Charcot–Marie–Tooth causing HSPB1 mutations increase Cdk5-mediated phosphorylation of neurofilaments

Mutations in the small heat shock protein HSPB1 (HSP27) are a cause of axonal Charcot–Marie–Tooth neuropathy (CMT2F) and distal hereditary motor neuropathy. To better understand the effect of mutations in HSPB1 on the neuronal cytoskeleton, we stably transduced neuronal cells with wild-type and mutant HSPB1 and investigated axonal transport of neurofilaments (NFs). We observed that mutant HSPB1 affected the binding of NFs to the anterograde motor protein kinesin, reducing anterograde transport of NFs. These deficits were associated with an increased phosphorylation of NFs and cyclin-dependent kinase Cdk5. As Cdk5 mediates NF phosphorylation, inhibition of Cdk5/p35 restored NF phosphorylation level, as well as NF binding to kinesin in mutant HSPB1 neuronal cells. Altogether, we demonstrate that HSPB1 mutations induce hyperphosphorylation of NFs through Cdk5 and reduce anterograde transport of NFs. Electronic supplementary material The online version of this article (doi:10.1007/s00401-013-1133-6) contains supplementary material, which is available to authorized users.


Introduction
Charcot-Marie-Tooth disease (CMT) is the most common inherited neurodegenerative disorder of the peripheral nervous system. CMT neuropathy is clinically and genetically heterogeneous, caused by mutations in a large number of genes with diverse functions. The genes associated with CMT disease may have a specific role in Schwann cells or in the peripheral neurons. Although some genes are expressed in every tissue and cell, the CMT-causing mutations selectively affect peripheral nerves [46].
Missense mutations in the small heat shock protein HSPB1 (HSP27) are causative of axonal CMT type 2F (CMT2F) and distal hereditary motor neuropathy (HMN) [26]. The HSPB1 protein is ubiquitously expressed and belongs to the family of highly conserved ATP-independent molecular chaperones [28,34]. We recently reported that some HSPB1 mutations show a higher chaperone activity than the wild-type protein, affect microtubule dynamics and impede axonal transport [5,7,22]. However, the pleiotropic nature of the HSPB1 protein suggests that some neuron-specific functions could contribute to peripheral neuropathy. Indeed, CMT-causing mutations in HSPB1 have been shown to cause aggregation of the neurofilament light protein, and therefore disruption of the neurofilament (NF) network [26,74].
Abstract Mutations in the small heat shock protein HSPB1 (HSP27) are a cause of axonal Charcot-Marie-Tooth neuropathy (CMT2F) and distal hereditary motor neuropathy. To better understand the effect of mutations in HSPB1 on the neuronal cytoskeleton, we stably transduced neuronal cells with wild-type and mutant HSPB1 and investigated axonal transport of neurofilaments (NFs). We observed that mutant HSPB1 affected the binding of NFs to the anterograde motor protein kinesin, reducing anterograde transport of NFs. These deficits were associated with an increased phosphorylation of NFs and cyclin-dependent kinase Cdk5. As Cdk5 mediates NF phosphorylation, inhibition of Cdk5/p35 restored NF phosphorylation level, as well as NF binding to kinesin in mutant HSPB1 neuronal Electronic supplementary material The online version of this article (doi:10.1007/s00401-013-1133-6) contains supplementary material, which is available to authorized users. Neurofilament light (NFL), together with neurofilament medium (NFM), neurofilament heavy (NFH) and α-internexin, are neuron-specific proteins that form the main cytoskeletal elements in mature neurons [73]. As their highest concentration is found along the axon, disruption of the NF network may underlie degeneration of peripheral nerves. Moreover, NFs in axons are extensively phosphorylated. Phosphorylation of their C-terminal domains modulates their structural dynamics and function [17,59] and is mainly regulated by the interplay of five proline-directed kinases: p42/44 mitogen-activated protein kinase (ERK1/2 MAPK), p38 MAPK, c-jun-N terminal kinase (JNK), glycogen synthetase kinase 3 (GSK3) and cyclin-dependent kinase 5 (Cdk5) [3,57,65]. Each kinase can phosphorylate distinct lysine-serine-proline (KSP) motifs in the C-terminal domains of NFM and NFH, suggesting their ability to differentially affect the functioning of NFs [2,16]. Here, we studied the effect of mutant HSPB1 on NF dynamics and phosphorylation.
The specificity of the antibodies against phosphorylated and non-phosphorylated NFs was verified using cell lysates treated with or without phosphatase inhibitor or arctic phosphatase. The SMI-31 antibody is directed against the phophorylated KSP repeats in the C-tail of NFH and to a lesser extent NFM, while the SMI-33 antibody is described to detect non-phosphorylated NFH and to a lesser extent NFM [49,53,60]. The arctic phosphatase treatment dephosphorylated NFH as indicated by a shift in electrophoretic mobility on the agarose gel [57]. As expected, the SMI-31 antibody did not probe NFH or NFM after treatment with arctic phosphatase, while the SMI-33 antibody still probed NFH and NFM after arctic phosphatase treatment (data not shown). The phosphorylation status of the NFs was therefore assessed with the SMI-31 antibody. The SMI-34 antibody was used to detect the phosphorylated S/TPXH/K/R repeat motif in the C-domains of NFH and NFM, specifically phosphorylated by Cdk5/p35 [9].
As inhibitors we used: SB203580 (p38 inhibitor, Enzo Life Technologies), SP600125 (JNK inhibitor, Enzo Life Technologies), U0126 (MEK1/2 inhibitor, Cell Signaling), TDZD-8 (GSK3β inhibitor, Sigma) and roscovitine (Cdk5 inhibitor, Cell Signaling). Specific kinase inhibitors were diluted to 10 μM directly in medium and cells were incubated for 16-24 h. Efficiency of all inhibitors was verified by WB by assessing the phosphorylation level of the kinase itself or a known downstream substrate unrelated to NFs (data not shown).

