ABCA1 p.Ser198Ala
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PMID: 21070853
[PubMed]
Huwait EA et al: "A novel role for c-Jun N-terminal kinase and phosphoinositide 3-kinase in the liver X receptor-mediated induction of macrophage gene expression."
No.
Sentence
Comment
142
The action of this phosphorylation was gene-specific as the expression of only some LXR targets was increased in cells expressing the S198A phosphorylation-deficient mutant compared to those for the wild-type receptor [27].
X
ABCA1 p.Ser198Ala 21070853:142:134
status: NEW141 The action of this phosphorylation was gene-specific as the expression of only some LXR targets was increased in cells expressing the S198A phosphorylation-deficient mutant compared to those for the wild-type receptor [27].
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ABCA1 p.Ser198Ala 21070853:141:134
status: NEW
PMID: 18250151
[PubMed]
Torra IP et al: "Phosphorylation of liver X receptor alpha selectively regulates target gene expression in macrophages."
No.
Sentence
Comment
8
Expression of some (AIM and LPL), but not other (ABCA1 or SREBPc1) established LXR target genes is increased in RAW 264.7 cells expressing the LXR␣ S198A phosphorylation-deficient mutant compared to those with WT receptors.
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ABCA1 p.Ser198Ala 18250151:8:138
status: NEWX
ABCA1 p.Ser198Ala 18250151:8:155
status: NEW9 Surprisingly, a gene normally not expressed in macrophages, the chemokine CCL24, is activated specifically in cells expressing LXR␣ S198A.
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ABCA1 p.Ser198Ala 18250151:9:139
status: NEW10 Furthermore, inhibition of S198 phosphorylation by 9cRA or by a CK2 inhibitor similarly promotes CCL24 expression, thereby phenocopying the S198A mutation.
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ABCA1 p.Ser198Ala 18250151:10:140
status: NEW46 LZRSpBMN-GFP retroviral vectors carrying the FLAG-tagged wild-type (WT) or S198A mutant LXR␣ cDNA were generated.
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ABCA1 p.Ser198Ala 18250151:46:75
status: NEW56 Recombinant retroviruses were produced by transfecting LZRSpBMN-GFP, LZRSpBMN-GFP/LXR␣, or LZRSpBMN-GFP/S198A into 293GP cells as described previously (66).
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ABCA1 p.Ser198Ala 18250151:56:111
status: NEW58 Cells infected with either the retroviral vector devoid of an LXR␣ sequence (RAW-VO [vector only]), the FLAG-tagged WT LXR␣ (RAW-LXR␣), or mutant S198A (RAW-S198A) were sorted for green fluorescent protein expression by fluorescence-activated cell sorting.
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ABCA1 p.Ser198Ala 18250151:58:167
status: NEWX
ABCA1 p.Ser198Ala 18250151:58:178
status: NEW82 For nuclear receptor corepressor (NCoR) coimmunoprecipitation assays, RAW-LXR␣ or RAW-S198A cells treated with vehicle or T0901317 for 2 h were cross-linked for 20 min in phosphate-buffered saline with 1.6 mM DSP [dithiobis(succinimidyl)propionate] (Pierce) prior to whole-cell extract preparation.
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ABCA1 p.Ser198Ala 18250151:82:93
status: NEW137 Specific immunoreactivity of the phospho-S198 antibody was demonstrated by its ability to recognize WT phosphorylated LXR␣, but not phosphorylation-deficient S198A LXR␣ (see Fig. S2A in the supplemental material).
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ABCA1 p.Ser198Ala 18250151:137:165
status: NEW142 Pools of cell clones stably expressing either WT or S198A-mutated LXR␣ were generated by retroviral infection of RAW 264.7 cells, which lack endogenous LXR␣ but express LXRbeta.
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ABCA1 p.Ser198Ala 18250151:142:52
status: NEWX
ABCA1 p.Ser198Ala 18250151:142:112
status: NEW143 Nuclear extracts from LXR␣-expressing RAW 264.7 cells loaded with cholesterol showed enhanced WT (and not S198A) LXR␣ phosphorylation compared to untreated cultures (Fig. 1B).
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ABCA1 p.Ser198Ala 18250151:143:113
status: NEW156 (B) RAW 264.7 cells infected with a retroviral vector only (VO) or stably expressing WT or S198A FLAG-hLXR␣ were treated with 40 g/ml cholesterol (Chol) in the form of soluble cholesterol-cyclodextrin complexes for 48 h.
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ABCA1 p.Ser198Ala 18250151:156:91
status: NEW175 Next, to determine the impact of S198 phosphorylation on LXR␣ function, we investigated LXR target gene expression in RAW 264.7 cells stably expressing the phosphorylation mutant S198A.
