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Modified Nucleosides and Cancer

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Cover of 'Modified Nucleosides and Cancer'

Table of Contents

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    Book Overview
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    Chapter 1 Organization and Expression of tRNA Genes in Drosophila Melanogaster
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    Chapter 2 Chemical Nature, Properties, Location, and Physiological and Pathological Variations of Modified Nucleosides in tRNAs
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    Chapter 3 Formation and Removal of Methylated Nucleosides in Nucleic Acids of Mammalian Cells
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    Chapter 4 Structural Modifications and Repair of DNA in Neuro-Oncogenesis by N-Ethyl-N-nitrosourea
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    Chapter 5 Role of Extent and Persistence of DNA Modifications in Chemical Carcinogenesis by Aromatic Amines
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    Chapter 6 Can DNA Methylation Regulate Gene Expression?
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    Chapter 7 tRNA Alterations in Cancer
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    Chapter 8 Tumor-Specific tRNA Modifications in Mouse Plasmacytomas and Other Tumors
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    Chapter 9 Alterations in Post-Transcriptional Modification of the Y Base in Phenylalanine tRNA from Tumor Cells
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    Chapter 10 Why Is Tumor tRNA Hypomodified with Respect to Q Nucleoside?
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    Chapter 11 The effects of growth factors on tRNALys modification.
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    Chapter 12 Perturbation of the mitochondrial lysine tRNA population by virus-induced transformation or stress of mammalian cells: functional properties and nucleotide sequence of a mitochondrially associated lysine tRNA.
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    Chapter 13 Involvement of tRNA in Retrovirus Expression: Biological Implications of Reverse Transcriptase-Primer tRNA Interactions
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    Chapter 14 Enzymatic Methylation of Chicken Erythrocyte DNA Modified by Two Carcinogens, 2-(N-Acetoxyacetylamino) Fluorene and Methylnitrosourea
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    Chapter 15 Inhibition of DNA Methylation by 5-Azacytidine
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    Chapter 16 Alteration of enzymatic DNA methylation by chemical carcinogens.
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    Chapter 17 Ethionine-Induced Alterations of tRNA Metabolism
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    Chapter 18 Processing of tRNA is accomplished by a high-molecular-weight enzyme complex.
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    Chapter 19 Alteration of tRNA Modification in Eukaryotes: Causes and Consequences
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    Chapter 20 Effects of Cortisol on tRNA Methylase Activities in Rat Mammary Carcinoma
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    Chapter 21 An approach to inhibition of viral replication: inhibition of mRNA methylation.
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    Chapter 22 Specific Effects of 5-Fluoropyrimidines and 5-Azapyrimidines on Modification of the 5 Position of Pyrimidines, in Particular the Synthesis of 5-Methyluracil and 5-Methylcytosine in Nucleic Acids
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    Chapter 23 New applications of urinary nucleoside markers.
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    Chapter 24 Multivariate analysis of urinary RNA catabolites in malignancies: cross-sectional and longitudinal studies.
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    Chapter 25 Evaluation of carcinoembryonic antigen, tissue polypeptide antigen, placental alkaline phosphatase, and modified nucleosides as biological markers in malignant lymphomas.
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    Chapter 26 Quantitative High-performance Liquid Chromatography Analysis of Modified Nucleosides in Physiological Fluids, tRNA, and DNA
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    Chapter 27 Modified Nucleosides in Body Fluids of Tumor-Bearing Patients
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    Chapter 28 Increasing Urinary Levels of Modified Nucleosides and Bases During Tumor Development in Mice
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    Chapter 29 Comparison of Urinary Modified Nucleosides and Bases in Rats with Hepatomas and Nephroblastomas
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    Chapter 30 Characterization and Analysis of Oncofetal tRNA and Its Possible Application for Cancer Diagnosis and Therapy
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    Chapter 31 Excretion of polyamines by children with leukemia during chemotherapy.
Attention for Chapter 11: The effects of growth factors on tRNALys modification.
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Chapter title
The effects of growth factors on tRNALys modification.
Chapter number 11
Book title
Modified Nucleosides and Cancer
Published in
Recent results in cancer research Fortschritte der Krebsforschung Progrès dans les recherches sur le cancer, January 1983
DOI 10.1007/978-3-642-81947-6_11
Pubmed ID
Book ISBNs
978-3-64-281949-0, 978-3-64-281947-6
Authors

B. J. Ortwerth, V. K. Lin, Ortwerth, B. J., Lin, V. K.

Abstract

The tRNALys population from tissue culture cells contains several isoaccepting species which are not present in the tRNALys population from tissue sources. These isoacceptors were isolated from mouse LM cells and tested for their coding properties in ribosomal binding assays and their ability to incorporate lysine into protein in a reticulocyte lysate. tRNALys5A and tRNALys6 eluted in the area of tRNALys5. All three species coded preferentially for AAA and bound with equal efficiency. tRNALys1, tRNALys3, tRNALys4, and tRNALys6 all transferred lysine into protein at a slower rate than tRNALys2 and tRNALys5, which are the native species. Several purified growth factors were tested for their ability to affect the levels of tRNALys4, a tRNA possibly associated with cell division. When Balb/c 3T3 cells were grown in medium containing plasma instead of serum, there was a decrease in tRNALys2, tRNALys3, tRNALys4 and an increase in tRNALys5 and tRNALys6. The addition of either FGF or PDGF returned the tRNALys profile to normal. The extent of the tRNALys changes depended upon the concentration of growth factor added. FGF was able to cause a 35% decrease in the tRNALys5 peak with a corresponding increase in tRNALys2 within 1 h of the addition of the factor. These data suggest that competence factors have the ability to stimulate the modification of specific tRNALys isoacceptors.

Mendeley readers

Mendeley readers

The data shown below were compiled from readership statistics for 4 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 4 100%

Demographic breakdown

Readers by professional status Count As %
Student > Ph. D. Student 2 50%
Researcher 1 25%
Student > Doctoral Student 1 25%
Readers by discipline Count As %
Agricultural and Biological Sciences 2 50%
Medicine and Dentistry 2 50%