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Plectin isoform 1b mediates mitochondrion–intermediate filament network linkage and controls organelle shape
Correspondence to G. Wiche: gerhard.wiche{at}univie.ac.at
Plectin is a versatile intermediate filament (IF)–bound cytolinker protein with a variety of differentially spliced isoforms accounting for its multiple functions. One particular isoform, plectin 1b (P1b), remains associated with mitochondria after biochemical fractionation of fibroblasts and cells expressing exogenous P1b. Here, we determined that P1b is inserted into the outer mitochondrial membrane with the exon 1b–encoded N-terminal sequence serving as a mitochondrial targeting and anchoring signal. To study P1b-related mitochondrial functions, we generated mice that selectively lack this isoform but express all others. In primary fibroblasts and myoblasts derived from these mice, we observe a substantial elongation of mitochondrial networks, whereas other mitochondrial properties remain largely unaffected. Normal morphology of mitochondria could be restored by isoform-specific overexpression of P1b in P1b-deficient as well as plectin-null cells. We propose a model where P1b both forms a mitochondrial signaling platform and affects organelle shape and network formation by tethering mitochondria to IFs.
© 2008 Winter et al. This article is distributed under the terms of an Attribution–Noncommercial–Share Alike–No Mirror Sites license for the first six months after the publication date (see http://www.jcb.org/misc/terms.shtml). After six months it is available under a Creative Commons License (Attribution–Noncommercial–Share Alike 3.0 Unported license, as described at http://creativecommons.org/licenses/by-nc-sa/3.0/).
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Introduction |
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 TopAbstract Introduction Results and DiscussionMaterials and MethodsReferences |
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The highly versatile IF-based cytolinker protein plectin (Wiche, 1998) would be an interesting candidate for mediating the interactions between IFs and mitochondria. The versatility of plectin is largely caused by complex splicing events in the N-terminal region of its gene that give rise to 11 alternatively spliced isoforms containing different first exons (1–1j; Elliott et al., 1997; Fuchs et al., 1999). The expression patterns of these isoforms are cell type–dependent, and some of the expressed variants have been shown to differ in their subcellular localization (Rezniczek et al., 2003). By forced expression in fibroblasts, isoform plectin 1b (P1b) was found to be specifically targeted to mitochondria (Rezniczek et al., 2003). Here, we analyzed the mode of P1b–mitochondrion interaction and show that this interaction affects the shape and network formation of mitochondria.
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Results and Discussion |
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TopAbstractIntroductionResults and DiscussionMaterials and MethodsReferences |
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P1b links IFs to mitochondria
To assess whether mitochondria-anchored P1b serves as a docking site for IFs, primary fibroblasts were transiently transfected with EGFP-tagged full-length P1b and analyzed using immunofluorescence microscopy. EGFP-tagged P1b was found to colocalize with mitochondria and to accumulate in discrete regions of vimentin (vim)-positive filaments (Fig. 3 A, a–e).
In cells with high level expression of P1b, a collapse of mitochondrial as well as of vim networks was observed (Fig. 3 A, f–j). Forced expression of P1, an isoform not associating with mitochondria, led to a collapse of IFs but not of mitochondria, which supports the notion that the latter phenotype was isoform 1b–specific (Fig. 3 B).
