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Sci Rep
2016 Jun 09;6:27647. doi: 10.1038/srep27647.
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Functional and pharmacological characterization of two different ASIC1a/2a heteromers reveals their sensitivity to the spider toxin PcTx1.
Joeres N
,
Augustinowski K
,
Neuhof A
,
Assmann M
,
Gründer S
.
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Acid Sensing Ion Channels (ASICs) detect extracellular proton signals and are involved in synaptic transmission and pain sensation. ASIC subunits assemble into homo- and heteromeric channels composed of three subunits. Single molecule imaging revealed that heteromers composed of ASIC1a and ASIC2a, which are widely expressed in the central nervous system, have a flexible 2:1/1:2 stoichiometry. It was hitherto not possible, however, to functionally differentiate these two heteromers. To have a homogenous population of ASIC1a/2a heteromers with either 2:1 or 1:2 stoichiometry, we covalently linked subunits in the desired configuration and characterized their functional properties in Xenopus oocytes. We show that the two heteromers have slightly different proton affinity, with an additional ASIC1a subunit increasing apparent affinity. Moreover, we found that zinc, which potentiates ASIC2a-containing ASICs but not homomeric ASIC1a, potentiates both heteromers. Finally, we show that PcTx1, which binds at subunit-subunit interfaces of homomeric ASIC1a, inhibits both heteromers suggesting that ASIC2a can also contribute to a PcTx1 binding site. Using this functional fingerprint, we show that rat cortical neurons predominantly express the ASIC1a/2a heteromer with a 2:1 stoichiometry. Collectively, our results reveal the contribution of individual subunits to the functional properties of ASIC1a/2a heteromers.
Figure 1. The two different ASIC1a/2a heteromers can be distinguished via their apparent affinity for protons.(a) Representative current traces of homo- and heteromeric ASICs, which were activated for 10âs with solutions of decreasing pH and allowed to recover for 50âs at pH 7.4. (b) Concentration-response curves of normalized currents. Maximal current amplitudes were 5.0â±â0.8âμA (ASIC1a), 16.1â±â2.7âμA (ASIC1a/2a), 13.3â±â3.4âμA (ASIC1a-2a-1a), 11.3â±â3.3âμA (ASIC1a-2a-2a), and 1.9â±â0.3âμA (ASIC2a), respectively. The EC50 values of ASIC1a-2a-1a and ASIC1a-2a-2a were significantly different (pâ<â0.001). There was also a slight significant difference in the Hill-coefficients (pâ<â0.05). Data are reported as meanâ±âSEM (nâ=â12â17 individual oocytes).
Figure 2. The two different ASIC1a/2a heteromers can be distinguished via their steady-state desensitization curves.(a) Representative current traces of homo- and heteromeric ASICs, which were activated for 10âs with pH 4.0 (pH 6.0 for ASIC1a) and allowed to recover for 120âs in a bath solution with decreasing pH. (b) Concentration-response curves of normalized currents. Maximal current amplitudes were 9.0â±â2.2âμA (ASIC1a), 22.9â±â2.3âμA (ASIC1a/2a), 25.7â±â2.1âμA (ASIC1a-2a-1a), 12.5â±â1.7âμA (ASIC1a-2a-2a), and 2.8â±â0.4âμA (ASIC2a), respectively. The curves of both concatamers differ in their IC50 values (pâ<â0.001) as well as in their Hill-coefficients (pâ<â0.001), which were similar to that of the dominant ASIC form in the constructs. Data are reported as meanâ±âSEM (nâ=â8â16 individual oocytes).
Figure 3. Tachyphylaxis is absent in ASIC1a/2a heteromers.ASICs were repeatedly activated for 10âs with pH 4.0 and allowed to recover for 50âs at pH 7.4. Only homomeric ASIC1a showed tachyphylaxis. Maximal current amplitudes were 30.6â±â3.6âμA (ASIC1a), 26.2â±â3.6âμA (ASIC1a/2a), 20.3â±â5.0âμA (ASIC1a-2a-1a), and 15.1â±â4.0âμA (ASIC1a-2a-2a), respectively. Data are reported as meanâ±âSEM (nâ=â4â9 individual oocytes; measurements for ASIC1a are from one week).