Neuronal differentiation of SH-SY5Y cells with retinoic acid
The protocol was adapted from Ammer and Schulz, 1994 [8,25]. Glass Bottom Culture Dishes (35 mm, thickness 1.5, 14 mm) (further referred to as 'imaging dishes') or 12-well plates were coated overnight with 0.1 mg/ml poly-l-ornithine (Sigma) at room temperature. Cells were seeded at a density of 10.000/cm 2 in medium with 1 % non-essential amino acids, 1 % glutamine, 2 % fetal calf serum and 10 μM retinoic acid (Sigma). Differentiation was performed in Neurobasal A medium (Life Technologies) containing 2 % B27 supplement (Life Technologies), 1 % glutamine and 20 μM retinoic acid. The medium was refreshed every other day. After 7 days of differentiation, cells were imaged, collected for WB or fixed in 4 % paraformaldehyde for immunocytochemistry.

Western blotting
Unless otherwise indicated, cells were lysed in E1A lysis buffer [20 mM HEPES (pH 7.9) with 1 % (vol/vol) NP-40, 250 mM NaCl, 1 mM EDTA, 20 mM β-glycerophosphate, 10 mM NaF, 1 mM Na 3 OVO 4 , 2 mM DTT] and Complete protease inhibitor mixture (Roche Applied Technologies, Vilvoorde, Belgium). Cells were sonicated for 10-30 s on ice using the U50-control sonicator (IkaLabortechnik, Staufen, Germany) and subsequently incubated for 30 min on ice. Protein concentrations were measured using the Bradford protein assay (Bio-Rad, Nazareth, Belgium) and equal amounts of protein extract were prepared for SDS-PAGE by addition of SDS-PAGE sample buffer and heating the samples at 95 °C for 10 min. Proteins were separated on NuPAGE gels (Life Technologies) and transferred to a nitrocellulose membrane (Hybond™-P, Amersham/ Pharmacia) using the wet blotting method. After blocking in 5 % milk powder in PBS or TBS, supplemented with 0.1 % (vol/vol) Tween-20, blots were incubated with a primary antibody overnight at 4 °C and 1 h with a secondary horseradish peroxidase-conjugated antibody. Blots were developed using the enhanced chemiluminescence Plus™ detection system (GE healthcare, Diegem, Belgium). In all experiments, except Triton-X 100 experiments, actin was used as loading control.
Band intensity was determined by quantifying the 'mean pixel gray' values using ImageJ software (http://rsbweb.nih. gov/ij/) after Gaussian blur and background subtraction on the inverted image. The 'mean pixel gray' values were measured in a rectangular region of interest. Band intensities were normalized to β-actin levels by dividing the 'mean pixel gray' values of the band of interest by the actin 'mean pixel gray' values. Data from multiple experiments are presented as relative quantities by normalizing to the non-transduced control.