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Generation of P1b-deficient mice enables isoform-specific assessment of mitochondrion–IF linkage
To prove that the interaction of mitochondria with IF networks was P1b-specific, we generated a mouse line that selectively lacks isoform 1b but expresses all others (Fig. S2, A–D, available at http://www.jcb.org/cgi/content/full/jcb.200710151/DC1). P1b-deficient (P1b–/–) mice were viable and fertile, and revealed no obvious phenotype when compared with their wt littermates (not depicted; for phenotypic analyses of P1b–/– fibroblasts, see Fig. S2, E–H). When fibroblasts isolated from these mutant mice were subjected to subcellular fractionation (Fig. 3 F), ATPS, actin, and vim were maintained in cell lysates at levels that were comparable to those of wt cells, which is reminiscent of the situation of P0 fibroblasts (Fig. 3 C). Contrary to P0 fibroblasts, the cytosolic fractions of P1b–/– cells contained no soluble vim. In the mitochondrial fraction of P1b–/– cells, the amount of vim was found decreased to 66% of the corresponding wt level (Fig. 3 G), validating that the interaction of mitochondria with the IF network was mediated by P1b. As the reduction was more prominent in P0 compared with P1b–/– mitochondrial fractions (39 vs. 66%), the additional lack of isoforms other than P1b in P0 cells apparently contributed to this reduction. To our knowledge, P1b is the first protein shown to act as a direct linker between IFs and the mitochondrial network.
P1b deficiency leads to elongation of mitochondria
Interactions between IFs and mitochondria have been suggested to contribute to organelle morphology and cytoplasmic distribution (Anesti and Scorrano, 2006). Thus, we monitored the shape of mitochondria in P1b–/–, P0, and wt fibroblasts using cyt c–specific immunostaining. As exemplified in Fig. 4 A, mitochondrial networks were classified as fragmented, intermediate, or tubular (for detailed classification criteria, see Materials and methods).
Interestingly, although in wt fibroblasts, 63, 30, and only 7% of the mitochondria exhibited intermediate, fragmented, and tubular morphology, respectively, in P1b–/– fibroblasts, the fragmented type was reduced to 9% and the tubular type increased to 37% (Fig. 4 B). Thus, in P1b–/– cells, there was a dramatic shift from the small and fragmented mitochondrial network type to the elongated type. In P0 fibroblasts, we found very similar alterations in mitochondrial morphology, with 13 and 36% of cells exhibiting fragmented and tubular mitochondrial networks, respectively (Fig. 4 B). This suggested that the observed alterations in mitochondrial morphology were entirely due to the lack of P1b, with no other isoform of plectin being involved. A similar phenotype was revealed in primary P1b–/– myoblasts (Fig. 4 C).
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P1b, a mitochondrial platform for signaling complexes?
It was conceivable that mitochondria become anchored to IFs via P1b primarily in those subcellular regions where they are needed most for metabolic or homeostatic reasons. To investigate P1b-dependent mitochondrial parameters, the membrane potential and mass of mitochondria in P1b–/–, wt, and P0 primary fibroblasts were comparatively assessed using MitoTracker and 10-N-nonyl-acridine orange (NAO) staining, respectively. No significant differences between the cell types were revealed, however (Fig. 5, A and B).
The same was true when the apoptotic predisposition of cells were analyzed after incubation with staurosporine (Fig. 5, C and D).
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To assess whether changes in mitochondrial fusion rates were a cause for differences in mitochondrial length, wt, P1b–/–, and P0 fibroblasts were transfected with a mitochondrial matrix–targeted photoactivatable GFP (mito-PAGFP; Karbowski et al., 2004). Selected regions of interest (ROIs) were activated using a short laser beam, and redistribution of the photoactivated protein out of the activated ROIs was monitored (Fig. 5 G). When changes of fluorescence intensities within activated and nonactivated ROIs were measured over a time period of 60 min, P1b–/– and P0 fibroblasts showed unaltered mitochondrial fusion dynamics compared with wt cells (Fig. 5, H and I). Furthermore, when fibroblasts expressing GFP-tagged full-length P1b were immunolabeled using antibodies to the mitochondrial fission site marker Drp-1, P1b showed partial colocalization with Drp-1-marked sites but did not appear to accumulate there (Fig. 5 J).
