Figures and data
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the Effect of overexpression of ABHD6 on the reduction of peak current in AMPARs.
(A) Plasmid abbreviations and variant combinations of AMPAR.
(B-D) Representative traces (left) and summary graphs of the peak amplitudes (right) of 10 mM glutamate-induced currents in HEK 293T cells transfected with GluA1-3 (black), GluA1-3 + ABHD6 (orange), GluA1-3 + TARP γ-2 (blue), GluA1-3 + TARP γ-2 + ABHD6 (red).
The statistical method was one-way ANOVA followed by a two-way comparison (*P < 0.05; **P < 0.01; ***P < 0.001. Table. EV1.2).
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Overexpression of ABHD6 accelerated the deactivation of AMPARs-TARP γ-2 complexes in HEK 293T cells.
The normalized traces, and the summary bar graphs of the τ w, deact of Glutamate (10 mM Glu, 1 ms) induced currents in the outside-out patch from HEK 293T cells transfected with GluA (black), GluA + ABHD6 (orange), GluA + TARP γ-2 (blue), and GluA + TARP γ-2 + ABHD6 (red). (A) GluA1i. (B) GluA1o. (C) GluA2(Q)i-R. (D) GluA2(Q)o-R. (E) GluA2(Q)i-G. (F) GluA2(Q)o-G. (G) GluA2(Q)i-R-TARP γ-2 tandem. (I) GluA1i-TARP γ-2 tandem. γ2-containing GluA receptors could be isolated when 50 μM spermine in the internal solution and recorded at +50 mV, the average traces and the normalized traces (right), and the summary bar graphs of the τ w, deact of Glutamate (10 mM Glu, 1 ms) induced currents in the outside-out patch recorded at +50 mV from HEK 293T cells transfected with GluA-TARP γ-2 tandem (blue), GluA-TARP γ-2 tandem + ABHD6 (red). (H) GluA2(Q)i-R-TARP γ-2. (J) GluA1i-TARP γ-2. The statistical method was one-way ANOVA followed by a two-way comparison (*P < 0.05; **P < 0.01; ***P < 0.001. Table. EV2.2).
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Overexpression of ABHD6 accelerated the desensitization of AMPARs-TARP γ-2 complexes in HEK 293T cells.
The normalized traces, and the summary bar graphs of the τ w, des of Glutamate (10 mM Glu, 100 ms) induced currents in the outside-out patch from HEK 293T cells transfected with GluA (black), GluA + ABHD6 (orange), GluA + TARP γ-2 (blue), and GluA + TARP γ-2 + ABHD6 (red).(A) GluA1i. (B) GluA1o. (C) GluA2(Q)i-R. (D) GluA2(Q)o-R. (E) GluA2(Q)i-G. (F) GluA2(Q)o-G. (G) GluA2(Q)i-R-TARP γ-2 tandem. (I) GluA1i-TARP γ-2 tandem. TARP γ-2-containing GluA receptors could be isolated when 50 μM spermine in the internal solution and recorded at +50 mV, the average traces and the normalized traces (right), and the summary bar graphs of the τ w, des and peak amplitude of Glutamate (10 mM Glu, 100 ms) induced currents in the outside-out patch recorded at +50 mV from HEK 293T cells transfected with GluA-TARP γ-2 tandem (blue), GluA-TARP γ-2 tandem + ABHD6 (red). (H) GluA2(Q)i-R-TARP γ-2. (J) GluA1i-TARP γ-2. The statistical method was one-way ANOVA followed by a two-way comparison (*P < 0.05; **P < 0.01; ***P < 0.001. Table. EV3.2).
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Overexpression of ABHD6 slows the recovery from desensitization of GluA1i-TARP γ-2 complexes in HEK 293T cells.
(A-F) Glutamate (Glu, 10 mM) induced currents in an outside-out patch excised from an HEK 293T cell transfected with GluA (black), GluA + ABHD6 (orange), GluA + TARP γ-2 (blue), and GluA+ TARP γ-2 + ABHD6 (red). The recovery ratio curves from desensitization, and the summary bar graphs of the τ w, rec. (A) GluA1i. (B) GluA1o. (C) GluA2(Q)i-R. (D) GluA2(Q)o-R. (E) GluA2(Q)i-G. (F) GluA2(Q)o-G. (G) GluA2(Q)i-R-TARP γ-2 tandem. (H) GluA1i-TARP γ-2 tandem. The statistical method was one-way ANOVA followed by a two-way comparison (*P < 0.05; **P < 0.01; ***P < 0.001. Table. EV4.2).
