PURA Syndrome-causing mutations impair PUR-domain integrity and affect P-body association

Marcel Proske; Robert Janowski; Sabrina Bacher; Hyun-Seo Kang; Thomas Monecke; Tony Köhler; Saskia Hutten; Jana Tretter; Anna Crois; Lena Molitor; Alejandro Varela-Rial; Roberto Fino; Elisa Donati; Gianni De Fabritiis; Dorothee Dormann; Michael Sattler; Dierk Niessing

doi:10.7554/eLife.93561.2

eLife assessment

This important study addresses the mechanisms by which mutations in the PURA protein, a regulator of gene transcription and mRNA transport and translation, cause the neurodevelopmental PURA syndrome. Based on convincing evidence from structural biology, molecular dynamics simulation, biochemical, and cell biological analyses, the authors show that the PURA structure is very dynamic, rendering it generally sensitive to structure-altering mutations that affect its folding, DNA-unwinding activity, RNA binding, dimerization, and partitioning into processing bodies. These findings are of substantial importance to cell biology, neurogenetics, and neurology alike, because they provide first insights into how very diverse PURA mutations can cause similar and penetrant molecular, cellular, and clinical defects.

https://doi.org/10.7554/eLife.93561.2.sa1

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Abstract

Mutations in the human PURA gene cause the neuro-developmental PURA syndrome. In contrast to several other mono-genetic disorders, almost all reported mutations in this nucleic acid binding protein result in the full disease penetrance. In this study, we observed that patient mutations across PURA impair its previously reported co-localization with processing bodies. These mutations either destroyed the folding integrity, RNA binding or dimerization of PURA. We also solved the crystal structures of the N- and C-terminal PUR domains of human PURA and combined them with molecular dynamics simulations and NMR measurements. The observed unusually high dynamics and structural promiscuity of PURA indicated that this protein is particularly susceptible to mutations impairing its structural integrity. It offers an explanation why even conservative mutations across PURA result in the full penetrance of symptoms in patients with PURA syndrome.

Introduction

The family of purine-rich element binding (PUR) protein is highly conserved from plants to humans (Molitor et al, 2021). Amongst the three vertebrate paralogs PURA, PURB, and PURG, the best-studied family member is PURA (Bergemann & Johnson, 1992; Haas et al, 1993; Haas et al, 1995). It is ubiquitously expressed and has been implicated in several cellular processes, including transcriptional and translational gene regulation as well as mRNA transport in neurons (Chepenik et al, 1998; Gallia et al, 2001; Haas et al., 1993; Haas et al., 1995; Johnson et al, 2006; Kobayashi et al, 2000; Mitsumori et al, 2017; Tretiakova et al, 1999). Results from two independent knock-out mouse models demonstrated that PURA is important for postnatal brain development (Hokkanen et al, 2012; Khalili et al, 2003).

Accordingly, PURA has been implicated as a modulator of neurodegenerative disorders, such as fragile X-associated tremor/ataxia syndrome (FXTAS), and the amyotrophic lateral sclerosis (ALS) frontotemporal dementia (FTD) spectrum disorder (Swinnen et al, 2020). PURA was reported to be present in the pathological RNA foci of both disorders and to protect against RNA toxicity upon ectopic overexpression (Mori et al, 2013; Rossi et al, 2015; Shen et al, 2018; Swinnen et al, 2018; Xu et al, 2013). In addition, PURA was shown to co-localize with an ALS-causing mutant variant of the FUS protein in stress granules of ALS patients. Importantly, overexpression of PURA reduced the toxicity of mutant FUS by preventing its mis-localization (Daigle et al, 2016).

In 2014, two studies reported that a monogenetic neurodevelopmental disorder is caused by sporadic mutations in the PURA gene (Hunt et al, 2014; Lalani et al, 2014). Hallmarks of this so-called PURA syndrome are developmental delay, moderate to severe intellectual disability, hypotonia, epileptic seizures, and feeding difficulties, amongst others (Reijnders et al, 2018) (Johannesen et al, 2021). Mutations causing PURA syndrome are often frame-shift events but also point mutations distributed over the entire sequence.

Based on the crystal structures of PURA from Drosophila melanogaster (dmPURA), three conserved sequence regions termed PUR repeats I, II, and III were identified to fold into globular domains (Graebsch et al, 2010; Graebsch et al, 2009; Weber et al, 2016). Whereas PUR repeat I and II assemble into an N-terminal PUR domain via intramolecular interactions, two C-terminal PUR repeats III from different molecules interact with each other and thus mediate dimerization of PURA. All these PUR domains belong to the class of the PC4-like protein family, which mainly bind single-stranded nucleic acids and can unwind double-stranded DNA and RNA (Janowski & Niessing, 2020). Although both PUR domains possess the typical PC4-like β-β-β-β-α-(linker)-β-β-β-β-α topology, the N-terminal domain has been suggested to be the main RNA/DNA interaction entity (Weber et al., 2016). In a previous study, homology models based on the dmPURA crystal structures (Graebsch et al., 2009; Weber et al., 2016) were used to predict in silico the effects of PURA syndrome-causing mutations on the structural integrity of the human PURA protein (Reijnders et al., 2018). While these mutations could be classified into groups that likely either do or do not impair the structural integrity of PURA, these predictions remained speculative (Reijnders et al., 2018). Surprisingly, in contrast to phenotypically related genetic diseases such as the Rett syndrome (Lombardi et al, 2015), no hot-spot regions could be identified in the protein sequence that trigger the PURA syndrome. With the exception of the unstructured N-terminal region and the very C-terminus, almost all mutations across the protein sequence appear to result in the full disease spectrum (Johannesen et al., 2021; Reijnders et al., 2018). To date, we fail to understand why there is such an underrepresentation of mild phenotypes in patients with PURA syndrome.

In this study, we experimentally assessed the structure and function of human PURA as well as the impact of representative PURA syndrome-causing mutations on the protein’s integrity. When studying the impact of patient mutations on PURA’s subcellular localization, we observed impaired processing body (P-body) association but normal localization to stress granules, indicating a potential importance of P-bodies for PURA-syndrome pathology. Two particularly interesting disease-causing mutations, K97E and R140P, were further analyzed by structural means. The results indicated that the N-terminal PUR domain is unusually flexible in its fold and prone to misfolding upon mutation. In summary, we provide a structure-based explanation for the underrepresentation of mutations with mild symptoms in patients and a rational approach for predicting and functionally testing mutations of uncertain significance.

Results

Effect of the mutations in hsPURA on stress granules association

Several patient-related mutations are frame-shift events and thus predictably destroy the integrity of PURA. In addition, a number of point and indel mutations have been reported for which the pathology-causing effects are less easy to predict (Johannesen et al., 2021; Reijnders et al., 2018). To understand the functional impact of such mutations, we decided to first study the effect of three known patient mutations, K97E, I206F, and F233del (Hunt et al., 2014; Lalani et al., 2014; Reijnders et al., 2018) (Fig 1A), on the subcellular localization of hsPURA.

Stress granule localization of hsPURA depends on its ability to bind RNA.
A Schematic overview of the hsPURA protein. Patient-derived mutations experimentally assessed in this study are marked in red.
B In HeLa cells stress granules were identified by G3BP1 immunostaining (magenta) and overexpressed hsPURA (yellow) by its N-terminal Flag-tag. Nuclei were stained with DAPI (blue). Representative stress granules are marked with red arrows in the zoomed-in area. Except for hsPURA m11, all overexpressed versions of hsPURA (wild-type and mutant) showed strong stress-granule localization.
C Box-Whiskers plot of quantified intensities of hsPURA staining in stress granules above cytoplasmic background levels upon arsenite-induced stress treatment (see A). Three biological replicates (indicated by different icons) with 66 stress granules each were quantified for each cell line. Box-Whiskers-Plot of average signal intensity per repeat in each cell line. No significant difference was detected between patient-related mutations and WT. Only for the m11 mutant protein the association to stress granules was significantly reduced (p=0.0064), indicating the requirement of RNA binding for stress-granule association. P-value were calculated using unpaired two-sided students t.test of mutant compared to WT Ctrl.

