The telomeric protein AKTIP interacts with A- and B-type lamins and is involved in regulation of cellular senescence

AKTIP is a shelterin-interacting protein required for replication of telomeric DNA. Here, we show that AKTIP biochemically interacts with A- and B-type lamins and affects lamin A, but not lamin C or B, expression. In interphase cells, AKTIP localizes at the nuclear rim and in discrete regions of the nucleoplasm just like lamins. Double immunostaining revealed that AKTIP partially co-localizes with lamin B1 and lamin A/C in interphase cells, and that proper AKTIP localization requires functional lamin A. In mitotic cells, AKTIP is enriched at the spindle poles and at the midbody of late telophase cells similar to lamin B1. AKTIP-depleted cells show senescence-associated markers and recapitulate several aspects of the progeroid phenotype. Collectively, our results indicate that AKTIP is a new player in lamin-related processes, including those that govern nuclear architecture, telomere homeostasis and cellular senescence.


Background
The nuclear lamina is a structure located between the nuclear membrane and the chromatin; it plays a scaffolding role within the nucleus and has been implicated in diverse processes including the control of nuclear architecture, DNA replication and repair, transcriptional regulation, and maintenance of telomere homeostasis [1][2][3][4][5][6]. A-and B-type lamins are the main components of the nuclear lamina; B-type lamins are expressed in most cell types, whereas lamin A/C expression is restricted to differentiated cells [7,8]. In interphase cells, lamins are mainly detected at the nuclear periphery, but are also found in discrete intranuclear aggregates associated with DNA replication foci or transcriptionally active areas [7]. At the onset of mitosis the lamina disassembles; B-type lamins concentrate in the spindle matrix, whereas A-type lamins remain diffuse in the cytoplasm. At the end of mitosis (telophase), the lamins reassemble to form the nuclear lamina [7,9,10].
In humans, there are three lamin genes: LMNA, LMNB1 and LMNB2. Lamins initially synthesized as precursors, known as prelamins, which are processed into mature lamins through a sequential series of post-translational modifications [1]. Mutations in the human lamin genes result in a wide range of diseases, including the Hutchinson-Gilford progeria syndrome (HGPS) [11] and mandibuloacral dysplasia type A (MADA) [12]. HGPS patients suffer from premature ageing; their cells exhibit an accumulation of a truncated form of lamin A, which causes early senescence, dismorphic nuclei, abnormal intranuclear chromatin distribution and telomere attrition [3,13]. MADA patients share with HGPS patients a premature ageing phenotype. MADA cells display an accumulation of prelamin A, an altered chromatin organization and dislocation of nuclear envelope-associated proteins [12,14].
Lamin-related functions and pathologies are largely dependent upon lamin interplay with multiple interacting partners. For example, the fact that the Ig-fold motif at the lamin C-terminus binds proliferating cell nuclear antigen (PCNA) suggests a mechanistic path for lamin implication in DNA replication [15]. Similarly, the lamin A/C interaction with 53BP1 to promote the DNA damage response (DDR) accounts for the DNA repair defects observed in lamin mutants [16]. The chromatin defects observed in HGPS patient cells probably reflect the interaction of lamins with the NURD chromatin remodelling complex [17]. Loss of another lamin-interacting protein, the Suv39h1 methyltransferase, has been shown to improve DNA repair and extend the lifespan of a progeroid mouse model with impaired prelamin A maturation, suggesting that HGPS causes Suv39h1-mediated epigenetic alterations in the chromatin [18]. Finally, lamin A/C interaction with the shelterin component TRF2 and the association of the laminaassociated polypeptide-a (LAP2a) with telomeres provide evidence for a role of lamin A and progerin in telomere homeostasis [6]. Although the biological significance of many of the lamins' interactions is not precisely defined, there is no doubt that further studies on these interactions and the discovery of new lamin-interacting partners will be instrumental to understand the mechanistic bases of the role of lamin in physiological and pathological processes [19].
