomycin pharmacology, Electrophoresis, Polyacrylamide Gel, L Cells metabolism, Molecular Weight, Polyribosomes drug effects, Polyribosomes metabolism, Sodium Dodecyl Sulfate, L Cells analysis, Polyribosomes analysis, Ribosomal Proteins biosynthesis, Ribosomal Proteins isolation & purification
Abstract

Three groups of proteins can be clearly discriminated in the total protein of L cell polysomes by selective labelling in the presence of low doses of actinomycin D and two-dimensional polyacrylamide/dodecylsulfate gel electrophoresis followed by autoradiography: (a) structural ribosomal proteins which are not labelled in the presence of actinomycin D and form stained non-radioactive spot in gels; (b) exchangeable ribosomal proteins which are labelled in the presence of actinomycin D and stained radioactive spots; (c) non-ribosomal proteins which are detectable only by autoradiography of gels. The large and small subunits of L cell ribosomes contain respectively 45 and 34 ribosomal proteins with molecular weights less than or equal to 50 000; seven of the large subunit proteins and nine of the small subunit proteins are exchangeable. Most of the non-ribosomal proteins migrate in the region of the related to the separation of the ribosomal proteins of mammalian cells and the possible significance of the presence of non-ribosomal proteins in polysomes are discussed.

Published
1979
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61. Mouse satellite DNA, centromere structure, and sister chromatid pairing.

Author

Lica LM, Narayanswami S, and Hamkalo BA

Subjects
Animals, Bisbenzimidazole pharmacology, Cell Line, Centromere drug effects, DNA Restriction Enzymes pharmacology, Fibroblasts drug effects, Fibroblasts ultrastructure, L Cells analysis, Mice, Mitosis drug effects, Centromere ultrastructure, Chromatids ultrastructure, Chromosomes ultrastructure, DNA, Satellite genetics, Mice, Inbred BALB C genetics
Abstract

The experiments described were directed toward understanding relationships between mouse satellite DNA, sister chromatid pairing, and centromere function. Electron microscopy of a large mouse L929 marker chromosome shows that each of its multiple constrictions is coincident with a site of sister chromatid contact and the presence of mouse satellite DNA. However, only one of these sites, the central one, possesses kinetochores. This observation suggests either that satellite DNA alone is not sufficient for kinetochore formation or that when one kinetochore forms, other potential sites are suppressed. In the second set of experiments, we show that highly extended chromosomes from Hoechst 33258-treated cells (Hilwig, I., and A. Gropp, 1973, Exp. Cell Res., 81:474-477) lack kinetochores. Kinetochores are not seen in Miller spreads of these chromosomes, and at least one kinetochore antigen is not associated with these chromosomes when they were subjected to immunofluorescent analysis using anti-kinetochore scleroderma serum. These data suggest that kinetochore formation at centromeric heterochromatin may require a higher order chromatin structure which is altered by Hoechst binding. Finally, when metaphase chromosomes are subjected to digestion by restriction enzymes that degrade the bulk of mouse satellite DNA, contact between sister chromatids appears to be disrupted. Electron microscopy of digested chromosomes shows that there is a significant loss of heterochromatin between the sister chromatids at paired sites. In addition, fluorescence microscopy using anti-kinetochore serum reveals a greater inter-kinetochore distance than in controls or chromosomes digested with enzymes that spare satellite. We conclude that the presence of mouse satellite DNA in these regions is necessary for maintenance of contact between the sister chromatids of mouse mitotic chromosomes.

Published
1986
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62. Purification and characterization of a major component from the cytoplasmic matrix of cultured murine L cells.

Author

Lanks KW and Kasambalides EJ

Subjects
Amino Acids analysis, Animals, Cyanogen Bromide, Cytoplasm analysis, Leukemia L1210 analysis, Mice, Molecular Weight, Neoplasm Proteins isolation & purification, Peptide Fragments analysis, Ultracentrifugation, L Cells analysis, Proteins isolation & purification
Abstract

This study describes the purification and preliminary characterization of a 94 000 molecular weight protein (S-94) previously known only as a major band in SDS-polyacrylamide gels of total proteins from cultured murine cells. Native S-94 is a soluble constituent of the cytoplasm and sediments at 5.0 S in sucrose gradients, behavior compatible with that of a 94 000 molecular weight monomer. S-94 is purified more than 20-fold from the 100 000 X g supernatant of murine L or L1210 lymphoma cells by DEAE-Sephadex (A-50) chromatography in the presence of 2-mercaptoethanol followed by Sephadex G-200 chromatography in 8 M urea. The protein prepared by this procedure is extensively aggregated, but is essentially homogeneous by SDS-polyacrylamide gel electrophoresis. S-94 preparations from the two types of murine cells behave identically during the purification procedure and are presumed to be the same protein. It appears that these cells contain only one major protein of 94 000 molecular weight. Purified S-94 yields a distinctive pattern of fragments following CNBr degradation, including one peptide of 36 100 molecular weight. The amino acid composition is distinguished by being relatively rich in threonine, glycine and lysine, but poor in valine, leucine and tyrosine.

Published
1979
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63. Isolation of L-cell messenger RNA which lacks poly(adenylate).