Previous studies in human cell cultures indicated that hsPURA localizes to stress granules upon cellular stress and may be essential for their formation (Daigle et al., 2016; Markmiller et al, 2018). To analyze whether the afore-mentioned patient-related mutations affect the localization of hsPURA to stress granules, the mutant and wild-type versions of full-length FLAG-tagged hsPURA were overexpressed in HeLa cells using a doxycycline-inducible expression cassette and cells were stressed for one hour with 500 µM sodium arsenite (Appendix Fig S1 and Fig 1B). To find out whether stress-granule localization of hsPURA depends on its nucleic-acids binding properties, we also utilized an RNA-binding deficient version of hsPURA bearing eleven structure-guided point mutations (m11) as a control (for rationale and design of this mutant, see Appendix Fig S2). Using an anti-FLAG tag antibody, we observed wild-type hsPURA to be distributed within the cytoplasm and accumulated in stress-granule structures, as seen by co-staining with the stress-granule marker G3BP1 (Fig 1B). In contrast, the nucleic acid-binding deficient mutant hsPURA m11 failed to co-localize to G3BP1-positive granules, indicating that RNA-binding by hsPURA is necessary for its co-localization with stress granules. Furthermore, all three versions of hsPURA bearing patient-derived mutations localized to stress granules upon cellular stress (Fig 1B). In all three patient-related mutations, no significant reduction of PURAs stress granule association was seen when compared to the wild-type control (Fig 1C).

To assess the previously reported influence of hsPURA on stress-granule formation at endogenous PURA levels (Daigle et al., 2016), we performed an siRNA-mediated knockdown of hsPURA in HeLa cells and stained with the stress-granule marker G3BP1 and PURA. Efficient knockdown of endogenous PURA levels was validated with western blot experiments, showing a significant reduction of PURA protein upon knockdown (S3A-C). As expected, endogenous hsPURA co-localized with G3BP1 upon stress treatment with 500 µM arsenite PURA (Appendix Fig S4A and S4B) and thus behaved similarly to overexpressed hsPURA. A PURA knockdown did not alter the total number of microscopically visible stress granules but resulted in a greater ratio of smaller stress granules (Appendix Fig S4C). Although this finding suggests that PURA is not essential for stress granule formation, it should be noted that the knockdown did not completely eliminate PURA levels and hence a stronger effect on stress granules could occur in a complete knockout of PURA. However, PURA-syndrome patients bear a heterozygous mutation, suggesting that an incomplete knockdown likely resembles the pathogenic situation more closely than a full knockout. Together these findings suggest that (i) reduced stress-granule association of mutant hsPURA variants may not be a core feature of the PURA syndrome and (ii) impaired stress-granule formation is not very likely to be directly responsible for the etiology of this disorder.

Localization of hsPURA to P-bodies is impaired by PURA syndrome-causing mutations

To assess the localization of hsPURA to cytoplasmic granules in unstressed conditions, we first recapitulated its recently reported localization to P-bodies (Molitor et al, 2023). Co-staining with the marker DCP1A indeed confirmed a co-localization of overexpressed hsPURA in P-bodies of HeLa cells (Fig 2A and 2B). As for stress granules, the PURA m11 mutant failed to accumulate in P-bodies, indicating that RNA binding of PURA contributes to its P-body localization. In addition, the K97E and F233del mutants of hsPURA showed significantly reduced co-localization to P-bodies (Fig 2A and 2B). In summary, these experiments indicate that P-body localization of hsPURA requires its RNA-binding activity, and that the majority of tested patient mutations result in impaired P-body localization. Furthermore, since F233del mutant has been predicted to have impaired dimerization properties (Reijnders et al., 2018), these findings suggest dimerization to be important for PURA’s P-body association.

Processing-body association of hsPURA in HeLa cells is impaired by patient-derived mutations.
A P-bodies were identified by immunostaining against DCP1A and against the N-terminal FLAG-tag of overexpressed hsPURA FL. Whereas their individual staining is shown in white, the overlay of DCP1A and FLAG is shown in magenta and yellow, respectively. Nuclei were stained with DAPI (blue). All cell lines show P-body formation, marked with red arrows in the zoomed area.
B Box-Whiskers plots of quantification of intensities of hsPURA staining in P-bodies above cytoplasmic background levels. For each cell line, three biological replicates (indicated by different icons) with each 100 P-bodies were quantified, and Box-Whiskers-Plot generated for each cell line. Significantly lower P-body localization was observed for mutant K97E (p = 0.0085), F2333del (P = 0.025) and m11 (p =0.011) variants of hsPURA. P-value were calculated using unpaired two-sided students t.test of mutant compared to WT Ctrl.

hsPURA does not readily undergo RNA-driven phase separation in vitro

hsPURA accumulates in an RNA-dependent fashion to stress granules as well as to P-bodies. Both types of granules are liquid-phase separated entities, indicating that the recruitment to such granules might occur via phase separation of RNA-bound hsPURA. Since hsPURA was recently shown to be required for P-body formation in HeLa cells and fibroblasts (Molitor et al., 2023), PURA-dependent liquid phase separation could potentially also directly contribute to the formation of these granules. Furthermore, a loss of such a function could potential contribute to the etiology of PURA syndrome. In order to test this hypothesis, we used a microscope-based approach to visualize the ability of RNA-bound hsPURA to phase separate in vitro. As a positive control for RNA-mediated liquid-phase separation, the protein FUS RGG3 was used (Hofweber et al, 2018). In contrast to this control, no indication of phase separation was observed for hsPURA either in the presence or absence of total HeLa cell RNA (Appendix Fig S5). These results indicate that hsPURA does not readily phase separate with total cellular RNA under the tested experimental conditions. Of note, this observation does not exclude the possibility that hsPURA can undergo phase separation under different experimental conditions, for instance in presence of additional co-factors. However, when putting this observation in perspective with previous reports, it seems unlikely that P-body formation directly depends on phase separation by hsPURA, but rather on its recently reported function as gene regulator of the essential P-body core factors LSM14a and DDX6 (Molitor et al., 2023).

Recombinant expression tests of PURA protein with disease-causing mutations

To understand the impact of mutations on the molecular and structural integrity of hsPURA, we recombinantly expressed the above-described mutant hsPURA proteins K97E, I206F, and F233del in E. coli. In addition, hsPURA with either of the mutations R140P, R199P, and R245P were recombinantly expressed (Fig 1A). All three mutations exchange an arginine against a proline, albeit in different positions of the protein and very different structural contexts. R140P was initially reported to be a disease-causing mutation (Lee et al, 2018) but later re-interpreted as a mutation for which it is unclear if it can trigger PURA Syndrome, i.e. of uncertain significance (https://www.ncbi.nlm.nih.gov/clinvar/variation/192343/). In contrast, the mutations R199P and R245P have been described as disease-causing, with matching symptoms for patients with PURA syndrome (Reijnders et al., 2018). Hence, R140P was chosen in this study to explore the diagnostic potential of our approach, whereas R199P and R245P served as a reference point for pathology-inducing mutations.

Even after extensive optimization, recombinantly expressed hsPURA fragments with the mutations R199P and I206F (full-length variant and N-terminal PUR domain consisting of repeats I-II; PURA I-II) as well as F233del and R245P (full-length variant and C-terminal PUR domain consisting of two repeats III; PURA III) could not be purified due to protein insolubility (Appendix Table S1). In contrast, N-terminal PUR domains (PURA I-II) with either of the two remaining mutations K97E and R140P were soluble and could be purified to near homogeneity. The observed solubility of recombinant hsPURA I-II K97E is also in agreement with the previous in silico prediction (Reijnders et al., 2018) as K97 has a surface-exposed side chain that is unlikely to cause folding issues upon mutation into another flexible, polar side chain. For the R140P mutation with unclear pathological significance, no conclusive prediction on its impact on protein folding could be made in the past.

The C-terminal dimerization PUR domain adopt a classical PC4-like fold

Several PURA-Syndrome-causing mutations have been reported to be located in the C-terminal, dimerization-mediating PUR domain (Johannesen et al., 2021; Reijnders et al., 2018). Due to the lack of an experimental structure of human PURA, previous predictions of the impact of patient mutations on the structural integrity of hsPURA had to rely on a human homology model derived from dmPURA (Reijnders et al., 2018). Since Drosophila and human PURA have a rather moderate sequence identity of 46%, we decided to establish a better experimental basis for predicting the structural effects of patient mutations and determined the crystal structure of the fragment P215-K280 (i.e. hsPURA III) at 1.7 Å resolution (Fig 3A and Appendix Table S2).

