ABCC7 p.Lys1041Arg
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PMID: 24777605
[PubMed]
Lee S et al: "Interference with ubiquitination in CFTR modifies stability of core glycosylated and cell surface pools."
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Sentence
Comment
6
The amount of CFTR in the K1041R mutant was drastically reduced and consisted of bands A/B, suggesting that the site in transmembrane 10 (TM10) was critical to further processing beyond the proteasome.
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ABCC7 p.Lys1041Arg 24777605:6:26
status: NEW73 We hypothe- TABLE 1 Primers for site-directed mutagenesis Mutation Directiona Sequence (5=-3=)b K14R F GGCCAGCGTTGTCTCCAGACTTTTTTTCAGCTGGACC R GGTCCAGCTGAAAAAAAGTCTGGAGACAACGCTGGCC K68R F GGCTTCAAAGAAAAATCCTAGACTCATTAATGCCCTTCGGCG R CGCCGAAGGGCATTAATGAGTCTAGGATTTTTCTTTGAAGCC K710R F CCAATCAACTCTATACGAAGATTTTCCATTGTGCAAAAG R CTTTTGCACAATGGAAAATCTTCGTATAGAGTTGATTGG K716R F GAAAATTTTCCATTGTGCAAAGGACTCCCTTACAAATGAATGG R CCATTCATTTGTAAGGGAGTCCTTTGCACAATGGAAAATTTTC K710/716R F CCAATCAACTCTATACGAAGATTTTCCATTGTGCAAAGGACTCCCTTACAAATGAATGG R CCATTCATTTGTAAGGGAGTCCTTTGCACAATGGAAAATCTTCGTATAGAGTTGATTGG K1041R F CCTCACAGCAATTCAGACAACTGGAATCTGAAG R CTTCAGATTCCAGTTGTCTGAGTTGCTGTGAGG K1080R F GAAACTCTGTTCCACAGAGCTCTGAATTTACATAC R GTATGTAAATTCAGAGCTCTGTGGAACAGAGTTTC K1218R F GATCTCACAGCAAGATACACAGAAGG R CCTTCTGTGTATCTTGCTGTGAGATC a F, forward; R, reverse.
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ABCC7 p.Lys1041Arg 24777605:73:598
status: NEW86 We generated K1041R and K1080R mutants and expressed them in IB3-1.
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ABCC7 p.Lys1041Arg 24777605:86:13
status: NEW89 Interference with residue 1080 drastically reduced CFTR but, in contrast to the K1041R mutation, significant band C continued to appear, similar to results with the R domain mutants.
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ABCC7 p.Lys1041Arg 24777605:89:80
status: NEW90 C-band expression was quantified by densitometry, as shown in Fig. 2B, and K1041R was the lowest although band B expression was higher than in the wt, further supporting a maturational block after band B and before C.
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ABCC7 p.Lys1041Arg 24777605:90:75
status: NEW104 The observed reduction in expression of K710R, K716R, K710/ 716R, K1041R, and K1080R CFTRs might be the consequence of disordered conformational structure or folding/assembly.
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ABCC7 p.Lys1041Arg 24777605:104:66
status: NEW106 The data in Fig. 3B show similar patterns of proteolytic digestion for wt and mutant CFTR; K1041R is the only mutant which shows significantly less CFTR at the final trypsin concentration.
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ABCC7 p.Lys1041Arg 24777605:106:91
status: NEW131 At steady state, the K1041R mutation in TM10 is almost completely lacking band C CFTR expression.
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ABCC7 p.Lys1041Arg 24777605:131:21
status: NEW151 The K1041R mutant was included to highlight the differences that will be explored further.
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ABCC7 p.Lys1041Arg 24777605:151:4
status: NEW156 Interestingly, MG132 treatment rescued only B band expression in the K1041R mutant form of CFTR, but this was not sufficient for trafficking beyond the ER.
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ABCC7 p.Lys1041Arg 24777605:156:69
status: NEW159 Prevention of proteolysis at the lysosome accumulates more C band K1041R and K1080R.
