ENZYMATICALLY PRODUCED SUBUNITS OF PROTEINS FORMED BY PLASMA CELLS IN MICE: I. gamma-GLOBULIN AND gamma-MYELOMA PROTEINS

doi:10.1084/jem.115.3.623

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The Journal of Experimental Medicine, Vol 115, 623-639, Copyright, 1962, by The Rockefeller Institute

ARTICLE

ENZYMATICALLY PRODUCED SUBUNITS OF PROTEINS FORMED BY PLASMA CELLS IN MICE : I. $gamma$ -GLOBULIN AND $gamma$ -MYELOMA PROTEINS

J. L. Fahey M.D.¹ and Brigitte A. Askonas Ph.D.¹

¹ From the Division of Immunology, National Institute for Medical Research, Mill Hill, London, and the Metabolism Service, National Cancer Institute, National Institutes of Health, Bethesda

Gamma globulin and antibody obtained from inbred C₃H mice aresplit by papain and cysteine into fragments roughly one-thirdthe size of the original Molecule (S_20,w = 3.5S). The papaindigests were characterized by starch gel electrophoresis andimmunological methods. The highly heterogeneous fragments couldbe divided into two groups with distinct antigenic determinants(S and F), which were separated by DEAE ion-exchange cellulosechromatography. Approximately two-thirds of the fragments hadS antigenic groupings and one-third had F antigenic groupings.These data are consistent with the view that mouse gamma globulinis split by papain and cysteine into three major fragments,two of which are of the S type and one of the F type.

Antibodyactivity of the original molecule was present in the S fragments.Although the S fragments did not precipitate the antigen (hemocyanin)they were shown to bind antigen specifically in the manner ofunivalent antibodies.

The S fragments of normal $gamma$ -globulin werevery heterogeneous with a broad spectrum of electrophoreticmobilities. Comparison of S fragments from slow and fast migratingglobulins showed that the mobilities of the original $gamma$ -globulinsamples were largely reflected in the mobilities of their Sfragments. Additional observations indicated that the F fragmentsalso may help to determine the electrophoretic mobility of intact $gamma$ -globulin molecules.

S fragments of differing electrophoreticmobility were shown to have the same antigenic determinants,indicating that the structural differences responsible for theelectrophoretic mobility differences were not involved in theantigenic groupings identified with rabbit antisera.

The F fragmentsof normal $gamma$ -globulin migrated more rapidly than the S fragments,were less heterogeneous, and showed several bands on starchgel electrophoresis. The F fragments differed antigenicallyfrom the S fragments, and had no antibody activity. Two groupsof F fragments (F and F') were detected with some antisera.

The $gamma$ -myeloma protein (5563) formed in a C₃H plasma cell tumor andsimilarly fragmented by treatment with papain and cysteine,produced much more discrete S and F components than were foundin the normal $gamma$ -globulin digest. The electrophoretic propertiesof the myeloma protein fragments were within the range observedfor normal $gamma$ -globulin fragments. Although the $gamma$ -myeloma proteinshares antigenic determinants with normal $gamma$ -globulins it lackssome of the antigenic groupings present in the $gamma$ -globulin preparation.Both S and F fragments from the myeloma protein share antigenicdeterminants with the corresponding fragments from normal $gamma$ -globulin.In addition, both S and F fragments of normal $gamma$ -globulin possessantigenic groupings not present in fragments of the $gamma$ -myelomaprotein, accounting for the antigenic deficiency observed oncomparison of the $gamma$ -myeloma protein with normal $gamma$ -globulins.

Submitted on October 16, 1961

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Mishell, R. I., Fahey, J. L. (1964). Molecular and Submolecular Localization of Two Isoantigens of Mouse Immunoglobulins. Science 143: 1440-1442 [Abstract]