Here, we provide a functional characterization of an additional lamin-interacting protein, AKTIP. AKTIP belongs to the ubiquitin E2 variant (UEV) enzyme subfamily, which comprises proteins that share sequence similarity with E2s but lack the conserved cysteine residue that is critical for the canonical E2 catalytic activity [20]. UEV functions are still ill defined; it has been suggested that they can act in combination with E2 conjugating enzymes in ubiquitylation processes [21,22]. We have recently shown that AKTIP and its Drosophila orthologue Pendolino (Peo) play roles at telomeres [23,24]. AKTIP directly binds the shelterin proteins TRF1 and TRF2 and interacts with the PCNA and RPA70 DNA replication factors, and its depletion results in general impairment of DNA synthesis and defective telomere replication. Collectively, our results indicate that AKTIP works in concert with TRF1 to ensure proper telomere replication.
The finding that both AKTIP and lamins interact with telomeres and with PCNA [3,6,23,25], along with the enrichment of AKTIP at the nuclear rim [23], prompted us to investigate whether AKTIP interacts with lamins. Here, we show that AKTIP co-purifies with A-and B-type lamins and partially colocalizes with lamins in interphase nuclei. In addition, we show that AKTIP depletion lowers lamin A expression and induces senescence hallmarks in human primary fibroblasts (HPFs).

Cells, vectors and virus
Human foreskin primary fibroblasts from healthy donors (provided by A. Orecchia, IDI, Rome, Italy) were used at early passages (from p5 to p10), unless otherwise specified. HeLa (ATCC CCL-2), 293T (ATCC CRL-11268), BJ-hELT cells and HPFs were cultured in DMEM (Invitrogen) supplemented with 10% FBS (Invitrogen). pCMV6-entry-AKTIP-MYC-FLAG (Origene), pTR-UF5 (provided by N. Muzyczka, University of Florida), or HDAC1-FLAG (Addgene, #13820) vectors were transfected in 293T cells according to Piersanti et al. [26]; cell extracts were analysed 72 h post-transfection, unless otherwise indicated. Second-generation recombinant lentiviruses (LVs) were produced and titrated for p24 antigen content and used for infections as previously described [26]. The LV-shAKTIP, LV-shTRF2 and LV-scramble (control, ctr) vectors were described previously [23]; the transfer vector pCDHblast MCSNard OST-LMNAD50 [17] (Addgene #22662) was used to produce LV-progerin. The multiplicity of infection (moi) used for all experiments was 3pg p24/cell on HPFs and 5pg p24/cell on HeLa cells. Transductions were performed in complete medium supplemented with 8 mg ml 21 polybrene (Sigma). After viral addition, cells were centrifuged for 30 min at 1800 r.p.m. at RT, incubated for 3 h at 378C, and then transferred to fresh complete medium. Seventy-two hours post-infection, cells transduced with LVs obtained with pLKO.1-derived transfer vectors were subjected to selection in complete medium supplemented with 2 mg ml 21 puromycin (Sigma) and kept under these conditions for further analyses. Seventy-two hours post-transduction, cells transduced with LV-progerin were subjected to selection in complete medium supplemented with 10 mg ml 21 blasticidin (Sigma) and kept under these conditions for further analyses.
HeLa cells were synchronized at the G1/S boundary by a double-thymidine block. Cells were treated with 2 mM thymidine for 14 h, released in fresh medium for 10 h and treated again with 2 mM thymidine for 14 h. After double-thymidine treatment, cells were released in fresh medium and collected at the indicated time points.
MADA skin fibroblasts were obtained from a 12-year-old patient carrying the Arg527His LMNA homozygous mutation. Cell cultures were established and grown in DMEM-F12 (Gibco, Life Technologies) supplemented with 10% fetal bovine serum (Gibco, Life Technologies), 1% penicillin/streptomycin and 1% L-glutamine. The experiments were performed on cells at p12. HGPS fibroblasts were obtained from a patient carrying the G608G LMNA mutation [27] and were maintained in culture in DMEM supplemented with 10% fetal calf serum (Gibco) and 1% penicillin/streptomycin. Skin biopsies were obtained from patients and donors according to local and EU ethical rules following informed consent.

