ABCC7 p.Asp836Arg
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PMID: 23060444
[PubMed]
Wang G et al: "Regulation of Activation and Processing of the Cystic Fibrosis Transmembrane Conductance Regulator (CFTR) by a Complex Electrostatic Interaction between the Regulatory Domain and Cytoplasmic Loop 3."
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12
Second, both K946D and D835R/D836R/E838R mutants were activated by ATP and curcumin to a different extent.
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ABCC7 p.Asp836Arg 23060444:12:29
status: NEWX
ABCC7 p.Asp836Arg 23060444:12:40
status: NEWX
ABCC7 p.Asp836Arg 23060444:12:141
status: NEW13 Third, R764A and R766A mutants enhanced the PKA-dependent activation.
X
ABCC7 p.Asp836Arg 23060444:13:9
status: NEW14 On the other hand, it is very exciting that D835R/D836R/E838R and K946D/H950D and H950R exhibited normal channel processing and activity while D835R/D836R/E838R/K946D/H950D was misprocessed and silent in response to forskolin.
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ABCC7 p.Asp836Arg 23060444:14:50
status: NEWX
ABCC7 p.Asp836Arg 23060444:14:149
status: NEW15 Further, D836R and E838R played a critical role in the asymmetric electrostatic regulation of CFTR processing and S768 phosphorylation may not be involved.
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ABCC7 p.Asp836Arg 23060444:15:9
status: NEW65 If this effect is due to a disruption of the putative electrostatic interaction between CL3 and NEG2, K946D or D835R/D836R/E838R should exhibit the similar effect in the presence of ATP.
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ABCC7 p.Asp836Arg 23060444:65:117
status: NEW67 In contrast, ATP and curcumin dramatically activated the D835R/D836R/E838R mutant.
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ABCC7 p.Asp836Arg 23060444:67:63
status: NEW70 It is interesting that ATP and curucmin only activated the K946D mutant by 40% but activated the D835R/D836R/E838R mutant completely (Fig. 3D).
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ABCC7 p.Asp836Arg 23060444:70:103
status: NEW80 However, neither K946D nor D835R/D836R/E838R was fully activated by ATP alone (Fig. 3B and 3C).
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ABCC7 p.Asp836Arg 23060444:80:33
status: NEW83 Fig. 4A indicates that when the whole-cell current was determined with D835R/D836R/E838R, the application of external forskolin to the bath solution increased the mutant current.
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ABCC7 p.Asp836Arg 23060444:83:77
status: NEW87 Because the D835R/D836R/E838R mutant exhibited the lower current with forskolin than H950R or WT CFTR, a cell capacitance was measured with WT and D835R/D836R/E838R CFTR constructs before and after forskolin was applied to evaluate the contribution of trafficking (20).
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ABCC7 p.Asp836Arg 23060444:87:18
status: NEWX
ABCC7 p.Asp836Arg 23060444:87:153
status: NEW88 Table 1 demonstrates that the cell capacitances of both WT and D835R/D836R/E838R were stable upon activation by forskolin.
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ABCC7 p.Asp836Arg 23060444:88:69
status: NEW90 Although both D835R/D836R/E838R and H950R were activated by forskolin and curcumin greatly, the introduction of K946D and H950D to D835R/D836R/E838R prevented the channel activation by forskolin and curcumin (Fig. 4C and 4D).
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ABCC7 p.Asp836Arg 23060444:90:20
status: NEWX
ABCC7 p.Asp836Arg 23060444:90:137
status: NEW92 In contrast, D835R/D836R/E838R and H950R failed to exhibit the basic activity (Fig. 4A and B).
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ABCC7 p.Asp836Arg 23060444:92:19
status: NEWX
ABCC7 p.Asp836Arg 23060444:92:33
status: NEW95 Upon normalization of the channel current to the cell capacitance, the insertion of K946D/H950D to D835R/D836R/E838R dramatically reduced the CFTR current density (Fig.4D).
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ABCC7 p.Asp836Arg 23060444:95:77
status: NEWX
ABCC7 p.Asp836Arg 23060444:95:105
status: NEW96 In contrast, D835R/D836R/E838R and K946D/H950D and H950R exhibited comparable current densities (Fig. 4D).
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ABCC7 p.Asp836Arg 23060444:96:19
status: NEW99 The putative electrostatic attraction between K946/H950R and D835/D836/E838 failed to inhibit the channel activity but the putative electrostatic attraction of D835R/D836R/E838R with K946D/H950D greatly suppressed the channel activity.
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ABCC7 p.Asp836Arg 23060444:99:166
status: NEW100 The asymmetric effects of R-CL3 electrostatic attractions on CFTR processing - To further determine if the reduction in the current density of K946D/H950D/D835R/D836R/E838R originates from the decrease in the channel expression or the single channel conductance, we carried out western-blotting analysis.
