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W1998849803 abstract "Article18 December 2003free access Identification of PKCζII: an endogenous inhibitor of cell polarity Scott J Parkinson Scott J ParkinsonCurrent address: Dana-Farber Cancer Institute, Division of Cancer Biology, Harvard Medical School, Boston 02115, USA. E-mail: [email protected]Search for more papers by this author J Anne Le Good J Anne Le GoodCurrent address: ISREC, Chemin des Boveresses 155, CH 1066 Epalinges, Switzerland Search for more papers by this author Richard DH Whelan Richard DH Whelan Search for more papers by this author Phil Whitehead Phil Whitehead Search for more papers by this author Peter J Parker Corresponding Author Peter J Parker Protein Phosphorylation Laboratory, Cancer Research UK, London Research Institute, London, UK Search for more papers by this author Scott J Parkinson Scott J ParkinsonCurrent address: Dana-Farber Cancer Institute, Division of Cancer Biology, Harvard Medical School, Boston 02115, USA. E-mail: [email protected]Search for more papers by this author J Anne Le Good J Anne Le GoodCurrent address: ISREC, Chemin des Boveresses 155, CH 1066 Epalinges, Switzerland Search for more papers by this author Richard DH Whelan Richard DH Whelan Search for more papers by this author Phil Whitehead Phil Whitehead Search for more papers by this author Peter J Parker Corresponding Author Peter J Parker Protein Phosphorylation Laboratory, Cancer Research UK, London Research Institute, London, UK Search for more papers by this author Author Information Scott J Parkinson, J Anne Le Good, Richard DH Whelan, Phil Whitehead and Peter J Parker 1 1Protein Phosphorylation Laboratory, Cancer Research UK, London Research Institute, London, UK *Corresponding author. Protein Phosphorylation Laboratory, Cancer Research UK, London Research Institute, 44 Lincoln's Inn Fields, London WC2A3PX, UK. Tel.: 020 7242 0200; Fax: 020 7269 3094; E-mail: [email protected] The EMBO Journal (2004)23:77-88https://doi.org/10.1038/sj.emboj.7600023 PDFDownload PDF of article text and main figures. ToolsAdd to favoritesDownload CitationsTrack CitationsPermissions ShareFacebookTwitterLinked InMendeleyWechatReddit Figures & Info A new member of the atypical protein kinase C (aPKC) family, designated PKCζII, is identified in this study. The gene contains no introns and is 98% homologous with the cDNA encoding PKCζ. The PKCζII coding region is frame-shifted with respect to the PKCζ open reading frame, resulting in expression of an aPKC regulatory domain without associated kinase activity. PKCζII mRNA is detected in various mouse tissues and an immunoreactive 45 kDa protein is present in epithelial cell cultures. PKCζII is shown to interact with the Par6 protein and functions in the development of cell polarity. HC11 epithelial cells express PKCζII and are maintained in a nondifferentiated state characterised by the absence of tight junctions and cell overgrowth. HC11 cells harbouring a PKCζII-specific RNAi, recruit ZO-1 and other tight junction markers to cell–cell boundaries and adopt a monolayer phenotype in the presence of growth factors. The data demonstrate a regulatory role for PKCζII in the maintenance of cell transformation and the development of cell polarity. Introduction Cell polarisation is a fundamental property of every cell type, with symmetric and/or asymmetric distribution of cellular components being essential for the development, cell division, cell migration, and maintenance of specialised compartments within cells. Atypical protein kinase (aPKC) is implicated in the development of cellular asymmetry and contributes to astrocyte migration and epithelial cell polarity (Joberty et al, 2000; Lin et al, 2000; Etienne-Manneville and Hall, 2001; Hirose et al, 2002). Epithelial cells are composed of distinct apical (lumenal) and basolateral domains separated by a specialised cellular structure known as the tight junction. The tight junction maintains a barrier that prevents diffusion of molecules across the epithelial cell layer (Dragsten et al, 1981). The protein components of the tight junction are beginning to be elucidated. The junctional adhesion molecules (JAMs) appear to be essential for tight junction assembly; monoclonal antibodies