Author

Greenberg JR

Subjects
Cell Fractionation, Centrifugation, Density Gradient, Edetic Acid pharmacology, Electrophoresis, Polyacrylamide Gel, L Cells metabolism, Polyribosomes drug effects, Polyribosomes metabolism, L Cells analysis, Poly A analysis, RNA, Messenger biosynthesis
Abstract

It has been found that centrifugation of (ethylenediamine)tetraacetic acid dissociated L-cell polyribosomes at 25 degrees C through preformed CS2SO4 density gradients containing 15% dimethyl sulfoxide resolves them into two distinct classes of particles that contain ribosomal and messenger RNA, respectively. Ribosomal RNA bands at a higher density than mRNA, presumably because it is more extensively stripped of protein by the action of CS2SO4 than mRNA. Undergraded RNA can be recovered from the gradients by trapping the particles on nitrocellulose filters and then eluting at 60 degrees C with a solution containing formamide and sodium dodecyl sulfate. When cells were labeled with [3H]adenosine, either in the presence or absence of a dose of actinomycin D which selectively inhibits rRNA synthesis, and their polyribosomes centrifuged through CS2SO4 density gradients, a large amount of the radioactivity recovered from the messenger-ribonucleoprotein region of the gradient had the size distribution of mRNA, but lacked poly(adenylate) (poly (A)). This material constituted 29-31% of the total mRNA. Histone mRNA was the most prominent component of poly(A)-lacking mRNA. However, 50-65% of the poly(A)-lacking mRNA was of larger size than histone mRNA.

Published
1976
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64. Characterization of the 5' termini of hn RNA in mouse L cells: implications for processing and cap formation.

Author

Schibler U and Perry RP

Subjects
Adenine analysis, Cytosine analysis, Guanine analysis, L Cells metabolism, Models, Biological, RNA, Messenger metabolism, Uracil analysis, L Cells analysis, RNA, Neoplasm metabolism, Transcription, Genetic
Abstract

An analysis of the phosphorylated and capped 5' termini of the heterogenous nuclear RNA of mouse L cells has revealed four types of structure: pppXp..., ppXp..., pXp..., and m7/GpppXmp.... The 5'triphosphate termini consists exclusively of pppGp... and pppAp..., whereas a large proportion of the 5' monophosphate termini are pUp.... The 5'diphosphate termini contain all four species of nucleotide in relative proportions that are roughly similar to those found at the Xm position of cap structures. These results indicate that initiation of hnRNA transcription occurre exclusively with purine nucleotides, and consequently that the hnRNA molecules containing pyrimidines at the 5' termini very probably arise by cleavages at internal sites of larger primary transcripts. Taken together with previous results relating cap structures of hnRNA and mRNA, the data favor a model in which some mRNA sequences are located at transcriptionally initiated proportions and others in internal regions of their precursors. According to this model, both the mRNA segments derived from initial 5' end, and those derived by cleavage at internal sites could be converted to diphosphate-terminated derivatives, which then condense with GTP to form cap structures according to the mechanism previously described for vaccinia and reovirus mRNA.

Published
1976
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65. Hybrid recombinant human leukocyte interferon inhibits differentiation in murine B-16 melanoma cells.

Author

Fisher PB, Hermo H Jr, Prignoli DR, Weinstein IB, and Pestka S

Subjects
Animals, Cell Differentiation drug effects, Cell Line, Interferon Type I genetics, L Cells analysis, Melanins biosynthesis, Melanocyte-Stimulating Hormones pharmacology, Melanoma metabolism, Mice, Tetradecanoylphorbol Acetate pharmacology, Two-Hybrid System Techniques, DNA, Recombinant, Interferon Type I pharmacology, Melanoma pathology
Abstract

We have investigated the effects of recombinant human leukocyte interferons (IFN-alpha A and IFN-alpha D) and various hybrid recombinant human leukocyte interferons on differentiation in B-16 mouse melanoma cells. Inhibition of both spontaneous and melanocyte hormone stimulated differentiation was observed with one hybrid construct, IFN-alpha A/D (Bgl) consisting of amino acids 1 to 62 from IFN-alpha A and amino acids 64 to 166 from IFN-alpha D. In contrast, the parental human interferons, IFN-alpha A and IFN-alpha D, when used alone or in combination, as well as other hybrid human leukocyte interferons, did not cause significant inhibition of melanogenesis in B-16 mouse cells. The tumor promoter 12-O-tetradecanoylphorbol-13-acetate (TPA) also inhibited B-16 differentiation and the combination of TPA with IFN-alpha A/D (Bgl) or mouse L-cell interferon was synergistic in delaying melanogenesis. These studies indicate that the IFN-alpha A/D (Bgl) hybrid that exhibits antiviral activity on mouse cells can also inhibit differentiation of murine cells.

Published
1984
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66. Cellular deoxyribonucleotide triphosphate pools levels and DNA synthesis.

Author

Skoog KL, Bjursell KG, and Nordenskjöld BA

Subjects
Adenosine Triphosphate analogs & derivatives, Adenosine Triphosphate analysis, Animals, Cells, Cultured, Cytosine Nucleotides analysis, Guanosine Triphosphate analogs & derivatives, Guanosine Triphosphate analysis, L Cells analysis, Mice, Thymine Nucleotides analysis, DNA biosynthesis, Deoxyribonucleotides analysis
Published
1974
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67. Monoclonal antibodies to cowpox virus: polypeptide analysis of several major antigens.

Author

Kitamoto N, Tanimoto S, Hiroi K, Ozaki M, Miyamoto H, Wakamiya N, Ikuta K, Ueda S, and Kato S

Subjects
Animals, Cell Line, Cross Reactions, HeLa Cells analysis, Humans, Kidney, L Cells analysis, Mice, Peptides analysis, Rabbits, Vaccinia virus immunology, Antibodies, Monoclonal, Antigens, Viral analysis, Vaccinia virus analysis, Viral Proteins analysis
Abstract

Monoclonal antibodies directed against major antigens induced by cowpox virus (CPV) were produced. The specificities of these antibodies were established by immunoprecipitation, immunoblotting and several serological analyses, and from the cross-reactivities of these antibodies with cells infected with various other poxviruses, ectromelia virus (EV), vaccinia virus and Shope fibroma virus. The antibodies defined included ones reacting with each of the known major antigens of poxviruses, i.e. the common antigen of all poxviruses (probably NP antigen), the Orthopoxvirus-specific antigen (probably LS antigen), the haemagglutinin, the cell surface antigen, the common A-type inclusions in CPV and EV, and the antigen involved in neutralization.

Published
1987
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68. Partial primary structures of human and murine macrophage colony stimulating factor (CSF-1).

