The Transmembrane Segment S6 Determines Cation versus Anion Selectivity of TRPM2 and TRPM8

Witschas

Journal of Biological Chemistry

et al. 2010

Self Cite

The closely related cation channels TRPM2 and TRPM8 show completely different requirements for stimulation and are regulated by Ca 2؉ in an opposite manner. TRPM8 is basically gated in a voltage-dependent process enhanced by cold temperatures and cooling compounds such as menthol and icilin. The putative S4 voltage sensor of TRPM8 is closely similar to that of TRPM2, which, however, is mostly devoid of voltage sensitivity. To gain insight into principal interactions of critical channel domains during the gating process, we created chimeras in which the entire S5-pore-S6 domains were reciprocally exchanged. The chimera M2-M8P (i.e. TRPM2 with the pore of TRPM8) responded to ADP-ribose and hydrogen peroxide and was regulated by extracellular and intracellular Ca 2؉ as was wild-type TRPM2. Single-channel recordings revealed the characteristic pattern of TRPM2 with extremely long open times. Only at farnegative membrane potentials (؊120 to ؊140 mV) did differences become apparent because currents were reduced by hyperpolarization in M2-M8P but not in TRPM2. The reciprocal chimera, M8-M2P, showed currents after stimulation with high concentrations of menthol and icilin, but these currents were only slightly larger than in controls. The transfer of the NUDT9 domain to the C terminus of TRPM8 produced a channel sensitive to cold, menthol, or icilin but insensitive to ADPribose or hydrogen peroxide. We conclude that the gating processes in TRPM2 and TRPM8 differ in their requirements for specific structures within the pore. Moreover, the regulation by extracellular and intracellular Ca 2؉ and the single-channel properties in TRPM2 are not determined by the S5-pore-S6 region.TRPM2 and TRPM8 display the highest sequence homology within the family of transient receptor potential (TRP) 2 cation channels (1). TRPM2 is gated mostly by intracellular ADP-ribose (ADPR) and possibly by oxidative stress, for which extracellular application of hydrogen peroxide is an experimental paradigm (2, 3). ADPR binds to the intracellular NUDT9 domain, forming the C-terminal part of the TRPM2 protein (2, 4, 5). Little is known about the further details of the gating mechanism initiated after binding of ADPR; no further protein domains have been identified that mediate gating by interaction with the pore. The resulting currents of TRPM2 show a linear I-V relation, indicating the absence of a voltage dependence of the gating process. In contrast, TRPM8 is, in principle, a voltage-gated channel, equipped with a voltage sensor in the S4-S5 region, in analogy to voltage-gated K ϩ channels (6, 7). Activation requires strongly depolarized membrane potentials. The physiological role of TRPM8 is, however, thought to be not the sensing of voltage but of cold and of some cooling agents such as menthol (1,8,9). It has been demonstrated that these physical and chemical stimuli shift the activation curve of TRPM8 into the negative voltage range corresponding to normal membrane potentials (6, 7). Interestingly, the S4-S5 regions of TRPM8 and TRPM2 are qui...

Section: Resultsmentioning

confidence: 73%

Section: Resultsmentioning

confidence: 99%

Contribution of the S5-Pore-S6 Domain to the Gating Characteristics of the Cation Channels TRPM2 and TRPM8

Witschas

Journal of Biological Chemistry

et al. 2010

Self Cite

American Journal of Physiology-Renal Physiology

“…Because the 563 position in the last transmembrane domain of TRPV5 is close to Asp 542 , it is likely that A563T substitution may affect the architecture of the pore and make it more accommodating for Ca 2ϩ ion permeation, although the lack of an accurate three-dimensional structure of TRPV5 precludes a precise prediction how this happens. It has been recently demonstrated that the substitution of a hydrophobic amino acid residue with a positively charged lysine in the last transmembrane domain of TRPM2 and TRPM8 converts the channels from cation selective to anion selective (20). This suggests that amino acid residues in the last transmembrane domain may participate in defining ion permeation properties directly or indirectly by affecting the conformation of the amino acid residues in the cation filter at the adjacent pore region.…”

Section: Discussionmentioning

confidence: 99%

The A563T variation of the renal epithelial calcium channel TRPV5 among African Americans enhances calcium influx