Mass spectrometry
Seventy-two hours after transfection with the AKTIP-FLAG, pTR-UF5 or HDAC1-FLAG (Addgene, #13820) vectors in 293T cells, extracts were obtained by lysing the cells with 20 mM Hepes pH 7.5, 150 mM NaCl, 5 mM MgCl 2 , 0.5 mM EGTA, 0.25% NP-40, 1 mM DTT, 0.5 mM PMSF, 0.5 mM Na 3 VO 4 in the presence of a protease inhibitor cocktail (Roche). Immunoprecipitation was performed by incubation of 2 mg of protein extract with 5 mg of anti-FLAG M2 antibody (Sigma) or 5 mg of mouse IgG (Sigma), both conjugated to Gsepharose four fast flow beads (GE Healthcare). Precipitated complexes were eluted using acid glycine ( pH 2.5) and 2% Triton X-100 (Sigma) and then resuspended in SDS/PAGE loading buffer (Invitrogen). For mass spectrometry (MS), samples were separated onto pre-cast 4-12% gradient acrylamide gels (NuPage, Invitrogen). Entire gel lanes were cut into 10 similar slices, subjected to in-gel tryptic digestion, and used for LC-MS/MS analysis. Raw spectra were analysed by BIOWORKS BROWSER 3.3.1. When proteins were present both in anti-FLAG and in anti-IgG antibody samples, they were selected by applying the emPAI ratio [28] equal or higher than 1.5. The UNIPROT IDs of putative AKTIP interactors were uploaded in the Protein Knowledgebase (UniProtKB) and categorized based on Gene Ontology (GO) annotation terms by using Cytoscape v 2.8.3 (see the electronic supplementary material for full MS methods).

GST pulldown
AKTIP-GST and AKTIP-GST truncations were previously described [23]. Protein purification and GST pulldown from 293T cell extracts were carried out as previously described [23]. Immunoblotting was performed as described above.
SA-b-gal staining was carried out according to Dimri et al. [29]. Cells at different days post-infection were plated on coverslips for 24 h and then stained using the Senescent cell Histochemical Staining Kit (Sigma).

Flow cytometry
5-bromo-deoxyuridine (BrdU) at a final concentration of 45 mM was added to the culture medium 30 min before harvesting the cells. Cells were fixed in 70% ethanol, washed twice in PBS þ 0.5% Tween 20, and incubated in 3 M HCl for 45 min. Cells were then exposed to anti-BrdU monoclonal antibody (Dako), to the secondary Alexa-Fluor488-conjugated antibody (Jackson) and counterstained with propidium iodide (PI, Sigma) in the presence of 1 mg ml 21 DNAse-free RNAse (Sigma) for 30 min at room temperature. Acquisition was carried out using a Beckman-Coulter Epics XL flow-cytometer and recorded data were analysed with the WINMDI software (developed by Joe Trotter; free download at http:// en.bio-soft.net/other/WinMDI.html).

mRNA quantification
One-week post-transduction, cells were lysed by addition of TRIzol reagent (Invitrogen) and RNA extracted according to the manufacturer's instructions. After DNase treatment (Invitrogen), RNA was reverse transcribed into cDNA using an oligo d(T) primer and the Omniscript RT kit (Qiagen). To quantify target gene expression, specific primers (electronic supplementary material, table S1) were selected using PRIMER EXPRESS software (Applied Biosystems). Reactions were carried out as previously described [30].