Author

Boosman A, Strickler JE, Wilson KJ, and Stanley ER

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Cells, Cultured, DNA genetics, Humans, L Cells analysis, Mice, Pancreatic Neoplasms analysis, Pancreatic Neoplasms genetics, Colony-Stimulating Factors genetics, Colony-Stimulating Factors isolation & purification
Abstract

Approximately 40 amino-terminal residues and 20 internal residues of CSF-1 purified from the media of cultured human pancreatic carcinoma (MIA PaCa) cells and of cultured murine L cells have been identified. Results indicated that the two subunits in each molecule of biologically active CSF-1 are identical in their amino-terminal portions. The twelve amino-terminal residues of MIA PaCa CSF-1 were found to be identical to those of human-urinary CSF-1, suggesting that the polypeptide portions of the two human proteins may be identical. Approximately 75% of the amino acids identified in both MIA PaCa CSF-1 and murine CSF-1 were found to be common to both. No homology to other proteins was observed. This study suggests a subunit polypeptide Mr nearer to 17K than to 26K predicted from cDNA.

Published
1987
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69. Heterogeneity of purified mouse interferons.

Author

Knight E Jr

Subjects
Animals, Chromatography, Gel, Chromatography, Ion Exchange, Drug Stability, Electrophoresis, Polyacrylamide Gel, Hydrogen-Ion Concentration, L Cells analysis, Macromolecular Substances, Mice, Molecular Weight, Interferons isolation & purification, Interferons pharmacology
Abstract

A procedure for obtaining highly purified stable interferon from mouse L cells is described. Interferon with a specific activity of 2.5 times 10-8 reference units/mg of protein is composed of 10 to 11 polypeptides. They differ in their molecular size as determined by electrophoresis on polyacrylamide gels containing sodium dodecyl sulfate. The molecular weight range is estimated to be from the smallest at 20, 000 to the largest at 32, 000. At least six of the polypeptides are glycoproteins and each of the polypeptides can be obtained as an apparent homogeneous entity and each has interferon activity.

Published
1975

70. The methylated constituents of L cell messenger RNA: evidence for an unusual cluster at the 5' terminus.

Author

Perry RP, Kelley DE, Friderici K, and Rottman F

Subjects
Adenine analogs & derivatives, Adenine analysis, Adenosine, Alkaline Phosphatase metabolism, Animals, Base Sequence, Chromatography, Ion Exchange, Methionine, Methylation, Mice, Nucleotidyltransferases metabolism, Oligonucleotides analysis, Polyribosomes analysis, Uridine, L Cells analysis, Nucleotides analysis, RNA, Messenger analysis
Abstract

An analysis of the methylated constituents of L cell mRNA by a combination of chromatographic methods and enzymatic treatments indicates that they comprise both 2'-O-methyl nucleosides and N6-methyl adenine, and/or 1-methyl adenine, and suggests that the 2'-O-methyl nucleotides, Ym, are part of an unusual class of sequences forming the 5' terminus of mRNA. These sequences seem to contain two 2'-O-methyl residues and a terminal residue that is not phosphorylated but, nevertheless, is blocked with respect to polynucleotid kinase reactivity. A strong candidate is a sequence of the type XppY1mpY2mpZp..., where X represents a blocking group which is itself occasionally methylated. The sequences isolated from total poly(A)+ mRNA contain all four species of 2'-O-methylated nucleoside, indicating some variability among different mRNA species. The methylated sequences do not appear to be enriched in the mRNA which hybridizes with repetitive DNA. The average L cell mRNA molecule also contains three residues of N6-methyl adenine. These residues are not part of the poly(A) segment, but appear to be located internal to the poly(A) near the 3' end of the mRNA molecules.

Published
1975
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71. Secondary structure maps of ribosomal RNA and DNA. I. Processing of Xenopus laevis ribosomal RNA and structure of single-stranded ribosomal DNA.

Author

Wellauer PK and Dawid IB

Subjects
Animals, Centrifugation, Density Gradient, HeLa Cells analysis, Hot Temperature, Kidney analysis, L Cells analysis, Microscopy, Electron, Nucleic Acid Conformation, Nucleic Acid Denaturation, Ribonucleotides analysis, Xenopus, DNA, Single-Stranded, RNA, Ribosomal, Ribosomes analysis
Published
1974
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72. Heterogeneity in nucleotide sequences adjacent to poly(riboadenylic acid) in L-cell messenger ribonucleic acid.

Author

Nichols JL and Eiden JJ

Subjects
Animals, Base Sequence, Cell Fractionation, Centrifugation, Density Gradient, Chromatography, Affinity, Electrophoresis, Paper, Electrophoresis, Polyacrylamide Gel, Mice, Molecular Weight, Oligonucleotides analysis, Osmolar Concentration, Pancreas enzymology, Phosphorus Radioisotopes, Ribonucleases, Ribonucleotides analysis, L Cells analysis, RNA, Messenger analysis, RNA, Messenger isolation & purification
Published
1974
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74. Analysis of gene structure and antigen determinants of DR2 antigens using DR gene transfer into mouse L cells.