Crystal structure of C-terminal PUR domain from hsPURA and effects of mutations on its function.
A Crystal structure of hsPURA III at 1.7 Å resolution (PDB ID: 8CHW). Two hsPURA III molecules (magenta and grey, respectively) form a homodimer. Like other PUR domains (e.g. hsPURA I-II), hsPURA repeat III consists of four β-sheets and one α-helix.
B In electrophoretic mobility shift *assays (EMSA)* the interaction of hsPURA FL and hsPURA III with a 24-mer (CGG)₈ RNA fluorescently labeled with Cy5 fluorophore at 5’end was observed. The amount of the RNA was kept constant at 8 nM while the protein concentration increased from 0 to 16 μM. The unbound RNA used for quantification (see E) is indicated with red arrows.
C Apparent affinities derived from EMSAs (C) indicate that the C-terminal PUR domain is also able to interact with the nucleic acids. Pairwise t-tests of the hsPURA fragments showed significantly lower RNA binding compared to the full-length protein (hsPURA III: p = 9.6E-4). Three replicates were measured for each experiment and protein variant, and the standard deviations have been calculated and shown as bars.
D, E Strand-separation activity of hsPURA. The graphs show the averaged values of three independent experiments as dots with standard deviations as error bars.
D The hsPURA III fragment shows sigmoidal increase of the ssDNA concentration measured as a fluorescent signal. For the quantification of the sigmoidal curves, we utilized Boltzmann function implemented in the Origin software. Calculated x₀, which corresponds to the Km in this assay yields 4.26 ± 0.74 µM.
E Strand-separation activity of full-length hsPURA was calculated with Michaelis-Menten kinetic, yielding an average Km value of 0.83 ± 0.05 µM, respectively. For both hsPURA samples at least three independent measurements have been performed.
F NanoBRET experiments in HEK293 cells with different hsPURA fragment-expressing constructs. Milli-BRET units (mBU) were measured for dimerization of hsPURA I-III with hsPURA I-III, hsPURA I-III F233del, and hsPURA I-III R245P. Pairwise t-tests of the mutant hsPURA I-III versions F233del and R245P yielded significantly lower signals compared to the wild-type protein (hsPURA I-III F233del: p = 3.3E-4; hsPURA I-III R245P: p = 1.5E-7), indicating impaired interactions between the proteins. Black horizontal line shows reference of mBU obtained for hsPURA I-II as negative control. Of note, since the BRET signal is the ratio of donor and acceptor signal, it does not require normalization for expression levels. Asterisks in (B) and (G) indicate significance level: *** for p ≤ 0.001.

This fragment corresponds to the domain boundaries suggested by the previously solved invertebrate dmPURA III structure (Weber et al., 2016). The structure of the C-terminal PUR domain possesses the typical four antiparallel β-strands and one α-helix. Like in the previously published dmPURA III structure (Weber et al., 2016), the C-terminal PUR domain of hsPURA is built from two PUR repeats III of independent protein chains that interact with each other to form an intermolecular homodimer. The hsPURA III dimer shows high structural similarity to dmPURA III with r.m.s.d. of 1.26 Å for 125 superimposed Cα atoms and 50% of sequence identity (Appendix Fig S6A).

Dimerization domain of hsPURA shows nucleic acid binding and unwinding activities

PUR repeats III adopt a classical PC4-like fold, suggesting that it might also bind to nucleic acids. Analysis of the crystal structure of the hsPURA III homodimer revealed electrostatic surface potentials favorable for interactions with nucleic acids (Appendix Fig S6B). When performing gel electrophoresis mobility shift assays (EMSAs) we indeed observed RNA binding (Fig 3B and 3C).

It had been previously reported that PURA can separate double-stranded (ds) nucleic acids in an ATP-independent fashion (Darbinian et al, 2001; Weber et al., 2016). This so-called unwindase activity has also been reported for several other PC4-like domains from different organisms (Janowski & Niessing, 2020). For dmPURA it had already been suggested that dsDNA strands are melted by intercalation of the β-ridge between both strands, followed by binding of both single strands to the cavities formed by the curved β-sheets on both sides of the β-ridge (Appendix Fig S7) (Weber et al., 2016). Since we had already observed RNA binding by PUR repeats III (Fig 3B and 3C), we examined its potential unwindase activity by utilizing a previously reported in vitro unwinding assay (Darbinian et al., 2001; Weber et al., 2016) with dsDNA 5’-end labelled with a FAM fluorophore and 3’-end labelled with Dabcyl quencher (Appendix Fig S8). In this assay, double-stranded DNA results in low fluorescence signal due to the proximity of the quencher to the fluorophore. Upon strand separation their distance and fluorescence signal increase. We indeed observed strand separation in presence of the hsPURA III fragment (Fig 3D). Of note, RNA binding as well as dsDNA strand separation by full-length hsPURA was much more efficient than by the PUR III domain (Fig 3D and 3E), indicating potential cooperativity of the N- and C-terminal PUR domains in unwinding double-stranded nucleic acids.

PURA syndrome-causing mutations in the C-terminal PUR domain impair dimerization

Next, we used the hsPURA III structure (Fig 3A and Table S2) to perform an in silico analysis of the impact of patient-derived mutations F233del and R245P on the structural integrity of the C-terminal PUR domain. While failure to obtain soluble recombinant PURA with F233del mutation prevented a direct biophysical assessment of its dimerization state in vitro (Appendix Table S1), this observation already indicated a misfolding of the C-terminal PUR domain upon mutation. Consistent with this observation is also the interpretation from homology modeling based on the previously published dmPURA III structure (Reijnders et al., 2018). There, the mutation was predicted to impair the structural integrity of the C-terminal hsPURA dimerization domain. F233 is part of the β-sheet and interacts with the α-helix of the other PUR repeat III within the PUR domain, contributing to dimerization (Appendix Fig S9A). Since in the PURA F233del variant, one residue is deleted, the orientation of all subsequent amino acids in the β-strand adopt the opposite orientation, likely resulting in a fold disruption of the β-sheet and possibly in impaired dimerization. In the case of R245P mutation (Appendix Fig S9B), the exchange into proline also likely impairs β-strand folding by introducing a kink, which could also impact dimerization.

To provide direct proof for impaired dimerization upon the introduction of patient-derived F233del and R245P mutations, we utilized the FRET-based NanoBRET assay in HEK293 cells (Fig 3F). With this assay, we assessed the ability of hsPURA bearing the F233del and R245P patient mutations to dimerize with wild-type hsPURA by measuring corresponding milli BRET Units (mBU). Of note, this combination of wild-type and mutant PURA protein is likely to recapitulate the heterozygous situation in patients. As a control for background signal, non-dimerizing hsPURA I-II was measured (negative control). As a control for positive interaction, hsPURA I-III was used. While for hsPURA I-III the signal intensities above the background level clearly indicated dimerization (Fig 3F), protein fragments with either the F233del or the R245P mutation showed strongly reduced signal intensities. This observation implies impairment of PURA dimerization in patients bearing either of these heterozygous mutations.

N-terminal PUR domain shows great flexibility in its domain fold

For a better understand of the structural impact of mutations in the N-terminal PUR domain (hsPURA I-II), we determined its structure (fragment E57-E212) by X-ray crystallography (Fig 4A and Appendix Table S2). The N-terminal PUR domain resembles the previously published PURA structure from D. melanogaster (Graebsch et al., 2009; Weber et al., 2016) (dmPURA I-II WT) with an average root mean square deviation (r.m.s.d.) of 1.2 Å (Appendix Fig S10). However, in contrast to this invertebrate structure, we observed for hsPURA I-II that the four molecules within its asymmetric unit of the crystal lattice showed marked differences in its loop regions and in particular at the edges of the β-sheets (Fig 4B). This suggested greater structural flexibility than average domain folds and most likely than its D. melanogaster ortholog.