against JAMs inhibit junction formation following Ca2+ switch (Liu et al, 2000). These transmembrane proteins associate as dimers in trans through their extracellular domains at sites of cell–cell contact and recruit intracellular scaffolding components to the tight junction (Kostrewa et al, 2001). The intracellular domains of JAMs bind directly to the first PDZ domain of the cell polarity protein Par3/Asip/Bazooka (Ebnet et al, 2001). Par3 also associates with Par6, Cdc42, and aPKC (Joberty et al, 2000; Lin et al, 2000) all of which contribute to tight junction formation. The JAMs, as well as the tight-junction-localised proteins occludin and the claudins, also associate with the PDZ domains of the ZO family of scaffolding proteins (Furuse et al, 1993, 1998; Fanning et al, 1998; Haskins et al, 1998, Itoh et al, 1999). aPKCs appear to be essential for the formation but not maintenance of tight junctions. MDCK cells expressing kinase-inactive aPKC mutants appear normal, however after Ca2+ depletion to disrupt cell–cell contacts, the localisation of the tight junction markers ZO-1, Par3, occludin, and claudin-1 is erratic following Ca2+ replacement (Suzuki et al, 2001). These and other observations led to the hypothesis that aPKCs catalyse the transition of premature cellular junctions into differentiated asymmetric structures (Suzuki et al, 2002). The aPKCs are activated by protein–protein interactions within the regulatory domains of the proteins. This serves the two purposes of destabilising the pseudosubstrate site interaction with the catalytic domain permitting binding/phosphorylation of substrate and tethering the kinase activity to specific regions of the cell (Moscat and Diaz-Meco, 2000). PKCζ and PKCλ/ι are homologous proteins that interact with Par6, a protein necessary for cellular asymmetry and asymmetric cell division. Interaction of aPKCs with Par6 restricts their localisation in the cell and activates their kinase activity (Joberty et al, 2000; Lin et al, 2000). In addition to the full-length aPKCs, there is also a PKCζ isoform (PKMζ) synthesised following transcription initiation of the PKCζ gene from a brain-specific promoter located in an intron (Marshall et al, 2000). This results in translation of an aPKC catalytic protein lacking the regulatory domain. The PKMζ transcript is implicated in long-term potentiation, likely as a result of its constitutive kinase activity (Sacktor et al, 1993, Osten et al, 1996). In this study, we describe the identification and characterisation of a distinct aPKC gene, designated PKCζII. This gene has a unique chromosomal localisation and is 98% identical with the cDNA encoding PKCζ. An immunoreactive protein corresponding to PKCζII is detected in cultured cell lines and RNA can be detected in many mouse tissues. Amongst the 29 bp differences with PKCζ, a deletion at nucleotide C1146 of PKCζII shifts the reading frame and results in truncation of the protein at amino acid 376. Therefore, PKCζII is composed of an aPKC regulatory domain without a functional catalytic domain. Recombinant PKCζII is partitioned in the nucleus, however its location changes when it interacts with proteins intrinsic to development of tight junctions. Expression of endogenous PKCζII in epithelial cells disrupts the assembly of tight junctions and promotes overgrowth of cells demonstrating its role in regulating aPKC-dependent functions. Results Cloning and identification of PKCζII A stringent screen of a mouse genomic library (using the 5′ end of the PKCζ cDNA as a probe) identified three hybridising clones. The three clones were identical by restriction analysis and Southern blotting. Clone 3, containing a 13 kb insert, was selected for further analysis. Sequencing revealed this clone to contain a DNA sequence homologous with PKCζ that was designated PKCζII (the genomic sequence has been annotated recently by the NCBI Annotation Project and is designated locus XM_124895). The genomic sequence of PKCζII was approximately 98% identical at the nucleotide level with the cDNA encoding ‘authentic’ murine PKCζ (Figure 1) and retained a 3′UTR containing AATAAA poly A addition signal and a poly A stretch (data not shown). The PKCζII genomic sequence contains 29 nucleotide divergencies with