Abstract
ARGINYL-tRNA-protein transferase is a soluble enzyme from mammalian tissues which catalyses the transfer of arginine from arginyl-tRNA into peptide linkage specifically with NH2-terminal aspartic or glutamic acid residues of protein acceptors1,2. Molar equivalents of arginine are transferred to appropriate NH2-terminal residues2. The reaction differs in many respects from the transfer of amino-acids associated with protein synthesis de novo and is thought to be a mechanism for regulating the activity of acceptor proteins3. Many immunoglobulins possess aspartic or glutamic acid in the NH2-terminal position, and it was interesting to examine whether arginylation of such residues might result in an alteration of activity of these proteins, for there is considerable evidence that the antibody-combining site is contained in the NH2-terminal region of both light4–7 and heavy8,9 chains.
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SOFFER, R., CAPRA, J. Enzymatic Probe for Accessibility of NH2-Terminal Residues in Immunoglobulins. Nature New Biology 233, 44–45 (1971). https://doi.org/10.1038/newbio233044a0
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DOI: https://doi.org/10.1038/newbio233044a0
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