Immunocytochemistry and immunofluorescence microscopy
Immunostaining was performed according to standard protocol. Briefly, cells were fixed in 4 % paraformaldehyde for 30 min and permeabilized with 0.1 % (vol/vol) Triton-X 100 in phosphate-buffered saline (PBS). Blocking was done with 5 % goat serum (Dako, Heverlee, Belgium) for 1 h, primary antibodies were incubated for 1 h and secondary antibodies for 30 min at room temperature. Nucleus staining was done with Hoechst33342 (Invitrogen), after which cells were mounted with Dako fluorescent mounting medium (Dako) and examined with an Axiovert200 fluorescence microscope, equipped with a CCD Axiocam camera and Axiovision software (Carl Zeiss, Zaventem, Belgium). Images were acquired with a 63× Plan-Apochromat objective (1.4NA) and standard fluorescence filters.
Laser scanning confocal microscopy of immunostained samples was performed on a Zeiss LSM700 microscope equipped with a 63× Plan-Apochromat objective (1.4 NA). Image stacks (sampled at Nyquist resolution in XY and Z) were deconvolved using the ImageJ Iterative Deconvolve 3D plugin with theoretically calculated point spread function, created with the ImageJ Diffraction PSF CD plugin.
Quantification of the number of V5-positive, or NFaggregate positive cells was performed manually by counting a minimum of 100 cells per experiment for each cell line. Cells were scored visually. For quantification of the mean fluorescence intensity, image fields were selected at random in the transmitted light mode, without exposure to the fluorescence excitation light. All images were captured with the same exposure time. In the soma or in neurites of respectively undifferentiated or differentiated SHSY-5Y cells, fluorescence intensity was quantified by measuring the 'mean pixel gray' value in a region with the same dimensions using ImageJ. All quantifications were performed blind for the treatment conditions and in triplicate.
Axonal transport studies with PAGFP-NFM Cells were seeded in an imaging dish and differentiated as explained above. The medium was changed right before imaging. All genotypes were imaged on the same day, during 7 days, for which three different differentiations were performed. Image time series were acquired on a Zeiss LSM700 inverted confocal laser scanning microscope equipped with temperature and CO 2 incubation. Imaging conditions and microscope settings were identical for all time series. Using a Plan-Apochromat 63×/1.4NA objective and laser light excitation at 1 % transmission of a 10 mW 488 nm diode laser, 512 × 512 images were acquired with a pixel dwell time of 3.15 μs and pixel size of 0.198 μm. Image fields containing several neurites were selected in transmitted light mode and, for photoactivation, a region of interest containing a 15 μm long neuritic segment was drawn in the Zeiss Zen 2009 software. Every time series consisted of (1) two prephotoactivation frames, (2) the photoactivation phase (2 iterations using the 5 mW 405 nm laser at 100 % transmission) and (3) 147 frames at 10.1 s time intervals. To specifically assess the directionality of movement, we counted the number of photoactivated neurofilaments that could unambiguously be discriminated as individual filaments that moved out of the photoactivated zone either anterogradely or retrogradely at high speed. To quantitatively assess movement of NFs in general, the leading edges of filaments moving out of the photoactivated neuritic segment were tracked by using the Manual Tracking plugin of ImageJ and by using the cell body as a reference point. The XY-coordinates of the filament tracks, originating from the ImageJ output file, were used to analyze the tracks in a custom-made script in R (http://www.rproject.org/). Briefly, the displacement of the leading edge between two consecutive frames was used to calculate the speed and directionality at each time point. A filament was considered in pause if the calculated speed was below 0.06 μm/s; this represents a displacement of three pixels during two consecutive time frames that we considered as the precision limit of our analysis. This value is consistent with earlier reports on analysis of NF movement [67]. These raw parameters were used to classify the speeds into different categories and to extract several parameters that describe the movement pattern. For the data that is presented, the mean parameters were calculated for each NF track, which was used to calculate the average and SEM for each genotype. In total, more than 120 time series, consisting of more than 600 tracks and 40,000 time points, were analyzed.