respect to the PKCζ cDNA sequence including deletion of nucleotides C1146, G1943, and a region flanking the PKCζ stop codon (C1779–G1819). Figure 1.Nucleotide alignment of murine PKCζII genomic DNA with murine PKCζ cDNA (accession number M94632). Predicted start codons are bold and overmarked with ***. Differences in nucleotide sequences are red and underlined. Stop codons for murPKCζII (green) and murPKCζ (blue) are also underlined. Download figure Download PowerPoint Translation of the putative coding region of PKCζII demonstrates a high degree of identity at the protein level with PKCζ (Figure 2). The start codon of PKCζ is conserved in PKCζII; however, the nucleotide deletion of C1146 in PKCζII results in a shift of the reading frame and termination of the putative coding region at nt1152 (Figure 1). Following translation, PKCζII would comprise a functional regulatory domain homologous with PKCζ. The differences between PKCζ and PKCζII in the catalytic region, however, are significant. In addition to loss of 60% of the catalytic domain, the shift in the PKCζII reading frame converts amino acid D356 to a threonine. This mutation ensures PKCζII lacks all catalytic activity since D356 is the catalytic base of PKCζ responsible for stabilising the serine/threonine oxyanion of the substrate prior to transfer of the γ phosphate from ATP (Protein Kinase Resource: www.sdsc.edu/kinases/). The frame shift also terminates the coding sequence in subdomain VIB (the catalytic loop) of the kinase domain suggesting that there is no catalytic function for this putative protein (see below). Figure 2.Amino acid alignment of murPKCζII with murPKMζ, murPKCζ (accession number M94632). The amino acid sequences of PKCζ and PKCζII were predicted from the nucleic acid sequence in Figure 1. The PKMζ sequence was derived from sequenced RT–PCR products in Figure 3 (below). Amino acid differences are underlined. The three shadowed sequences define the three domains of the protein; in order from the amino-terminus of PKCζ these are PB1, C1, and kinase domains. Download figure Download PowerPoint Fluorescence in situ hybridisation (FISH) was performed to map the location of PKCζ and PKCζII on mouse metaphase spreads stained with specific chromosome paints (Figure 3A, A′). Probes specific for PKCζII (X7; see Materials and methods) hybridised strongly to chromosome 7(A2–3 region). PKCζ-specific hybridising probes (pZ-X5; see Materials and methods) hybridised with chromosome 4(E2 region). These locations were also confirmed by analysis of the Celera mouse genome database using the nucleotide sequences in Figure 1 (J Sgouros and S Parkinson, unpublished). Thus PKCζII has a unique chromosomal location on chromosome 7. Figure 3.The gene encoding PKCζII is on mouse chromosome number 7 and is transcribed and translated in various tissues and cell lines. (A) Chromosome localisation of the PKCζII gene. FISH was performed with a specific probe recognising the PKCζII 3′UTR and chromosomal paints recognising chromosome 7. Hybridising regions of the PKCζII probe are indicated with red arrows and correlate with the highlighted chromosome 7s (right panel). (A′) Chromosome localisation of the PKCζ gene. FISH was performed with a specific probe recognising an intron sequence from the murine PKCζ gene and chromosomal paints recognising chromosome 4. Fluorescent-tagged PKCζ hybridising regions are indicated with a red arrow and correlate with the presence of chromosome 4 in the right panel. (B) Transcription of aPKCs detected in mouse tissues by RT–PCR. Total RNA was isolated from the indicated Balb/C mouse tissues and treated with DNAse. All RNAs were free of DNA contamination as demonstrated by a lack of visible β-actin or PKCζII product in the absence of reverse transcriptase (not shown). The specific primers used to detect PKCζ, PKMζ, and PKCζII are indicated in Materials and methods. (C) In vitro transcription/translation of isolated PKCζII genomic clone and detection of a 45 kDa protein. Genomic DNA encoding PKCζII was added to a rat reticulocyte lysate and transcribed and translated in vitro in the presence of 35S methionine. The following templates were used: lane 1—PKCζII no ATG, lane 2—PKCζII no 5′-UTR, lane 3—PKCζII with 5′ and 3′ UTR, lane 4—PKCζII 