ABCMdb

ABCB1 p.Met68Arg

None has been submitted yet.

Publications

PMID: 18596043 [PubMed] Loo TW et al: "Arginines in the first transmembrane segment promote maturation of a P-glycoprotein processing mutant by hydrogen bond interactions with tyrosines in transmembrane segment 11."

No. Sentence Comment

48 The most efficient rescue was observed with the M68R mutant. Login to comment
55 For disulfide cross-linking analysis, the cDNA of mutant L339C(TM6)/F728C(TM7) (16) was modified to also encode the G64R, M68R, or V71R mutations. Login to comment
103 Mutants M68R and L65R showed the highest increase in maturation efficiency (85 and 60% mature 170-kDa mature, respectively) (Fig. 2). Login to comment
118 Mutants G251V, V53R/G251V (inhibited maturation) and M68R/G251V (enhanced maturation) were subjected endoglycosidase H or F digestion to determine whether the alterations in mobility of the mutant P-gps were indeed due to changes in the glycosylation state of the protein. Login to comment
125 Because the M68R mutation was most efficient in promoting maturation of the G251V processing mutant, we tested whether it could also promote maturation of a different processing mutant. Login to comment
126 Accordingly, the M68R mutation was introduced into the ⌬NBD2- P-gp processing mutant (20). Login to comment
128 Mutants ⌬NBD2- P-gp, M68R/⌬NBD2-P-gp, and ⌬NBD2-P-gp lacking the three glycosylation sites (N91A, N94A, N99A) were expressed in HEK 293 cells, and whole cell SDS extracts were subjected to immunoblot analysis. Login to comment
129 Fig. 4 shows that the M68R mutant yielded an extra P-gp protein that corresponded in size to the mature protein (Fig. 4). Login to comment
130 Treatment with endoglycosidases H and F showed that the immature form (100 kDa) was sensitive to endoglycosidases H and F, whereas the slower migrating M68R protein (115 kDa) was sensitive to endoglycosidase F but not endoglycosidase H (data not shown). Login to comment
138 Whole cell SDS extracts of HEK 293 cells expressing A52-tagged mutants G251V, V53R/G251V, or M68R/G251V were treated with endoglycosidase Hf (H),peptideN-glycosidaseF(F)ornoendoglycosidase(-).Equivalentamountsweresubjectedtoimmunoblot analysis. Login to comment
149 Mutants L65R and M68R yielded mature 170-kDa P-gp as the major product in the absence of drug substrates. Login to comment
155 Effect of Suppressor Arginine Mutations on P-gp-Drug Interactions-Because mutant M68R/G251V showed efficient maturation (about 85%) when expressed in the absence of drug substrates (Fig. 2), we tested whether Arg-68 affected P-gp- drug interactions in disulfide protection assays using mutant L339C(TM6)/F728C(TM7) as described previously (9). Login to comment
159 Effect of the M68R mutation on maturation of the ⌬NBD2 processing mutant. Login to comment
160 Whole cell extracts of HEK 293 cells expressing mutants ⌬NBD2-P-gp with no changes (None), the M68R mutation, or N91A, N94A and N99A changes to the glycosylation sites (Unglycos) were subjected to immunoblotanalysis.Thepositionsofmature,immature,andunglycosylated(Unglycos) forms of ⌬NBD2 P-gp are indicated. Login to comment
165 TABLE 1 Effects of drug substrates on the maturation of TM1 arginine mutants containing the G251V mutation Mutation (G251V ؉) No drug Cyclosporin A Verapamil Vinblastine Rhodamine None - 111a,c 111 111 11 V52R -a,b 111 111 111 11 V53R 2 - - - - G64R 2 - - - - T55R 2 - - - - L56R 2 - - - - A57R 2 - - - - A58R 2 - - - - I59R 2 - - - - I60R 2 - - - - H61R - 111 1 1 1 G62R 2 - - - - A63R 2 - - - - G64R 1 111 1 1 11 L65R 11 111 11 11 11 P66R 2 1 - - - L67R - 111 111 111 11 M68R 111 111 111 111 111 M69R - 111 - 11 111 L70R - 111 111 111 11 V71R 1 111 111 111 11 F72R 2 1 1 1 1 a Change in the amount of mature (170 kDa) protein in the presence of drug substrate relative to that in the absence of drug substrate. Login to comment
173 Membranes were prepared from HEK 293 cells expressing mutants L339C(TM6)/F728C(TM7), G64R/ L339C(TM6)/F728C(TM7), M68R/ L339C(TM6)/F728C(TM7), and V71R/L339C(TM6)/F728C(TM7). Login to comment
177 A representative example of the effects of various concentrations of vinblastine on cross-linking of mutant M68R/L339C(TM6)/ F728C(TM7) by M14M is shown in Fig. 6. Login to comment
179 The M68R/ L339C(TM6)/F728C(TM7) mutant, however, required 266 ␮M vinblastine (Ͼ500-fold increase) to inhibit cross-linking by 50%. Login to comment
183 The G64R, L65R, and M68R mutations preferentially affected P-gp-vinblastine interactions. Login to comment
188 Effect of the M68R mutation on inhibition of cross-linking by vinblastine. Login to comment
189 A, membranes were prepared from HEK 293 cells expressing mutants L339C(TM6)/F728C(TM7) or M68R/L339C(TM6)/F728C(TM7). Login to comment
194 TABLE 2 Concentrations of drug substrates required to inhibit cross-linking by 50% Mutant Vinblastine Cyclosporin A Rhodamine B ␮M ␮M ␮M L339C/F728C 0.5 Ϯ 0.2a 0.8 Ϯ 0.3 52 Ϯ 14 G64R/L339C/F728C 53 Ϯ 15b 1.5 Ϯ 0.4 61 Ϯ 10 M68R/L339C/F728C 266 Ϯ 62b 1.3 Ϯ 0.3 57 Ϯ 7 V71R/L339C/F728C 0.6 Ϯ 0.2 0.8 Ϯ 0.2 57 Ϯ 10 a Each value is the mean Ϯ S.D. (n ϭ 3-4 separate cross-linking experiments). Login to comment
