Abstract
Background: Epitope tags and fluorescent fusion proteins have become indispensable molecular tools for studies
in the fields of biochemistry and cell biology. The knowledge collected on the subdomain organization of the two
subunits of the adhesion complex dystroglycan (DG) enabled us to insert the 10 amino acids myc-tag at different
locations along the α-subunit, in order to better visualize and investigate the DG complex in eukaryotic cells.
Results: We have generated two forms of DG polypeptides via the insertion of the myc-tag 1) within a flexible
loop (between a.a. 170 and 171) that separates two autonomous subdomains, and 2) within the C-terminal domain
in position 500. Their analysis showed that double-tagging (the β-subunit is linked to GFP) does not significantly
interfere with the correct processing of the DG precursor (pre-DG) and confirmed that the α-DG N-terminal domain
is processed in the cell before α-DG reaches its plasma membrane localization. In addition, myc insertion in position
500, right before the second Ig-like domain of α-DG, proved to be an efficient tool for the detection and
pulling-down of glycosylated α-DG molecules targeted at the membrane.
Conclusions: Further characterization of these and other myc-permissive site(s) will represent a valid support for
the study of the maturation process of pre-DG and could result in the creation of a new class of intrinsic
doubly-fluorescent DG molecules that would allow the monitoring of the two DG subunits, or of pre-DG, in cells
without the need of antibodies.
Original language | English |
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Pages (from-to) | 14-21 |
Number of pages | 8 |
Journal | BMC Biochemistry |
Volume | 2012 |
DOIs | |
Publication status | Published - 2012 |
Keywords
- dystroglycan