3′UTR only, lane 5—luciferase control. (D) myc-PKCξ or PKCξII were expressed in Cos7 cells and immunopurified. Activity was determined against myelin basic protein (MBP) as described in Materials and methods. (E) Detection of endogenous PKCζII protein in various cell lines. The indicated cell lines were grown to confluence, trypsinised, counted, and lysed in sample buffer. Lysate from the equivalent of 106 cells was loaded on 12.5% PAGE gel, transferred to PVDF and incubated with an antibody directed against the C-terminus to detect full-length aPKCs (λ/ι/ζ) (top panel) or an antibody directed against the N-terminus to detect PKCζII (bottom panel) (see Materials and methods for specificity). Lysate from Cos7 cells expressing a PKCζII cDNA plasmid (Cos7 (PKCζII)) is included as a migration control. Download figure Download PowerPoint The data indicate that a PKCζ-like gene on chromosome 7, lacking any introns, encodes a protein with an atypical PKC regulatory domain. To determine if this PKCζ-homologous region is simply a nonexpressed pseudogene, Balb/c mouse RNA was extracted from various organs in order to assess PKCζII transcription by RT–PCR (Figure 3B). Since PKCζII genomic DNA contains no introns, extreme care was taken to ensure there was no DNA contamination of the extracted RNAs. Specific primers were designed that only amplified PKCζ, PKMζ, or PKCζII, as determined in control reactions. RNA encoding PKCζ was detected primarily in muscle, heart, lung, kidney, and liver. PKMζ RNA was abundant in the brain and could not be detected in other tissues. RNA derived from PKCζII was abundant in bone, lung, kidney, and liver, however it could be detected in most of the tissues tested. This demonstrates that PKCζII is transcribed from its locus on chromosome 7. Next, we sought to address whether the RNA detected (Figure 3B) could be translated, generating this putative novel aPKC protein. In vitro transcription/translation of the open reading frame of the PKCζII genomic sequence identified the expected 45 kDa protein following autoradiography (Figure 3C). Detection was dependent on the ATG homologous to the PKCζ open reading frame and, as expected, the T7-dependent product was disrupted by the presence of the 5′UTR. No product was detected from the 3′UTR only, demonstrating that the identified protein product derives from translation of the predicted open reading frame identified in Figure 2. Expression and immunoprecipitation of PKCζII or PKCζ as a positive control demonstrated conclusively that PKCζII had no intrinsic catalytic activity (Figure 3D). In order to determine whether PKCζII was expressed in vivo, an antibody recognising the amino terminus of PKCζ (kindly provided by Dr T Sacktor) was used to determine the expression of PKCζII in various cell lines. PKCζII and PKCζ contain virtually identical N-termini. Therefore, detection of an immunoreactive 45 kDa band would indicate the presence of a PKCζII-related protein (Figure 3E). Various cell lines were grown to confluence, the number of cells determined and lysates analysed by Western blot using the N-terminal PKCζ antibody or C-terminal aPKC antibody. A C-terminal antibody that does not distinguish between the aPKC subtypes (ζ/ι/λ) (71 kDa; Figure 3E, top panel) gave a signal following Western blot analysis of total cell lysates. NIH and U251 cells also gave a signal following longer exposure of the film. An N-terminal PKCζ-specific antibody detected a 45 kDa band that comigrated with that detected in lysates from Cos7 cells transfected with a plasmid encoding PKCζII. Full-length PKCζ could also be detected by the N-terminal antibody in these epithelial cell lines. This data support the conclusion that the PKCζII genomic locus on mouse chromosome 7A2–3 encodes a new member of the aPKC family. An equivalent protein species is detected in human (293, Hela, MCF10A, MCF7), green monkey (Cos7), mouse (NIH3T3, HC11) and canine (MDCK)-derived cells suggesting PKCζII is expressed across mammalian species. PKCζII interacts with Par6 and PKMζ To determine the potential for PKCζII to interact with candidate partners, we exploited the fact that ectopic expression of tagged PKCζII in COS7 cells produced an accumulation of the fusion protein in nuclei, such that the