AKTIP binds nuclear envelope and nuclear matrix proteins
As a first step towards the identification of AKTIP-interacting partners, we analysed by MS the proteins that co-purify with rsob.royalsocietypublishing.org Open Biol. 6: 160103 AKTIP. 293T cells were transfected with a vector encoding an AKTIP-FLAG fusion protein [23], or a control HDAC1-FLAG expression plasmid, or an empty pTR-UF5 vector. Previous work has shown that AKTIP-FLAG accumulates at the nuclear rim just as the untagged AKTIP protein [23] (see also electronic supplementary material, figure S1A). The AKTIP-FLAG fusion protein also displayed the expected molecular weight and was detected by both anti-FLAG and anti-AKTIP antibodies (electronic supplementary material, figure S1b). Seventy-two hours after transfection, we precipitated AKTIP-FLAG from whole-cell extracts using an anti-FLAG antibody; MS was carried out on immunoprecipitates following polyacrylamide gel electrophoresis (electronic supplementary material, figure S1B). To detect AKTIP bona fide interactors and eliminate false positives, we filtered raw data from three independent experiments using the BIOWORKS BROWSER 3.3.1 software (see Material and methods). These analyses led to the identification of 45 AKTIP-interacting proteins (figure 1a and electronic supplementary material, figure S2). Using UniProtKB, we found that these proteins localize in the nucleus (31%), in the nucleus and the cytoplasm (13%), in the cytoplasm (29%) or in the mitochondria (25%) (figure 1b). Cytoscape enrichment analysis further revealed that the nucleus and especially the nuclear lamina are GO categories significantly overrepresented among AKTIPinteracting partners (figure 1c). AKTIP-interacting proteins included lamins B1, B2 and A/C (figure 1a), importin 7, a nuclear-pore-associated b-family import receptor [31] and matrin 3, an internal nuclear matrix component that interacts with lamin A [32] (electronic supplementary material, figure S2).
To validate these MS data, we performed a pulldown assay using bacterially purified AKTIP-GST to capture proteins from 293T cell extracts. Consistent with the MS data, precipitates included lamins B1 and A/C, matrin 3 and importin 7. In addition, we found that an anti-FLAG antibody precipitates lamin B1 from AKTIP-FLAG-expressing 293T cells (figure 2a-c).
We next determined the AKTIP region(s) that interact with the nuclear envelope proteins. We used three AKTIP truncations fused with GST including the N-terminal disordered region (aa 1-70), the central region comprising the UEV portion (aa 70-189) and the C-terminus consisting of 2 a-helices and a distal disordered portion (aa 190-292) (figure 2d) [23]. GST pulldown showed that only the central region of AKTIP interacts with A-and B-type lamins, importin 7 and matrin 3 (figure 2e,f).

AKTIP partially co-localizes with lamins
Previous work has shown that A-and B-type lamins form two prominent nuclear meshworks with points of co-localization during interphase [33]. During mitosis, after dissolution of the nuclear lamina, A-type lamins exhibit a diffuse localization. By contrast, B-type lamins associate with the spindle matrix, where they are thought to provide a scaffold to promote microtubule assembly and lamina reorganization at the nuclear periphery at the end of mitosis [9,10]. Given the interaction between AKTIP and lamins, we investigated AKTIP localization. We immunostained with an anti-AKTIP antibody HeLa cells harvested at different times after release from synchronization at the G1-S boundary by a double-thymidine block. We found that at all time points tested AKTIP was enriched at the nuclear rim, suggesting that this localization pattern is dominant during the cell cycle (figure 3a).
We next investigated whether AKTIP co-localizes with Aand B-type lamins in interphase nuclei. The analysis of HPFs stained for both AKTIP and lamin B1 showed that the two proteins have multiple co-localization points, both at the nuclear rim and in the nucleoplasm (figure 3b). Double staining of HPFs for AKTIP and either lamin A or lamin A/C showed a partial co-localization of AKTIP with A-type   rsob.royalsocietypublishing.org Open Biol. 6: 160103 lamins at the nuclear periphery (figure 3b). We also observed partial colocalization of AKTIP intranuclear signals with lamin A/C signals (figure 3b).