Author

Kawai J, Ando A, Sato T, Nakatsuji T, Tsuji K, and Inoko H

Subjects
Absorption, Animals, Chromosome Mapping, Chromosomes, Human, Pair 6, Cloning, Molecular, Cytotoxicity Tests, Immunologic, HLA-DR Antigens analysis, HLA-DR2 Antigen, Humans, Mice, Polymorphism, Genetic, Epitopes analysis, Genes, MHC Class II, HLA-DR Antigens genetics, L Cells analysis, Transfection
Abstract

Three HLA class II DR beta genes and one DR alpha gene from the DR2 haplotype were cloned in cosmid vectors. The DR beta II gene might be a pseudogene lacking the first exon that encodes the leader peptide. The DR beta I and DR beta III genes were expressed, together with the DR alpha-chain, after transfection into mouse L cells. Restriction enzyme mapping of the DR beta genomic clones and reactivity of their products expressed on the L cell transfectant against mAb showed that the DR beta I and DR beta III genes encoded the nonpolymorphic and polymorphic DR beta chain, respectively. This arrangement is the reverse of that observed in other haplotypes, such as DR3, 4 and 6. The alignment of the HLA class II genes including the DR beta genes on the chromosome 6, however, was consistent with other haplotypes, e.g., centromere-DX beta-DX alpha-DV beta-DQ beta-DQ alpha-DR beta I-DR beta II- DR beta III-DR alpha-telomere. These results suggest that the susceptibility to mutations or gene conversions responsible for genetic polymorphisms depends on the gene itself and not on its location. Furthermore, absorption experiments of anti-DR2 allosera by the DR alpha/DR beta transfectants revealed that the so-called DR2 specificities were determined by multiple epitopes although both the DR beta I and DR beta III genes behaved similarly with DR2-specific antibodies.

Published
1989

75. Analysis of D2d: a D-region class I gene.

Author

Hedley ML, Hunt SW 3rd, Brorson KA, Andris JS, Hood L, Forman J, and Tucker PW

Subjects
Amino Acid Sequence, Animals, Base Sequence, Biological Evolution, Cytoplasm analysis, H-2 Antigens isolation & purification, L Cells analysis, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Promoter Regions, Genetic, Genes, MHC Class I, H-2 Antigens genetics
Abstract

The mouse major histocompatibility complex is composed of several genes arranged into the K, D, Qa, and Tla regions. The D region of the BALB/c mouse includes genes D2d, D3d, and D4d, in addition to H-2Dd and H-2Ld. We have determined the DNA sequence of the D2d gene and compared it with the known sequences of several class I genes. The exon/intron structure of the D2d gene is similar to other class I genes. It also contains similar 5' regulatory elements. A frameshift occurs in exon seven, resulting in a gene product with a truncated cytoplasmic tail. To examine the surface expression of the D2d molecule, we generated an exon-shuffled construct containing the promoter and exons 1-3, encoding the signal peptide, alpha 1, and alpha 2 external domains of the D2d gene linked to exons 4-8, encoding the alpha 3, transmembrane and cytoplasmic domains, of the H-2Dd gene. The construct was transfected into mouse L cells, and a protein was detected at the cell surface by a monoclonal antibody (mAb) specific for the alpha 3 domain of H-2Dd, as well as by other class I-specific mAbs. Although D2d is expressed at low levels, it may be a functional class I gene that most probably evolved from a Qa region gene.

Published
1989
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76. The ribosomal proteins of L cells. A comparative analysis of the ribosomal proteins split off by KCl, the core proteins, the proteins transferable between the two subunits and the proteins labelled in absence of ribosomal synthesis.

Author

Cazillis M and Houssais JF

Subjects
Animals, Edetic Acid, Electrophoresis, Polyacrylamide Gel, L Cells analysis, L Cells metabolism, Macromolecular Substances, Mice, Molecular Weight, Peptides analysis, Potassium Chloride, Puromycin, Ribosomal Proteins biosynthesis, Ribosomal Proteins analysis
Published
1981
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77. DNA-mediated transfer of complex I genes into three different respiration-deficient Chinese hamster mutant cell lines with defects in complex I of electron transport chain.

Author

Garnett KE, Simmons WA, Wing MS, and Breen GA

Subjects
Animals, Antimycin A analogs & derivatives, Antimycin A pharmacology, Carbohydrate Metabolism, Cell Line, Citric Acid Cycle, Cricetinae, Cricetulus, DNA genetics, Fibroblasts metabolism, HeLa Cells analysis, Humans, L Cells analysis, Mitochondria metabolism, Mutation, NAD(P)H Dehydrogenase (Quinone), Oxidative Phosphorylation drug effects, Oxygen Consumption, Rotenone pharmacology, NADH, NADPH Oxidoreductases genetics, Quinone Reductases genetics, Transformation, Genetic
Abstract

We have used genomic DNA from human or mouse cells as a calcium phosphate precipitate to transfect three different respiration-deficient Chinese hamster mutant cell lines with defects in complex I of the electron transport chain. Transformants were selected in DMEM containing galactose, a medium in which respiration-deficient cells do not grow. Evidence for the DNA-mediated transformation of these respiration-deficient cells with a putative complex I gene includes: the clones are respiration-positive and respire at rates comparable to those of wild-type human, hamster, or mouse cells; the clones have rotenone-sensitive NADH oxidase activities, indicating a functional complex I of the electron transport chain; and the clones appear to be true transformants, as demonstrated by hybridization and Southern blot analyses. These experiments provide the basis for the isolation and subsequent characterization of several of the genes involved with complex I of the mammalian electron transport chain.

Published
1985
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78. Long pyrimidine tracts of L-cell DNA: localization to repeated DNA.

Author

Straus NA and Birnboim HC

Subjects
Animals, Base Sequence, Chromatography, DNA, Neoplasm metabolism, Electrophoresis, Polyacrylamide Gel, Female, HeLa Cells analysis, Humans, Hydroxyapatites, Mice, Nucleic Acid Denaturation, Nucleic Acid Renaturation, Oligonucleotides isolation & purification, Thymidine metabolism, Tritium, DNA, Neoplasm analysis, L Cells analysis, Polynucleotides analysis, Pyrimidine Nucleotides analysis
Abstract

Like HeLa DNA, L-cell DNA contains a significant number of unexpectedly long pyrimidine tracts. 1.3% of the thymidine residues of L-cell DNA are found in these long polypyrimidine tracts. Analysis of L-cell DNA fractions with different rates of reassociation indicates that polypyrimidine tracts are associated with "repeated" DNA. Longer pyrimidine tracts appear to have a higher repetition frequency than shorter tracts, and some may be repeated as many as 5 x 10(4) times in L-cell DNA.