197 Therefore, we measured drug stimulation of ATPase activity of mutants G64R and M68R using various concentrations of verapamil to test whether the apparent affinity for verapamil of the P-gp mutants was altered. Login to comment
200 Accordingly, mutations G64R or M68R were introduced into a wild-type P-gp that contained a histidine tag at the COOH-terminal end. Login to comment
201 Histidine-tagged wild-type and mutants G64R and M68R P-gps were expressed in HEK 293 cells, and the proteins were isolated by nickel-chelate chromatography. Login to comment
205 Verapamil also stimulated the ATPase activities of mutants G64R and M68R (1.6 and 1.8 ␮mol Pi/min/mg of protein, respectively). Login to comment
206 Although both mutants G64R and M68R showed relatively high activation of ATPase activity with verapamil, their apparent affinities for verapamil were reduced by about 19-and 4-fold, respectively. Login to comment
207 Half-maximal activation of the ATPase activities of mutants G64R and M68R required 540 ␮m and 120 ␮M verapamil, respectively, compared with 29 ␮m for wild-type P-gp. Login to comment
208 Effect of TM11 Mutations on Rescue of Mutant G251V Containing the L65R and M68R Changes-One reason that Arg-68 caused the largest increase in maturation of mutant G251V is that the arginine residue may promote packing of the TM segments. Login to comment
214 To test if Tyr-950 or Tyr-953 influences the ability of the M68R mutation to promote maturation of the G251V mutant, we introduced the Y950A or Y953A mutations into mutant M68R/ G251V mutant. Login to comment
216 Fig. 8 shows the maturation efficiencies compared with the M68R/G251V parent. Login to comment
218 Not all mutations in TM11, however, affected maturation of the M68R/G251V mutant. Login to comment
219 The presence of mutations Q946A, M948A, M949A, F951A, or S952A did not appear to affect the maturation of the M68R/ G251V mutant (Fig. 8A, lanes 2-5, 7, and 8). Login to comment
222 In contrast, both Y950A and Y953A affected the maturation efficiency of the M68R/G251V mutant. Login to comment
229 Mutants L65R/G251V/Y950F, M68R/G251V/ Y950A/Y953A, and M68R/G251V/Y950F/Y953F were constructed, and the cDNAs were expressed in HEK 293 cells. Login to comment
231 Immunoblot analysis shows the Y950A/Y953A and Y950F/Y953F changes in M68R/G251V (Fig. 8A, lanes 11 and 12) or Y950F change in L65R/G251V (Fig. 8B, lane 5) reduced maturation to levels similar to that observed in the G251V parent. Login to comment
233 Verapamil-stimulated ATPase activities of wild-type and mutant G64R and M68R P-gps. Login to comment
264 Effect of TM11 mutations on maturation of M68R/G251V and L65R/G251V mutants. Login to comment
265 A, HEK 293 cells were transfected with mutants M68R/G251V (lanes 2-12) or G251V (lanes 1, 13-15) containing the indicated TM11 mutations. Login to comment
276 Mutants H61R/G251V or M69R/G251V showed little drug rescue with verapamil (Fig. 5), and mutants G64R and M68R in a wild-type background showed reductions in apparent affinity for verapamil in ATPase assays (Fig. 7). Login to comment
280 The observation that the M68R mutation can reduce the apparent affinities for the drug substrates verapamil and vinblastine would be unexpected because it appears that P-gp initially interacts with drug substrates in the inner leaflet of the bilayer (44). Login to comment
281 One explanation is that the M68R mutation causes an indirect effect on the vinblastine and verapamil binding sites. Login to comment
282 The structural alterations may be small because the M68R change did not appear to affect P-gp interactions with cyclosporin A or rhodamine B (Table 2). Login to comment
283 Another explanation is that the M68R mutation has altered the predicted "OFF-sites" of P-gp. Login to comment
285 Because the OFF-sites would be involved in drug release, they may be located in the outer portions of P-gp and would be sensitive to mutations such as M68R. Login to comment
298 Some mutations such as G64R, L65R, M68R, and V71R actually promoted maturation of the G251V mutant. Login to comment
299 The L65R and M68R mutations were particularly effective in promoting maturation as they increased maturation efficiency of the G251V mutant from about 20 to 60-85%. Login to comment
304 An alternative possibility to explain why the L65R and M68R mutations were particularly effective in promoting maturation of the G251V mutant is that they promoted packing of the TM segments by forming hydrogen bonds with Tyr-950 and/or Tyr-953 located in TM11. Login to comment
308 This possibility is supported by the observations that the conservative Y950F and Y953F mutations reduced maturation of the M68R/G251V mutant to levels observed with the G251V parent. Login to comment
314 In P-gp, the introduction of the L65R or M68R mutations appears to promote folding by enhancing TM1-TM11 interactions through hydrogen bond formation with the Tyr-950 and/or Tyr-953 in TM11. Login to comment

