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Proteolytic Shedding of ST6Gal-I by BACE1 Regulates the Glycosylation and Function of α4β1 Integrins
Differentiation of monocytes into macrophages is accompanied by increased cell adhesiveness, due in part to the activation of α4β1 integrins. Here we report that the sustained α4β1 activation associated with macrophage differentiation results from expression of β1 integrin subunits that lack α...
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Published in: | The Journal of biological chemistry 2008-09, Vol.283 (39), p.26364 |
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Main Authors: | , , , , |
Format: | Article |
Language: | English |
Online Access: | Get full text |
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Summary: | Differentiation of monocytes into macrophages is accompanied by increased cell adhesiveness, due in part to the activation
of α4β1 integrins. Here we report that the sustained α4β1 activation associated with macrophage differentiation results from
expression of β1 integrin subunits that lack α2â6-linked sialic acids, a carbohydrate modification added by the ST6Gal-I sialyltransferase.
During differentiation of U937 monocytic cells and primary human CD14 + monocytes, ST6Gal-I is down-regulated, leading to β1 hyposialylation and enhanced α4β1-dependent VCAM-1 binding. Importantly,
ST6Gal-I down-regulation results from cleavage by the BACE1 secretase, which we show is dramatically up-regulated during macrophage
differentiation. BACE1 up-regulation, ST6Gal-I shedding, β1 hyposialylation, and α4β1-dependent VCAM-1 binding are all temporally
correlated and share the same signaling mechanism (protein kinase C/Ras/ERK). Preventing ST6Gal-I down-regulation (and therefore
integrin hyposialylation), through BACE1 inhibition or ST6Gal-I constitutive overexpression, eliminates VCAM-1 binding. Similarly,
preventing integrin hyposialylation inhibits a differentiation-induced increase in the expression of an activation-dependent
conformational epitope on the β1 subunit. Collectively, these results describe a novel mechanism for α4β1 regulation and further
suggest an unanticipated role for BACE1 in macrophage function. |
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ISSN: | 0021-9258 1083-351X |
DOI: | 10.1074/jbc.M800836200 |