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ABCA1 p.Ser198Ala 18250151:175:4
status: NEWX
ABCA1 p.Ser198Ala 18250151:175:186
status: NEW176 RAW-S198A macrophages showed a dramatically enhanced ligand-dependent expression of LPL and AIM compared to the WT LXR␣-transduced cells (Fig. 3A), indicating that S198 phosphorylation exerts an inhibitory effect on the LXR␣-regulated transcription of these genes.
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ABCA1 p.Ser198Ala 18250151:176:4
status: NEW179 Consistent with the gene expression data, the activities of WT and S198A receptors were similar when tested in transient-transfection experiments on an ABCA1 promoter fragment containing the LXRE (reference 10 and data not shown).
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ABCA1 p.Ser198Ala 18250151:179:17
status: NEWX
ABCA1 p.Ser198Ala 18250151:179:67
status: NEW180 Furthermore, the S198A mutant displayed no major difference in expression (Fig. 3B) or subcellular localization (see Fig. S3C in the supplemental material) compared to the WT and thus cannot account for the observed differential gene expression.
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ABCA1 p.Ser198Ala 18250151:180:17
status: NEW187 (A) RAW cells stably expressing FLAG-hLXR␣ (WT or S198A) were incubated with or without 5 M T0901317 ligand for 2 h.
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ABCA1 p.Ser198Ala 18250151:187:57
status: NEW195 (A) RAW-LXR␣ (WT or S198A) cells were incubated with vehicle or T0901317 ligand (T) at the indicated concentrations for 24 h.
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ABCA1 p.Ser198Ala 18250151:195:27
status: NEW199 (B) Protein expression levels of LXR␣ in RAW 264.7 cells infected with a retroviral vector only (VO) or FLAG-hLXR␣ (WT or S198A) incubated in the presence or absence of T0901317, as in panel A.
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ABCA1 p.Ser198Ala 18250151:199:136
status: NEW213 Remarkably, in RAW-S198A macrophages, CCL24 basal expression was markedly induced compared to WT LXR␣-expressing cells (Fig. 5A) and was further dramatically increased by T0901317 in a dose-dependent manner (Fig. 5B).
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ABCA1 p.Ser198Ala 18250151:213:19
status: NEW221 The induction of CCL24 expression by DMAT was not observed in RAW-S198A cells, indicating that this effect is due to LXR␣ dephosphorylation by the CK2 inhibitor.
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ABCA1 p.Ser198Ala 18250151:221:66
status: NEW232 RAW-VO (VO) and RAW-LXR␣ (WT or S198A) cells were incubated for 24 h in medium with vehicle or 1 M (A) or the indicated concentrations (B) of T0901317 LXR ligand.
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ABCA1 p.Ser198Ala 18250151:232:39
status: NEW235 Indeed, in the presence of the RXR ligand 9cRA, CCL24 induction by T0901317 in the RAW LXR␣ cells was markedly enhanced (Fig. 7A), reaching expression levels similar to those observed in untreated RAW-S198A cells (see Fig. S5 in the supplemental material).
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ABCA1 p.Ser198Ala 18250151:235:208
status: NEW239 Importantly, the synergistic action of T0901317 and 9cRA on CCL24 expression was lost in RAW-S198A cells (16-fold versus 2.7-fold over T0901317 alone in WT and S198A cells, respectively), suggesting that it is S198 phosphorylation that mediates this effect (see Fig. S5A in the supplemental material).
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ABCA1 p.Ser198Ala 18250151:239:93
status: NEWX
ABCA1 p.Ser198Ala 18250151:239:160
status: NEW294 We thus explored the possibility that activation of CCL24 gene expression by S198A is mediated by NCoR.
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ABCA1 p.Ser198Ala 18250151:294:77
status: NEW296 However, no detectable binding to the phosphorylation mutant S198A was observed, despite the fact FIG. 8. Identification of an LXR/RXR-responsive region in the CCL24 gene.
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ABCA1 p.Ser198Ala 18250151:296:61
status: NEW307 that similar amounts of LXR␣ protein were immunoprecipitated and NCoR expression levels were similar in WT and S198A cells (not shown).
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ABCA1 p.Ser198Ala 18250151:307:118
status: NEW312 In agreement with this observation, NCoR was barely present at the d1.6 region in RAW-S198A cells compared to RAW-LXR␣ WT cells under similar conditions.
