GENETIC-HETEROGENEITY IN ACID ALPHA-GLUCOSIDASE DEFICIENCY

Abstract

Several clinical forms of acid .alpha.-glucosidase deficiency were described. Differences at the molecular level were identified in acid .alpha.-glucosidase deficiency. Of 9 fibroblast strains derived from patients with the infantile form of the disease, 8 were crossreacting material (CRM)-negative and 1 CRM-positive. This was demonstrated by both agar immunodiffusion and immunotitration. No difference in apparent enzymatic activityw as observed between CRM-negative and CRM-positive infantile acid .alpha.-glucosidase deficiency fibroblasts. In 2 fibroblast strians with the adult form of acid .alpha.-glucosidase deficiency, rocket immunoelectrophoresis demonstrated a reduction in the amount of enzyme protein, which was directly proportional to the reduction in enzyme activity. In another fibroblast strain obtained from a patient with the adult form of the disease, the activity was within the range of the infantile form and no CRM could be identified. Fibroblasts with phenotype 2 of acid .alpha.-glucosidase, considered a normal variant, showed a reduction both in the amount of enzyme protein and in the ability of the enzyme to cleave glycogen. The catalytic activity for maltose was normal. Extensive genetic heterogeneity was demonstrated in acid .alpha.-glucosidase deficiency. Molecular differences were identified both between the clinical forms of the disease and within the infantile and the adult forms of acid .alpha.-glucosidase deficiency. It remains unknown whether or not the enzyme deficiency in homozygotes for isozyme 2 of acid .alpha.-glucosidase will be sufficient to cause glycogen accumulation and lead to the development of muscular dystrophy-like disease later in life.