PMID: 26507655 [PubMed] Loo TW et al: "Mapping the Binding Site of the Inhibitor Tariquidar That Stabilizes the First Transmembrane Domain of P-glycoprotein."

No. Sentence Comment

175 In the N-terminal TMD1 domain, the largest number of arginine mutations predicted to line the drug-binding pocket that inhibited tariquidar rescue were located in TM1 (H61R, G64R, L65R, M68R, M69R, and F72R) and TM5 (F303R, I306R, Y307R, S309R, and Y310R) (Fig. 4, A and E). Login to comment
193 It was found that 16 of the 28 mutants resembled the G251V/I868R mutant as expression in the presence of 5 òe;M cyclosporine A yielded mature P-gp as the major product in TM1 (H61R, G64R, L65R, M68R, and M69R), TM5 (F303R, I306R, and S309R), TM7 (Q725R and F728R), TM10 (I868R and G872R), TM11 (F942R, T945R, and Q946R), and TM12 (V982R) (Fig. 7). Login to comment
212 Seventeen of the 30 G251V/arginine mutants (M68R, M69R, and F72R in TM1; I306R, Y307R, S309R, and Y310R in TM5; F336R in TM6; F728R and F732R in TM7; I868R and G872R in TM10; F942R, T945R, M949R, and S952R in TM11; and V982R in TM12) that could not be rescued with tariquidar showed little or no stimulation of ATPase activity with tariquidar (Fig. 8A). Login to comment
283 We identified 13 additional arginine mutations (H61R, G64R, L65R, and M68R in TM1; A129R in TM2; I306R and S309R in TM5; F343R in TM6; F942R, T945R, Q946R, and Y950R in TM11; and L975R in TM12) (Fig. 11A) that were not predicted to lie within 4.5-&#c5; of the predicted site 3 tariquidar-binding site (9). Login to comment