Specific amino-acid residues in the N-terminus and TM3 implicated in channel function and oligomerization compatibility of connexin43

doi:10.1242/jcs.00604

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doi: 10.1242/10.1242/jcs.00604

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Journal of Cell Science 116, 3189-3201 (2003)
doi: 10.1242/jcs.00604

Research Article

Specific amino-acid residues in the N-terminus and TM3 implicated in channel function and oligomerization compatibility of connexin43

Valérie Lagrée¹^,*, Karin Brunschwig¹^,, Patricia Lopez¹, Norton B. Gilula¹^,, Gabriele Richard² and Matthias M. Falk¹^,¶

¹ Department of Cell Biology, The Scripps Research Institute, 10550 North Torrey Pines Road, La Jolla, CA 92037, USA
² Department of Dermatology and Cutaneous Biology, and Jefferson Institute of Molecular Medicine, Thomas Jefferson University, Philadelphia, PA, USA

^¶ Author for correspondence (e-mail: mfalk{at}scripps.edu)

Accepted 9 April 2003

To identify signals that convey connexin oligomerization compatibility,we have aligned amino-acid sequences of ${alpha}$ and ß groupconnexins (Cx) and compared the physico-chemical propertiesof each homologous amino-acid residue. Four positions were identifiedthat consistently differed between ${alpha}$ and ß-type connexins;two are located in the N-terminal domain (P1 and P2, correspondingto residues 12 and 13 of the Cx43 sequence), and two in thethird trans-membrane-spanning domain TM3 (P3 and P4, correspondingto residues 152 and 153 of the Cx43 sequence). Replacement ofeach of these residues in Cx43 (an ${alpha}$ -type connexin) with thecorresponding residues of Cx32 (a ß-type connexin)resulted in the assembly of all variants into gap junctions;however, only the P4 variant was functional, as indicated by luciferyellow dye transfer assays. The other three variants exerteda moderate to severe dose-dependent, dominant-negative effecton co-expressed wild-type (wt) Cx43 channel activity. Moreover,a significant dose-dependent, trans-dominant inhibition of channelactivity was observed when either one of the N-terminal variantswas co-expressed with wt Cx32. Assembly analyses indicated thatdominant and trans-dominant inhibitory effects appeared to be basedon the oligomerization of wt and variant connexins into mixedconnexons. Interestingly, the identified N-terminal amino acidscoincide with the position of naturally occurring, disease-causingmissense mutations of several ß-connexin genes (Cx26,Cx30, Cx31, Cx32). Our results demonstrate that three of theidentified discriminative amino-acid residues (positions 12,13 and 152) are crucial for Cx43 channel function and suggest thatthe N-terminal amino-acid residues at position 12/13 are involvedin the oligomerization compatibility of ${alpha}$ and ß connexins.

Key words: Gap junction diseases, Gap junctions, Green fluorescent protein, Membrane channels, Oligomeric proteins, Connexin subunit assembly

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