Increasing evidence indicates that plectin serves the cell not merely as a structural element but also as a scaffolding platform of proteins involved in signaling. Among others, plectin was shown to bind and sequester the receptor for activated C kinase 1 (RACK1) to the cytoskeleton, thereby influencing PKC signaling pathways (Osmanagic-Myers and Wiche, 2004). Given that the various plectin isoforms are targeted to different cellular locations, it is quite conceivable that P1b, as a mitochondrial outer membrane protein, could act as a scaffolding platform for signaling molecules proximal to mitochondria. To test this hypothesis, we prepared cellular subfractions from P1b–/– and wt fibroblasts that had been exposed (or not) to the PKC activator PMA. A quantitative analysis of autophosphorylated (activated) PKC (pan), PKC
/βII, and PKC
, as well as of RACK1 and AMP-activated protein kinase (AMPK) β1/2, levels in total lysate fractions revealed no differences between the two cell types (Fig. S3, A and B, available at http://www.jcb.org/cgi/content/full/jcb.200710151/DC1). Interestingly, however, in the mitochondrial fraction from PMA-treated P1b–/– cells, activated PKC was decreased to nearly 70% of wt levels (Fig. S3, C and D), whereas all other proteins tested remained unaffected. Thus, P1b seemed to be at least partially involved in recruiting activated PKC to mitochondria.
Conclusions
With P1b, a ubiquitously expressed isoform of plectin, we have identified the first cytolinker protein capable of physically interlinking mitochondria with the IF network system of cells. By generating a mouse line selectively lacking this isoform, combined with the phenotypic analysis of primary fibroblasts derived from these animals, we were able to establish a direct link between P1b expression and mitochondrial shape. Mitochondrial morphology might be regulated by anchoring mitochondrial membranes or membrane-associated molecules to the IF cytoskeleton. IF-based P1b could either provide a scaffolding platform for signaling proteins – which establish and/or maintain mitochondrial morphology on the surface of the organelle, such as proteins involved in fusion/fission events – or the interlinkage between mitochondria and IFs mediated by P1b could play a mechanical role in shaping the organelle. Future studies will be aimed at elucidating the precise molecular mechanism underlying this phenomenon and its applicability to other cell types expressing different IF networks systems. It will also be of interest to investigate whether other cytolinker proteins play a similar role and whether P1b-mediated cross talk between mitochondria and the cytoskeleton is affected in plectin-related epidermolysis bullosa simplex and other human diseases involving mitochondrial dysfunctions.
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Materials and Methods |
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TopAbstractIntroductionResults and DiscussionMaterials and MethodsReferences |
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For generating cell lines stably expressing fusion proteins of EGFP and N-terminal fragments of P1b, P1, or EGFP alone, we used immortalized P0 fibroblasts and the Phoenix retroviral expression system as described previously (Gregor et al., 2006).
Expression plasmids encoding full-length P1b and P1 have been described previously (Rezniczek et al., 2003). For generating plasmids harboring only the exon 1b sequence, the corresponding cDNA (Rezniczek et al., 2003) was cloned into expression vectors pEGFP-N1 and pEGFP-C1 (Clontech Laboratories, Inc.). For transfections, FuGENE 6 transfection reagent (Roche) was used.
Cellular and mitochondrial subfractionation
Cells were scraped off in 250 mM sucrose, 10 mM MOPS-KOH, pH 7.2, and 1 mM EDTA (SME); homogenized using a Dounce tissue grinder (Wheaton), and centrifuged at 700 g for 10 min. The supernatant was collected and the pellet was resuspended in SME and recentrifuged (nuclear pellet). Pooled supernatants were centrifuged at 15,000 g for 15 min to obtain a cytosolic fraction and a mitochondrial pellet, which was dissolved in SME.
Mitochondria were subjected to extraction in 100 mM Na2CO3, pH 11.5, for 30 min on ice. Membranes were isolated by centrifugation at 100,000 g for 30 min at 4°C, and proteins in the supernatant were precipitated using trichloroacetic acid. Alternatively, mitochondria were solubilized with 1% Triton X-100 or left untreated and then incubated with increasing concentrations of proteinase K (Roche) for 30 min on ice.
