Structural basis of Na super(+)-independent and cooperative substrate/product antiport in CaiT

Transport of solutes across biological membranes is performed by specialized secondary transport proteins in the lipid bilayer, and is essential for life. Here we report the structures of the sodium-independent carnitine/butyrobetaine antiporter CaiT from Proteus mirabilis (PmCaiT) at 2.3-Aa and from Escherichia coli (EcCaiT) at 3.5-Aa resolution. CaiT belongs to the family of betaine/carnitine/choline transporters (BCCT), which are mostly Na super(+) or H super(+) dependent, whereas EcCaiT is Na super(+) and H super(+) independent. The three-dimensional architecture of CaiT resembles that of the Na super(+)-dependent transporters LeuT and BetP, but in CaiT a methionine sulphur takes the place of the Na super(+) ion to coordinate the substrate in the central transport site, accounting for Na super(+)-independent transport. Both CaiT structures show the fully open, inward-facing conformation, and thus complete the set of functional states that describe the alternating access mechanism. EcCaiT contains two bound butyrobetaine substrate molecules, one in the central transport site, the other in an extracellular binding pocket. In the structure of PmCaiT, a tryptophan side chain occupies the transport site, and access to the extracellular site is blocked. Binding of both substrates to CaiT reconstituted into proteoliposomes is cooperative, with Hill coefficients up to 1.7, indicating that the extracellular site is regulatory. We propose a mechanism whereby the occupied regulatory site increases the binding affinity of the transport site and initiates substrate translocation.