ABCC1 p.Pro255Ala

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PMID: 12948592 [PubMed] Ito K et al: "Mutation of proline residues in the NH(2)-terminal region of the multidrug resistance protein, MRP1 (ABCC1): effects on protein expression, membrane localization, and transport function."
No. Sentence Comment
107 The seven single (P196A, P205A, P207A, P209A, P235A, P255A, and P272A) and two multiply substituted CL3 mutants (P196/205/207/209A and P235/255A) could also be stably expressed in HeLa cells.
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ABCC1 p.Pro255Ala 12948592:107:53
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147 GFP-tagged MRP1 proteins are shown in green; nuclei were stained with propidium iodide and are shown in red. (C) HeLa cells stably expressing wild-type MRP1, MRP1-P235A, MRP1-P255A, MRP1-P235/255A, and MRP1-P196/205/207/209A were cultured and processed for immunofluorescence and confocal microscopy as described in panel A.
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ABCC1 p.Pro255Ala 12948592:147:175
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149 Duplicate immunoblots of the P235A, P255A, P235/255A, and P272A MRP1 mutants probed with MAb QCRL-1 and MAb MRPr1 indicated that detection of the P255A and P235/P255A mutant MRP1 proteins relative to wild-type MRP1 by MAb MRPr1 was lower than that by MAb QCRL-1 (not shown).
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ABCC1 p.Pro255Ala 12948592:149:36
status: NEW
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ABCC1 p.Pro255Ala 12948592:149:146
status: NEW
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ABCC1 p.Pro255Ala 12948592:149:161
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151 When MRP1-P235A was detected with MAb QCRL-1, the signal intensity was approximately 1.8-fold higher than that for wild-type MRP1, while the signal intensity for MRP1-P235/P255A was approximately 2.3-fold higher (Fig. 5A).
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ABCC1 p.Pro255Ala 12948592:151:172
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153 Thus, MRP1-P235A Fig. 5.
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ABCC1 p.Pro255Ala 12948592:153:106
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154 Dot blot analyses of MRP1 expression in membranes from HeLa cells expressing CL3 mutants MRP1-P235A, MRP1-P255A, and MRP1-P235/255A.
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ABCC1 p.Pro255Ala 12948592:154:106
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156 MRP1-P235A and MRP1-P235/255A mutants probed with (A) MAb QCRL-1 and (B) MAb MRPr1.
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ABCC1 p.Pro255Ala 12948592:156:5
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157 MRP1-P255A and MRP1-P235/255A mutants probed with (C) MAb QCRL-1 and (D) MAb MRPr1.
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ABCC1 p.Pro255Ala 12948592:157:5
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159 (A and B) Wild-type MRP1 (n); MRP1-P235A (E); MRP1-P235/255A (z).
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ABCC1 p.Pro255Ala 12948592:159:35
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160 (C and D) Wild-type MRP1 (n); MRP1-P255A (E); MRP1-P235/255A (z).
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ABCC1 p.Pro255Ala 12948592:160:35
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162 We next compared the immunoreactivity of the double mutant MRP1-P235/255A and the single mutant MRP1-P255A.
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ABCC1 p.Pro255Ala 12948592:162:61
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ABCC1 p.Pro255Ala 12948592:162:101
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163 When detected with MAb QCRL-1, the signal intensity for MRP1-P255A was approximately 1.3-fold higher than that for wild-type MRP1 (Fig. 5C).
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ABCC1 p.Pro255Ala 12948592:163:42
status: NEW
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ABCC1 p.Pro255Ala 12948592:163:61
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164 In contrast, the signal intensity of MRP1-P255A detected with MAb MRPr1 was only 50% that of wild-type MRP1 detected with the same MAb (Fig. 5D).
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ABCC1 p.Pro255Ala 12948592:164:42
status: NEW
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ABCC1 p.Pro255Ala 12948592:164:53
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165 Overall, these findings suggest that substitution of Pro255 with Ala might introduce a change in the structure of this region of MRP1 such that the MRPr1 epitope is less accessible to the MAb.
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ABCC1 p.Pro255Ala 12948592:165:53
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167 Plasma membrane localization of CL3 MRP1-Pro mutants is unchanged in transfected HeLa cells The changes in immunoreactivity of the MRP1-P255A and MRP1-P235/255A mutant proteins suggested that the Pro255 to Ala substitution introduced a conformation change in CL3.
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ABCC1 p.Pro255Ala 12948592:167:87
status: NEW
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ABCC1 p.Pro255Ala 12948592:167:136
status: NEW
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ABCC1 p.Pro255Ala 12948592:167:196
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168 To determine whether this change might also affect plasma membrane trafficking of MRP1-P255A, transfected HeLa cells expressing this mutant as well as the MRP1-P235A and MRP1-P235/255A mutants were examined by confocal microscopy as before.
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ABCC1 p.Pro255Ala 12948592:168:26
status: NEW
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ABCC1 p.Pro255Ala 12948592:168:87
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169 Like wild-type MRP1, MRP1-P255A as well as MRP1-P235A and MRP1-P235/ 255A localized mostly to the plasma membrane of confluent HeLa cells (Fig. 4C).