Na¹,

Zhang²,

Jiang³

et al. 2009

The transient receptor potential cation channel, subfamily V, member 5 (TRPV5) gene, which encodes the Ca 2ϩ channel in the apical membrane of distal convoluted tubule and connecting tubule of the kidney, exhibits an unusually high frequency of nonsynonymous single nucleotide polymorphisms (SNPs) among African Americans. To assess the functional impacts of the nonsynonymous SNP variations in TRPV5, these variants were analyzed with radiotracer 45 (15,16,27). Mice lacking Trpv5 resulted in a 6-to 10-fold increase in urinary Ca 2ϩ excretion, and ultimately in defects in bone mineralization (16).Urinary Ca 2ϩ excretion is an important factor for kidney stone formation and bone health. For instance, urine Ca 2ϩ excretion correlates with bone loss in calcium-stone-forming patients with idiopathic hypercalciuria (3). Interestingly, African Americans exhibit lower urinary Ca 2ϩ excretion than whites (8,25,29,34,35,40,45), and the risk of kidney stones in African American is lower than that in whites (32,36,38). Furthermore, African Americans have higher bone mass (5, 41) and lower incidence of osteoporosis-related fractures than whites (4, 6, 7). The mechanism underlying the lowered urinary Ca 2ϩ in African Americans is not well understood. A lower 25-hydroxyvitamin D concentration in African Americans could result in an increased parathyroid hormone level and in turn renal Ca 2ϩ conservation. However, Braun and colleagues (8) observed significantly lower urinary Ca 2ϩ excretion in adolescent African American girls than white girls in a wide range of controlled Ca 2ϩ intake, whereas the 25-hydroxyvitamin D, 1,25-dihydroxyvitamin D and parathyroid hormone values were not significantly different between the two groups. The difference in bone mass and urinary Ca 2ϩ excretion between blacks and whites is not restricted to Americans; a similar finding was reported in South Africa (10). Thus genetic rather than social and environmental factors may play a major role in the superior renal Ca 2ϩ conservation mechanism in African descendents.Because TRPV5 is a key protein that regulates Ca 2ϩ reabsorption, genetic variations of TRPV5 may influence urinary Ca 2ϩ excretion. Interestingly, TRPV5 gene is one of the four contiguous genes, including EPHB6, TRPV6, TRPV5, and KEL, in chromosome 7q34-35 with striking evidence of a recent selective sweep in European Americans based on the analysis on the single nucleotide polymorphisms (SNPs) of over 100 genes from 24 African Americans and 23 European Americans provided by SeattleSNPs program (1, 37). Akey and colleagues (2) further showed that the TRPV6 haplotype, defined by three nonsynonymous SNPs, is nearly fixed in populations outside Africa, suggesting that these variations may confer a selective advantage, e.g., efficiency in Ca 2ϩ absorption from dairy products or resistance to a pathogen, after early humans migrated out of Africa. The TRPV6 variant with the three nonsynonymous SNPs exhibited increased Ca 2ϩ transport ability and may play a role in absorptive hypercalciuria and ki...

“…TM4 and the TM4-TM5 linker in TRPM8 determines its sensitivity to voltage, temperature and menthol , while the distal part of TM6 determines cation versus anion selectivity, at least in TRPM2 and TRPM8 channels (Kuhn et al, 2007).…”

Section: Structurementioning

confidence: 99%

Pharmacology of transient receptor potential melastatin channels in the vasculature

Zholos¹

2010

British J Pharmacology

Mammalian transient receptor potential melastatin (TRPM) non-selective cation channels, the largest TRP subfamily, are widely expressed in excitable and non-excitable cells where they perform diverse functions ranging from detection of cold, taste, osmolarity, redox state and pH to control of Mg 2+ homeostasis and cell proliferation or death. Recently, TRPM gene expression has been identified in vascular smooth muscles with dominance of the TRPM8 channel. There has been in parallel considerable progress in decoding the functional roles of several TRPMs in the vasculature. This research on native cells is aided by the knowledge of the activation mechanisms and pharmacological properties of heterologously expressed TRPM subtypes. This paper summarizes the present state of knowledge of vascular TRPM channels and outlines several anticipated directions of future research in this area.