Structure and nucleic-acids interaction of the N-terminal PUR domain.
A Crystal structure of wild-type hsPURA repeat I (green) and II (blue) at 1.95 Å resolution. Protein fragment for which no electron density was visible is shown as a grey dotted line.
B Ribbon presentation of the overlay of all four chains (shown in different colors) of hsPURA I-II in the asymmetric unit of the crystal. There are three regions showing greater differences in folding between these individual molecules, indicating that they are flexible and likely adopt several conformations also in solution.
C In electrophoretic mobility shift assays, (EMSA) the interaction of different hsPURA I-II variants with 24-mer RNA (CGG)₈ labeled with Cy5-fluorophore was observed. The amount of labeled RNA was kept constant at 8 nM while the protein concentration increased from 0 to 16 μM. The unbound RNA was used for quantification (see D) and is indicated with the red arrow. Above the unbound RNA a second band of free RNA is visible, which might constitute a different conformation or RNA dimer.
D Quantification of the RNA interactions of different hsPURA I-II variants from EMSAs shown in (C). The RNA-binding affinity of wild-type hsPURA was normalized to 100%. Pairwise t-test was used to assess differences in RNA binding compared to the hsPURA I-II. The mutants K97E and m11 showed significantly lower relative affinities (p = 1.5E-05 and p = 4.6E-09, respectively). In contrast, the mutation R140P did not alter binding affinity (p = 0.5).
E Strand-separation activity of different hsPURA variants. For each hsPURA sample at least three measurements have been performed. The graphs show the averaged values as points as well as the standard deviations as error bars. The strand-separation activity shows linear increase within the used concentration range.
F Quantitative representation of strand-separating activity of the hsPURA I-II variants. The strand-separating activity of hsPURA I-II was quantified from the slope in (E) and normalized to 100%. Except for R140P (p = 0.07), pairwise t-tests of the hsPURA I-II mutants showed significantly lower relative activity (K97E p = 3.9E-16 and m11 p = 9.2E-16) than hsPURA I-II. For each experiment and each protein variant three replicates were measured, the standard deviations were calculated and are shown as bars. Asterisks in (D) and (F) indicate significance level: * for p ≤ 0.05, *** for p ≤ 0.001; n.s. for p > 0.05.

Effects of patient mutations in the N-terminal PUR domain on RNA binding

To assess the interaction of hsPURA I-II with nucleic acids and to understand how selected patient-derived mutations affect this function, we performed EMSAs for this protein fragment (Fig 4C and 4D). While hsPURA I-II quantitatively bound a 24-mer CGG-repeat RNA, the hsPURA I-II K97E mutant protein showed moderately but significantly decreased RNA binding (Fig 4C and 4D). Impaired RNA binding upon K97E mutation is not surprising as a change of the surface electrostatic potential from positive to negative may impact its interaction with nucleic acids (Appendix Fig S6B). In contrast, hsPURA I-II R140P did not show impaired RNA binding (Fig 4C and 4D). This finding indicates that R140P might be a benign mutation and does not have disease-causing properties. As a negative control, the N-terminal PUR domain containing eleven selected point mutations was employed (hsPURA I-II m11; Appendix Fig S2). Since these mutations were introduced to abolish the interaction of hsPURA with nucleic acids, this mutant protein showed no detectable RNA binding in EMSA.

PURA-dependent strand separation of dsDNA is affected by disease-causing mutations

We recapitulated the previously reported unwindase activity (Darbinian et al., 2001; Weber et al., 2016) with human PURA I-II and asked if patient-derived mutations in this domain impair PURA’s strand-separating activity. In vitro unwinding experiments with dsDNA were performed for hsPURA I-II and compared to the patient mutants hsPURA I-II K97E and hsPURA I-II R140P as well as the hsPURA I-II m11 variant. While hsPURA I-II showed considerable strand-separating activity in this assay, the nucleic acid-binding deficient m11 mutant variant expectedly failed to separate dsDNA (Fig 4E and 4F). With an effect considerably stronger than observed for RNA binding (Fig 4C and 4D), the hsPURA I-II K97E variant showed a loss of strand-separation activity by 90% (Fig 4E and 4F). In contrast, hsPURA I-II R140P mutant showed wild-type-like separation of dsDNA (Fig 4E and 4F), further supporting our previous interpretation from RNA-binding analyses that the mutation R140P is likely functional.

CD spectroscopic measurements indicate impaired domain folding upon mutations

In order to confirm the structural integrity of the soluble hsPURA variants, we performed circular dichroism (CD) spectroscopy experiments. The spectra for both, hsPURA I-II as well as hsPURA I-II R140P mutant showed a typical alpha-beta profile (Fig 5A), suggesting a proper folding of the protein. In contrast, the spectrum for hsPURA I-II K97E indicated a strongly altered secondary-structure content. This observation was unexpected as we had predicted that this surface mutation would not affect the protein’s structural integrity (this study and (Reijnders et al., 2018). It also indicates that more detailed structural information of hsPURA I-II is needed to better understand its susceptibility to disease-causing mutations of surface-exposed residues.

Structural analysis of hsPURA I-II bearing the K97E patient mutation.
A Circular dichroism (CD) spectroscopic analyses of hsPURA I-II, K97E, and R140P mutant. Shown are the mean of three CD measurements for each of the proteins (n = 3). The spectra of hsPURA I-II K97E show a very different profile, indicating an altered fold of this mutant compared to the wild-type form.
**B, C** Crystal structures of hsPURA K97E repeat I (green) and II (blue) at 2.45 Å resolution, showing a high overall similarity to hsPURA (**Fig 4A**). Two independent hsPURA I-II K97E chains (A and B) in the asymmetric unit are shown in (B) and (C), respectively. The mutated amino acid K97E is indicated as red sticks.
**D, E** Positional shifts of amino acids in β5 (D) and β6 (E) strands of the chain B in the crystal structure of hsPURA I-II K97E. 2Fo-Fc electron density map (contour 1σ) is shown for the selected fragment of β5 and β6 strands in chain B (light pink). The superimposed chain A (grey) shows a register shift in chain B by +1 amino acid in the β5 strand and by +2 in the β6 strand.
F NMR experiment with wild-type hsPURA I-II and hsPURA I-II K97E. Overlay of the ¹H, ¹⁵N-HSQC spectra of hsPURA I-II (red) and K97E (black). Blue boxes indicate examples of changes between both spectra.

hsPURA bearing mutation R140P with uncertain clinical significance shows wild-type-like domain folding

The mutation R140P had been previously described to be of uncertain clinical significance and it remained to be shown if this mutation affects the protein’s domain folding. CD spectra had already suggested that this mutation has no dramatic effect on the overall domain folding (Fig 5A). To assess if this mutation has a rather local effect on the structural integrity of PURA that may not be detectable by CD spectroscopy, we solved the crystal structure of hsPURA I-II R140P at 2.15 Å resolution (Appendix Fig S11A, S11B and Table S2). The crystals of R140P mutant protein exhibited the same space group, unit cell parameters, and crystal packing as the wild-type protein (Appendix Table S2). The R140P mutation is located at the end of the flexible linker between PUR repeat I and II connecting helix α1 to the strand β5 (Fig 1A, Appendix Fig S11A and S11B). Because of its position in a flexible region, the mutated residue is partially visible only in one out of four PURA chains in the asymmetric unit. The overlap of the R140P mutant structure with the PURA I-II WT fragment confirmed our previous observation about the unusually high flexibility of the strands β4 and β8 forming the β-ridge (Appendix Fig S11A and S11B). Since no major structural differences were visible between hsPURA I-II WT and R140P mutant (average r.m.s.d. of 0.89 Å for 133 Cα atoms aligned, Appendix Fig S11C), we concluded that this mutation is unlikely to impair the structural integrity of hsPURA.

hsPURA I-II with the patient mutation K97E reveals promiscuous domain folding

To understand how exactly the surface-exposed K97E mutation alters the domain folding of PURA (Fig 5A), we solved the crystal structure of hsPURA I-II K97E (Fig 5B-E, Appendix Table S2). The asymmetric unit of the crystal contained two molecules of hsPURA I-II K97E and showed good overall fold similarity to the hsPURA I-II structure (Fig 5B and 5C). However, an overlay of both molecules of the K97E-mutant protein from the asymmetric unit also revealed unusual differences between them with r.m.s.d of 1.48 Å for 125 superimposed Cα atoms. While one of these molecules (chain A, Fig 5B) showed a fold very similar to hsPURA I-II (average r.m.s.d. 1.09 Å, Appendix Fig S12A), the second molecule (chain B) displayed much greater structural changes (average r.m.s.d. 1.61 Å, Fig 5C and Appendix Fig S12A). These differences were especially pronounced in PUR repeat II (Fig 5D-E), where we observed a shift of register in the β-sheet by one amino acid in strand β5 (Fig 5D) and by two amino acids in strand β6 (Fig 5E). More C-terminally, the loop linking β6 and β7 is shorter by two residues, thereby correcting again the sequence register within the next β-strands (β7 and β8).

