ABCC3 p.Trp1242Ala
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PMID: 14965249
[PubMed]
Haimeur A et al: "The MRP-related and BCRP/ABCG2 multidrug resistance proteins: biology, substrate specificity and regulation."
No.
Sentence
Comment
402
Effects of Non-conservative and Conservative Substitutions of MRP1-Trp1246, MRP2-Trp1254 and MRP3-Trp1242 on Transport of Common Substrates MRP-Related Amino Acid Substitution % Wild-type MRP Transport Activity* Transporter LTC4 E217βG MTX MRP1-Trp 1246 Ala Tyr 100 100 < 10 < 10 < 10 10 MRP2-Trp 1254 Ala Tyr < 10 30 < 10 100 14 1 MRP3-Trp 1242 Ala Tyr 70 65 250 700 20 20 * data are from References [125, 284, 324] directly involved in forming the binding site for this modulator [284].
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ABCC3 p.Trp1242Ala 14965249:402:343
status: NEW
PMID: 12388190
[PubMed]
Oleschuk CJ et al: "Substitution of Trp1242 of TM17 alters substrate specificity of human multidrug resistance protein 3."
No.
Sentence
Comment
59
Mutations for Trp1242 substitutions (underlined), silent DraI restriction sites (italicized), and their corresponding oligonucleotides were as follows: W1242A (5Ј-G CAG GTG ACA TTC GCT TTA AAC GCG ATG ATA CGA ATG ATG TCA G-3Ј), W1242C (5Ј-G CAG GTG ACA TTC GCT TTA AAC TGC ATG ATA CGA ATG ATG TCA G-3Ј), W1242F (5Ј-G CAG GTG Fig. 1.
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ABCC3 p.Trp1242Ala 12388190:59:152
status: NEW103 These included nonconservative substitutions with a nonaromatic nonpolar amino acid (Ala; W1242A-MRP3) and a nonaromatic polar amino acid (Cys; W1242C-MRP3), as well as conservative substitutions with aromatic polar (Tyr; W1242Y-MRP3) and nonpolar (Phe; W1242F-MRP3) amino acids.
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ABCC3 p.Trp1242Ala 12388190:103:90
status: NEW106 As shown in Fig. 2, wild-type MRP3 and the four mutants (W1242A-, W1242C-, W1242F-, and W1242Y-MRP3) were expressed at similar levels.
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ABCC3 p.Trp1242Ala 12388190:106:57
status: NEW108 Mean expression levels of the mutant MRP3 proteins relative to wild-type MRP3 were as follows: W1242A, 1.1 Ϯ 0.3; W1242C, 1.0 Ϯ 0.2; W1242Y, 1.0 Ϯ 0.1; W1242F, 1.0 Ϯ 0.3; and W1242P, 0.6 Ϯ 0.2 (4-6 independent transfections).
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ABCC3 p.Trp1242Ala 12388190:108:95
status: NEW110 Time courses of ATP-dependent [3 H]E217betaG uptake were determined for the W1242A-, W1242C-, W1242F-, W1242Y-, and W1242P-MRP3 mutants by using inside-out membrane vesicles prepared from transfected HEK293T cells (Fig. 3A).
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ABCC3 p.Trp1242Ala 12388190:110:76
status: NEW111 Unexpectedly, four of the five mutants (W1242A-, W1242C-, W1242F-, and W1242Y-MRP3) transported this glucuronide substrate at levels that were substantially higher than those of wild-type MRP3.
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ABCC3 p.Trp1242Ala 12388190:111:40
status: NEW113 At 3 min, [3 H]E217betaG uptake in membrane G282 CONSERVED TRP AND MRP3 (ABCC3) SUBSTRATE SPECIFICITY AJP-Gastrointest Liver Physiol • VOL 284 • FEBRUARY 2003 • www.ajpgi.org atUnivofNorthCarolina-AcqSrvcsonOctober,2012http://ajpgi.physiology.org/Downloadedfrom vesicles enriched for W1242A-, W1242C-, and W1242F-MRP3 was 2.5-to 3-fold higher than for wild-type MRP3, whereas [3 H]E217betaG uptake by the most conservatively substituted mutant, W1242Y-MRP3, was ϳ7-fold higher (Fig. 3B).
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ABCC3 p.Trp1242Ala 12388190:113:306
status: NEW120 [3 H]LTC4 uptake by the W1242A-, W1242F-, and W1242Y-MRP3 mutants was somewhat less than the wild-type MRP3 transport activity (Fig. 4A).
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ABCC3 p.Trp1242Ala 12388190:120:24
status: NEW128 At 10 min, ATP-dependent [3 H]MTX uptake levels by the W1242A, W1242C, W1242F, and W1242Y Fig. 3.
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ABCC3 p.Trp1242Ala 12388190:128:55
status: NEW130 A: time course of ATP-dependent [3 H]E217betaG uptake in membrane vesicles prepared from HEK293T cells transfected with empty vector (ᮀ), wild-type MRP3 (s), and mutant [W1242A (), W1242C (}), W1242F (F), W1242Y (Œ), and W1242P (ƒ)] cDNA expression vectors.
