Abstract
Hyperphosphatasia mental retardation syndrome (HPMR), an autosomal recessive disease characterized by mental retardation and elevated serum alkaline phosphatase (ALP) levels, is caused by mutations in the coding region of the phosphatidylinositol glycan anchor biosynthesis, class V (PIGV) gene, the product of which is a mannosyltransferase essential for glycosylphosphatidylinositol (GPI) biosynthesis. Mutations found in four families caused amino acid substitutions A341E, A341V, Q256K, and H385P, which drastically decreased expression of the PIGV protein. Hyperphosphatasia resulted from secretion of ALP, a GPI-anchored protein normally expressed on the cell surface, into serum due to PIGV deficiency. In contrast, a previously reported PIGM deficiency, in which there is a defect in the transfer of the first mannose, does not result in hyperphosphatasia. To provide insights into the mechanism of ALP secretion in HPMR patients, we took advantage of CHO cell mutants that are defective in various steps of GPI biosynthesis. Secretion of ALP requires GPI transamidase, which in normal cells, cleaves the C-terminal GPI attachment signal peptide and replaces it with GPI. The GPI-anchored protein was secreted substantially into medium from PIGV-, PIGB-, and PIGF-deficient CHO cells, in which incomplete GPI bearing mannose was accumulated. In contrast, ALP was degraded in PIGL-, DPM2-, or PIGX-deficient CHO cells, in which incomplete shorter GPIs that lacked mannose were accumulated. Our results suggest that GPI transamidase recognizes incomplete GPI bearing mannose and cleaves a hydrophobic signal peptide, resulting in secretion of soluble ALP. These results explain the molecular mechanism of hyperphosphatasia in HPMR.
Highlights
Hyperphosphatasia was observed with glycosylphosphatidylinositol (GPI) deficiency due to mutation in PIGV, but not the PIGM gene
Using mutant Chinese hamster ovary (CHO) cells that are defective in various GPI biosynthesis steps, we show that secretion of alkaline phosphatase (ALP) requires GPI transamidase, which is activated by GPI bearing at least one mannose
To analyze the activities of these mutant PIGV proteins, we transfected PIGV-deficient CHO cells with plasmids bearing mutant PIGV driven by the strong SR␣ promoter or by the weak promoter containing only a TATA box and analyzed surface expression of CD59, a GPI-anchored proteins (GPI-APs), by FACS
Summary
Hyperphosphatasia was observed with glycosylphosphatidylinositol (GPI) deficiency due to mutation in PIGV, but not the PIGM gene. Hyperphosphatasia mental retardation syndrome (HPMR), an autosomal recessive disease characterized by mental retardation and elevated serum alkaline phosphatase (ALP) levels, is caused by mutations in the coding region of the phosphatidylinositol glycan anchor biosynthesis, class V (PIGV) gene, the product of which is a mannosyltransferase essential for glycosylphosphatidylinositol (GPI) biosynthesis. Hyperphosphatasia resulted from secretion of ALP, a GPI-anchored protein normally expressed on the cell surface, into serum due to PIGV deficiency. PIGM deficiency is caused by a mutation in the PIGM gene promoter region that encodes the first mannosyltransferase, which is essential for GPI biosynthesis [12] To explain this difference, we considered the possibility that the pathogenesis of hyperphosphatasia is critically dependent on the step of GPI biosynthesis that is defective. Using mutant CHO cells that are defective in various GPI biosynthesis steps, we show that secretion of ALP requires GPI transamidase, which is activated by GPI bearing at least one mannose
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