Published
1974
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79. Rapid size determination of mRNAs complementary to cloned DNA sequences: plaque and colony hybrid-selection of cDNAs.

Author

Shaw PH, Carneiro M, and Schibler U

Subjects
Animals, Base Sequence, Cloning, Molecular, Genetic Vectors, L Cells analysis, Liver analysis, Mice, Mice, Inbred A, Molecular Weight, Nucleic Acid Hybridization, Parotid Gland analysis, Plasmids, RNA, Messenger genetics, RNA-Directed DNA Polymerase metabolism, DNA metabolism, RNA, Messenger isolation & purification
Abstract

We describe a novel screening method for the rapid size determination of mRNAs. This method has been used successfully to identify the cDNA and genomic DNA clones that had been constructed using the plasmid vector pBR322 or phage vectors M13mp7 and lambda EMBL3. Poly(A) RNA is reverse-transcribed into 32P-labeled cDNA under conditions that yield a high proportion of full-length cDNA copies. This radioactive cDNA is then hybridized in situ to bacterial colonies or phage plaques harboring recombinant DNA molecules. Colonies or plaques containing sequences complementary to abundant or moderately abundant mRNAs are detected by autoradiography and excised from nitrocellulose filters. The hybridized cDNA is eluted from the filter by alkaline denaturation and sized directly by alkaline agarose gel electrophoresis. The mRNAs characterized thus far by this technique measure between 450 and 2100 nucleotides and account for 0.03% to 15% of the mass of cytoplasmic poly(A) RNA.

Published
1984
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80. Stable transfer and restricted expression of a cloned class I gene encoding a secreted transplantation-like antigen.

Author

Barra Y, Tanaka K, Isselbacher KJ, Khoury G, and Jay G

Subjects
Animals, Cell Line, Cloning, Molecular, DNA, Recombinant isolation & purification, Enhancer Elements, Genetic, Epithelium, Gene Expression Regulation, Humans, L Cells analysis, Liver immunology, Liver Neoplasms, Experimental, Mice, Organ Specificity, Transfection, Antigens genetics, Mice, Inbred BALB C genetics, Mice, Inbred C57BL genetics
Abstract

The identification of a unique major histocompatibility complex class I gene, designated Q10, which encodes a secreted rather than a cell surface antigen has led to questions regarding its potential role in regulating immunological functions. Since the Q10 gene is specifically activated only in the liver, we sought to define the molecular mechanisms which control its expression in a tissue-specific fashion. Results obtained by transfection of the cloned Q10 gene, either in the absence or presence of a heterologous transcriptional enhancer, into a variety of cell types of different tissue derivations are consistent with the Q10 gene being regulated at two levels. The first is by a cis-dependent mechanism which appears to involve site-specific DNA methylation. The second is by a trans-acting mechanism which would include the possibility of an enhancer binding factor. The ability to efficiently express the Q10 gene in certain transfected cell lines offers an opportunity to obtain this secreted class I antigen in quantities sufficient for functional studies; this should also make it possible to define regulatory sequences which may be responsible for the tissue-specific expression of Q10.

Published
1985
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81. Bone marrow differentiation in vitro.

Author

Schrader JW

Subjects
20-Hydroxysteroid Dehydrogenases metabolism, Animals, Antigens, Ly genetics, Antigens, Ly immunology, Antigens, Surface genetics, Antigens, Surface immunology, B-Lymphocytes cytology, B-Lymphocytes immunology, Blood Physiological Phenomena, Bone Marrow anatomy & histology, Bone Marrow immunology, Cell Differentiation, Cell Line, Cell Transformation, Viral, Colony-Stimulating Factors biosynthesis, Colony-Stimulating Factors immunology, Colony-Stimulating Factors physiology, Culture Media, Cytotoxicity, Immunologic, DNA Nucleotidylexotransferase metabolism, Hematopoietic Stem Cells classification, Histocompatibility Antigens classification, Histocompatibility Antigens Class II immunology, Immunoglobulin mu-Chains genetics, Interferon-gamma physiology, Interleukin-3, Killer Cells, Natural cytology, Killer Cells, Natural immunology, L Cells analysis, Langerhans Cells cytology, Lung analysis, Lymphocyte Activation, Lymphocytes, Null cytology, Lymphocytes, Null immunology, Lymphokines biosynthesis, Lymphokines isolation & purification, Lymphokines physiology, Macrophages cytology, Macrophages immunology, Mast Cells cytology, Mice, Mice, Inbred BALB C, Mice, Nude, Molecular Weight, Monocytes cytology, Rats, T-Lymphocytes cytology, T-Lymphocytes immunology, Thy-1 Antigens, Time Factors, Bone Marrow Cells, Colony-Forming Units Assay, Hematopoiesis, Hematopoietic Stem Cells cytology
Abstract

In vitro techniques have proven particularly fruitful for the study of the differentiation of the hemopoietic cells in bone marrow. Progenitor cells can be readily obtained in suspension and in many cases can be induced to grow and differentiate as isolated clones in vitro. At least in vitro, growth and differentiation appear to be regulated by a series of soluble molecules. Recent advances in immunology (the production of inducible T-cell hybridomas and specific T-cell clones) have defined the T-cell as a source of a number of these soluble regulators. Study of the generation of lymphocytes from bone-marrow precursors in vitro, however, remains a challenge.

Published
1983

82. The RNA fractions of chromatin from L-cells.

Author

Monahan JJ and Hall RH

Subjects
Animals, Carbon Radioisotopes, Cell Nucleus analysis, Cell Nucleus metabolism, Centrifugation, Density Gradient, Chromatin metabolism, Chromatography, DEAE-Cellulose, Electrophoresis, Electrophoresis, Polyacrylamide Gel, Isotope Labeling, L Cells metabolism, Mice, Molecular Weight, Phosphorus Radioisotopes, Polysaccharides, Time Factors, Tritium, Uridine metabolism, Chromatin analysis, L Cells analysis, RNA analysis, RNA biosynthesis, RNA isolation & purification
Published
1974
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83. The 7S RNA common to oncornaviruses and normal cells is associated with polyribosomes.