influence of coexpressed proteins could be investigated. Recombinant PKCζII and candidate binding partners were expressed in Cos7 cells tagged with the fluorescent proteins, CFP or YFP. YFP-PKCζII (Figure 4A; top left) was found primarily in the nucleus and could also be observed at cell contacts (Figure 4A; top left, arrow). This was in contrast to YFP-PKMζ (Figure 4A; bottom right) and YFP-PKCζ (not shown), which were located almost exclusively in the cytoplasm. Figure 4.Characterisation of PKCζII localisation and protein interactions. (A) Localisation of PKCζII, PKCζIIA119E, PKCζ, and Par6c by live-cell confocal microscopy. YFP-tagged plasmids encoding PKCζII (top left), PKCζIIA119E (bottom left), PKMζ (bottom right) and Par6c (top right) were transfected into Cos7 cells and visualised (pseudocolour red) by confocal microscopy (bar=50 μM). (B) PKCζII and PKMζ colocalise in the cytoplasm of coexpressing cells. Cos7 cells (phase, top right) expressing YFP-PKMζ (red) and CFP-PKCξII (green) were observed by live-cell confocal microscopy (merge, bottom right) (bar=50 μM). (C) PKCζII and Par6c colocalise in the cytoplasm of coexpressing cells. Cos7 cells (phase, top right) expressing YFP-PKCζII (red) and CFP-Par6c (green) were visualised by live-cell confocal microscopy (merge, bottom right) (bar=30 μM). (D) Interaction with PKMζ stabilises PKCζII in the cytoplasm. Cos7 cells (Cont) expressing mycPKCζII (mycζII), PKMζ (PKMζ) or coexpressing mycPKCζII and PKMζ (mycζII+PKMζ) were lysed and nuclear-rich fractions obtained as described in Materials and methods. Equivalent volumes of nuclear (N) or cytoplasmic (C) fractions in sample buffer were run on a 12.5% PAGE gel, transferred to PVDF and immunoblotted with 9E10 (anti-myc) or aPKC C-terminal (aPKC C-term) antibodies. PKCλ/ι is endogenously expressed in Cos7 cells. (E) The intensity of the indicated bands (PKCλ/ι, PKMζ, or mycζII) from Figure 4D were quantitated (NIH ImageQuant) from three independent experiments and the percentage of protein in the nuclear (open bars) or cytoplasmic (closed bars) fractions was quantified (±s.d.). (F) PKCζII forms a complex with Par6c or PKMζ that is not dependent on the pseudosubstrate site. Cos7 cells (lane 1) expressing PKMζ (lane 2), flagPar6c (lane 3), mycPKCζIIA119E (lane 4), mycPKCζIIA119E+PKMζ (lane 5), mycPKCζIIA119E+flagPar6c (lane 6) mycPKCζII (lane 7), mycPKCζII+PKMζ (lane 8) or mycPKCζII+flagPar6c (lane 9) were lysed and the detergent-soluble fraction was incubated with Protein G Sepharose-coupled 9E10 (αmyc) antibody. Detergent soluble (LOAD; bottom panels; 1:25 of total) and immunoprecipitates (mycIP; top panels) were run on 12.5% gels, transferred to PVDF and associated proteins were detected by probing with anti-aPKC C-terminal (PKMζ), anti-flag (flagPar6c), or anti-myc (mycPKCζII/mycζIIA119E) primary antibodies. Download figure Download PowerPoint PKCζII retains the regulatory domains predicted to be required for interaction with the aPKC catalytic domain (PKMζ) and also with regulatory protein Par6. Expressed alone, PKCζII and PKMζ are located in nonoverlapping regions of the cell (Figure 4A). However, when CFP-PKCζII and YFP-PKMζ were coexpressed in Cos7 cells, CFP-PKCζII was observed in the cytoplasm in proportion to the relative PKMζ expression (Figure 4B). In high YFP-PKMζ-expressing cells (single arrowhead) CFP-PKCζII was observed in the cytoplasm. In relatively low YFP-PKMζ-expressing cells (double arrowhead) CFP-PKCζII still accumulated in the nucleus. PKMζ and full-length PKCζ express identical catalytic domains. Despite the presence of its own regulatory domain, PKCζ could also stabilise PKCζII in the cytoplasm although this required significantly higher expression levels for PKCζ than those for PKMζ (data not shown). These data suggest that the PKCζ catalytic domain can interact with PKCζII. Expressed alone, Par6c (Figure 4A; top right) could be detected in both the cytoplasm and nucleus of cells while, as noted above, PKCζII (Figure 4A; top left) was primarily nuclear. In low expressing CFP-Par6c cells, YFP-PKCζII retained its nuclear localisation (single arrowheads; Figure 4C), however in high CFP-Par6c-expressing cells YFP-PKCζII resided in the cytoplasm (Figure 4C; double arrowhead) suggesting that