Co-immunoprecipitation
Cells were lysed in NP-40 buffer (PBS, 0.5 % (vol/vol) Nonidet P-40, 20 mM β-glycerophosphate, 10 mM NaF, 1 mM Na 3 OVO, 2 mM DTT) and Complete protease inhibitor mixture (Roche Applied Science) and left on ice for 30 min [50,69,70,72]. We considered the insolubility of the NF proteins and therefore worked with total cell lysates. No harsh detergent was added to the lysates before IP. Protein measurement was performed to equalize protein concentration from different cell lines before immunoprecipitation (IP). Sepharose 6B (Sigma-Aldrich) and protein G beads (GE Healthcare) were used and the anti-SMI-31 antibody was incubated overnight at 4 °C, after which the beads were pulled down by centrifugation. The beads were repeatedly washed before preparing SDS-polyacrylamide electrophoreses.
Preparation of Triton-X 100-soluble/-insoluble fractions Cells were lysed in a 1 % Triton-X 100 buffer (50 mMTris (pH 6.8) with 1 % (vol/vol) Triton-X 100, 5 mM EDTA, 50 μg/ml leupeptin, 1 mM Na 3 OVO 4 , 20 mM β-glycerophosphate, 10 mM NaF) and Complete protease inhibitor mixture (Roche Applied Science), by pipetting up and down and leaving them on ice for 20 min. After centrifugation at 15,000×g for 20 min at 4 °C, the supernatant was collected as 'Triton-X 100-soluble fraction' and the pellet fraction ('Triton-X 100-insoluble fraction') was resuspended in E1A lysis buffer and sonicated for 30 s. On both fractions, protein concentrations were measured and equal concentrations were subjected to WB. The amyloid precursor protein (APP) was used as a positive control to determine if the experiment was accurately executed, as it is supposed to be Triton-X 100 soluble.

Transmission electron microscopy
Cells were grown on poly-l-ornithine-coated eight-well chambered Permanox slides (Nunc, Lab-Tek) and treated for neuronal differentiation as described above. Cells were fixed in 0.1 M sodium cacodylate-buffered (pH 7.

Statistical analysis
For all experiments, results are shown as average ± standard error of the mean (SEM). GraphPad Prism 5 software was used for statistical calculations. One-way ANOVA with post hoc Bonferroni's multiple comparison test was used for statistical analysis; p values are indicated.

Mutation in HSPB1 reduces anterograde axonal transport of neurofilaments
To test if mutations in HSPB1 affect axonal transport of NFs, we performed live cell imaging of axonal segments of wild-type (WT) and mutant HSPB1 cells expressing NFM coupled to a photoactivatable GFP (PAGFP-NFM) [20]. This method allowed us to visualize the photoactivated fluorescent filaments moving into non-photoactivated axonal regions (Fig. 1a). We used human neuroblastoma cells (SH-SY5Y) because these cells express all NF subunits endogenously. The SH-SY5Y cells were transduced with lentiviral vectors containing WT or mutant HSPB1 as described in "Materials and methods". When cells expressed only PAGFP-NFM or PAGFP-NFM and WT HSPB1, the majority of filaments moved anterogradely, whereas cells expressing PAGFP-NFM and mutant HSPB1-P182L showed a higher frequency of filaments moving retrogradely, and a lower frequency of filaments moving anterogradely (Fig. 1b). To determine whether this effect was a consequence of a decrease in axonal transport rates, we compared the speed at which NFs were transported in cells expressing WT and mutant HSPB1. The NF axonal transport velocity results from rapid anterograde or retrograde movements interrupted by long periods of pause  [47,67]. We therefore evaluated NF movement velocity, pausing frequency and the frequency of switches made between retrograde and anterograde movements, but could not observe any statistical difference between cells expressing the different HSPB1 constructs (Table 1). We conclude that mutant HSPB1 decreases the frequency of anterograde transport of NFs in favor of retrograde transport.