Already the different molecules of wild-type hsPURA I-II in the crystal unit cell revealed considerable conformational freedom (Fig 4B, Appendix Fig S12B and S12C), not only for narrow movements of the loops but also in the folding of the β-strands. For instance, in some of the molecules in the asymmetric unit of the wild-type hsPURA I-II crystal, β4 and β8 strands formed bulges (Fig 4B, Appendix Fig S12B and S12C). From all the areas of the structure, the β-ridge appears to be structurally the most divergent part. It is surprising that the K97E point mutation, which is located on the β4 strand of the β-ridge, induces the observed unusual change in the β-sheet arrangement (Fig 5C-E) without destroying the domain’s overall scaffold. Together these findings indicate great structural flexibility of the N-terminal PUR domain and promiscuity in folding, which results in misfolding upon mutation of a surface-exposed residue. While CD measurements suggest a difference in folding between wild-type and K97E mutated PURA (Fig 5A) and the crystal structure of hsPURA I-II K97E indicates folding promiscuity (Fig 5C-E), these data do not fully exclude unfolding of the domain in solution. To distinguish between a mutation-induced unfolding and an altered folded state, we performed NMR measurements with the ¹⁵N-isotope-labeled samples of wild-type and K97E mutant hsPURA I-II (E57-E212 fragment). First, ¹H,¹⁵N-correlation spectra (HSQC) of both wild-type and K97E constructs showed a clear presence of the structured core, as evidenced by the well-dispersed resonances, with a significant number of residues adopting strand conformation (¹H 8.5 - 9.5 ppm) (Fig 5F). Next, we carefully compared the two HSQC spectra for individual resonances/residues. When the two spectra were overlaid, we observed that a significant number of resonances, especially in the region corresponding to the β-strand, were perturbed, which is clearly more extensive than just affecting the residues adjacent to the mutational site of residue 97 (Fig 5F). Finally, we performed the ¹⁵N-heteronuclear NOE experiment on the K97E mutant to measure the residue-level backbone dynamics (Appendix Fig S13A). The overlaid spectra of the absence (control) and presence (NOE) of ¹H-saturation shows most resonances retaining their signal intensities (rigid, hetNOE ∼ 0.8), while the resonances corresponding to the dynamic regions, likely N-/C-terminal & loop regions, with significantly reduced signal intensities or even negative (flexible). Importantly, all the resonances perturbed upon K97E mutation remained in the presence of ¹H-saturation, confirming that the structural rearrangement does not induce protein unfolding. Together, this shows that the K97E mutation does not induce global unfolding of hsPURA I-II, but rather triggers structural rearrangements mostly in the β-strand region.

To obtain a better understanding of the intrinsic dynamics of hsPURA I-II we performed in silico molecular dynamics simulations. The hsPURA I-II WT and K97E showed a similar overall profile (Appendix Fig S13B), where most of the flexibility or fluctuations are concentrated in the loops connecting strands β3 with β4 and β7 with β8. However, there are some statistically significant differences between the two proteins. The most significant differences concentrate on the two ends of the α1 helix, as well as the β5, β6, and β7 segments. In these regions, the K97E mutant shows higher flexibility than the WT, with the N-terminal part of the α1 helix and the C-terminal end of β5 and β6 having the greatest gap between the two variants. The movie (S1 for hsPURA I-II WT and S2 for hsPURA I-II K97E) of the simulation confirms a large degree of fluctuation in this area, which can adopt many different conformations in both WT and mutant. Finally, there is one region where the WT displays a higher flexibility than the mutant, the loop connecting β7 with β8 (residues 175 to 185), although only a few of those differences are significant. Of note, while these simulations are consistent with the increased flexibility suggested by the crystal structure, the time window of these simulations was too short to observe alterations between the two folding states as seen in this experimental structure.

Discussion

Currently, more than 270 different pathogenic mutations in the PURA gene have been identified in over 600 patients with confirmed PURA syndrome (personal communication: PURA Foundation Australia). The aim of this study was to understand how mutations causing this neurodevelopmental disorder affect the functional and structural integrity of the hsPURA protein. Towards this goal, we performed cellular, biophysical, and structural analysis with wild-type hsPURA as well as with versions of hsPURA bearing representative patient-derived mutations.

To understand how PUR-syndrome-causing mutations affect the subcellular localization of hsPURA, we performed immunofluorescence microscopic analyses in HeLa cells by overexpressing full-length hsPURA as well as variants bearing a disease-causing mutation in each of the three PUR repeats, i.e. K97E, I206F, and F233del. Consistent with previous reports (Daigle et al., 2016; Markmiller et al., 2018), we observed that hsPURA co-localizes to stress granules in HeLa cells (Fig 1B and 1C). As we did not observe significant changes in the association of patient-related mutations of hsPURA to stress granules, it is suggested that this feature may not constitute a major hallmark of the PURA syndrome. It should be noted however that this interpretation must be considered with some caution as the experiments were performed in a PURA wild-type background.

What is more, the knockdown of PURA resulted in reduced sizes of those stress granules (Appendix Fig S4), indicating that PURA indeed does have an influence on these granules. Future experiments will be necessary to unambiguously clarify the importance of PURA’s localization to stress granules for the etiology of PURA syndrome.

Very recently, hsPURA was reported to localize to P-bodies and that a PURA knockdown leads to a significant reduction in HeLa cells (Molitor et al., 2023). While we recapitulated co-localization of hsPURA to P-bodies (Fig 2), hsPURA K97E and F233del mutants failed to fully localize to P-bodies. Since the F233del mutation impairs the dimerization of hsPURA (Fig 3F), this finding suggests the requirement of dimerization for efficient P-body association.

To address the question of what drives hsPURA accumulation in these phase-separated granules, we utilized a hsPURA version lacking RNA-binding activity (m11, Appendix Fig S2). This mutant failed to localize to stress granules or P-bodies, indicating that RNA binding is essential for both co-localization events. A potential RNA-dependent mechanism to recruit hsPURA into stress granules or P-bodies could be liquid phase separation of hsPURA when bound to RNAs. In vitro experiments testing this potential property of hsPURA failed to yield phase-separated droplets. In summary, these findings indicate that RNA binding of hsPURA is important for its co-localization into stress granules and P-bodies, while we have no evidence that phase separation of hsPURA plays a role.

In a recent study, it was shown that a hsPURA knock-down in HeLa and in fibroblast cells resulted in down-regulation of the essential P-body proteins LSM14a and DDX6 and, most likely as a direct consequence, in strongly impaired P-body formation (Molitor et al., 2023). In light of this report, our finding that patient-derived mutations impair the P-body association of hsPURA (Fig 2) provide further evidence for a potential role of P-body localization of hsPURA for the etiology of PURA syndrome.

It has been reported that protein domains with PC4-like fold interact with RNA and DNA and are responsible for the separation of the double-stranded nucleic acids (Darbinian et al., 2001; Weber et al., 2016) (reviewed in (Janowski & Niessing, 2020). In this study, we show that both, the N- and C-terminal PUR domains of human PURA can separate double-stranded nucleic acids (Fig 4E, 4F and 3D) and to bind single-stranded nucleic acids (Fig 4C, 4D, 3B and 3C). We also tested patient-derived mutant versions of hsPURA to find out whether they exhibit impaired interaction with nucleic acids. For the K97E mutated version, we observed in EMSAs a reduced affinity to RNA (Fig 4C and 4D). Similar behavior of the K97E mutant was observed in the strand-separation assay where it showed an almost complete loss of activity (Fig 4E and 4F). The latter is of interest since previous experiments had demonstrated that strand separation contributes to the neuroprotective activity of PURA in a Drosophila FXTAS disease model (Weber et al., 2016). It is therefore also probable that loss of strand-separation activity contributes to cellular abnormalities in hsPURA patients harboring the K97E mutation.