Par6c interacts with PKCζII in vivo. The effects on cellular localisation of PKCζII were also assessed by cell fractionation (Figure 4D, E). Crude nuclear and cytoplasmic fractions were isolated from Cos7 cells expressing mycPKCζII, PKMζ or mycPKCζII, and PKMζ and the distribution of the expressed proteins was evaluated in the two fractions. Endogenous PKCλ/ι and exogenous PKMζ were primarily cytoplasmic in the presence or absence of mycPKCζII. MycPKCζII was detected primarily in the nucleus when expressed alone in Cos7 cells. However, it appeared mainly in the cytoplasmic fraction when coexpressed with PKMζ. This cell fractionation supports the fluorescent microscopy results presented in Figure 4B. These data, exploiting the subcellular location observed on overexpression of PKCζII, indicate that PKCζII can interact with aPKCs and with aPKC regulatory proteins mutually regulating their cellular location. The pseudosubstrate site of PKCζII is a potential regulatory site that mediates interaction with the catalytic domain of the aPKCs. In addition, Par6 interacts with the N-terminal 120 amino acids of the aPKCs that includes the pseudosubstrate site. Interestingly, mutation of the PKCζII pseudosubstrate site (A119E) stabilises the protein in the cytoplasm (Figure 4A; bottom left). This indicates that the pseudosubstrate site determines the nuclear location of the overexpressed protein. To investigate this further, mycPKCζII or mycPKCζIIA119E was expressed in Cos7 cells with flagPar6c or PKMζ and their association was examined following immunoprecipitation with the anti-myc 9E10 antibody (Figure 4F). The flagPar6c and PKMζ detected in immunoprecipitates were specific for mycPKCζII-expressing cells. Notably, mutation of the mycPKCζII pseudosubstrate site (mycζIIA119E) had no effect on the interaction between PKCζII and PKMζ or flagPar6c (see Discussion). This indicates that while the pseudosubstrate site contributes to nuclear localisation it is not required for binding to PKCζ or Par6. It is likely however that PKCζII binding to these proteins blocks recognition of its pseudosubstrate site, leading to inefficient nuclear import. PKCζII inhibits tight junction formation in mammary epithelial cells PKCζII protein interacts with the cell polarity protein Par6 (Figure 4). This suggests that PKCζII could play a role in development of cellular junctions. It was previously reported that aPKC activity was required for the formation but not maintenance of tight junctions presumably via aPKC interaction with Par6 (Suzuki et al, 2001). PKCζII lacks any catalytic activity and could compete with aPKCs for binding to Par6 (Figure 4) inhibiting tight junction formation. Therefore, the role of endogenous PKCζII in the development of cell junctions was investigated using an RNAi approach. HC11 cells are a mouse mammary epithelial cell line endogenously expressing PKCζII (Figure 3B). They are normally maintained in an undifferentiated state in the presence of EGF and insulin. However, they form tight junctions and become differentiated in response to lactogenic hormones and produce β-casein and other differentiation markers (Stelwagen et al, 1999; Xie et al, 2002). Preliminary experiments demonstrated that the selected RNAi sequence specifically inhibited expression of recombinant PKCζII but not PKCζ in 293T cells (data not shown). HC11 cells were infected with an ecotropic retrovirus driving transcription of this RNAi molecule complementary and specific to PKCζII. RNA was extracted from HC11 cells infected with the PKCζII RNAi retrovirus (pSRII) or control virus (pSR), and the expression of PKCζ, PKCζII, and β-actin was assessed by RT–PCR (Figure 5A). HC11 pSRII cells showed a significant loss of PKCζII message in all conditions tested while the detection of PKCζ was unaffected demonstrating the specificity of the targeting sequence. The levels of expressed proteins were also assessed in the two cell lines (Figure 5B). Western blot analysis revealed a loss of the 45 kDa immunoreactive band (PKCζII) in pSRII cells while no significant difference in the 70 kDa band (PKCζ) was observed between pSR and pSRII HC11 lysates. These data demonstrate that the PKCζII gene identified here is expressed and further that PKCζII is translated