Mutation in HSPB1 decreases neurofilament binding to kinesin
Anterograde transport of NFs along the axon is mediated by the motor protein kinesin, while dynein allows both anterograde and retrograde transport [64]. To determine whether the altered axonal transport in mutant HSPB1 SH-SY5Y cells is caused by a deficit in the interaction between NFs and their motor proteins, we co-immunoprecipitated (co-IP) phosphorylated NFs and kinesin or p150glued, a component of the dynactin-dynein complex [17,49]. We used the SMI-31 antibody that recognizes phosphorylated NFs that are able to interact with kinesin [66]. The SMI-31 antibody usually detects four separate signals in the SH-SY5Y cells, of which the upper three bands probably correspond to different phospho-forms of NFH and the single lower band corresponds to phospho-NFM. The interaction between NFs and kinesin was significantly reduced in all cell lines expressing a mutant HSPB1 construct (Fig. 1c, d). In contrast, HSPB1 mutations did not affect NF binding to p150glued (Supplementary Fig. 1). These results suggest that mutant HSPB1 may affect axonal transport of NF by altering the NFskinesin interaction.

Mutation in HSPB1 increases NF-NF interaction
The axonal transport of neurofilaments is mediated by continued shuttling between mobile and stationary states (reviewed in [29]). In the stationary phase, bundles of NFs are closely apposed, phosphorylated NFs that gained higher binding affinity for each other [17,19]. Hence, the decreased interaction between the NFs and kinesin, observed in cells with mutant HSPB1, is likely to coincide with an increase in NF bundling. Therefore, we compared NF-NF interactions in cells expressing WT and mutant HSPB1. By co-IP we observed an increased interaction between the NFs in mutant HSPB1 cell lines compared to non-transduced or HSPB1-WT controls (Fig. 2a-d).
As NF bundles form polymers that are insoluble compared to their monomeric counterparts, we assessed NF solubility using the Triton-X 100 detergent. In cells stably expressing mutant HSPB1-S135F and HSPB1-P182L, the phosphorylated NFs were more retained in the insoluble pellet fraction compared to control cells ( Fig. 3a-b), suggesting that NFs could be trapped in NF bundles or aggregates. We tested this hypothesis by analyzing NF morphology in the different cell lines by staining for NFH, often used as a neuronal marker (Fig. 4a). However, we could detect neither NF-positive aggregates nor any significant morphological differences between WT and mutant HSPB1 expressing cells. The NFs were present in a filamentous network independently of the evaluated HSPB1 genotype, and no differences in NF bundling were detected (Fig. 4b-c). To evaluate the intermediate filaments at the ultrastructural level, we next performed transmission electron microscopy on the axonal neurites of the SH-SY5Y cells. However, we were unable to detect differences in the intermediate filament distribution between WT and mutant HSPB1 cells (Fig. 4d).

