Testis-enhanced gene transfer family
The testis-enhanced gene transfer (TEGT) family (TC# 1.A.14) is part of the TOG superfamily and includes members represented in all three domains of life. They include the testis-enhanced gene transfer proteins of mammals, which are expressed at high levels in the testis, the putative glutamate/aspartate binding proteins of plants and animals, the YccA protein of Escherichia coli and the YetJ protein of Bacillus subtilis. These proteins are about 200-250 residues in length and exhibit 7 TMSs.[1]
Homology
Homologues are found in a variety of Gram-negative and Gram-positive bacteria, yeast, fungi, plants, animals and viruses. The E. coli genome encodes three paralogues, YbhL, YbhM and YccA. Distant homologues found in Drosophilia melanogaster and the rat are the N-methyl-D-aspartate receptor-associated protein (NMDARAI) and the N-methyl-D-aspartate receptor glutamate binding chain, respectively. Two others are the rat neural membrane protein 35 and the Arabidopsis thaliana Bax inhibitor-1 (BI-1) protein capable of suppressing Bax-induced cell death in yeast.
BI-1
One of these proteins, TEGT or the Bax Inhibitor-1 (TC# 1.A.14.1.1), has a C-terminal domain that forms a Ca2+-permeable channel.[2] BI-1 is an ER-localized protein that protects against apoptosis and ER stress. BI-1 has been proposed to modulate ER Ca2+ homeostasis by acting as a Ca2+-leak channel. These proteins are distantly related to the ionotropic glutamate-binding protein of the N-methyl D-aspartate (NMDA) receptor of man. Homologues include a putative cold shock inducible protein and a SecY stabilizing protein.[1]
Function
Based on experimental determination of the BI-1 topology, Bultynck et al. proposes that its C-terminal α-helical 20 amino acid peptide catalyzes Ca2+ flux both in vivo and in vitro.[2] The Ca2+-leak properties were conserved among animal, but not plant and yeast orthologs. By mutating one of the critical aspartate residues (D213) in the proposed Ca2+-channel pore in full-length BI-1, D213 proved to be essential for BI-1 dependent ER Ca2+-leak.
Structure
Chang et al. published crystal structures of a bacterial homolog, YetJ (TC# 1.A.14.2.3) at 1.9 Å resolution and characterized its calcium leak activity. Its seven-transmembrane-helix fold features two triple-helix sandwiches wrapped around a central C-terminal helix.[3] Structures obtained in closed and open conformations are reversibly interconvertible by changes in the pH. A hydrogen-bonded perturbed pair of conserved aspartyl residues explains the pH dependence of this transition, and the pH regulates calcium influx in proteoliposomes. Homology models for human BI-1 provided insight into its cytoprotective activity.[3]
Transport Reaction
The generalized reaction catalyzed by TEGT channels is:
- cations (out) ⇌ cations (in)
References
- 1 2 van Stelten, Johna; Silva, Filo; Belin, Dominique; Silhavy, Thomas J. (2009-08-07). "Effects of antibiotics and a proto-oncogene homolog on destruction of protein translocator SecY". Science (New York, N.Y.). 325 (5941): 753–756. doi:10.1126/science.1172221. ISSN 1095-9203. PMC 2832214
. PMID 19661432. - 1 2 Bultynck, Geert; Kiviluoto, Santeri; Henke, Nadine; Ivanova, Hristina; Schneider, Lars; Rybalchenko, Volodymyr; Luyten, Tomas; Nuyts, Koen; De Borggraeve, Wim (2012-01-20). "The C terminus of Bax inhibitor-1 forms a Ca2+-permeable channel pore". The Journal of Biological Chemistry. 287 (4): 2544–2557. doi:10.1074/jbc.M111.275354. ISSN 1083-351X. PMC 3268414. PMID 22128171.
- 1 2 Chang, Yanqi; Bruni, Renato; Kloss, Brian; Assur, Zahra; Kloppmann, Edda; Rost, Burkhard; Hendrickson, Wayne A.; Liu, Qun (2014-06-06). "Structural basis for a pH-sensitive calcium leak across membranes". Science (New York, N.Y.). 344 (6188): 1131–1135. doi:10.1126/science.1252043. ISSN 1095-9203. PMC 4119810. PMID 24904158.
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