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ABCC1 p.Pro255Ala 12948592:169:26
status: NEW
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ABCC1 p.Pro255Ala 12948592:169:82
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170 Thus, despite the apparent change in conformation of MRP1 proteins containing the Pro255-Ala substitution, their expression at the plasma membrane remained unchanged.
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ABCC1 p.Pro255Ala 12948592:170:82
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188 Results were expressed relative to wild-type Table 1 Kinetic parameters of [3 H]LTC4 uptake by membrane vesicles prepared from transfected HeLa cells expressing MRP1-Pro mutants Transfected cell line Km (nM) Vmax (pmol minÀ 1 mgÀ 1 ) Normalized Vmax MSD1 mutants WT-MRP1 128 80 80 P42A 139 35 41 P51A 109 55 50 P42/51A 103 15 48 P69A 142 46 42 P110A 150 73 124 CL3 mutants WT-MRP1 88 57 57 P196A 143 25 52 P205A 63 14 88 P207A 81 75 110 P209A 112 121 85 P196/205/207/209A 90 87 94 P235A 91 45 30 P255A 99 110 67 P235/255A 97 81 35 P272A 80 59 109 The kinetic parameters of [3 H]LTC4 uptake were determined by regression analysis of the Eadie-Hofstee transformed data.
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ABCC1 p.Pro255Ala 12948592:188:506
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242 Indeed, substitution of Pro255 with Ala caused a significant decrease in MRP1 reactivity with MAb MRPr1 but not MAb QCRL-1, presumably reflecting some conformational change in this region of the protein.
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ABCC1 p.Pro255Ala 12948592:242:24
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243 Nevertheless, neither the P255A mutant nor the P235/255A double mutant showed major changes in plasma membrane localization or organic anion transport.
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ABCC1 p.Pro255Ala 12948592:243:26
status: NEW
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ABCC1 p.Pro255Ala 12948592:243:49
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244 The change in MAb MRPr1 reactivity caused by the P255A substitution was unexpected.
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ABCC1 p.Pro255Ala 12948592:244:49
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146 GFP-tagged MRP1 proteins are shown in green; nuclei were stained with propidium iodide and are shown in red. (C) HeLa cells stably expressing wild-type MRP1, MRP1-P235A, MRP1-P255A, MRP1-P235/255A, and MRP1-P196/205/207/209A were cultured and processed for immunofluorescence and confocal microscopy as described in panel A.
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ABCC1 p.Pro255Ala 12948592:146:175
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148 Duplicate immunoblots of the P235A, P255A, P235/255A, and P272A MRP1 mutants probed with MAb QCRL-1 and MAb MRPr1 indicated that detection of the P255A and P235/P255A mutant MRP1 proteins relative to wild-type MRP1 by MAb MRPr1 was lower than that by MAb QCRL-1 (not shown).
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ABCC1 p.Pro255Ala 12948592:148:36
status: NEW
X
ABCC1 p.Pro255Ala 12948592:148:146
status: NEW
X
ABCC1 p.Pro255Ala 12948592:148:161
status: NEW
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150 When MRP1-P235A was detected with MAb QCRL-1, the signal intensity was approximately 1.8-fold higher than that for wild-type MRP1, while the signal intensity for MRP1-P235/P255A was approximately 2.3-fold higher (Fig. 5A).
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ABCC1 p.Pro255Ala 12948592:150:172
status: NEW
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161 We next compared the immunoreactivity of the double mutant MRP1-P235/255A and the single mutant MRP1-P255A.
X
ABCC1 p.Pro255Ala 12948592:161:101
status: NEW
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166 Plasma membrane localization of CL3 MRP1-Pro mutants is unchanged in transfected HeLa cells The changes in immunoreactivity of the MRP1-P255A and MRP1-P235/255A mutant proteins suggested that the Pro255 to Ala substitution introduced a conformation change in CL3.
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ABCC1 p.Pro255Ala 12948592:166:136
status: NEW
X
ABCC1 p.Pro255Ala 12948592:166:196
status: NEW
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187 Results were expressed relative to wild-type Table 1 Kinetic parameters of [3 H]LTC4 uptake by membrane vesicles prepared from transfected HeLa cells expressing MRP1-Pro mutants Transfected cell line Km (nM) Vmax (pmol min 1 mg 1 ) Normalized Vmax MSD1 mutants WT-MRP1 128 80 80 P42A 139 35 41 P51A 109 55 50 P42/51A 103 15 48 P69A 142 46 42 P110A 150 73 124 CL3 mutants WT-MRP1 88 57 57 P196A 143 25 52 P205A 63 14 88 P207A 81 75 110 P209A 112 121 85 P196/205/207/209A 90 87 94 P235A 91 45 30 P255A 99 110 67 P235/255A 97 81 35 P272A 80 59 109 The kinetic parameters of [3 H]LTC4 uptake were determined by regression analysis of the Eadie-Hofstee transformed data.
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ABCC1 p.Pro255Ala 12948592:187:494
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241 Indeed, substitution of Pro255 with Ala caused a significant decrease in MRP1 reactivity with MAb MRPr1 but not MAb QCRL-1, presumably reflecting some conformational change in this region of the protein.
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ABCC1 p.Pro255Ala 12948592:241:24
status: NEW
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