Mutant HSPB1 increases neurofilament phosphorylation
Thus far, we have demonstrated that in SH-SY5Y cell lines transduced with CMT-associated HSPB1 mutants, NFs undergo less anterograde transport and interact less with kinesin, but bind more to each other. Interestingly, each of these properties can be regulated by the same event: phosphorylation of the large NF subunits [1,70,71]. Through the numerous KSP repeat motifs in their long C-terminal tail domain, NFH and NFM can be highly phosphorylated and play a crucial role in NFs properties [32,59]. We investigated the phosphorylation status of NFs in SH-SY5Y cells expressing WT or mutant HSPB1 using the SMI-31 antibody. When cells were transduced with mutant forms of HSPB1, the level of phosphorylated neurofilament was slightly but significantly increased (Fig. 5a-b). The same effects were observed when cells were subjected 0.021 ± 0.001 0.020 ± 0.002 0.021 ± 0.001 to neuronal differentiation with retinoic acid (Fig. 5e, f). Subsequently, the undifferentiated and differentiated SH-SY5Y cell lines were immunostained for phosphorylated NFs, and quantification of the mean fluorescence intensity confirmed the significant increase in phosphorylated NFs in the mutant HSPB1-S135F and HSPB1-P182L cell  (Fig. 5d-g). It is important to note that the transduction of cells with an HSPB1 construct (WT or mutant) increased the expression of the NFs, compared to nontransduced control cells. We observed a positive correlation between the protein expression levels of HSPB1 and nonphosphorylated NFs (Pearson correlation for linear measures: R = 0.6084; p value: 0.0358; n = 12). This increase reflects a more general effect of HSPB1 on the expression level of the NFs. However, when calculating the ratio of phosphorylated versus non-phosphorylated NFs, we found that the increase in phospho-NFs was independent of the increase in non-phosphorylated NFs (Fig. 5c). There was no positive correlation between the protein expression level of HSPB1 and phosphorylated NFs. We therefore conclude that mutant HSPB1 induces an increase in phospho-NFs and this increase is not attributable to HSPB1 levels.

Increased NF phosphorylation in HSPB1 mutant cells is mediated by Cdk5
Because of the observed effects of mutant HSPB1 on the phosphorylation of NFs, we searched for the protein kinase responsible for the increased NF phosphorylation in mutant HSPB1 cells. Five proline-directed kinases have previously been shown to be able to phosphorylate the KSP repeat motifs in the C-tail domains of NFM and NFH: ERK1/2, p38, JNK, GSK3β and Cdk5 [3,9,15,65]. Here, we selectively inhibited the activity of these five kinases and found that only roscovitine, a Cdk5/p35 inhibitor, prevented NF hyperphosphorylation in mutant HSPB1 cell lines. The data for roscovitine is shown in Fig. 6a, b. We confirmed these results in a second experiment where Cdk5 was silenced using a specific shRNA construct (sh3) that knocked down the expression of Cdk5 to 20 % in WT and mutant HSPB1 cell lines (Fig. 6c-e). Two major phosphorylation sites in Cdk5 have been shown to regulate its activity. Phosphorylation of Thr14 inhibits the activity of Cdk5, while phosphorylation of Tyr15 increases its activity [23]. To determine whether HSPB1 mutations could affect Cdk5 activity, we compared Cdk5 phosphorylation in WT and mutant HSPB1 cell lines. We found an increased phosphorylation of Cdk5 at the Tyr15 site in mutant HSPB1 cell lines (S135F and P182L), compared to controls (Fig. 7a-b), while the level of the Cdk5 protein was unaltered (Fig. 7c). We conclude that Cdk5 activity is increased in HSPB1 mutants.
To further assess the role of the increased Cdk5 activity, we compared the interaction of Cdk5 with the NFs in WT and mutant HSPB1 cells. Accordingly, our results showed an increased binding of Cdk5 to the phosphorylated NFs in protein extracts from the mutant HSPB1 cell lines (Fig. 2a, e). Furthermore, the HSPB1-S135F and P182L mutant cell lines displayed an increased phosphorylation of the S/TPXH/K/R repeat motif in the C-domains of NFH and NFM, a site specifically targeted by Cdk5/p35, which can be detected by the SMI-34 antibody specifically (Fig. 7d-e). Together, these results suggest that increased phosphorylation of NFs in HSPB1 mutant neuronal cells is mediated by an increased activity of Cdk5.

Silencing of Cdk5 restores NF-kinesin interaction and NF solubility in HSPB1 mutants
To further assess the role of Cdk5 in mutant HSPB1 cell lines, we tested if silencing of Cdk5 with shRNA could prevent the atypical NF properties: decreased binding of NFs to kinesin, increased NF-Cdk5 interaction and increased NF solubility. As expected, when Cdk5 was constitutively silenced, no difference in NF-Cdk5 interaction could be observed between WT and mutant Cdk5-silenced cells (Fig. 8a, c). Furthermore, silencing of Cdk5 also prevented the decreased binding of NFs with kinesin formerly seen in HSPB1 mutant cell lines (Fig. 8a, b). Additionally, no differences could be seen in NF solubility between WT and mutant cell lines (Fig. 8d, e). These experiments suggest that silencing Cdk5 can prevent the aberrant NF phenotype observed in cells expressing mutant HSPB1.

