The CFTR chloride channel is tightly regulated by phosphorylation at multiple serine residues. Recently it has been proposed that its activity is also regulated by tyrosine kinases, however the tyrosine phosphorylation sites remain to be identified. In this study we examined 2 candidate tyrosine residues near the boundary between the first nucleotide binding domain and the R domain, a region which is important for channel function but devoid of PKA consensus sequences. Mutating tyrosines at positions 625 and 627 dramatically reduced responses to Src or Pyk2 without altering the activation by PKA, suggesting they may contribute to CFTR regulation

Billet, Arnaud

Chang, Xiu-Bao

Hanrahan, John W.

Hou, Yue-Xian

Jensen, Timothy J.

Jia, Yanlin

Riordan, John R.

English

PubMed

Carolina Digital Repository

ARTICLE ADDENDUMPotential sites of CFTR activation by tyrosine kinasesArnaud Billeta,b, Yanlin Jiaa,b, Timothy J. Jensenc, Yue-Xian Houc, Xiu-Bao Changc, John R. Riordanc,and John W. Hanrahana,b,daDepartment of Physiology, McGill University, Montreal, Quebec, Canada; bCF Translational Research Center, McGill University, Montreal,Quebec, Canada; cDepartment of Biochemistry and Biophysics & CF Research Center, UNC Chapel Hill, Chapel Hill, NC, USA; dResearch Instituteof the McGill University Hospital Center, Montreal, Quebec, CanadaARTICLE HISTORYReceived 19 November 2015Revised 23 November 2015Accepted 23 November 2015ABSTRACTThe CFTR chloride channel is tightly regulated by phosphorylation at multiple serine residues.Recently it has been proposed that its activity is also regulated by tyrosine kinases, however thetyrosine phosphorylation sites remain to be identified. In this study we examined 2 candidatetyrosine residues near the boundary between the first nucleotide binding domain and the Rdomain, a region which is important for channel function but devoid of PKA consensus sequences.Mutating tyrosines at positions 625 and 627 dramatically reduced responses to Src or Pyk2 withoutaltering the activation by PKA, suggesting they may contribute to CFTR regulation.KEYWORDSCFTR regulation; cysticfibrosis; phosphotyrosine;Pyk2; SrcIntroductionCystic Fibrosis is caused bymutations in the cystic fibro-sis transmembrane conductance regulator (CFTR)anion channel. Like other members of the ATP-bindingcassette (ABC) transporter family, CFTR channel activ-ity is regulated by the binding and hydrolysis of ATPmolecules by the Nucleotide Binding Domains(NBDs).1,2 In addition, CFTR catalytic activity is initi-ated and regulated by phosphorylation of its unique,intrinsically disordered regulatory region or R-domain.The phosphorylation state of CFTR is controlled byboth kinases and phosphatases3 and many serines liewithin consensus sequences for phosphorylation byPKA and PKC.4 Several studies have suggested thattyrosine kinases may also influence CFTR gatingeither directly or indirectly. Direct tyrosine kinase reg-ulation was suggested by exposing excised membranepatches to c-Src kinase5 and by the sensitivity of mus-carinic stimulation of CFTR to tyrosine kinase inhibi-tors.6 Indirect regulation through a mechanism inwhich tyrosine phosphorylation unmasks a potentialCasein Kinase 2 (CK2) phospho-acceptor site(Ser511) in NBD1 has also been reported.7,8 Werecently reported that that tyrosine phosphorylationcan be a potent and direct (PKA/C-independent)stimulus for CFTR activation.9 Moreover, we foundthat the tyrosine kinases c-Src and Pyk2 are both ableto phosphorylate CFTR on tyrosine residues, and acti-vate chloride currents which are 80% as large as thosestimulated by PKA.The serine/threonine phosphorylation sites onCFTR have been identified10,11 and their contributionsto channel regulation have been characterized indetail,12-14 however the tyrosine residues that mediatedirect regulation of channel activity remain unknown.We have attempted to identify these sites using massspectrometry but so far that approach has not beensuccessful despite clear radiolabeling after incubationwith Src and [g-32P]-ATP and detection of a CFTRband in immunoprecipitates when immunoblots areprobed with anti-phosphotyrosine antibody. In thepresent work, we used a site-directed mutagenesis/functional assay approach, focusing on 2 candidatetyrosine residues near the c-terminal end of NBD1(Y625 and Y627). We found that substituting these2 tyrosine residues with phenylalanine (CFTR-YY625,627FF mutant) dramatically reduced (but didnot abolish) tyrosine kinase stimulated currents with-out altering those stimulated by PKA.CONTACT Arnaud Billet arnaud.billet@mail.mcgill.caAddendum to: Billet A, et al. Regulation of the Cystic Fibrosis Transmembrane conductance Regulator (CFTR) anion channel by tyrosine phosphorylation. FASEB J.2015; 29(9):3945-53. http://dx.doi.org/10.1096/fj.15-273151.