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[[Phospholipase C]] (PLC) is an enzyme that is known to cleave the phospho-glycerol bond found in GPI-anchored proteins. Treatment with PLC will cause release of GPI-linked proteins from the outer cell membrane. The [[T-cell]] marker Thy-1 and [[acetylcholinesterase]], as well as both intestinal and placental alkaline phosphatases, are known to be GPI-linked and are released by treatment with PLC. GPI-linked proteins are thought to be preferentially located in [[lipid raft]]s, suggesting a high level of organization within plasma membrane microdomains.
[[Phospholipase C]] (PLC) is an enzyme that is known to cleave the phospho-glycerol bond found in GPI-anchored proteins. Treatment with PLC will cause release of GPI-linked proteins from the outer cell membrane. The [[T-cell]] marker Thy-1 and [[acetylcholinesterase]], as well as both intestinal and placental alkaline phosphatases, are known to be GPI-linked and are released by treatment with PLC. GPI-linked proteins are thought to be preferentially located in [[lipid raft]]s, suggesting a high level of organization within plasma membrane microdomains.


==GPI-anchor synthesis deficiencies==
Defects of ''GPI anchors'' occur in the rare disease [[paroxysmal nocturnal hemoglobinuria]]. In this disease, [[decay-accelerating factor]] (DAF) and [[CD59]] are not properly anchored to [[red blood cell]]s because of the faulty GPI linkage. Without these proteins linked to the cell surface, the [[complement system]] can lyse the cell, and high numbers of RBCs are destroyed, leading to [[hemoglobinuria]]. Other cells are not affected because they have transmembrane forms of DAF and CD59.
Defects in the ''GPI anchors'' synthesis occur in the rare diseases [[paroxysmal nocturnal hemoglobinuria|paroxysmal nocturnal hemoglobinuria PNH]] and [[hyperphosphatasia_with_mental_retardation_syndrome|hyperphosphatasia with mental retardation syndrome, (HPMR)]]. In PNH a clonal defect in blood stem cells in the gene [[PIGA]], that is required for GPI synthesis, results in faulty GPI linkage of [[decay-accelerating factor]] (DAF) and [[CD59]] in [[red blood cell]]s. Without these proteins linked to the cell surface, the [[complement system]] can lyse the cell, and high numbers of RBCs are destroyed, leading to [[hemoglobinuria]].




==External links==
==External links==

Revision as of 16:09, 11 December 2010

Glycosylphosphatidylinositol (pronunciation) (GPI anchor) is a glycolipid that can be attached to the C-terminus of a protein during posttranslational modification. It is composed of a phosphatidylinositol group linked through a carbohydrate-containing linker (glucosamine and mannose glycosidically bound to the inositol residue) to the C-terminal amino acid of a mature protein. The two fatty acids within the hydrophobic phosphatidyl-inositol group anchor the protein to the cell membrane.

Glypiated (GPI-linked) proteins contain a signal peptide, thus directing them into the endoplasmic reticulum (ER). The C-terminus is composed of hydrophobic amino acids that stay inserted in the ER membrane. The hydrophobic end is then cleaved off and replaced by the GPI-anchor. As the protein processes through the secretory pathway, it is transferred via vesicles to the Golgi apparatus and finally to the extracellular space where it remains attached to the exterior leaflet of the cell membrane. Since the glypiation is the sole means of attachment of such proteins to the membrane, cleavage of the group by phospholipases will result in controlled release of the protein from the membrane. The latter mechanism is used in vitro; i.e., the membrane proteins released from the membranes in the enzymatic assay are glypiated protein.

Phospholipase C (PLC) is an enzyme that is known to cleave the phospho-glycerol bond found in GPI-anchored proteins. Treatment with PLC will cause release of GPI-linked proteins from the outer cell membrane. The T-cell marker Thy-1 and acetylcholinesterase, as well as both intestinal and placental alkaline phosphatases, are known to be GPI-linked and are released by treatment with PLC. GPI-linked proteins are thought to be preferentially located in lipid rafts, suggesting a high level of organization within plasma membrane microdomains.

GPI-anchor synthesis deficiencies

Defects in the GPI anchors synthesis occur in the rare diseases paroxysmal nocturnal hemoglobinuria PNH and hyperphosphatasia with mental retardation syndrome, (HPMR). In PNH a clonal defect in blood stem cells in the gene PIGA, that is required for GPI synthesis, results in faulty GPI linkage of decay-accelerating factor (DAF) and CD59 in red blood cells. Without these proteins linked to the cell surface, the complement system can lyse the cell, and high numbers of RBCs are destroyed, leading to hemoglobinuria.


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