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ABCC7 p.Lys1041Arg 24777605:159:66
status: NEW169 (C) The results from expression of control vector, wt CFTR, K1041R, K1080R, and K1218R with and without proteasomal or lysosomal inhibition are shown in representative blots similar to the results show in panel A. MG132 rescues band B from K1041R to some extent, as well as a small portion of band C.
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ABCC7 p.Lys1041Arg 24777605:169:60
status: NEWX
ABCC7 p.Lys1041Arg 24777605:169:240
status: NEW175 Therefore, these data suggest that K1041R and K1080R mutants are degraded at the proteasome and lysosome, respectively.
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ABCC7 p.Lys1041Arg 24777605:175:35
status: NEW185 For K1041R the reduced Ub-K63 immunoblot signal likely derives from the reduced amount of immunoprecipitated product.
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ABCC7 p.Lys1041Arg 24777605:185:4
status: NEW194 K14R, K1080R, and K1218R but not K1041R reach the cell surface.
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ABCC7 p.Lys1041Arg 24777605:194:33
status: NEW200 There were decreased levels of cell surface CFTR detection in the K68R, K710R, K716R, K710/ K716R, and K1041R mutant forms of CFTR, but the wild-type, K14R, K1080R, and K1218R mutants accumulated similar levels of visible cell surface CFTR.
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ABCC7 p.Lys1041Arg 24777605:200:103
status: NEW215 On the other hand, prevention of ubiquitination at 1041 by making the K1041R construct promotes degradation primarily by the proteasome.
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ABCC7 p.Lys1041Arg 24777605:215:70
status: NEW218 Control vector, wt CFTR, K14R, K68R, K710R, K716R, K710/716R, K1041R, K1080R, and K1218R were expressed in IB3-1 cells for 48 h. CFTR was immunoprecipitated (IP) with M3A7 as described in Materials and Methods and separated by SDS-PAGE.
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ABCC7 p.Lys1041Arg 24777605:218:62
status: NEW226 FIG 6 K-to-R mutation alters the stability of CFTR protein, and wt CFTR, K14R, K1080R, and K1218R, but not K1041R, are detectable at the cell surface.
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ABCC7 p.Lys1041Arg 24777605:226:107
status: NEW236 As expected, CFTR is virtually undetectable in cells expressing control vector or K1041R.
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ABCC7 p.Lys1041Arg 24777605:236:82
status: NEW237 CFTR is easily detected HDAC6 must interact with CFTR to promote trafficking beyond the ER, then we predict that K1041R would interact preferentially with VCP and that K1218R would interact preferentially with HDAC6.
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ABCC7 p.Lys1041Arg 24777605:237:114
status: NEW261 Band C was most reduced in K1041R and highest in the wt, K1080R, and K1218R, consistent with data in panels A and B.
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ABCC7 p.Lys1041Arg 24777605:261:27
status: NEW268 Interestingly, higher-molecular-weight forms of K1041R were pulled down from the biotinylated surfaces of cells treated with proteasomal or lysosomal inhibition.
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ABCC7 p.Lys1041Arg 24777605:268:48
status: NEW275 Since ZO-1 interacts with PDZ domains, the reduced interactions in K14R, K68R, K710R, K716R, K710/716R, and K1041R and the absence of interactions with K1080R and K1218R raise the issue of alternative trafficking routes that are not dependent on the C-tail PDZ domain.
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ABCC7 p.Lys1041Arg 24777605:275:108
status: NEW278 Poly- or monoubiquitination in K14, K68, K710, K716, 1041, K1080, and K1218 sites allows CFTR to pass through its regular quality control process, producing adequate band C. K710R, K716R, K710/K716R, and K1080R mutants undergo some proteasome- and some lysosome-dependent degradation, whereas K1041R is primarily degraded by the proteasome.
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ABCC7 p.Lys1041Arg 24777605:278:293
status: NEW296 Interestingly, ZO-1 was highly abundant in complexes formed with wt CFTR; K14R, K68R, K710R, K716R, K710/716R, and K1041R mutants bound less ZO-1, whereas K1080R and K1218R mutant complexes had none.
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ABCC7 p.Lys1041Arg 24777605:296:115
status: NEW