To establish a structural framework for these observations, we solved the crystal structures of hsPURA III (Fig 3A) and of hsPURA I-II (Fig 4A). These human structures were overall very similar to previously published crystal structures from dmPURA (Appendix Fig S6A and S10) (Graebsch et al., 2009; Weber et al., 2016). Based on the crystal structures of hsPURA III (Fig 3A) we were able to predict folding defects in the C-terminal PUR domain (hsPUR III) that are caused by the patient-derived mutations F233del and R245P (Appendix Fig S9). Deletion of phenylalanine 233 within the β2-strand changes the orientation of all subsequent side chains within the β-sheet and likely destroys the interaction network required for the assembly of this secondary structure. A mutation of arginine 245 into proline likely disrupts β-strand folding by introducing a kink. Since repeat III mediates homodimer formation through swapping of its α-helices, the dimerization of hsPURA is potentially affected by folding defects induced by either the F233del or the R245P mutation. Indeed, we could experimentally confirm by nanoBRET measurements in HEK293 cells that dimerization of hsPURA I-III F233del and hsPURA I-III R245 is impaired when compared to wild-type hsPURA (Fig 3F).

Determination of the crystal structure of hsPURA I-II revealed larger flexible regions than the previously reported invertebrate structures (Graebsch et al., 2010; Graebsch et al., 2009; Weber et al., 2016), with considerable differences in the four molecules of hsPURA I-II in the asymmetric unit of the crystals (Fig 4B, Appendix Fig S12B and S12C). These observations provide clear evidence that in particular strands β4 and β8 of the N-terminal PUR domain are dynamic and can adopt considerable local differences within the β-sheet. This flexibility already suggests structural promiscuity of PUR domains. It also indicates that they can at least partially compensate for structural perturbance by mutations, resulting in folded domains of mutant proteins. However, since these mutations were reported to cause PURA syndrome, such modest structural alterations must nevertheless result in functional impairment.

The interpretation of structural flexibility and folding promiscuity of PUR domains found experimental support from the crystal structure of its K97E variant, whose mutated residue has a solvent-exposed side chain (Fig 5B-E). The corresponding structure shows in the β5 strand a shift by one (Fig 5D) and in the β6 strand by two amino acids (Fig 5E) in one of the molecules of the asymmetric unit. Surprisingly, these structural distortions did not result in major unfolding events of this PUR domain. Furthermore, NMR measurements with the ¹⁵N- and ¹H-labeled N-terminal PUR domain yielded many spectral differences between the wild-type and K97E variants in particular within their β-sheets (Fig 5F and Appendix Fig S13A). Despite these considerable structural changes, the NMR data also confirmed that the K97E-mutant protein remains folded in solution and indicates that PUR domains may be able to partially compensate for mutations by folding promiscuity. These findings were further supported by molecular dynamics simulations, indicating high intrinsic motions of the N-terminal PUR domain (Appendix Fig S13B).

Instead of hot-spot regions for disease-causing mutations, as reported for other genetic disorders such as neurodevelopmental Rett syndrome (Lombardi et al., 2015), mutations of PURA-syndrome patients are found along the entire protein sequence (Johannesen et al., 2021; Reijnders et al., 2018). Also, in contrast to disorders such as the Rett syndrome, most of these mutations cause the full spectrum of disease symptoms. Our findings suggest that the flexibility and promiscuity of hsPURA domain folding render this protein particularly susceptible to mutations, even when amino-acid substitutions impose only moderate changes to the local charge and stereochemistry. This property of PUR domains might offer a structural explanation for why so many mutations across the sequence of hsPURA result in the full disease spectrum.

Not in all cases is the pathogenic effect of a given mutation as clear as in the case of K97E. For instance, the replacement of arginine 140 by proline in hsPURA was initially reported to cause PURA syndrome (Lee et al., 2018). Even though the corresponding patient did show symptoms, the severity and type of symptoms raised doubts about this initial diagnosis. In our assessment, neither the functional in vitro experiments nor the structural assessment of hsPURA I-II R140P yielded any significant differences from the wild-type protein (Fig 4C-F and Appendix Fig S11). These experimental findings are consistent with R140P being rather a benign mutation. Furthermore, after the initial description of R140P to be causative for PURA Syndrome (Lee et al., 2018), subsequent genomic assessment of a relative of this patient uncovered that this person had the same mutation without any clear symptoms. Consequently, the R140P mutation is now listed in the NCBI ClinVar database to be of “uncertain significance” (https://www.ncbi.nlm.nih.gov/clinvar/variation/192343/). Our data clearly suggest that this mutation is rather benign. In summary, an assessment of the different mutations in hsPURA indicates a clear correlation between defects observed in in vitro analyses and the reported pathogenicity in patients. Hence, in future such in vitro analyses may serve as a diagnostic tool to distinguish pathogenic from benign mutations.

Recently, two publications resorted to in silico predicted, AI-based structures to model the potential impact of PURA-syndrome mutations on the structural integrity of hsPURA. Instead of assessing the physiologically correct dimer consisting of two PUR repeats, both publications analyzed in silico-predicted hsPURA half-structure consisting of a single PUR repeat III with incomplete dimerization domain (Dai et al, 2023; Lopez-Rivera et al, 2022). Such half PURA structures are very unlikely to exist in solution and hence predictions based on them are of very limited value or worse, prone to yield wrong interpretations. We expect that our experimentally determined structures of the human N-and C-terminal PUR domains offer more physiological structural reference points for future assessments of novel hsPURA mutations and their potential pathogenicity in patients.

In summary, this study provides the first functional and experimental structural assessment of the effects of PURA-syndrome causing mutations on folding, nucleic-acid binding, and unwinding, as well as on subcellular localization to stress granules and P-bodies. Some of the selected patient variants of hsPURA were previously predicted to have folding defects (Reijnders et al., 2018). Of note, for all these cases expression tests with recombinant proteins resulted in insoluble samples, indicating that these mutant proteins indeed have impaired folding (Appendix Table S1). Whereas predictions of such misfolding events appear reliable, the examples of R140P (benign) and K97E (pathogenic) indicate that structural predictions of surface-exposed residues seem more complicated. In fact, the observed great promiscuity of folding of PUR domains indicates that also moderate surface mutations such as K97E can result in promiscuous folding and the full spectrum of disease symptoms. Our study may serve as proof-of-principle that in vitro and structural studies are suitable tools to classify mutations in the hsPURA gene as potentially pathogenic or benign.

Materials and methods

In-depth descriptions of the sample preparation techniques and comprehensive details of the experimental procedures can be found in the Appendix section of this document.

Acknowledgements

We acknowledge the use of the X-ray Crystallography Platform at Helmholtz Munich, the Core Facility Bioimaging of the BMC of the Ludwig-Maximilians University Munich, as well as the Bavarian NMR Centre (BNMRZ). We would like to thank Vera Roman for her excellent technical support as well as Melinda Anderson from the PURA Foundation Australia and the PURA Syndrome Foundation for their precious support.

Funding

Deutsche Forschungsgemeinschaft FOR2333 sub-project Ni-1110/6-2 (DN) Care-for-Rare Science Award (DN)

Author contributions

MP performed structural and biophysical analysis as well as most cell-culture studies, RJ performed X-ray measurements, structural analysis, in vitro RNA and DNA binding tests. SB performed staining and analysis of stress granules in HeLa cells under PURA knock-down conditions. SH participated in biophysical analysis as well as cell-based studies. H-S K performed NMR experiments and analysis. TK and AC performed NanoBRET experiments and LM, SB, and JT produced the cell lines. A V-R, R F, E D, and G D F performed and analyzed molecular dynamics simulations. TM performed phase separation experiments. DD, MS and DN supervised and discussed the project. The manuscript was written by MP, RJ, SB, and DN. All authors participated in the discussion, interpreted the results, and commented on the manuscript.

Disclosure and competing interests statement

Authors declare that they have no competing interests.

Data and materials availability

All data are available in the main text or the supplementary materials. Structural models and diffraction data are available at the Protein Data Base (PDB; https://www.rcsb.org/) under the accession codes 8CHT (hsPURA I-II), 8CHU (hsPURA I-II K97E), 8CHV (hsPURA I-II R140P) and 8CHW (hsPURA III).