To determine AKTIP localization during mitosis, we used a fixative containing 0.25% Triton X-100. This fixative results in a high level of protein extraction allowing a clear visualization of AKTIP, but it does not fully preserve spindle microtubules. We analysed AKTIP localization in BJ-hELT (BJ fibroblasts expressing hTERT and SV40 Large T) and HeLa cells and HPFs (figure 3ce and electronic supplementary material, figure S4). In all cell types, antibody staining detected specific AKTIP-enriched mitotic structures, which were absent in AKTIP-depleted cells (shAKTIP) (figure 3d; see the electronic supplementary material, figure S3 for analysis of RNAi efficiency). The AKTIP signal was associated with structures at the cell poles that overlapped the spindle microtubules and the centrosomes. In addition, AKTIP concentrated to the midbody, a transient structure that connects the two daughter cells at the end of cytokinesis. The midbody contains microtubules that overlap in a narrow region at the centre of the structure. This region often appears dark after tubulin immunostaining (dark zone), because it is tightly associated with proteins that block antibody binding to tubulin [34]. Remarkably, AKTIP precisely encircles the dark zone of the midbody (figure 3d), suggesting a possible role of AKTIP in cytokinesis.
To ask whether AKTIP co-localizes with lamins during mitosis, we co-immunostained HPFs for AKTIP and either lamin A or B. As expected from previous work [9], lamin A did not co-localize with the AKTIP-enriched structures and was instead diffuse (figure 3e). By contrast, lamin B1 accumulated at the centrosomes and partially co-localized with

Functional relationships between lamins and AKTIP
Given the connection between AKTIP and lamins, we investigated the functional relationships between these proteins. We first asked whether mutations in lamin genes affect AKTIP localization. We analysed AKTIP localization in HPFs from patients affected by HGPS or MAD type A (MADA). The HGPS mutation exposes a cryptic splice site in the LMNA gene, leading to a lamin A form deleted of 50 aa and permanently farnesylated [35,36]. MADA cells, which carry the R527H LMNA mutation that replaces an arginine with a histidine at position 527, are characterized by accumulation of prelamin A and progeroid traits [37]. In addition, we examined AKTIP localization in HPFs transduced with a progerin-coding lentivector (LV-progerin; electronic supplementary material, figure S5). Immunostaining for AKTIP showed that in untreated control cells AKTIP is enriched in both the cytoplasm and the nucleus ( particularly at the nuclear rim), while in detergent-extracted control cells AKTIP localization was  rsob.royalsocietypublishing.org Open Biol. 6: 160103 restricted to the nucleus ( figure 4a,b). In unextracted LVprogerin cells expressing both endogenous lamin A and progerin, and more effectively in unextracted HGPS cells, which are heterozygous for the LMNA mutation, the AKTIP signal in the cytoplasm was reduced and the nuclear rim staining was weaker and more discontinuous than in controls (figure 4a); the defective AKTIP localization at the nuclear rim of these cells was more evident in preparations extracted with Triton X-100 (figure 4b). In MADA cells, homozygous for the LMNA mutation, AKTIP was almost undetectable (figure 4a,b). We next investigated whether loss of AKTIP affects lamin expression. We reduced the AKTIP level by RNAi in early passage HPFs and HeLa cells (electronic supplementary material, figure S3). Western blotting performed on extracts from both cell types collected at 7 days post-infection showed that AKTIP depletion results in a substantial decrease in lamin A compared with control cells, without affecting lamin C and lamin B1 levels (figure 5a-d). In addition, Q-PCR-mediated mRNA quantification in HeLa cells at 7 days after shAKTIP infection showed a significant decrease in the lamin A mRNA level compared to control (figure 5e). However, AKTIP deficiency did not affect the level of lamin C mRNA, which is the main alternative splicing product of the LMNA gene. Consistent with these results, lamin A immunostaining in AKTIP-depleted HeLa cells showed a substantial reduction of the lamin A signal, which, however, maintained its normal association with the nuclear rim (figure 5f).
