Your search keyword '"L Cells analysis"' showing total 6 results

1. The purification and quantitation of myosin from cultured cells.

Author

Ostlund RE and Pastan I

Subjects

Adenosine Triphosphatases analysis, Animals, Cell Line, Female, HeLa Cells analysis, L Cells analysis, Methods, Mice, Myosins isolation & purification, Uterus analysis, Myosins analysis

Abstract

Myosin has been purified from the following cultured cell lines: normal rat kidney fibroblast (NRK), HeLa-Rhino (HeLa), human choriocarcinoma, human acute lymphoblastic leukemia, rat hepatoma (HTC), monkey kidney (VERO), pigmented mouse melanoma, Y-1 rat adrenal cortex, and growth hormone-secreting GH-1. Myosin constitutes 0.5-5.4% of the protein of these cells. It was not detected in washed human erythrocytes or in two types of mouse plasmacytoma cells. Two methods for the purification of myosin from cultured cells have been employed. With Method I highly purified myosin was prepared by Sepharose 4B and DEAE-cellulose chromatography from 10(10) L-929 cells as well as from mouse uterus. Those myosins have similar molecular and subunit weights as well as ATPase activity but are immunologically distinct. Method II involving ultracentrifugation and Sepharose 4B chromatography, is suitable for the production of moderately pure myosin in good yield from as few as 5-10(7) cells (five 100-mm Petrie dishes).

Published

1976

2. Sequence studies on mouse L-cell satellite DNA by base-specific degradation with T4 endonuclease IV.

Author

Harbers K and Spencer JH

Subjects

Base Sequence, Coliphages enzymology, Endonucleases metabolism, Oligodeoxyribonucleotides analysis, DNA genetics, DNA, Satellite genetics, L Cells analysis

Abstract

The base sequence of mouse L-cell satellite DNA was investigated by degradation of the two separated complementary strands with the base specific enzyme, T4 endonuclease IV. Digestion of the heavy strand DNA released a limited number of oligonucleotides which were separated by ionophoresis/homochromatography, isolated, and sequenced by the 'wandering spot' method. The light strand DNA was resistant to digestion with T4 endonuclease IV and no detectable amounts of oligonucleotides were released. The oligonucleotides obtained from the heavy strand were related in sequence, indicating that mouse satellite DNA derived from a short tandemly repeated sequence. The sequence of part of the original repeat unit is proposed to be C-A-T-T-T-T-T-C. Five major oligonucleotides were identified, all of which differ from the proposed original sequence by single base changes. The five major oligonucleotides occur with about equal frequency and together comprise approximately 50% of the oligonucleotides released by T4 endonuclease IV from the heavy strand DNA. In addition to the five major oligonucleotides, several oligonucleotides were found to occur in lesser amounts. Since these oligonucleotides are related to the major oligonucleotides, it is likely that they have arisen from them by mutation.

Published

1978

3. 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

4. Membranes of animal cells. 8. Distribution of sialic acid, hexosamines and sialidase in the L cell.

Author

Glick MC, Comstock CA, Cohen MA, and Warren L

Subjects

Acid Phosphatase analysis, Animals, Cell Fractionation, Cell Line, Cell Membrane analysis, Cell Membrane enzymology, Cell Nucleus analysis, Glycolipids analysis, Glycoproteins analysis, L Cells cytology, L Cells enzymology, Lysosomes analysis, Lysosomes enzymology, Membranes analysis, Methods, Mice, Microscopy, Electron, Microsomes analysis, Mitochondria analysis, Mitochondria enzymology, Proteins analysis, Solubility, Zinc, Hexosamines analysis, L Cells analysis, Neuraminic Acids analysis, Neuraminidase analysis

Published

1971

5. Isopeptide bonds in membrane proteins from eukaryotic cells.

Author

Birckbichler PJ, Dowben RM, Matacic S, and Loewy AG

Subjects

Adenosine Triphosphatases analysis, Aminopeptidases, Animals, Carbon Isotopes, Cell Fractionation, Cell Membrane enzymology, Dialysis, Fibroblasts, Glutamine analysis, Hydrolysis, L Cells enzymology, Lysine analysis, Mice, Microsomes analysis, Neuraminidase analysis, Peptides analysis, Potassium, Sodium, Tritium, Cell Membrane analysis, L Cells analysis

Published

1973

6. Ribosomal proteins in rapidly growing and non-proliferating mouse cells.

Author

Rodgers A

Subjects

Animals, Brain cytology, Brain Chemistry, Cell Line, Electrophoresis, Polyacrylamide Gel, Intestines analysis, Intestines cytology, Kidney analysis, Kidney cytology, L Cells analysis, Liver analysis, Liver cytology, Mice, Organ Specificity, Carcinoma, Ehrlich Tumor metabolism, Proteins analysis, Ribosomes analysis

Published

1973