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ABCA1 p.Ser198Ala 18250151:312:86
status: NEWX
ABCA1 p.Ser198Ala 18250151:312:198
status: NEW313 These data also indicate that in the absence of ligand, this transcriptional corepressor is present at higher levels on this regulatory sequence in the CCL24 gene in WT-expressing cells than in the S198A cells, which could explain, at least in part, higher CCL24 levels in cells expressing the phosphorylation-deficient mutant.
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ABCA1 p.Ser198Ala 18250151:313:198
status: NEW328 The authors also present two forms of LXR␣ bearing double mutations (S195A and S196A, the latter being equivalent to S198A in the human sequence, and T290 and S291) that show resistance to PKA inhibition of SREBP-1c promoter FIG. 9.
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ABCA1 p.Ser198Ala 18250151:328:124
status: NEW330 ChIP assays were performed using chromatin isolated from RAW-LXR␣ (WT) (A) or WT and RAW-S198A (S198A) cells (B) treated as described in the legend to Fig. 7.
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ABCA1 p.Ser198Ala 18250151:330:96
status: NEWX
ABCA1 p.Ser198Ala 18250151:330:103
status: NEW341 Although we did not study phosphorylation of LXR␣ by PKA, our mass spectrometry assays detected S198A as the only phosphorylated residue in LXR␣.
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ABCA1 p.Ser198Ala 18250151:341:103
status: NEW343 Concerning the effects of LXR␣ phosphorylation on DNA binding and its heterodimerization with RXR, we did not observe reduced binding of the S198A mutant to different LXREs or impaired interaction between RXR and LXR␣ upon changes in LXR␣ phosphorylation by gel shift assays (not shown).
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ABCA1 p.Ser198Ala 18250151:343:148
status: NEW7 Expression of some (AIM and LPL), but not other (ABCA1 or SREBPc1) established LXR target genes is increased in RAW 264.7 cells expressing the LXRॷ S198A phosphorylation-deficient mutant compared to those with WT receptors.
X
ABCA1 p.Ser198Ala 18250151:7:154
status: NEW45 LZRSpBMN-GFP retroviral vectors carrying the FLAG-tagged wild-type (WT) or S198A mutant LXRॷ cDNA were generated.
X
ABCA1 p.Ser198Ala 18250151:45:75
status: NEW55 Recombinant retroviruses were produced by transfecting LZRSpBMN-GFP, LZRSpBMN-GFP/LXRॷ, or LZRSpBMN-GFP/S198A into 293GP cells as described previously (66).
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ABCA1 p.Ser198Ala 18250151:55:110
status: NEW57 Cells infected with either the retroviral vector devoid of an LXRॷ sequence (RAW-VO [vector only]), the FLAG-tagged WT LXRॷ (RAW-LXRॷ), or mutant S198A (RAW-S198A) were sorted for green fluorescent protein expression by fluorescence-activated cell sorting.
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ABCA1 p.Ser198Ala 18250151:57:164
status: NEWX
ABCA1 p.Ser198Ala 18250151:57:175
status: NEW81 For nuclear receptor corepressor (NCoR) coimmunoprecipitation assays, RAW-LXRॷ or RAW-S198A cells treated with vehicle or T0901317 for 2 h were cross-linked for 20 min in phosphate-buffered saline with 1.6 mM DSP [dithiobis(succinimidyl)propionate] (Pierce) prior to whole-cell extract preparation.
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ABCA1 p.Ser198Ala 18250151:81:92
status: NEW136 Specific immunoreactivity of the phospho-S198 antibody was demonstrated by its ability to recognize WT phosphorylated LXRॷ, but not phosphorylation-deficient S198A LXRॷ (see Fig. S2A in the supplemental material).
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ABCA1 p.Ser198Ala 18250151:136:164
status: NEW141 Pools of cell clones stably expressing either WT or S198A-mutated LXRॷ were generated by retroviral infection of RAW 264.7 cells, which lack endogenous LXRॷ but express LXRbeta.
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ABCA1 p.Ser198Ala 18250151:141:52
status: NEW155 (B) RAW 264.7 cells infected with a retroviral vector only (VO) or stably expressing WT or S198A FLAG-hLXRॷ were treated with 40 òe;g/ml cholesterol (Chol) in the form of soluble cholesterol-cyclodextrin complexes for 48 h.
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ABCA1 p.Ser198Ala 18250151:155:91
status: NEW174 Next, to determine the impact of S198 phosphorylation on LXRॷ function, we investigated LXR target gene expression in RAW 264.7 cells stably expressing the phosphorylation mutant S198A.
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ABCA1 p.Ser198Ala 18250151:174:185
status: NEW178 Consistent with the gene expression data, the activities of WT and S198A receptors were similar when tested in transient-transfection experiments on an ABCA1 promoter fragment containing the LXRE (reference 10 and data not shown).