Immunoblotting
For immunoblotting (Rezniczek et al., 2004), antiserum No. 9 recognizing all plectin isoforms (Andrä et al., 2003) and antibodies to P1b, P1 (Abrahamsberg et al., 2005), ATPS (Invitrogen), cyt c (BD Biosciences), porin (Invitrogen), actin (Sigma-Aldrich), vim (from P. Traub, University of Bonn, Bonn, Germany), phospho-PKC (kit 9921), AMPKβ1/2 (both from Cell Signaling Technology Inc.), and RACK1 (BD Biosciences) were used in combination with HRP-conjugated secondary antibodies (Jackson ImmunoResearch Laboratories).
Immunofluorescence and time-lapse video microscopy
Cells were fixed with 4% PFA, permeabilized with 0.1% Triton X-100, and immunostained using antibodies to GFP (Invitrogen), cyt c, Drp-1 (both from BD Biosciences), and vim (P. Traub) in combination with donkey anti–rabbit IgG Alexa Fluor 488 (Invitrogen), donkey anti–mouse IgG Rhodamine red, donkey anti–mouse IgG Cy5, and donkey anti–goat IgG Texas red (all from Jackson ImmunoResearch Laboratories). Microscopy was performed at room temperature using a confocal microscope (LSM 510; Carl Zeiss, Inc.) equipped with a Plan-Apochromat 63x 1.4 NA objective lens (Carl Zeiss Inc.). Images were recorded using the LSM510 module and the LSM software (Carl Zeiss Inc.) and processed using the Photoshop 7.0 (Adobe) software package.
Mitochondrial morphologies were classified as fragmented (individual round- or rod-shaped organelles, >80% displaying an axial length of <5 µm), intermediate (majority 
5 µm), or tubular (often interconnected in branched networks, >80% displaying a length of >5 µm). Because of their smaller size, myoblast mitochondria were classified as fragmented (round, <2 µm) or elongated (tubular, >2 µm).
Cells expressing mito-PAGFP (from R.J. Youle, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, MD) were kept in a closed POCmini cultivation system (Carl Zeiss, Inc.). Photoactivation of mito-PAGFP was performed as described previously (Karbowski et al., 2004), using a confocal microscope (LSM Live DuoScan) and a Plan-Apochromat 63x 1.4 NA objective lens (Carl Zeiss, Inc.).
Fibroblasts were transfected with cDNA encoding ATPS subunit 9 presequence (provided by N. Pfanner, Institute of Biochemistry and Molecular Biology, University of Freiburg, Freiburg, Germany) fused to EGFP (mito-GFP), and live-cell imaging was performed using an inverted microscope (Axiovert S100TV; Carl Zeiss, Inc.) as described previously (Osmanagic-Myers et al., 2006). Frames were collected with a Plan-Apochromat 100x 1.4 NA objective lens (Carl Zeiss, Inc.) and individual mitochondria were tracked using Metamorph 6.3 software (MDS Analytical Technologies).
Flow cytometry
Cells were resuspended in medium containing 1 µM NAO or 0.1 µM MitoTracker red CMXRos, incubated for 15 min at 37°C in the dark, and analyzed using a cytometer (LSR1; BD Biosciences).
Online supplemental material
Fig. S1 shows the subcellular localization of isoform 1b. Fig. S2 depicts the targeted disruption of P1b for generating knockout mice, Southern blot analysis, and PCR to identify mutant ES cell clones and mouse lines, as well as an RNase protection assay and the analyses of adhesion, migration, and proliferation properties of P1b–/– fibroblasts. Details about the generation of P1b–/– mice are provided in the legend. Fig. S3 presents a subcellular fractionation after PMA treatment. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200710151/DC1.
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Acknowledgments |
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This work was supported by grants F 006-11 and P17862-B09 from the Austrian Science Research Fund.
Submitted: 22 October 2007
Accepted: 13 May 2008
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