© 2016 Taylor & FrancisCHANNELS2016, VOL. 10, NO. 3, 247–251http://dx.doi.org/10.1080/19336950.2015.1126010ResultsNone of the 40 tyrosine residues on CFTR are situatedin canonical strong sites for phosphorylation by Src orother tyrosine kinases.15 As a first step toward localiz-ing the critical tyrosines we examined the ability ofSrc to phosphorylate CFTR peptide fragments (Fig. 1).Polypeptides corresponding to full-length CFTR (a.a.1-1480, lane 1and2), first membrane domain C NBD1(a.a. 1-640, lane 3&4), first membrane domain CNBD1 C R domain (a.a. 1-830, lane 5&6) or all of theCFTR sequence that is distal to the fourth transmem-brane segment (a.a. 281-1480, lane 7&8) were stablyexpressed in BHK cells. Peptides were immunopreci-pitated from the control (¡) or v-Src expressing (C)cells using a mouse monoclonal antibody against anti-phosphotyrosine, and immunoblots were probed withthe anti-CFTR antibody L12B4. When co-expressedwith the consitutively active tyrosine kinase v-Src, allCFTR peptides could be immunoprecipitated by anti-phosphotyrosine antibody as indicated by bands attheir predicted molecular weights (Fig. 1 blackarrows). Tyrosine phosphorylation of all 3 peptidesmight be explained by the phosphorylation of one ormore tyrosines between a.a. 281-640, the region ofCFTR which is shared by these peptides, which werefer to as the “optimistic hypothesis”. Alternatively,the results are also consistent with the presence ofmultiple phosphotyrosines distributed throughout themolecule.We tested the optimistic hypothesis (i.e., thatphosphotyrosine is detectable on all the peptidesbecause it is situated in the region of overlap) bysubstituting the most likely candidate tyrosine resi-dues, Y625 and Y627, simultaneously with phenylala-nine. Silent patches were excised from BHK stablyexpressing the double mutant (CFTR-YY625,627FF)and exposed to active phospho-Src or to the catalyticdomain of Pyk2 (30U/ml for both kinases). Wt-CFTR current was strongly activated by both tyrosinekinases. Figure 2A and B show representative tracesof wt-CFTR activity induced by Src and Pyk2, respec-tively. By contrast, CFTR channel activation by the 2tested tyrosine kinases was strongly decreased in thedouble mutant compared to the normal responses toPKA (75 nM), which was added at the end of eachexperiment (Fig. 2C and D). Strong activation byPKA confirmed the presence of mutant CFTR chan-nels in the patch and indicate that substituting phe-nylalanine at Y625 and Y627 did not grossly affectchannel function.To compare the activation by different kinases weadded the non-hydrolysable ATP analog AMP-PNP(1mM) at the end of experiments and calculated thecurrent ratio to help normalize for variation in thenumber of channels per patch as described previ-ously.9 Figure 2E shows a histogram of the currentratios obtained in presence of 30U/ml Src, Pyk2, or75nM PKA. The ratios revealed a dramaticallydecrease in the activation of YY625,627FF CFTR bySrc or Pyk2 (current ratios 0.20 and 0.13 respectively,n D 3) compared to wild-type CFTR. This contrastedwith the current ratio during application of PKA,which was similar for mutant (current ratio 0.51,n D 5) and wild-type channels. These data stronglysuggest that phosphorylation of one or both tyrosinescontributes to CFTR activation by Src and Pyk2,although part (25 – 40%) of the response is apparentlydue to other sites which remain to be identified.Figure 1. Phosphorylation of CFTR by Src kinase. Blot of anto-phosphotyrosine immunoprecipitates probed with the anti-CFTRmonoclonal antibody L12B4. CFTR peptides (identified by theboundary amino acid numbers indicated above each pair oflanes) co-expressed with or without v-Src and precipitated usingmonoclonal antibody against phosphotyrosine. Black arrows indi-cate the positions of CFTR phosphopeptides. The bands at~50 and~100 kDa observed in every lane indicate mono- and dimericheavy chains of the immunoprecipitating IgG, which are recog-nized by the secondary antibody used for immunoblotting. Blackarrows indicate CFTR fragments. A representative of 2 experi-ments is shown.248 A. BILLET ET AL.DiscussionIn a previous study we found that the tyrosine kinasesSrc and Pyk2 can activate wild-type CFTR, producingcurrents that reach 80% of those stimulated by PKA.9Here we observed a dramatic decrease in tyrosinekinase-activated currents when Y625 and Y627 weremutagenized to phenylalanine (YY625,627FF) in full-length CFTR. Since PKA stimulation was not alteredin the double mutant, one or both tyrosine residuesmay contribute to CFTR activation by tyrosinekinases.As a first approach toward localizing the site wecoexpressed peptides corresponding to differentregions of CFTR together with v-Src and examinedtheir in vivo phosphorylation by immunoprecipitationwith anti-phosphotyrosine antibody and blotting withanti-CFTR antibody. Phosphotyrosine was detectedon all 3 peptides, therefore we focused on tyrosines inthe region of overlap (amino acids 281 – 640), whichoccur in the sequence KILI[LHEGSSY625]FY627GTF.Based on the preferential phosphorylation ofsequences in a peptide library, E(2-3)-I/V-Y- G/Figure 2. Effect of Src