Cloning of genes for bacteriophage T5 stable RNAs.
Biochim Biophys Acta, 1982/5/31;697(2):235-42.
Ksenzenko VN, Kamynina TP, Kazantsev SI, Shlyapnikov MG, Kryukov VM, Bayev AA
PMID: 6285979
Abstract
One EcoRI-generated fragment (440 basepairs) and two EcoRI/HindIII fragments (220 and 960 basepairs) from the deletion region of T5 phage have been inserted into the phage lambda XIII and the plasmid pBR322 as vectors. Recombinant DNA molecules were studied by hybridization with in vivo 32P-labeled T5 4-5 S RNAs on nitrocellulose filters. Two-dimensional polyacrylamide gel electrophoretic fractionation and fingerprint analysis of the RNAs eluted from the filters were carried out to identify RNAs coded by cloned fragments. For the accurate localization of the genes for these RNAs, RNA-DNA hybrids were treated with T1 and pancreatic RNAases, and the eluted RNA fragments stable against RNAase action were electrophoresed. It was shown that the EcoRI 440 fragment contains the gene for tRNA 10 (tRNAAsp), the EcoRI/HindIII 220 fragment contains the gene for RNA III (107 bases) and parts of the genes for RNA I (107 bases) and tRNA 12 (tRNAHis), and the EcoRI/HindIII 960 fragment contains only a part of the gene for tRNA 9 (tRNAGln). The arrangement of these genes on the physical map of T5 phage was as follows: -tRNAGln-tRNAHis-RNA III-RNA I-...-tRNAAsp.
MeSH terms
Bacteriophage lambda; Base Composition; Base Sequence; Cloning, Molecular; DNA Restriction Enzymes; DNA, Recombinant; Deoxyribonuclease EcoRI; Escherichia coli; Genes, Viral; Nucleic Acid Hybridization; RNA, Viral; T-Phages
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