Functional analysis of plasma alpha(2)-macroglobulin from Alzheimer's disease patients with the A2M intronic deletion

Functional analysis of plasma alpha(2)-macroglobulin from Alzheimer's disease patients with the A2M intronic deletion

alpha(2)-Macroglobulin (alpha(2)M) is an abundant plasma/extracellular space protein implicated in clearance of amyloid beta (Abeta), a key constituent of Alzheimer's disease (AD) plaques. alpha(2)M also regulates proteinase and growth factor activities. In recent years, there have been >30...

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Bibliographic Details
Published in:Neurobiology of disease Vol. 14; no. 3; pp. 504 - 512
Main Authors: Hope, Caroline, Mettenburg, Joseph, Gonias, Steven L, DeKosky, Steven T, Kamboh, M Ilyas, Chu, Charleen T
Format: Journal Article
Language:English
Published: United States 01-12-2003
Subjects:
Aged
alpha-Macroglobulins - deficiency
alpha-Macroglobulins - genetics
alpha-Macroglobulins - metabolism
Alzheimer Disease - blood
Alzheimer Disease - genetics
Alzheimer Disease - immunology
Amyloid beta-Peptides - metabolism
Binding Sites - genetics
Blood Proteins - deficiency
Blood Proteins - genetics
Gene Deletion
Humans
Introns - genetics
Mutation - genetics
Protein Binding - genetics
Radioligand Assay
Sequence Deletion
Transforming Growth Factor beta - metabolism
Transforming Growth Factor beta1
Trypsin - metabolism
Up-Regulation - genetics
Up-Regulation - immunology
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Summary:alpha(2)-Macroglobulin (alpha(2)M) is an abundant plasma/extracellular space protein implicated in clearance of amyloid beta (Abeta), a key constituent of Alzheimer's disease (AD) plaques. alpha(2)M also regulates proteinase and growth factor activities. In recent years, there have been >30 genetic studies debating the controversial role of a five-base-pair intronic deletion in the A2M gene in late-onset AD. However, little is known about potential effects of the deletion upon alpha(2)M function. In this study, we examined the subunit and conformational structure of alpha(2)M in AD plasma samples, and its capacity to bind trypsin, transforming growth factor-beta1, and Abeta. Plasma from patients homozygous for the deletion (DD) showed normal alpha(2)M subunit size, conformation, and proteinase inhibitory activity. Interestingly, plasma alpha(2)M from two DD patients showed markedly increased TGF-beta1 binding. Moreover, methylamine-treated DD plasma samples showed modest, but significant, elevations in Abeta binding to alpha(2)M* compared with samples from patients lacking the deletion. These observations suggest a possible functional basis by which the A2M deletion may influence multifactorial AD pathogenesis.
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ISSN:0969-9961
DOI:10.1016/j.nbd.2003.08.005