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Article and author information

Author information

Marcel Proske
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany, Institute of Pharmaceutical Biotechnology, Ulm University, 89081 Ulm, Germany
ORCID iD: 0000-0002-1570-7231
- These authors contributed equally to this study
Robert Janowski
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany
ORCID iD: 0000-0002-9940-2143
- These authors contributed equally to this study
Sabrina Bacher
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany
Hyun-Seo Kang
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany, Chemistry Department, Biomolecular NMR and Center for Integrated Protein Science Munich, Technical University of Munich, 85748 Garching, Germany
ORCID iD: 0000-0003-4029-5096
Thomas Monecke
Institute of Pharmaceutical Biotechnology, Ulm University, 89081 Ulm, Germany
Tony Köhler
Institute of Pharmaceutical Biotechnology, Ulm University, 89081 Ulm, Germany
Saskia Hutten
Biocenter, Institute of Molecular Physiology, Johannes Gutenberg-Universität (JGU), 55128 Mainz, Germany
Jana Tretter
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany
Anna Crois
Institute of Pharmaceutical Biotechnology, Ulm University, 89081 Ulm, Germany
ORCID iD: 0009-0001-0791-5719
Lena Molitor
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany
Alejandro Varela-Rial
Acellera Labs SL, 08005 Barcelona, Spain
ORCID iD: 0000-0002-6918-1765
Roberto Fino
Acellera Labs SL, 08005 Barcelona, Spain
ORCID iD: 0000-0001-5323-4562
Elisa Donati
Acellera Labs SL, 08005 Barcelona, Spain
ORCID iD: 0000-0001-7073-1974
Gianni De Fabritiis
Acellera Labs SL, 08005 Barcelona, Spain
ORCID iD: 0000-0003-3913-4877
Dorothee Dormann
Biocenter, Institute of Molecular Physiology, Johannes Gutenberg-Universität (JGU), 55128 Mainz, Germany, Institute of Molecular Biology (IMB), 55128 Mainz, Germany
ORCID iD: 0000-0002-9260-2775
Michael Sattler
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany, Chemistry Department, Biomolecular NMR and Center for Integrated Protein Science Munich, Technical University of Munich, 85748 Garching, Germany
Dierk Niessing
Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich, 85764 Neuherberg, Germany, Institute of Pharmaceutical Biotechnology, Ulm University, 89081 Ulm, Germany
ORCID iD: 0000-0002-5589-369X
- Correspondence should be addressed to dierk.niessing@uni-ulm.de

Version history

Preprint posted: September 20, 2023
Sent for peer review: November 8, 2023
Reviewed Preprint version 1: January 24, 2024
Reviewed Preprint version 2: March 20, 2024
Version of Record published: April 24, 2024

Copyright

This article is distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use and redistribution provided that the original author and source are credited.

Revised: This Reviewed Preprint has been revised by the authors in response to the previous round of peer review; the eLife assessment and the public reviews have been updated where necessary by the editors and peer reviewers.

Reviewing Editor
Nils Brose
Max Planck Institute of Experimental Medicine, Göttingen, Germany
Senior Editor
Volker Dötsch
Goethe University Frankfurt, Frankfurt am Main, Germany

Joint Public Review:

The present study focuses on the structure and function of human PURA, a regulator of gene transcription and mRNA transport and translation whose mutation causes the neurodevelopmental PURA syndrome, characterized by developmental delay, intellectual disability, hypotonia, epileptic seizures, a.o. deficits. The authors combined structural biology, molecular dynamics simulation, and various cell biological assays to study the effects of disease-causing PURA mutations on protein structure and function. The corresponding data reveal a highly dynamic PURA structure and show that disease-related mutations in PURA cause complex defects in folding, DNA-unwinding activity, RNA binding, dimerization, and partitioning into processing bodies. These findings provide first insights into how very diverse PURA mutations can cause penetrant molecular, cellular, and clinical defects. This will be of substantial interest to cell biologists, neurogeneticists, and neurologists alike.

A particular strength of the present study is the structural characterization of human PURA, which is a challenging target for structural biology approaches. The molecular dynamics simulations are state-of-the-art, allowing a statistically meaningful assessment of the differences between wild-type and mutant proteins. The functional consequences of PURA mutations at the cellular level are fascinating, particularly the differential compartmentalization of wild-type and mutant PURA variants into certain subcellular condensates.

https://doi.org/10.7554/eLife.93561.2.sa0

Author Response

The following is the authors’ response to the original reviews.

Public Review

[...] A particular strength of the present study is the structural characterization of human PURA, which is a challenging target for structural biology approaches. The molecular dynamics simulations are state-of-the-art, allowing a statistically meaningful assessment of the differences between wild-type and mutant proteins. The functional consequences of PURA mutations at the cellular level are fascinating, particularly the differential compartmentalization of wild-type and mutant PURA variants into certain subcellular condensates.

Weaknesses that warrant rectification relate to (i) The interpretation of statistically non-significant effects seen in the molecular dynamic simulations.

We removed from the manuscript the sentence which indicated that we analyzed statistically non-significant effects. Therefore, the above statement has been resolved.

(ii) The statistical analysis of the differential compartmentalization of PURA variants into processing bodies vs. stress granules, and

We re-analyzed all cell-biological data and adjusted the statistical analysis of P-bodies and Stress-granule intensity analysis. The new, and improved statistics have replaced the original analyses in the corresponding figures (Figs. 1C and 2B).

(iii) Insufficient documentation of protein expression levels and knock-down efficiencies.

Quantification of protein expression levels by Western blotting is shown in Appendix Figure S1. Quantification of knock-down efficiencies by Western blot experiments (Appendix Figure S3).

Recommendations for the authors: Reviewer #1

Concerns and Suggested Changes

(a) I have only one concern about the computational part and that is about statements such as "There are also large differences in the residue surrounding the mutation spot (residues 90 to 100), where the K97E mutant also shows much greater fluctuation. However, these differences are not significant due to the large standard deviations." If the differences are not statistically significant, then I would suggest either removing such a statement or increasing the statistics.

We agree with the Reviewer’s comment. We removed this sentence from the text.

Recommendations for the authors: Reviewer #2

General Comments

This is a challenging structural target and the authors have made considerable efforts to determine the effect of several mutations on the structure and function. Many of the constructs, however, could not be expressed and/or purified in bacteria. However, it is not clear to what extent other expression systems (e.g. Drosophila or human) were considered and if this would have been beneficial.

We did not use other expression systems because the wild-type protein is well-behaved when expressed in E. coli. In case a mutant variant cannot be expressed or does not behave well in E. coli, this constitutes a clear indication that the respective mutation impairs the protein’s integrity. Thus, by using *E. coli *as a reference system for all the variants of PURA protein, we could assess the influence of the mutations on the structural integrity and solubility. Only for the variants that did not show impairment in E. coli expression, we continued to assess in more detail why they are nevertheless functionally impaired and cause PURA Syndrome.

Concerns and Suggested Changes

(a) The schematic in Figure 3A would have been helpful for interpreting the mutations discussed in Figures 1 and 2. I would suggest moving it earlier in the text.

We changed the figure according to the Reviewer’s suggestion.

(b) I believe the RNA used for binding studies in Figures 3C and D was (CGG)8. Are the two "free" RNA bands a monomer and a dimer (duplex?)?

Although we do not know for certain, it is indeed likely that the two free RNA bands represent either different secondary structures of the free RNA or a duplex of two molecules. Of note, PURA binds to both “free” RNA bands, indicating that it either does not discriminate between them or melts double-stranded RNA in these EMSAs.

There also seems to be considerable cooperativity in the binding, so I wonder if a shorter RNA oligonucleotide might facilitate the measurement of Kds.

The length of the used RNA was selected based on the estimated elongated size of the full-length PURA and the presence of 3 PUR repeats. Assuming that one PUR repeat interacts with about 6-7 bases (data from the co-structure of Drosophila PURA with DNA; PDB-ID: 5FGP) and that full-length PURA forms a dimer consisting of three PUR repeats, the full-length protein in its extended form should cover a nucleic-acid stretch of about 24 bases.

Also, it is not clear how the affinities were measured particularly for hsPURA III since free band is never fully bound at the highest protein concentration.

It was not our goal to measure Kds for the interaction of PURA variants with RNA. The EMSA experiments were conducted to detect relative differences in the interaction between PURA variants and RNA. To estimate the differences, we measured total intensity of the bound (shifted) and unbound RNA. The intensities of the bands observed on the scanned EMSA gels were quantified with FUJI ImageJ software. We calculated the percentage of the shifted RNA and normalized it. hsPURA III fragment shows much lower affinity therefore it does not fully shift RNA with the highest protein concentration when compared to the full-length PURA and to PURA I-II.