We have previously shown that AKTIP is required for telomere replication and that its depletion generates telomereassociated DNA repair foci [23]. Depletion of the TRF2 shelterin component, which physically interacts with lamin A/C [6], also causes telomere dysfunction and triggers the DDR [38]. We thus wondered whether lamin A reduction observed in AKTIP-depleted cells could be generated by dysfunctional telomeres. To test this possibility, we monitored lamin expression in shTRF2 HeLa cells. TRF2 depletion did not result in lamin A/C reduction, indicating that the effect of AKTIP depletion on lamin A is specific and not a general consequence of DDR triggered by dysfunctional telomeres (electronic supplementary material, figure S6).

AKTIP depletion results in cell senescence
Lamin mutations cause defects in nuclear structure, variations in heterochromatic marks and cell senescence [3]. These findings prompted us to inquire whether AKTIP depletion generates the same phenotypic traits elicited by LMNA mutations. Cell labelling with the empirical senescence marker SA-bgal [29] revealed that early passage HPFs (p6) at 11 and 13 days after shAKTIP infection (electronic supplementary material, figure S3a) exhibit a significant increase in senescent cells compared with controls ( figure 6a,b). We next analysed K9 trimethylation of histone H3 (trimethyl H3K9), an epigenetic marker of cell senescence that is reduced in prematurely ageing lamin-defective cells [39]. Early passage wild-type cells show a clustered intranuclear distribution of trimethyl H3K9, while senescent cells exhibit a more diffuse distribution of this trimethylated histone [14,37,39]. Early (p6) and mid-late (p12) passage AKTIP-depleted HPFs (electronic supplementary material, figure S3a) displayed higher frequencies of nuclei with diffuse trimethyl H3K9 distribution than passage-matched controls ( figure 6c,d). In addition, Western blotting showed that in AKTIP-depleted early passage (p6) HPFs, the trimethyl H3K9 level was reduced with respect  rsob.royalsocietypublishing.org Open Biol. 6: 160103 to controls and was comparable to that observed in naturally aged HPFs at p22 (figure 6e). Previous studies on naturally aged cells have shown that they accumulate unprocessed lamin A ( prelamin A) [40]. This accumulation exacerbates the disease traits in HGPS and MADA patients, and eventually leads to nuclear deformation [12,14]. To ask whether AKTIP depletion results in a similar phenotype, we treated HPFs at different passages ( p6 and p22) with shAKTIP (electronic supplementary material, figure S3a) and examined 7 days post-infection cells immunostained with the C20 antibody, which specifically reacts with prelamin A. shAKTIP HPFs at p22 displayed a higher frequency of prelamin A-positive cells than passage-matched control HPFs ( figure 7a,b). We also examined AKTIPdeficient HPFs for distorted nuclei, which have been described in lamin mutant cells [12,14,39]. We found that AKTIP-depleted HPFs at p22 exhibit a significantly higher frequency of distorted nuclei than control cells ( figure 7c,d).
Taken together, these data indicate that AKTIP depletion results in phenotypic traits that are characteristically associated with lamin A mutations.

Discussion
We have recently shown that AKTIP interacts with the PCNA and RPA70 components of the DNA replication machinery and with the shelterin subunits TRF1 and TRF2. Consistent with these results, we found that AKTIP is required for both general DNA replication and telomere replication [23]. Our MS experiments have shown that AKTIP also interacts with A-and B-type lamins, matrin 3, importin 7 and several mitochondrial proteins. The AKTIP interaction with lamins, matrin 3 and importin 7 was further validated by GST pulldown.
We focused on the relationships between AKTIP and lamins and found that these proteins exhibit similar localization patterns in interphase nuclei, with AKTIP enriched at the nuclear rim, showing partial co-localization with both the A-and B-lamin meshworks. We also found that AKTIP is enriched in structures that partially co-localize with the centrosomes and the spindle of mitotic cells. In addition, AKTIP forms a ring around the midbody during late cytokinesis. Previous studies in different cell types have shown that lamin B is also enriched at the centrosomes and spindle poles [10,41,42] as well as at the midbody [43]. It has been suggested the lamin network is part of the spindle matrix, a membranous network that favours spindle morphogenesis [10,42]. Thus, it appears that AKTIP and lamins are enriched in the same cellular compartments, a finding that suggests a functional interaction among these proteins.