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ABCC7 p.Asp836Arg 23060444:100:161
status: NEW102 The similar cases were seen with D835R/D836R/E838R and H950R and K946D/H950D (Fig.5).
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ABCC7 p.Asp836Arg 23060444:102:39
status: NEW103 However, the insertion of K946D/H950D to D835R/D836R/E838R clearly reduced the fractional mature Band C by 50%.
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ABCC7 p.Asp836Arg 23060444:103:47
status: NEW105 On the other hand, the channel activity of D835R/D836R/E838R/K946D/H950D was still very low (Fig. 4D).
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ABCC7 p.Asp836Arg 23060444:105:18
status: NEWX
ABCC7 p.Asp836Arg 23060444:105:49
status: NEWX
ABCC7 p.Asp836Arg 23060444:105:151
status: NEW108 Therefore, we prepared a control mutant S768D/K946D/H950D to exclude this putative H-bond.
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ABCC7 p.Asp836Arg 23060444:108:20
status: NEWX
ABCC7 p.Asp836Arg 23060444:108:137
status: NEW110 The introduction of D835R to this mutant failed to change the current density.
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ABCC7 p.Asp836Arg 23060444:110:19
status: NEW111 However, the insertion of D836R or E838R to S768D/K946D/H950D dramatically reduced the CFTR current density (Fig.4D).
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ABCC7 p.Asp836Arg 23060444:111:26
status: NEW112 Fig.5 further demonstrates that the fractions of the mature Band C of S768D/K946D/H950D/D836R and S768D/K946D/H950D/E838R were also significantly decreased by 45%.
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ABCC7 p.Asp836Arg 23060444:112:88
status: NEW117 Because R764X and R766M were reported with CF patients (www.genet.sickkids.on.ca/cftr/app), we investigated if missense alanine mutation of R764 and R766 alters the channel processing and activity.
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ABCC7 p.Asp836Arg 23060444:117:175
status: NEW118 Fig. 4D demonstrates that both R764A and R766A exhibited a normal channel density.
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ABCC7 p.Asp836Arg 23060444:118:164
status: NEW121 The K1/2 for PKA activation of R764A and R766A increased from 10 units/ml to 25 and 44 units/ml, respectively.
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ABCC7 p.Asp836Arg 23060444:121:47
status: NEW123 To support this hypothesis, we determined if S832C is closed enough to S768C to form a detectable disulfide-bond crosslinking based on the Cys-free CFTR construct.
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ABCC7 p.Asp836Arg 23060444:123:47
status: NEW139 Second, the curcumin sensitivity was also increased for K946A, K946D and D835R/D836R/E838R (Fig.3).
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ABCC7 p.Asp836Arg 23060444:139:79
status: NEW140 Finally, it is very exciting that the putative electrostatic attraction between K946D/H950D and D835R/D836R/E838R dramatically suppressed the channel activity by stopping the channel processing or opening(10).
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ABCC7 p.Asp836Arg 23060444:140:102
status: NEW150 Otherwise, a putative electrostatic attraction of CL3 (K946D/H950D) with both NEG2 (D836R or E838R) and the S768 phosphorylation site (R764 or R766) may result in misprocessing and low channel activity (Fig.8B).
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ABCC7 p.Asp836Arg 23060444:150:43
status: NEWX
ABCC7 p.Asp836Arg 23060444:150:84
status: NEWX
ABCC7 p.Asp836Arg 23060444:150:112
status: NEW10 Second, both K946D and D835R/D836R/ E838R mutants were activated by ATP and curcumin to a different extent.
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ABCC7 p.Asp836Arg 23060444:10:29
status: NEW69 If this effect is due to a disruption of the putative electrostatic interaction between CL3 and NEG2, K946D or D835R/D836R/ E838R should exhibit a similar effect in the presence of ATP.
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ABCC7 p.Asp836Arg 23060444:69:117
status: NEW79 Asymmetric Electrostatic Regulation of CFTR NOVEMBER 23, 2012ߦVOLUME 287ߦNUMBER 48 JOURNAL OF BIOLOGICAL CHEMISTRY 40485 cally activated the D835R/D836R/E838R mutant.
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ABCC7 p.Asp836Arg 23060444:79:160
status: NEW82 It is interesting that ATP and curcumin only activated the K946D mutant by 40% but activated the D835R/ D836R/E838R mutant completely (Fig. 3D).
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ABCC7 p.Asp836Arg 23060444:82:104
status: NEW106 Table 1 demonstrates that the cell capacitances of both WT and D835R/D836R/E838R were stable upon activation by forskolin.
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ABCC7 p.Asp836Arg 23060444:106:69
status: NEW113 Upon normalization of the channel current to the cell capacitance, the insertion of K946D/H950D to D835R/D836R/ E838R dramatically reduced the CFTR current density (Fig. 4D).
