Analysis of a sequence region of 5S RNA fromE. colicross-linkedin situto the ribosomal protein L25

Abstract

70S ribosomes from E. coli were chemically cross-linked under conditions of in vitro protein biosynthesis. The ribosomal RNAs were extracted from reacted ribosomes and separated on sucrose gradients. The 5S RNA was shown to contain the ribosomal protein L25 covalently bound. After total RNase T₁ hydrolysis of the covalent RNA-protein complex several high molecular weight RNA fragments were obtained and identified by sequencing. One fragment, sequence region U₁₀₃ to U12O, was shown to be directly linked to the protein first by protein specific staining of the particular fragment and second by phosphor cellulose chromato-graphy of the covalent RNA-protein complex. The other two fragments, U₈₉ to G₁₀₆ and A₃₄ to G₅₁, could not be shown to be directly linked to L25 but were only formed under cross-linking conditions. While the fragment U₈₉ to G₁₀₆ may be protected from RNase T₁ digestion because of a strong interaction with the covalent RNA-protein complex, the formation of the fragment A34 to G51 is very likely the -result of a double monovalent modification of two neighbouring guanosines in the 5S RNA The RNA sequences U₁₀₃ to U_12O established to be in direct contact to the protein L25 within the ribosome falls into the sequence region previously proposed as L25 binding site from studies with isolated 5S RNA-protein complexes