Author

Walker TA, Pace NR, Erikson RL, Erikson E, and Behr F

Subjects
Animals, Cell Fractionation, Centrifugation, Density Gradient, Chromatography, Cycloheximide pharmacology, Dimethyl Sulfoxide, Electrophoresis, Polyacrylamide Gel, Fibroblasts analysis, HeLa Cells analysis, Humans, L Cells analysis, Mice, Molecular Weight, Subcellular Fractions, Oncogenic Viruses analysis, Polyribosomes analysis, RNA Viruses analysis, RNA, Neoplasm analysis, RNA, Ribosomal analysis, RNA, Viral analysis
Abstract

The 7S RNA species first demonstrated in avian and murine oncornaviruses and later in normal, uninfected cells is found associated in part with cellular polyribosomes. A molar ratio of 7S RNA to 5S ribosomal RNA of 0.05 indicates that there is approximately one mole of 7S RNA per mole of messenger RNA. Dissociation of polyribosomes with dimethylsulfoxide results in a marked decrease in the sedimentation rate of the 7S RNA. The dimethylsulfoxide-induced dissociation of polyribosomes and the concomitant movement of the 7S RNA from the polyribosome region into lighter regions of a sucrose gradient are both inhibited by cycloheximide, indicating that the 7S RNA is indeed associated with polyribosomes and not with a ribonucleoprotein particle sedimenting with polyribosomes.

Published
1974
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84. Methylation pattern of mouse mitochondrial DNA.

Author

Pollack Y, Kasir J, Shemer R, Metzger S, and Szyf M

Subjects
5-Methylcytosine, Animals, Base Sequence, Cytosine analysis, DNA Restriction Enzymes, L Cells analysis, Methylation, Mice, Mitochondria analysis, Mitochondria, Liver analysis, Nucleic Acid Hybridization, Plasmids, Cytosine analogs & derivatives, DNA, Mitochondrial analysis
Abstract

The pattern of methylation of mouse mitochondrial DNA (mtDNA) was studied using several techniques. By employing a sensitive analytical procedure it was possible to show that this DNA contains the modified base 5-methylcytosine (m5Cyt). This residue occurred exclusively at the dinucleotide sequence CpG at a frequency of 3 to 5%. The pattern of methylation was further investigated by determining the state of methylation of several MspI (HpaII) sites. Different sites were found to be methylated to a different extent, implying that methylation of mtDNA is nonrandom. Based on the known base composition and nucleotide sequence of mouse mtDNA, the dinucleotide sequence CpG was found to be underrepresented in this DNA. The features of mtDNA methylation (CpG methylation, partial methylation of specific sites and CpG underrepresentation) are also characteristic of vertebrate nuclear DNA. This resemblance may reflect functional relationship between the mitochondrial and nuclear genomes.

Published
1984
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85. Use of antibodies to nucleosides and nucleotides in studies of nucleic acids in cells.

Author

Erlanger BF, Klein WJ Jr, Dev VG, Schreck RR, and Miller OJ

Subjects
Animals, Cell Division, Chromosomes analysis, Chromosomes ultrastructure, Fluoresceins, Fluorescent Antibody Technique, Humans, L Cells analysis, Methods, Mice, Nucleic Acid Denaturation, Rabbits immunology, Sheep immunology, Antibodies, DNA analysis, Nucleosides immunology, Nucleotides immunology, RNA analysis
Published
1975
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87. Sequence organization and cytological localization of the minor satellite of mouse.

Author

Wong AK and Rattner JB

Subjects
Animals, Base Sequence, Centromere analysis, Centromere physiology, DNA, Satellite physiology, L Cells physiology, Metaphase, Mice, Molecular Sequence Data, Nucleic Acid Conformation, Nucleic Acid Hybridization, Repetitive Sequences, Nucleic Acid, DNA, Satellite isolation & purification, L Cells analysis
Abstract

A complete 120 bp genomic consensus sequence for the mouse minor satellite has been determined from enriched L929 centromeric sequences. The extensive sequence homology existing between the major and minor satellite suggests an evolutionary relationship. Some sequences flanking the minor satellite has also been identified and they provide insight into centromeric DNA organization. Isotopic in situ hybridization analysis of the minor satellite to mouse L929 and Mus musculus metaphase spreads showed that this repetitive DNA class is localized specifically to centromeres of all chromosomes of the karyotype. With the use of high resolution non-isotopic fluorescence in situ hybridization the minor satellite is further localized to the outer surface of the centromere in a discrete region at or immediately adjacent to the kinetochore. Our cytological data suggests that the minor satellite might play a role in the organization of the kinetochore region rather than, as previously suggested, sites for general anchoring of the genome to the nuclear matrix.

Published
1988
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88. Myosin in cultured fibroblasts.

Author

Ostlund RE, Pastan I, and Adelstein RS

Subjects
Actins analysis, Animals, Bucladesine pharmacology, Buffers, Cell Fractionation, Cell Line, Cell Nucleus analysis, Cell Transformation, Neoplastic, Electrophoresis, Disc, Fibroblasts drug effects, Fibroblasts growth & development, Gammaretrovirus, Kidney analysis, L Cells analysis, Membranes analysis, Mice, Mice, Inbred Strains embryology, Microtubules analysis, Myosins isolation & purification, Proteins analysis, Rats, Sodium Dodecyl Sulfate, Subcellular Fractions analysis, Theophylline pharmacology, Fibroblasts analysis, Myosins analysis
Published
1974

89. Some structural, biochemical and biophysical characteristics of L-929 cells growing in the presence of hyperosmotic sorbitol concentrations.