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ABCC7 p.Asp836Arg 23060444:113:105
status: NEW114 In contrast, D835R/D836R/E838R and K946D/H950D and H950R exhibited comparable current densities (Fig. 4D).
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ABCC7 p.Asp836Arg 23060444:114:19
status: NEW120 Similar cases were seen with D835R/ D836R/E838R and H950R and K946D/H950D (Fig. 5).
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ABCC7 p.Asp836Arg 23060444:120:36
status: NEW127 Macroscopic currents across inside-out membrane patches excised from transfected HEK-293T cells expressing CFTR mutants K946A (A), K946D (B) and D835R/D836R/E838R (C) by using a ramp protocol (afe;80 mV) are shown.
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ABCC7 p.Asp836Arg 23060444:127:151
status: NEW131 The relative activity of K946D was significantly smaller than that of D835R/D836R/E838R (n afd; 3-4; *, p b0d; 0.05, unpaired t test); error bars, S.E. Asymmetric Electrostatic Regulation of CFTR NOVEMBER 23, 2012ߦVOLUME 287ߦNUMBER 48 JOURNAL OF BIOLOGICAL CHEMISTRY 40487 The Effects of Ser-768 Phosphorylation on the Asymmetric NEG2-CL3 Electrostatic Regulation of the CFTR Activity and Processing-Although previous studies demonstrated that Ser-768 phosphorylation had no electrostatic contribution to the channel gating, nonphosphorylated Ser-768 may form a strong putative H-bond with H950D to affect the CL3-NEG2 electrostatic interaction (10).
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ABCC7 p.Asp836Arg 23060444:131:76
status: NEW135 However, the insertion of D836R or E838R to S768D/K946D/H950D dramatically reduced the CFTR current density (Fig. 4D).
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ABCC7 p.Asp836Arg 23060444:135:26
status: NEW136 Fig. 5 further demonstrates that the fractions of the mature Band C of S768D/K946D/H950D/D836R and S768D/K946D/H950D/ E838R were also significantly decreased by 45%.
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ABCC7 p.Asp836Arg 23060444:136:89
status: NEW146 Effects of electrostatic interactions on current densities of CFTR mutants at the R-CL3 interface. A-C, whole cell currents from transfected HEK-293T cells expressing CFTR mutants D835R/D836R/E838R (A), H950R (B), and K946D/H950D/D835R/D836R/E838R (C) recorded by using a ramp protocol (afe;40 mV).
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ABCC7 p.Asp836Arg 23060444:146:186
status: NEWX
ABCC7 p.Asp836Arg 23060444:146:236
status: NEW151 The currents mediated by S768D/K946D/H950D/D836R and S768D/K946D/H950D/E838R were statistically smaller than the S768D/K946D/H950D current (n afd; 3,*, p b0d; 0.05, unpaired t test); error bars, S.E. TABLE 1 WholecellcurrentsIm (picoamperes)andcapacitancesCm (picofarads) of HEK-293T cells expressing CFTR constructs in response to forskolin Constructs Stimulated Im Control Cm Stimulated Cm n WT-CFTR 701.6 afe; 9.0 17.4 afe; 0.9 16.4 afe; 1.1 3 D835R/D836R/E838R 539.5 afe; 5.3 15.0 afe; 1.0 16.2 afe; 0.8 3 Asymmetric Electrostatic Regulation of CFTR 40488 JOURNAL OF BIOLOGICAL CHEMISTRY VOLUME 287ߦNUMBER 48ߦNOVEMBER 23, 2012 at SEMMELWEIS UNIV OF MEDICINE on December , The K1/2 for PKA activation of R764A and R766A increased from 10 units/ml to 25 and 44 units/ml, respectively.
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ABCC7 p.Asp836Arg 23060444:151:43
status: NEWX
ABCC7 p.Asp836Arg 23060444:151:468
status: NEW168 Second, the curcumin sensitivity was also increased for K946A, K946D, and D835R/ D836R/E838R (Fig. 3).
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ABCC7 p.Asp836Arg 23060444:168:81
status: NEW169 Finally, it is very exciting that the putative electrostatic attraction between K946D/H950D and D835R/D836R/E838R dramatically suppressed the maximal channel activity by stopping the channel processing or opening (10).
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ABCC7 p.Asp836Arg 23060444:169:102
status: NEW189 Otherwise, a putative electrostatic attraction of CL3 (K946D/H950D) with both NEG2 (D836R or E838R) and the Ser-768 phosphorylation site (Arg-764 or Arg-766) may result in misprocessing and low channel activity (Fig. 8B).
X
ABCC7 p.Asp836Arg 23060444:189:84
status: NEW