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Overexpression of ABHD6 accelerated the deactivation and desensitization of GluA1i/GluA2(R)i-G receptors-TARP γ-2 complexes in HEK 293T cells, slowed the recovery of GluA1i/GluA2(R)i-G receptors in the presence and absence of TARP γ-2.
(A) The normalized traces and the summary bar graphs of the τ w, deact of Glutamate (10 mM Glu, 1 ms) induced currents in the outside-out patch recorded at -60 mV from HEK 293T cells transfected with GluA1i/GluA2(R)i-G (black), GluA1i/GluA2(R)i-G + ABHD6 (orange), GluA1i/GluA2(R)i-G + TARP γ-2 (blue), and GluA1i/GluA2(R)i-G + TARP γ-2 + ABHD6 (red).
(B) The normalized traces and the summary bar graphs of the τ w, des and peak amplitude of Glutamate (10 mM Glu, 100 ms) induced currents in the outside-out patch recorded at -60 mV from HEK 293T cells transfected with GluA1i/GluA2(R)i-G (black), GluA1i/GluA2(R)i-G + ABHD6 (orange), GluA1i/GluA2(R)i-G + TARP γ-2 (blue), and GluA1i/GluA2(R)i-G + TARP γ-2 + ABHD6 (red).
(C) Glutamate (Glu, 10 mM) induced currents in an outside-out patch excised from an HEK 293T cell transfected with GluA1i/GluA2(R)i-G (black), GluA1i/GluA2(R)i-G + ABHD6 (orange), GluA1i/GluA2(R)i-G + TARP γ-2 (blue), and GluA1i/GluA2(R)i-G + TARP γ-2 + ABHD6 (red). The first application of 100 ms glutamate was followed by a second glutamate application at increasing pulse intervals at -60 mV. The recovery ratio curves from desensitization (C1), and the summary bar graphs of the τ w, rec (C2). The statistical method was one-way ANOVA followed by a two-way comparison (*P < 0.05; ***P < 0.01; ***P < 0.001. Table. EV5.2)
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Schematic illustration of the AMPAR subunit and the Sequence alignment of RNA splice variants and editing of AMPAR.
(A) Topology of a single AMPAR subunit in the plasma membrane. Each subunit consists of an extracellular N-terminal domain (NTD), a ligand-binding domains (LBD), a transmembrane domain (TMD, M1–4) and an intracellular C-terminal domain (CTD), the flip/flop splice variants and the RNA editing sites (Q/R and R/G) are also shown.
(B) Sequence alignment of RNA splice variants and editing. Q/R editing sites (red letters) (GluA2), R/G editing sites (purple letters) (GluA2, A3), flip/flop splice variants (Grey box) (GluA1–A3). Complete sequences can be found in UniProt. Sequences are homologous and conserved in mouse, rat and human.
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Average traces of deactivation of AMPAR with overexpression of ABHD6 in HEK 293T cells.
The average traces of Glutamate (10 mM Glu, 1 ms) induced currents in the outside-out patch from HEK 293T cells transfected with GluA (black), GluA + ABHD6 (orange), GluA + TARP γ-2 (blue), and GluA + TARP γ-2 + ABHD6 (red). (A) GluA1i. (B) GluA1o. (C) GluA2(Q)i-R. (D) GluA2(Q)o-R. (E) GluA2(Q)i-G. (F) GluA2(Q)o-G. (G, H) GluA2(Q)i-R-TARP γ-2 tandem. (I, J) GluA1i-TARP γ-2 tandem.
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Average traces of desensitization of AMPAR with overexpression of ABHD6 in HEK 293T cells.