and Pyk2 on activity of the CFTR double mutant YY625,627FF. (A–D): Effect of Src (A & C) and Pyk2 (B & D) onchannel activity in patch excised from cell expressing wt (A&B) or YY625,627FF (C & D) CFTR. (E): Comparison of the mean ratio of thekinase- stimulated currents measured before and after addition of 1 mM AMP-PNP. Error bars show SE for number of cells indicated. ,p< 0.05; , p< 0.01 with student t-test. The wt-CFTR results from Billet et al 20159 obtained under identical conditions are reproducedhere for comparison with YY625,627FF-CFTR mutant.CHANNELS 249E-X-F15 was proposed to be the ideal Src consensus.The three residues following Y627 fit this consensus,however the non-polar residue and 2 or 3 upstreamglutamates are lacking. This divergence from the idealconsensus may explain why high activity, i.e., heterol-ogous expression of constitutively active v-Src, wasneeded to be able to detect tyrosine phosphorylationin intact cells. We cannot exclude other explanationshowever as the specificity may depend on factors otherthan the primary sequence, and Src kinases are knownto phosphorylate a range of target sequences.16 Thesequence upstream of Y625 and Y627 bears someresemblance to the generic protein tyrosine kinase(PTK) consensus R/K-[X(2/3)-D/E-X(3/2)-Y], sug-gesting these sites in CFTR might also be a substratesfor other tyrosine kinases under physiological condi-tions. The lack of PKA sites near these sites reinforcethe notion that phosphotyrosine acts specificallyrather than as a surrogate for phosphoserine.Interestingly, Y625 and Y627 are situated at thejunction between NBD1 and the R domain, a regionin which structural integrity is crucial for channel reg-ulation and pharmacology.17,18 Further studies oftyrosine kinase regulation may provide a betterunderstanding of R domain structure and the confor-mational changes associated with CFTR channelregulation.MethodsPlasmid and cell cultureBaby hamster kidney (BHK) cells stably expressingwild-type CFTR or the YY625,627FF-CFTR mutant10were plated on plastic coverslips at low density and cul-tured in MEM (Life Technologies, Burlington, ON,Canada) containing 5% FBS and the selecting drugmethotrexate (300-500 mM) for 2 days with 5% CO2 at37C. To express peptides comprising different regionsof CFTR, cDNAs encoding amino acids 1-640, 1-830,and 281- 1480 were prepared by PCR mutagenesis,inserted into the pNUT vector, and stably transfectedinto BHK cells. The role of tyrosines 625 and 627 ofCFTR in the activation by Src was examined by substi-tuting them with phenylalanines using site-directedmutagenesis. An expression plasmid containing v-SrccDNA was kindly provided by Dr. R. Huganir (Depart-ment of Neuroscience, Johns Hopkins University) andco-transfected with large T antigen plasmid into BHKcells using calcium phosphate co-precipitation.Tyrosine phosphorylationTo detect phosphotyrosine on CFTR, cells in 25 cm2dishes were transiently transfected using calcium phos-phate coprecipitation with 5 mg of v-Src plasmid DNAand 1 mg of a large T-antigen expressing plasmid. Twodays after Src transfection, cells were lysed in RIPAbuffer and subjected to sequential immunoprecipitationand immunoblotting. For immunoprecipitation weused an anti-phosphotyrosine monoclonal antibody,which recognizes an epitope between residues 1365 and1395 of CFTR. The monoclonal antibody L12B4, whichrecognizes an epitope between residues 386 and 412 ofCFTR, was used for immunoblotting.Patch clampMicroscopic CFTR currents were recorded frominside-out patches as previously described.9 The ratioof currents activated by kinase in the absence vs pres-ence of AMP-PNP (which further increases openprobability to near Po D 1.0) allowed CFTRresponses to be normalized for variations in thenumber of channels per patch. Recombinant Src(30U/ml) was from EMD Millipore; the catalyticdomain of Pyk2(30U/ml) was from Cedarlane (Bur-lington, ON, Canada); PKA (final concentration,75 nM–30 U) was from Promega (Madison, WI,USA); MgATP (1 mM) was from Sigma-Aldrich, andAMP-PNP (1 mM) was from Sigma-Aldrich (St.Louis, MO, USA).AcknowledgmentsAB was supported by fellowships from the Groupe d’Etude desProteines Membranaire (GEPROM), the Groupe de RechercheAxe sur la Structure des Proteines (GRASP), the McGill CIHRProgram in Chemical Biology and the McGill Faculty of Medi-cine. YJ was supported by the Respiratory Health Network ofCenters of Excellence and fellowships from the Canadian LungAssociation/Medical Research Council and Canadian CysticFibrosis Foundation.Disclosure of potential conflicts of interestNo potential conflicts of interest were disclosed.FundingThis work was funded by grants from the NIH and CIHR toJRR and JWH, respectively.250 A. 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Potential sites of CFTR activation by tyrosine kinases

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Potential sites of CFTR activation by tyrosine kinases

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