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Research Article Free access | 10.1172/JCI106204

Immunochemical studies in four cases of alpha chain disease

Maxime Seligmann, Edith Mihaesco, Daniel Hurez, Constantin Mihaesco, Jean-Louis Preud'homme, and Jean-Claude Rambaud

1Laboratory of Immunochemistry, Research Institute on Blood Diseases, Hôpital Saint-Louis, Paris 10e., France

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1Laboratory of Immunochemistry, Research Institute on Blood Diseases, Hôpital Saint-Louis, Paris 10e., France

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1Laboratory of Immunochemistry, Research Institute on Blood Diseases, Hôpital Saint-Louis, Paris 10e., France

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1Laboratory of Immunochemistry, Research Institute on Blood Diseases, Hôpital Saint-Louis, Paris 10e., France

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1Laboratory of Immunochemistry, Research Institute on Blood Diseases, Hôpital Saint-Louis, Paris 10e., France

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1Laboratory of Immunochemistry, Research Institute on Blood Diseases, Hôpital Saint-Louis, Paris 10e., France

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Published December 1, 1969 - More info

Published in Volume 48, Issue 12 on December 1, 1969
J Clin Invest. 1969;48(12):2374–2389. https://doi.org/10.1172/JCI106204.
© 1969 The American Society for Clinical Investigation
Published December 1, 1969 - Version history
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Abstract

Studies of a number of properties of the pathological γA-proteins in the first four cases of the recently recognized alpha-chain disease demonstrate that, as in γ-heavy-chain disease, the abnormal protein is devoid of light chains and represents a portion of the α-heavy chain related to the Fc-fragment. In two patients, serum electrophoresis showed a broad abnormal band, whereas in the two others the pathological protein was not noticeable on the electrophoretic pattern. The diagnosis of α-chain disease can be established without purification of the protein by immuno-electrophoresis and gel diffusion experiments using selected antisera to γA and a reference α-chain disease protein. All four proteins belonged to the α1-subclass, displayed electrophoretic heterogeneity, and showed a strong tendency to polymerize. The polymers occurred in vivo and were held together both by disulfide bonds and by strong noncovalent forces. Two of the three purified proteins had a very high carbohydrate content. The abnormal protein was always found in concentrated urines in variable but generally low amounts. It was not detected in parotid saliva but was present in significant amounts in jejunal fluid of all four patients. The α-chain disease protein was shown to be associated with the secretory piece in external secretions of two patients.

The clinicopathological features were strikingly similar in the four patients. All patients were affected with a neoplastic and mostly plasmacytic proliferation involving primarily the whole length of the small intestine and the mesenteric nodes and all exhibited a severe malabsorption syndrome. While Israeli authors have emphasized the frequency of this type of abdominal lymphoma in young Arabs and non-Ashkenazi Jews, two of our patients were Kabyles, one a Syrian Arab, and one an Eurasian. Cellular studies showed that the pathological protein was synthesized by the proliferating cells in the lymphoid tissue of the digestive tract and in the mesenteric nodes, and that there was no detectable light-chain synthesis at the intracellular level.

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