Author

Clegg JS, Gallo J, and Gordon E

Subjects
Animals, Biological Transport, Cell Division, Culture Media, Glucose metabolism, Kinetics, L Cells analysis, L Cells cytology, L Cells drug effects, L Cells metabolism, Mice, Microscopy, Electron, Organoids ultrastructure, Osmolar Concentration, Osmotic Pressure, Oxygen Consumption, Sorbitol metabolism, Time Factors, Water analysis, L Cells physiology, Sorbitol pharmacology
Abstract

Mouse L-929 cells (a fibroblast-like line) were transferred from normal growth medium to one supplemented with 0.3 M sorbitol, doubling the normal external osmotic pressure. After a short lag phase and minimal cell death, the cells began to grow, and the growth rate reached that of controls after about one week. These chronically grown cells (S) have been compared to those of control cultures (C) with regard to general morphology, ability to reverse when returned to normal condition, water content, volume and selected metabolic parameters. S-cell cultures exhibited considerable heterogeneity but most contained vesicle-like cytoplasmic structures, sometimes in abundance. These structures do not appear to be completely bounded by membranes, but that is uncertain. S cells become larger and contain more water than C cells; however, the ratio of total water to total dry mass is indistinguishable from controls suggesting regulation at that level. S and C cells were found to be remarkably similar, on a per cell basis, with regard to their rate of respiration and the incorporation of glucose into metabolites and macromolecules. These results are interpreted in terms of current views on the composition and organization of the aqueous compartments of animal cells.

Published
1986
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90. Repeat array in Epstein-Barr virus DNA is related to cell DNA sequences interspersed on human chromosomes.

Author

Heller M, Henderson A, and Kieff E

Subjects
Animals, Burkitt Lymphoma, Cell Line, DNA Restriction Enzymes, Humans, L Cells analysis, Mice, Nucleic Acid Hybridization, Plasmids, Repetitive Sequences, Nucleic Acid, Species Specificity, Cell Transformation, Viral, Chromosomes, Human analysis, DNA genetics, DNA, Recombinant analysis, DNA, Viral genetics, Herpesvirus 4, Human genetics
Abstract

The third internal repeat (IR3) simple repeat array in Epstein-Barr virus (EBV) DNA has a high degree of homology to a reiterated component of cell DNAs. 32P-Labeled human or mouse DNAs hybridize to the IR3 sequence on Southern blots of viral DNA. EBV IR3 probe identifies many restriction enzyme fragments on Southern blots of human and mouse DNAs that have extensive homology to IR3. Cytological hybridization shows that IR3 is homologous to at least one region on each human chromosome except the Y chromosome.

Published
1982
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91. Purification of mouse L cell interferon. Essentially pure preparations with associated cell growth inhibitory activity.

Author

Iwakura Y, Yonehara S, and Kawade Y

Subjects
Cell Division drug effects, Interferons pharmacology, Molecular Weight, Newcastle disease virus, Interferons isolation & purification, L Cells analysis
Abstract

Mouse L cell interferon induced by Newcastle disease virus was purified by a combination of salt precipitation, ion exchange chromatography, gel filtration, and affinity chromatography using anti-interferon anti-body. The preparation was labeled with 125I at a later step of purification, which served as an index of protein concentration. Two main species of interferon molecules differing in molecular weight were separated from each other, and the final preparations obtained were shown to be essentially pure by polyacrylamide gel electrophoresis in the absence as well as in the presence of sodium dodecyl sulfate. The highest specific activities obtained were 2.6 X 10(9) and 7.3 X 10(8) international units/mg of protein (determined by 125I radioactivity) for the 40,000- and 24,000-dalton species, respectively. The preparations at different steps of purification, including those of the highest purity, were tested for the anti-cell growth activity. Their activities were found to be indistinguishable from each other when compared at the same antiviral doses, indicating that the anti-cell growth activity is carried by the interferon molecules themselves.

Published
1978

92. Evidence for nystatin micelles in L-cell membranes from fluorescence photobleaching measurements of diffusion.

Author

O'Neill LJ, Miller JG, and Petersen NO

Subjects
Animals, Diffusion, Kinetics, L Cells analysis, Mice, Micelles, Phosphatidylethanolamines, Photochemistry, Spectrometry, Fluorescence methods, Cell Membrane analysis, Nystatin analogs & derivatives, Nystatin analysis
Abstract

Diffusion of a nitrobenzoxadiazole derivative of the polyene antibiotic nystatin in the membranes of L cells is found to depend on the concentration of nystatin in the membrane. Its diffusion coefficient measured by fluorescence photobleaching decreases hyperbolically as the concentration of nystatin is increased. This behavior is reproduced when the concentration of the derivative is increased. In contrast, diffusion of a nitrobenzoxadiazole derivative of a phospholipid is insensitive to the nystatin concentration under these conditions. The nystatin-specific diffusion changes can be understood if nystatin exists in a monomer-micelle equilibrium within the membrane but cannot be accounted for by binding or phase partitioning.

Published
1986
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93. Analysis of polyadenylate . protein complex of polysomal messenger RNA from mouse L cells.

Author

Bernd A, Zahn RK, Maidhof A, and Müller WE

Subjects
Animals, L Cells analysis, Mice, Molecular Weight, Nucleoproteins analysis, Poly A analysis, Polyribosomes metabolism, RNA, Messenger analysis, Ribonucleoproteins analysis, Ribosomal Proteins analysis
Abstract

The organization of polysomal poly(A)-ribonucleoprotein complex [poly(A)-RNP] was studied. The poly(A)-associated proteins were liberated directly from the poly(A)-RNP complex. Polysomal mRNA was isolated from L5178y mouse lymphoma cells by oligo (dT)-cellulose chromatography; poly(A)-RNP was prepared by nuclease digestion. The poly(A)-RNP fraction was considered to be pure basing on the size of its poly(A) component which was determined to consist of 155 AMP moieties. By radiolabeling with [3H]dansyl chloride, two poly(A)-associated proteins with molecular masses of 77,000 Da (P77) and 54,000 Da (P54) were identified. In a quantitative approach, it was shown that the polysomal poly(A)-RNP complex is composed of approximately 4 molecules P54 and 2 molecules P77. Digestion experiments with dimers and tetramers containing ribonuclease A indicated that P54 covers 15-20 AMP residues and P77 a sequence of 40-45 ribonucleotides on the poly(A)--155 stretch of polysomal poly(A)-RNP.

