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Structure of methemerythrin at 5 A resolution.
Authors:R E Stenkamp  L C Sieker  L H Jensen  J S Loehr
Affiliation:The Rockefeller University, New York, N.Y. 10021, U.S.A.;Molecular Cytology Laboratory Sloan-Kettering Institute for Cancer Research New York, N.Y. 10021, U.S.A.
Abstract:Rabbit globin messenger RNA was labelled in vitro with 125I to specific activities in the range 20 to 200 × 106 cts/min per μg. This 125I-labelled mRNA bound to rabbit reticulocyte ribosomes with the kinetics and sensitivity to inhibitors expected from its participation in the normal process of the initiation of protein synthesis. Furthermore, when modified in 25% of its cytidine residues with unlabelled iodide, the mRNA coded for the same series of initiation peptides as did the unmodified mRNA. Using the techniques of RNA fingerprinting, the binding reaction was shown to select against contaminants and against “globin mRNA” molecules which lack a particular oligonucleotide implicated in the initiation process. When the 125I-labelled mRNA was bound to ribosomes, both the initiating 40 S subunits and the 80 S ribosomes protected a fraction of the mRNA from digestion by pancreatic ribonuclease. Fingerprint analysis showed that highly specific regions of the mRNA were protected by the 40 S subunits and 80 S ribosomes and that these two protected regions were not identical.
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