Figure 4. Both concatamers of ASIC1a/2a are potentiated by Zn2+.Concentration-response curves for normalized currents with and without Zn2+. The EC50 values of ASIC1a/2a (pâ=â0.045), ASIC1a-2a-1a () and ASIC1a-2a-2a (pâ<â0.01) were significantly left-shifted in the presence of 300âμm Zn2+. There was also a significant increase in the Hill-coefficient of ASIC1a-2a-1a (pâ<â0.001) and ASIC1a/2a (pâ<â0.01) but not of ASIC1a-2a-2a (pâ=â0.8). Maximal current amplitudes were 14.5â±â3.1âμA (ASIC1a/2a), 20.3â±â3.5âμA (ASIC1a/2a + Zn2+), 14.2â±â3.1âμA (ASIC1a-2a-1a), 17.6â±â3.4âμA (ASIC1a-2a-1a + Zn2+), 12.3â±â1.8âμA (ASIC1a-2a-2a) and 11.9â±â3.3âμA (ASIC1a-2a-2a + Zn2+), respectively. Data are reported as meanâ±âSEM (nâ=â10â13 individual oocytes).
Figure 5. Inhibition by PcTx1 can distinguish between the two ASIC1a/2a heteromers.(a) Representative current traces showing the inhibition of different ASICs by PcTx1. ASICs were activated with pH 4.0 (pH 6.0 for homomeric ASIC1a) for 10 s and allowed to recover for 120âs in pH 6.95 (pH 7.4 for ASIC1a). 50ânM PcTx1 was applied in the conditioning solution before the second activation. (b) Comparison of the inhibition by PcTx1 of the different ASICs. The difference between ASIC1a-2a-1a and ASIC1a-2a-2a (pâ<â0.001) as well as the difference between ASIC1a-2a-1a and ASIC1a/2a (pâ<â0.001) were significant. There was no significant difference between ASIC1a/2a and ASIC1a-2a-2a. Maximal current amplitudes were 9.6â±â1.9âμA (ASIC1a), 15.2â±â1.7âμA (ASIC1a/2a), 12.9â±â2.8âμA (ASIC1a-2a-1a), and 9.1â±â1.4âμA (ASIC1a-2a-2a), respectively. Data are reported as meanâ±âSEM (nâ=â8â10).
Figure 6. PcTx1 inhibits ASIC1a/2a heteromers in rat cortical neurons.(a) Representative current trace showing the inhibition of ASICs by PcTx1 at conditioning pH 6.95. ASICs were activated with pH 6.0 for 15 s and allowed to recover for 60âs in pH 6.95. 50ânM PcTx1 was applied in the conditioning solution before the third activation. (b) Quantitative analysis of six measurements like the one shown in (a). Symbols represent six individual neurons, bars represent mean and SD, respectively. Conditioning pH 6.95 desensitized homomeric ASIC1a and heteromeric ASIC1a/2b. Co-application of PcTx1 revealed the PcTx1-sensitivity of the remaining ASIC1a/2a heteromers in these neurons.
Figure 7. Possible interactions of PcTx1 with subunit interfaces of the ASIC1a-2a-2a heteromer.The homology model of the heteromer with ASIC1a (blue) and ASIC2a (red) is shown in cartoon and PcTx1 (green) in solvent-accessible surface representation. Boxes illustrate the amino acids (stick and spheres representation) in the ASIC1a/2a subunit interfaces that interact with PcTx1, namely Gly214, Gly216, Glu236, Thr238, Glu241, and Glu352 in rASIC2a and Gly215, Gly217, Asp237, Thr239, Glu242, Asp349, and Glu353 in rASIC1a. Five interacting amino acids are completely conserved between cASIC1, rASIC1a and rASIC2a. Numbers of amino acids refer to rASIC1a and rASIC2a, respectively.
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