Discussion
In this study, we show that CMT-causing mutations in HSPB1 reduce the anterograde axonal transport of NFs, which might be a consequence of decreased affinity of NFs for the anterograde motor protein kinesin in mutant cell lines. We demonstrated that the impaired NF-kinesin binding is in part attributable to an increase in phosphorylation of KSP sites of NFs. Although NF hyperphosphorylation was subtle and transient, we showed that in mutant cell lines, NFs displayed known characteristics of hyperphosphorylation, as their insolubility and affinity toward each other were increased. Finally, we demonstrated that these effects were at least partially mediated by the prolinedirected kinase Cdk5.
Our results, showing that NF axonal transport is associated with NF phosphorylation, are in line with previous studies [37,41]. Our time lapse imaging showed that NFs underwent both anterograde and retrograde transport interrupted by pausing periods, as previously described [47,67]. It is reported that 73-80 % of NFs are generally in pause [47,67], while we observed only 54-59 % of the NFs pausing. However, with our imaging method only those NFs leaving the photoactivated zone (and pausing at some point) are monitored and not those that remain in the Anterograde axonal transport of NFs is known to be mediated by kinesin [69] and we found that NF interaction with kinesin is phospho-dependent, confirming several studies [33,37,41,70]. Our results suggest that the affected anterograde axonal transport observed in our mutant cell lines might play a crucial role in the pathomechanisms of CMT neuropathy.
Our results strongly suggest a central role for NFH and NFM phosphorylation in the NF atypical properties observed in HSPB1 mutants. Our strongest evidence comes from the demonstration that knocking down Cdk5 prevents NF hyperphosphorylation and interaction with kinesin. Inhibition and knockdown of Cdk5/p35 did not completely prevent NF phosphorylation, suggesting the involvement of other proline-directed kinases. The increased NF phosphorylation in cells only expressing the Cdk5 shRNA construct suggests that some compensatory mechanism by other kinases known to phosphorylate NF [51] may take place. Further support for the role of Cdk5 in NF axonal transport has been shown in literature [54]. Our study suggests a connection between the activity of Cdk5, NF hyperphosphorylation and the consequences on NF binding and dynamics b-c Quantitative analysis of the co-IP experiment for kinesin (b) and Cdk5 (c). d Repetition of the Triton-X 100 experiment as shown in Fig. 3, but performed with the sh3 double-transduced SH-SY5Y cell lines. e Quantifications of the insoluble/soluble ratios of the Triton-X 100 experiments as previously described (n = 3). **p < 0.01 in mutant HSPB1 cells. However, the intermediates in this molecular cascade are missing. Although HSPB1 and Cdk5/p35 are not known to interact with each other, they are involved in many common pathways such as apoptosis, reorganization of the cytoskeleton, cell growth and differentiation [35]. HSPB1 and Cdk5 have also been shown to be upregulated by Heat Shock Factor 2 [18,27]. However, to our knowledge no direct or indirect interaction between the two proteins has been described. As HSPB1 is known to bind to the p38 mitogen-activated protein kinase [58], its indirect effect, through ERK1/2, on Cdk5 is a plausible hypothesis that is yet to be tested.
Although the three mutations studied here induce a decreased interaction between NFs and the motor protein kinesin, the NF-NF and NF-Cdk5 interactions were not significantly increased in the HSPB1-R127W mutant cells. This observation indicates that various mutations may differentially affect HSPB1 structure and function. Indeed, in a previous work we demonstrated differences in the binding affinity of various HSPB1 mutants according to the localization of the mutation in the protein [5]. Subsequently, it is possible that each mutation differentially affects HSPB1 post-translational modification and interaction with molecular targets, resulting in the initiation of different signaling cascades. In patients, the various mutations in the HSPB1 gene result in differences in the severity of the disease, the involvement of the sensory and motor functions and the age of onset, which may also suggest differences in the pathomechanisms involved.