Indeed, we found that AKTIP knockdown results in a specific reduction of lamin A at both the mRNA and the protein level. A specific downregulation of A-type lamins has been also found in other systems. For example, in   rsob.royalsocietypublishing.org Open Biol. 6: 160103 mouse brains both lamin A and progerin expression is downregulated by miR-9, a brain-specific microRNA; miR-9 targets prelamin A 3 0 -UTR but not the lamin C transcript [44]. Lamin A and prelamin A downregulation and autophagic degradation have been also detected in response to retinoic acid and rapamycin treatments, in the absence of concomitant lamin C variations [27,45]. Our current results do not allow us to envisage a precise model to explain how AKTIP-deficient cells specifically downregulate lamin A expression. It is possible that loss of AKTIP lowers the production of lamin A by affecting the splicing of LMNA RNA or by controlling both prelamin A degradation and LMNA gene expression [46]. It is also conceivable that the prelamin A mRNA is downregulated by a microRNA. However, this hypothetical microRNA cannot be miR-9, because it was not found in HeLa cells [44]. The most intriguing aspect of the AKTIP-mediated regulation of prelamin A mRNA is that AKTIP interacts physically with both lamin A/C and lamin B. This finding raises the enthralling possibility that AKTIP regulates prelamin A mRNA expression through an interaction with one or more lamin types. We also found a modest increase (from 3 to 9%) in the frequency of prelamin A-positive cells in late passage samples of AKTIP-depleted cells. This finding is in apparent contrast with the downregulation of lamin A observed in in early passage AKTIP-depleted cells. However, it should be considered that prelamin A accumulation reflects a slowdown in prelamin A processing, a phenomenon that characterizes the senescent phenotype associated with physiological and premature ageing [47]. It is thus possible that the accelerated senescence of AKTIP-depleted cells strongly affects prelamin A processing leading to an accumulation of this protein even in cells in which level of lamin A mRNA was initially reduced compared with controls.
We showed that AKTIP is mislocalized in LV-progerin and HGPS cells and in cells from MADA patients that accumulate prelamin A [12,14,39]. These findings raise the possibility of a role of AKTIP in progerin-induced pathogenesis. Another possible contributing factor to HGPS pathogenesis is the lamin A-interacting LAP2a protein [48,49]. It has been also shown that LAP2a transiently binds telomeres [50] and that progerin has the ability to reduce LAP2a association with telomeres [48]. Here, we have not addressed the relationships between AKTIP and LAP2a but we have shown that in HGPS cells the nuclear localization of AKTIP is strongly reduced compared with controls, suggesting a possible effect on proper telomere replication. These data, together with the cellular senescence observed in AKTIP-depleted cells, reinforce the idea of a functional interconnection between lamins and AKTIP and support the hypothesis of a possible involvement of AKTIP in progeroid syndromes.
Our MS analyses, in addition to lamins, identified matrin 3, importin 7 and several mitochondrial proteins as AKTIP partners. The functional relationships between AKTIP and these interacting partners deserve further investigation. In this respect, it should be noted that previous studies have shown that proteins involved in telomere maintenance such as the ATM kinase and the shelterin subunit TIN2 localize to mitochondria and regulate mitochondrial activity [14,51].
Altogether, our results identify AKTIP as a new lamin interactor, expanding the connection between telomeres and lamins and, more in general, between telomeres and nuclear envelope. In addition, the interplay between AKTIP and both lamin A and its aberrant forms responsible for HGPS and MADA suggests a possible involvement of AKTIP in the pathogenesis of these diseases.
Ethics. Skin biopsies were obtained from patients and donors according to local and EU ethical rules following informed consent.
Data accessibility. The datasets supporting this article have been uploaded as part of the electronic supplementary material.