from an mRNA distinct from PKCζ. Figure 5.PKCζII inhibits formation of tight junctions in HC11 cells. (A) PKCζII RNAi specifically reduces PKCζII, but not PKCζ RNA. RT–PCR detection of PKCζII, PKCζ, and β-actin message in control HC11 cells (pSR) and PKCζII RNAi-expressing HC11 cells (pSRII). Cells were grown to confluence on 6 cm2 plates under standard growth conditions (EGF, INS, and SER). Following confluence, parallel cultures were switched to 2% serum for 24 h (serum) and then treated with prolactin/hydrocortisone (prolactin) for 72 h to induce differentiation (Xie et al, 2002). Cells grown under these different conditions were harvested, RNA extracted, DNAse treated and the indicated message amplified with specific primers. For clarity, the images shown are negatives. Differentiation was confirmed by β-casein mRNA expression (not shown). DNA contamination was minimal as detected by the lack of amplification of β-actin in the absence of reverse transcriptase using the specified primers (β-actin – RT). (B) Western blot detection of PKCζ and PKCζII in HC11 pSR (control) and HC11 pSRII (PKCζII RNAi) cells. HC11 pSR and pSRII cells were grown for 72 h postconfluence and the proteins extracted in lysis buffer. Lysates were run on 10% PAGE gels, transferred to PVDF membrane and immunoblotted with rabbit antibodies against the N-terminus of PKCζ or the C-terminus of atypical PKCs. PKCζII is recognised by the N-terminal but not C-terminal antibody and is decreased in HC11 pSRII (PKCζII RNAi) versus pSR (control) cells. The asterisk denotes a nonspecific immunoreactive band. (C) Immunostaining of adherence and tight junction markers in HC11 pSR (control) and HC11 pSRII (PKCζII RNAi) cells. Cells were seeded on glass coverslips and grown to confluence in EGF, insulin, and 10% serum. After 72 h, cells were fixed in MeOH and stained to detect β-catenin, β-actin, and ZO-1. Single confocal sections (0.5 μm) are shown for the two cell lines (bar=50 μm). (D) PKCζII is necessary for the transformed phenotype of HC11 cells. HC11 pSR or pSRII cells were grown for 72 h postconfluence and stained with propidium iodide to identify nuclei (red) and an antibody against ZO-1 (green). Z stack profiles (top, bar=10 μm) of stained cells are shown above confocal images in the X–Y plane (bottom, bar=50 μM). Download figure Download PowerPoint Using the RNAi cell lines characterised in Figure 5A and B, we investigated the role of PKCζII in the development of cell polarity. HC11 pSR and HC11 pSRII cells were seeded on coverslips, allowed to grow to confluence, fixed and stained for various junction markers (Figure 5C). Loss of PKCζII in pSRII cells correlated with the appearance of contiguous staining of ZO-1 in the apical plane. This contrasts with pSR cells where ZO-1 staining is punctate throughout the cytoplasm and disjointed at cell junctions. A similar pattern of behaviour was observed for the tight junction marker claudin-1 (data not shown). The β-actin staining was consistent with the ZO-1 localisation. Bundled cortical actin could be observed in the apical plane of pSRII but not pSR cells. The adherens junction marker β-catenin was located at cell–cell contacts in both cell lines suggesting that PKCζII did not regulate adherens junction formation. These results suggest that PKCζII specifically inhibits the development of tight junctions in HC11 cells. In growth media containing EGF and insulin, HC11 cells adopt a transformed phenotype. They are characteristically rounded and grow in multiple layers losing contact inhibition (pSR cells, Figure 5D). However, in pSRII cells, loss of PKCζII correlates with a monolayer phenotype as demonstrated in Z stacks of cells stained with propidium iodide to label nuclei. The loss of cell overgrowth (ie monolayer growth) can also be observed in orthogonal sections of cells stained with E-cadherin and β-catenin (Figure 6). The adherens junction marker localises to areas of cell–cell contact and multiple layers of cells can be observed. Blocking PKCζII expression repressed the transfo" @default.
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W1998849803 title "Identification of PKCζII: an endogenous inhibitor of cell polarity" @default.
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