The average traces of Glutamate (10 mM Glu, 500 ms) induced currents in the outside-out patch from HEK 293T cells transfected with GluA (black), GluA + ABHD6 (orange), GluA + TARP γ-2 (blue), and GluA + TARP γ-2 + ABHD6 (red). (A) GluA1i. (B) GluA1o. (C) GluA2(Q)i-R. (D) GluA2(Q)o-R. (E) GluA2(Q)i-G. (F) GluA2(Q)o-G. (G, H) GluA2(Q)i-R-TARP γ-2 tandem. (I, J) GluA1i-TARP γ-2 tandem.
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Typical traces of the recovery from desensitization of AMPAR in HEK 293T cells.
(A-F) Glutamate (Glu, 10 mM) induced currents in an outside-out patch excised from an HEK 293T cell transfected with GluA (black), GluA + ABHD6 (orange), GluA + TARP γ-2 (blue), and GluA+ TARP γ-2 + ABHD6 (red). The first application of 100 ms glutamate was followed by a second glutamate application at increasing pulse intervals at -60 mV. The typical traces from a cell are normalized and aligned to the peak. The typical traces of the recovery from desensitization. (A) GluA1i. (B) GluA1o. (C) GluA2(Q)i-R. (D) GluA2(Q)o-R. (E) GluA2(Q)i-G. (F) GluA2(Q)o-G. (G) GluA2(Q)i-R-TARP γ-2 tandem. (H) GluA1i-TARP γ-2 tandem.
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Average traces of the deactivation, desensitization and recovery from desensitization of GluA1i/GluA2(R)i-G receptors-TARP γ-2 complexes in HEK 293T cells.
(A) The average traces of the τ w, deact of Glutamate (10 mM Glu, 1 ms) induced currents in the outside-out patch recorded at -60 mV from HEK 293T cells transfected with GluA1i/GluA2(R)i-G (black), GluA1i/GluA2(R)i-G + ABHD6 (orange), GluA1i/GluA2(R)i-G + TARP γ-2 (blue), and GluA1i/GluA2(R)i-G + TARP γ-2 + ABHD6 (red).
(B) The average traces of the τ w, des and peak amplitude of Glutamate (10 mM Glu, 100 ms) induced currents in the outside-out patch recorded at -60 mV from HEK 293T cells transfected with GluA1i/GluA2(R)i-G (black), GluA1i/GluA2(R)i-G + ABHD6 (orange), GluA1i/GluA2(R)i-G + TARP γ-2 (blue), and GluA1i/GluA2(R)i-G + TARP γ-2 + ABHD6 (red).
(C) The typical trace of recovery from desensitization. Glutamate (Glu, 10 mM) induced currents in an outside-out patch excised from an HEK 293T cell transfected with GluA1i/GluA2(R)i-G (black), GluA1i/GluA2(R)i-G + ABHD6 (orange), GluA1i/GluA2(R)i-G + TARP γ-2 (blue), and GluA1i/GluA2(R)i-G + TARP γ-2 + ABHD6 (red). The first application of 100 ms glutamate was followed by a second glutamate application at increasing pulse intervals at -60 mV.
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Pearson’s correlation between natural logarithm peak amplitude (pA) and the τ w, deact and τ w, des coexpression with various GluA subunits.
(A-J) Pearson’s correlation and Local Polynomial Regression (loess) with 95% confidence intervals between natural logarithm peak amplitude (pA) and the τ w, deact (ms) of Glutamate (10 mM Glu, 1 ms) induced currents and τ w, des (ms) of Glutamate (10 mM Glu, 100 ms) induced currents in the outside-out patch from HEK 293T cells transfected with various GluA subunits.
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Summary of peak amplitude(pA) of GluAs when co-transfected with/without γ-2 or/and ABHD6.
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Summary of P values for comparison of peak amplitude.
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Summary of τ w, deact (ms) of GluAs when co-transfected with/without γ-2 or/and ABHD6.
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Summary of P values for comparison of τ w, deact.
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Summary of τ w, des (ms) of GluAs when co-transfected with/without γ-2 or/and ABHD6.
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Summary of P values for comparison of τ w, des.
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Summary of τ w, rec (ms) of GluAs when co-transfected with/without γ-2 or/and ABHD6.
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Summary of P values for comparison of τ w, rec.
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Summary of GluA1i/GluA2(R)i-G receptors when co-transfected with/without γ-2 or/and ABHD6.
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