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ABCA1 p.Ser198Ala 18250151:178:67
status: NEW186 (A) RAW cells stably expressing FLAG-hLXRॷ (WT or S198A) were incubated with or without 5 òe;M T0901317 ligand for 2 h.
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ABCA1 p.Ser198Ala 18250151:186:56
status: NEW194 (A) RAW-LXRॷ (WT or S198A) cells were incubated with vehicle or T0901317 ligand (T) at the indicated concentrations for 24 h.
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ABCA1 p.Ser198Ala 18250151:194:26
status: NEW198 (B) Protein expression levels of LXRॷ in RAW 264.7 cells infected with a retroviral vector only (VO) or FLAG-hLXRॷ (WT or S198A) incubated in the presence or absence of T0901317, as in panel A.
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ABCA1 p.Ser198Ala 18250151:198:134
status: NEW212 Remarkably, in RAW-S198A macrophages, CCL24 basal expression was markedly induced compared to WT LXRॷ-expressing cells (Fig. 5A) and was further dramatically increased by T0901317 in a dose-dependent manner (Fig. 5B).
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ABCA1 p.Ser198Ala 18250151:212:19
status: NEW220 The induction of CCL24 expression by DMAT was not observed in RAW-S198A cells, indicating that this effect is due to LXRॷ dephosphorylation by the CK2 inhibitor.
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ABCA1 p.Ser198Ala 18250151:220:66
status: NEW231 RAW-VO (VO) and RAW-LXRॷ (WT or S198A) cells were incubated for 24 h in medium with vehicle or 1 òe;M (A) or the indicated concentrations (B) of T0901317 LXR ligand.
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ABCA1 p.Ser198Ala 18250151:231:38
status: NEW234 Indeed, in the presence of the RXR ligand 9cRA, CCL24 induction by T0901317 in the RAW LXRॷ cells was markedly enhanced (Fig. 7A), reaching expression levels similar to those observed in untreated RAW-S198A cells (see Fig. S5 in the supplemental material).
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ABCA1 p.Ser198Ala 18250151:234:207
status: NEW238 Importantly, the synergistic action of T0901317 and 9cRA on CCL24 expression was lost in RAW-S198A cells (16-fold versus 2.7-fold over T0901317 alone in WT and S198A cells, respectively), suggesting that it is S198 phosphorylation that mediates this effect (see Fig. S5A in the supplemental material).
X
ABCA1 p.Ser198Ala 18250151:238:93
status: NEWX
ABCA1 p.Ser198Ala 18250151:238:160
status: NEW293 We thus explored the possibility that activation of CCL24 gene expression by S198A is mediated by NCoR.
X
ABCA1 p.Ser198Ala 18250151:293:77
status: NEW295 However, no detectable binding to the phosphorylation mutant S198A was observed, despite the fact FIG. 8. Identification of an LXR/RXR-responsive region in the CCL24 gene.
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ABCA1 p.Ser198Ala 18250151:295:61
status: NEW306 that similar amounts of LXRॷ protein were immunoprecipitated and NCoR expression levels were similar in WT and S198A cells (not shown).
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ABCA1 p.Ser198Ala 18250151:306:117
status: NEW311 In agreement with this observation, NCoR was barely present at the d1.6 region in RAW-S198A cells compared to RAW-LXRॷ WT cells under similar conditions.
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ABCA1 p.Ser198Ala 18250151:311:86
status: NEW327 The authors also present two forms of LXRॷ bearing double mutations (S195A and S196A, the latter being equivalent to S198A in the human sequence, and T290 and S291) that show resistance to PKA inhibition of SREBP-1c promoter FIG. 9.
X
ABCA1 p.Ser198Ala 18250151:327:123
status: NEW329 ChIP assays were performed using chromatin isolated from RAW-LXRॷ (WT) (A) or WT and RAW-S198A (S198A) cells (B) treated as described in the legend to Fig. 7.
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ABCA1 p.Ser198Ala 18250151:329:95
status: NEWX
ABCA1 p.Ser198Ala 18250151:329:102
status: NEW340 Although we did not study phosphorylation of LXRॷ by PKA, our mass spectrometry assays detected S198A as the only phosphorylated residue in LXRॷ.
X
ABCA1 p.Ser198Ala 18250151:340:102
status: NEW342 Concerning the effects of LXRॷ phosphorylation on DNA binding and its heterodimerization with RXR, we did not observe reduced binding of the S198A mutant to different LXREs or impaired interaction between RXR and LXRॷ upon changes in LXRॷ phosphorylation by gel shift assays (not shown).
X
ABCA1 p.Ser198Ala 18250151:342:147
status: NEW