In addition to a deficit in NF axonal transport, increased Cdk5 activation and hyperphosphorylation of NFs might as well directly affect axonal degeneration in HSPB1 mutants as both events have been associated with neurodegenerative diseases [10,42,75]. Hyperphosphorylation of NFs is an early event observed in many neurodegenerative disorders, such as Alzheimer's disease (AD), amyotrophic lateral sclerosis (ALS), and Parkinson's disease (PD), for which they are used as early biomarkers [13,14,24,44,52]. Changes in the phosphorylation status of NFM and NFH have been shown to affect axonal transport and axon caliber [55], and phosphorylation of the KSP repeats in the tail domain of NFH modifies the binding properties of the NFs [56]. Hyperphosphorylation of NFs has also been linked specifically to axonal damage [45]. While normally phosphorylated NFs are found in the distal part of the axon [49,60], hyperphosphorylated NFs are found within protein accumulations called 'spheroids' in the proximal axons and neuronal cell body [32,56]. An increased amount of hyperphosphorylated NF bundles could destabilize the axonal cytoskeleton and negatively affect the axonal transport of other cargos [31,36,43,68]. It was hypothesized that NF aggregates entrap kinesin and dynein motors and thus jeopardize overall axonal transport [21,63]. However, we were unable to detect cell body modifications including NF aggregates or differences in the distribution of intermediate filaments despite the reported correlation between NF hyperphosphorylation, NF-NF interaction and bundles [37,61]. Although significant, the NF hyperphosphorylation seen in our study might not be strong or sustained enough to support an increased bundling of NF. The apparent contradiction between the absence of aggregates in this study and the aggregates reported in a previous study using a similar cellular model [4,74] can be explained by the level of expression of HSPB1. Indeed, the overexpression of mutant HSPB1 leads to aggregation of the protein (data not shown). While the studies previously cited used cells transiently overexpressing HSPB1, we favored a stable cell model where the transgene was expressed at a moderate level and formation of aggregates was prevented.
Another possibility is that the effect of mutant HSPB1 on NFs causes cytoskeleton dynamic deficits indirectly, through the interaction of NFs to microtubules (MTs). We recently showed that some CMT-causing HSPB1 mutations stabilized the MT network and reduced MT dynamics by binding more strongly to MTs than wild-type HSPB1 [6,7]. On the other hand, NFs have also been shown to bind unassembled tubulin, inhibit MT polymerization and directly modulate MT assembly in the axon in vivo [12,30,76]. Interestingly, the interaction between NFs and tubulin was shown to be lost upon Cdk5-mediated phosphorylation of NFH [40]. The Cdk5-dependent hyperphosphorylation of NFs could therefore affect NF regulation of MT polymerization. Thus, HSPB1 mutations could reduce neuronal maintenance by contributing to global transport defects affecting the MT network directly and indirectly, through deregulation of the level of phospho-NFs. Both MT overstabilization [7] and NF hyperphosphorylation could contribute to the destabilization of the cytoskeleton, affect axonal transport and compromise the overall integrity of the axon.
Patients carrying an HSPB1 mutation are characterized by an axonal peripheral neuropathy associated with a decrease in the amplitude of the compound muscle action potentials, which is consistent with the observed decrease in the amount, density and diameter of myelinated nerve fibers [11,38,39,62]. Among the few reports of biopsy of CMT2F patients, one [11] describes a single patient with an HSPB1-S135C mutation showing loss of NFs with a simultaneous increase in MT density in the sural nerve biopsy, underlining some correlation between these structures and the pathomechanisms. However, a causal link between deficits in the structure, density or function of NF and the degeneration of the peripheral axons still needs to be demonstrated.
In conclusion, we have shown that mutations in HSPB1, a stress protein with ubiquitous functions, affect NF properties, and each of these properties have a direct or indirect effect on NF axonal transport. Our present and previous works suggest that degeneration of long peripheral nerves associated with CMT results from the deleterious combination of different pathomechanisms affecting axonal transport. Importantly, our study contributes to the unraveling of common pathomechanisms linking mutations in HSPB1 and NFL to CMT diseases.