CONTROLLED PROTEOLYSIS OF NASCENT POLYPEPTIDES IN RAT LIVER CELL FRACTIONS: I. Location of the Polypeptides within Ribosomes

doi:10.1083/jcb.45.1.130

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CONTROLLED PROTEOLYSIS OF NASCENT POLYPEPTIDES IN RAT LIVER CELL FRACTIONS : I. Location of the Polypeptides within Ribosomes

G. Blobel ¹ and D. D. Sabatini ¹

¹ From The Rockefeller University, New York 10021

Free ribosomes containing nascent polypeptide chains labeledin vitro were submitted to proteolysis at 0° by a mixtureof trypsin and chymotrypsin. Sucrose gradient analysis showedthat polysome patterns are retained even after 24 hr of proteolysisin the cold, while messenger RNA-free ribosomes (generated progressivelyduring in vitro incorporation) are, within 2 hr, completelydissociated into subunits by trypsin. Although ribosomes andsubunits are not extensively degraded into smaller fragmentsduring low temperature proteolysis, changes in the acrylamidegel electrophoresis pattern showed that most ribosomal proteinsare accessible to and are partially degraded by the proteases.Ribosome-bound nascent polypeptides are partially resistantto proteolysis at 0°, although they are totally digestedat 37° or when the ribosomal subunit structure is disruptedby other means. Radioactivity incorporated into nascent chainsduring incubation times shorter than 3 min was mostly resistantto digestion at 0°. A larger fraction of the initial radioactivitybecame degraded in ribosomes which incorporated for longer times.In these ribosomes, the amount of radioactivity which was resistantto proteolysis was constant and independent of the initial value,which reflects the labeled length of the nascent chains. Theseresults suggest that the growing end of the nascent polypeptideis resistant to digestion and is protected from proteolyticattack by the ribosomal structure. A pulse and chase experimentconfirmed this suggestion, showing that the protected segmentis located at the carboxy-terminal end of the nascent chain.The protected segment was contained in the large ribosomal subunitand had a length of $sim$ 39 amino acid residues, as estimated bychromatography on Sephadex G-50.

Submitted on September 24, 1969
Revised on November 3, 1969

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