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ABCC3 p.Trp1242Ala 12388190:130:177
status: NEW135 Top: MRP3 expression in membrane vesicles prepared from human embryonic kidney (HEK) 293T cells transfected with empty vector [pcDNA3.1(ϩ)], wild-type (WT-MRP3), and mutant (W1242A, W1242C, W1242F, W1242Y, and W1242P) MRP3 cDNAs was determined by immunoblotting with MAb M3II-9, and relative levels of expression were estimated by densitometry.
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ABCC3 p.Trp1242Ala 12388190:135:180
status: NEW147 To determine if Trp1242 substitutions also affected MRP3-mediated transport of the latter substrate, [3 H]leucovorin uptake into membrane vesicles prepared from transfected cells expressing wild-type MRP3 and W1242A-, W1242C-, W1242F-, and W1242Y-MRP3 mutants was examined.
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ABCC3 p.Trp1242Ala 12388190:147:209
status: NEW151 Time course of [3 H]methotrexate (MTX) uptake and MTX- mediated inhibition of [3 H]E217betaG uptake by wild-type and Trp1242 mutant MRP3 proteins. A: ATP-dependent uptake of [3 H]MTX was measured in membrane vesicles prepared from HEK293T cells transfected with empty pcDNA3.1(ϩ) vector (ᮀ), wild-type (s), and mutant [W1242A (), W1242C (}), W1242F (F), and W1242Y (Œ)] MRP3 cDNA expression vectors. Membrane vesicles were incubated at 37°C with 1 M [3 H]MTX and ATP or AMP in transport buffer.
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ABCC3 p.Trp1242Ala 12388190:151:332
status: NEW161 Taurocholate uptake by the W1242A-, W1242C-, W1242F-, and W1242Y-MRP3 mutants was then examined and, in all cases, was not significantly different from uptake by wild-type MRP3 (Fig. 7B).
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ABCC3 p.Trp1242Ala 12388190:161:27
status: NEW162 Consistent with this observation, [3 H]E217betaG uptake by W1242A-, W1242C-, W1242F-, and W1242Y-MRP3 could still be inhibited by taurocholic acid (40-60%) at concentrations of 50 and 100 M (Fig. 7C).
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ABCC3 p.Trp1242Ala 12388190:162:59
status: NEW170 Cells were transfected with empty vector [pcDNA3.1(ϩ)], wild-type, and mutant (W1242A, W1242C, W1242F, and W1242Y) MRP3 cDNA expression.
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ABCC3 p.Trp1242Ala 12388190:170:85
status: NEW171 C: membrane vesicles from cells expressing wild-type and W1242A, W1242C, W1242F, and W1242Y mutant MRP3 were incubated at 37°C with 400 nM [3 H]E217betaG in transport buffer and other components for 3 min in the absence (open bars) or presence of taurocholic acid (50 M, grey bar; 100 M, solid bar).
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ABCC3 p.Trp1242Ala 12388190:171:57
status: NEW173 [3 H]leucovorin uptake by wild-type and Trp1242 mutant MRP3 proteins. A: uptake of [3 H]leucovorin was measured in membrane vesicles prepared from HEK293T cells transfected with empty vector [pcDNA3.1(ϩ)], wild-type, and Trp1242 mutant (W1242A, W1242C, W1242F, and W1242Y) MRP3 cDNA expression vectors. Membrane vesicles were incubated at 37°C with 250 M [3 H]leucovorin and ATP or AMP in transport buffer for 20 min.
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ABCC3 p.Trp1242Ala 12388190:173:243
status: NEW193 Effects of nonconservative (Ala) and conservative (Tyr) substitutions of MRP1-Trp1246 , MRP2-Trp1254 , and MRP3-Trp1242 on transport activity of common substrates Transporter Substitution %Wild-type MRP Transport Activity LTC4 E217betaG MTX MRP1-Trp1246 Ala 100 Ͻ10 Ͻ10* Tyr 100 Ͻ10 10* MRP2-Trp1254 Ala Ͻ10 Ͻ10 14 Tyr 30 100 1 MRP3-Trp1242 Ala 70 250 20 Tyr 65 700 20 Data are from Ito et al. (17, 18) and the present study, with exceptions (*) noted (I. Letouneau, C. J. Oleschuk, R. G. Deeley, and S. P. C. Cole, unpublished observations).
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ABCC3 p.Trp1242Ala 12388190:193:363
status: NEW196 Membrane vesicles from cells expressing wild-type MRP3 (WT-MRP3) and W1242A, W1242C, W1242F, and W1242Y mutant MRP3 were incubated at 37°C with 400 nM [3 H]E217betaG in transport buffer and other components for 3 min in the absence (open bars) or presence of glycocholate (50 M, grey bar; 100 M, solid bar).
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ABCC3 p.Trp1242Ala 12388190:196:69
status: NEW199 Transport activities of variously substituted MRP3-Trp1242 mutants Substrate Transport Activity W1242A W1242C W1242F W1242Y W1242P E217betaG 1 1 1 11 222 LTC4 2 22 2 2 222 MTX 222 222 222 222 n.d.
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ABCC3 p.Trp1242Ala 12388190:199:96
status: NEW