Published
1982
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95. [Non-mitochondrial DNA in cytoplasm].

Author

Erepreĭs IaG

Subjects
Animals, Balantidium analysis, Cycloheximide pharmacology, DNA Replication, Entamoeba histolytica analysis, Female, HeLa Cells analysis, Histones physiology, Humans, L Cells analysis, Liver analysis, Liver enzymology, Male, Membranes analysis, Mitosis, Neoplasms, Experimental analysis, Nucleic Acid Precursors analysis, Oocytes analysis, Spermatocytes analysis, Cytoplasm analysis, DNA analysis
Published
1976

97. Potential for clinical use of the analytical laser microprobe for element measurement.

Author

Glick D and Marich KW

Subjects
Adenocarcinoma analysis, Animals, Carcinoma, Hepatocellular analysis, Carcinoma, Small Cell analysis, Colonic Neoplasms analysis, Evaluation Studies as Topic, Fibroblasts analysis, Gold analysis, Humans, L Cells analysis, Liver Neoplasms, Lung Neoplasms analysis, Lysosomes analysis, Lysosomes ultrastructure, Methods, Mice, Microchemistry, Microscopy, Electron, Neoplasm Metastasis, Phagocytes analysis, Phagocytes ultrastructure, Sarcoma analysis, Time Factors, Lasers, Metals analysis, Trace Elements analysis
Abstract

Use of the laser microprobe for rapid emission spectroscopic analysis of elements in microscopic samples of biological material is described. The technique depends on vaporization of the microsample with a focused laser beam at a temperature that renders the vapor incandescent for spectrochemical analysis. Spectral line intensities are recorded photographically with densitometry of the negatives or photoelectrically. Current capability permits analysis of about 10(-8) to 10(-10) g of tissue, with detection limits of 10-12 to 10-15 g of element. Groups of elements can be simultaneously analyzed. Minimum sample preparation is required, and the analysis is done on the stage of a light microscope, usually on an air-dried sample on a plastic slide. We exemplify the technique in analysis of gold in cultured fibroblasts treated with gold salts and in human skin after treatment with gold salts for rheumatoid arthritis, in element changes in biopsies of transplanted human hearts, and in unique profiles of groups of elements in human cancer tissue.

Published
1975

98. The reaction of cells with anti-actin sera in relation to the amount of cellular actin.

Author

Norberg R, Biberfeld G, Fagraeus A, Lidman K, Thorstensson R, and Utter G

Subjects
Actins immunology, Animals, Antibodies, Cell Line, Electrophoresis, Polyacrylamide Gel, Fluorescent Antibody Technique, L Cells analysis, Lymphoma, Non-Hodgkin analysis, Mice, Mice, Inbred BALB C, T-Lymphocytes analysis, Thymus Gland analysis, Actins analysis
Abstract

The staining pattern of anti-actin sera on various cells smeared on glass was compared to the relative amount of cellular actin estimated by SDS-polyacrylamide-gel electrophoresis with subsequent scanning of the gel. Although the cells showed a varying stainability the actin content was fairly constant. Thus, the staining differences reflected changes in the organization of cellular actin rather than actual differences in the amount of actin.

Published
1977

99. Characterization of polypyrimidines in Drosophila and L-cell DNA.

Author

Birnboim HC, Straus NA, and Sederoff RR

Subjects
Animals, Base Sequence, Cells, Cultured, Chromatography, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Hydroxyapatites, Mice, Nucleic Acid Hybridization, DNA analysis, Drosophila melanogaster analysis, L Cells analysis, Polynucleotides analysis, Thymine analysis
Abstract

Unusually long pyrimidine tracts (polypyrimidines), ranging from 100 to over 1000 nucleotides in length, have been found in Drosophila melanogaster DNA. They are compared to shorter pyrimidine tracts (25-150 nucleotides) which have previously been found in L-cell DNA. Both species were able to anneal to homologous DNA; Drosophila polypyrimidines formed stable hybrids while L-cell polypyrimidines formed hybrids of lower thermal stability. In both cases, the kinetics of the reaction was rapid, suggesting that these tracts are part of highly repeated DNA.

Published
1975
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100. A sandwich enzyme-linked immunoadsorbent assay for detection of murine macrophage colony-stimulating factor (CSF-1).

Author

Lokeshwar BL and Lin HS

Subjects
Animals, Antibodies, Monoclonal, Colony-Stimulating Factors immunology, Granulocyte-Macrophage Colony-Stimulating Factor, Growth Substances analysis, L Cells analysis, Macrophage Colony-Stimulating Factor, Mice, Species Specificity, Colony-Stimulating Factors analysis, Enzyme-Linked Immunosorbent Assay
Abstract

A simple three-layer sandwich enzyme-linked immunoadsorbent assay (sandwich-ELISA) has been developed for murine macrophage colony-stimulating factor-1 (CSF-1) using the two monoclonal antibodies on which we recently reported (J. Immunol. (1988) 141, 483). The anti-CSF-1 monoclonal antibodies used in this assay recognize different epitopes of the same antigen, thereby permitting the detection of low amounts of CSF-1. This assay is specific to murine CSF-1. Recombinant human macrophage colony-stimulating factor, murine GM-CSF, or IL-3, either alone or together with CSF-1, does not interfere with the assay. The advantage of this assay over other reported immunoassays for CSF-1 is that radiolabeled or large quantities of purified CSF-1 are not required. This sandwich-ELISA compares favorably with other assays in its rapidity, simplicity, and sensitivity.

Published
1989
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