(c) Do the human PURA I+II and dmPURA I+ II crystallize in the same space group and have similar packing? Can the observed structural flexibility be due to crystal contacts?

hsPURA I+II and dmPURA I+II crystallize in different space groups with different crystal packing. In both cases, the asymmetric unit contains 4 independent molecules with the flexible part of the structure composed of the β4 and β8 (β ridge) exposed to solvent. In the case of the Drosophila structure, we do not observe any flexibility of both β-strands. In contrast, for the human PURA structure the β ridge exhibits lots of flexibility and it adopts different conformations in all 4 molecules of the asymmetric unit. We observe similar flexibility of the β4 and β8 (β ridge) in the structure of K97E mutant which contains 2 molecules in the asymmetric unit. We would like to add that we expect crystal contacts to rather stabilize than destabilize domains.

Similarly, can the conformations observed for the K97E mutant be partially explained by packing?

Regarding the sequence shift observed for the β5 and β6 strands in hsPURA I+II K97E variant: although the β5 strand with shifted amino acid sequence is involved in the contact with the symmetry-related molecule with another β5 strand we don’t consider this interaction as a source of the shift. To be sure that the shift is not forced by the crystallization, we had performed NMR measurement which confirmed that in solution there is a strong change in the β-stands comparing WT and K97E mutant. This is an unambiguous indication that the structural changes observed in the crystal structure are also happening in solution. In addition, the MD simulations provide additional confirmation of our interpretation that K97E destabilizes the corresponding PUR domain. Taken together, we provide proof from three different angles that the observed differences indeed affect the integrity and hence function of the protein.

(d) Perhaps, it is my misunderstanding, but I find the NMR data on the Arg sidechains for the K97E confusing. If they are visible for K97E and not WT, doesn't this indicate that there is an exchange between two conformations or more dynamics in the WT structure? This does not seem to be the opposite of the expectation if K97E is thought to have more conformational flexibility.

Due to a technical issue (peak contour level), arginine side chain resonances were not clearly visible in the WT spectrum. The figure 5F has been updated. Now, they do correspond to those seen in the mutant spectrum. However, to prevent any confusion or mis/overinterpretation, we removed the sentence regarding arginine side chain: "Intriguingly, arginine side chain resonances Nε-Hε were only visible in the K97E variant, while they were broadened out in the wild-type spectrum."

(e) The most speculative part of the paper is the interpretation of SG and PB localization of PURA in Fig 1 and 2. There is an important issue with the statistics that must be clarified because it would appear that statistical significance was determined using each SG or PB as an independent measurement. This is incorrect and significance should be measured by only using the means of three biological replicates. This is well described here. It is not clear at this time if the reported P values will be confirmed upon reanalysis, and this may require reinterpretation of the data.

We are grateful for this clarifying comment and agree that the statistical analysis of P-body and stress granule was misleading. Of note, while the figures depicted all the values independent of the biological repeats, the statistical analyses were done on the mean value of each replicate of each cell line and not all raw data points.

We prepared new Plots, only showing the mean value of each replicate, and also re-calculated P-values. The values have changed only slightly in this new analysis because we now also included the previously labeled outliers (red points) to better demonstrate that significance still exists even when considering them.

In the new analysis of stress-granule association, only the value of the K97E mutant lost its significance, indicating that its association to stress granules is not lost. Therefore, we adjusted the following sentences in the manuscript.

Results:

Original: "While quantification showed a reduced association of hsPURA K97E mutant with G3BP1-positive granules (Fig 1B), the two other mutants, I206F and F233del, showed the same co-localization to stress granules as the wild type control."

Corrected: "In all the patient-related mutations, no significant reduction in stress granule association was seen when compared to the wild type control (Fig 1C)."

Original: "The observation that only one of the patient-related mutations of hsPURA, K97E, showed reduced stress granule association indicates that this feature may not constitute a major hallmark of the PURA syndrome. It should be noted however that this interpretation must be considered with some caution as the experiments were performed in a PURA wild-type background."

Corrected: "As we did not observe significant changes in the association of patient-related mutations of hsPURA to stress granules, it is suggested that that this feature may not constitute a major hallmark of the PURA syndrome. It should be noted however that this interpretation must be considered with some caution as the experiments were performed in a PURA wild-type background."

(f) A western blot showing the level of overexpression of the PURA proteins should be shown in Figure 1 as well as the KD of endogenous PURA for Figure S2?

As requested, a Western blot showing the level of overexpression of the different PURA proteins has been added as Appendix Figure S1.

A Western blot of the siRNA-mediated knock-down experiments of PURA and their corresponding control has been added to Appendix Figure S3. Quantification of three biological repeats showed a significant reduction of PURA protein levels upon knock down.

(g) While I appreciate that rewriting is time-consuming, I would recommend considering restructuring the manuscript because I think that it would aid the overall clarity. I think the foundation of the work is the structural characterization and would suggest beginning the paper with this data and the biochemical characterization. The co-localization with SGs and PBs and how this may be relevant to disease is much more speculative and is therefore better to present later. While I appreciate that the structural interpretation of why some mutants localize to PBs differently is not entirely clear, I do think that this would provide some context for the discussion.

In the initial version of the manuscript we first presented the structural characterization of PURA and afterwards the co-localization with SGs and PBs. As this reviewer stated him-/herself in (e), we also noticed that the SG and PB interpretation is the most speculative part of this manuscript. We felt that having this at the end of the results section would weaken the manuscript. On the other hand, we consider that the structural interpretation of mutations is much stronger and has a greater impact for future research. After long discussion we decided to swap the order to leave the most important results for the end of the manuscript.

Recommendations for the authors: Reviewer #3

Concerns and Suggested Changes:

(a) For the characterization of G3BP1-positive stress granules in HeLa cells upon depletion of PURA, it remains unclear what is the efficiency of siRNA? The authors should provide a western blot to indicate how much the endogenous levels were reduced.

We completely agree with the stated concern and addressed it accordingly. We had performed this experiment prior to submission but for some unknown reason it was not included in the manuscript.

The Western blot of siRNA-mediated knock-down experiments of PURA and their corresponding control is now shown in Appendix Figure S3. Quantification of three biological repeats, showed a significant reduction of PURA protein levels upon knock down.

(b) How does knocking down PURA affect DCP1A-positive structures in HeLa cells? Would P bodies be formed even in the absence (or reduction) of total PURA?

Indeed, the stated question is very interesting. In fact, we have already shown in our recent publication (Molitor et al., 2023) that a knock down of PURA in HeLa and NHDF cells leads to a significant reduction of P-bodies. We actually referred to this finding on page 6:

"Since hsPURA was recently shown to be required for P-body formation in HeLa cells and fibroblasts (Molitor et al. 2023), PURA-dependent liquid phase separation could potentially also directly contribute to the formation of these granules."

On the same page, we also refer to the underlying molecular mechanism:

"However, when putting this observation in perspective with previous reports, it seems unlikely that P-body formation directly depends on phase separation by hsPURA, but rather on its recently reported function as gene regulator of the essential P-body core factors LSM14a and DDX6 (Molitor et al., 2023)."

https://doi.org/10.7554/eLife.93561.2.sa2

Significance of findings

Strength of evidence

Abstract

Introduction

Results

Effect of the mutations in hsPURA on stress granules association

Stress granule localization of hsPURA depends on its ability to bind RNA.

Localization of hsPURA to P-bodies is impaired by PURA syndrome-causing mutations

Processing-body association of hsPURA in HeLa cells is impaired by patient-derived mutations.

hsPURA does not readily undergo RNA-driven phase separation in vitro

Recombinant expression tests of PURA protein with disease-causing mutations

The C-terminal dimerization PUR domain adopt a classical PC4-like fold

Crystal structure of C-terminal PUR domain from hsPURA and effects of mutations on its function.

Dimerization domain of hsPURA shows nucleic acid binding and unwinding activities

PURA syndrome-causing mutations in the C-terminal PUR domain impair dimerization

N-terminal PUR domain shows great flexibility in its domain fold

Structure and nucleic-acids interaction of the N-terminal PUR domain.

Effects of patient mutations in the N-terminal PUR domain on RNA binding

PURA-dependent strand separation of dsDNA is affected by disease-causing mutations

CD spectroscopic measurements indicate impaired domain folding upon mutations

Structural analysis of hsPURA I-II bearing the K97E patient mutation.

hsPURA bearing mutation R140P with uncertain clinical significance shows wild-type-like domain folding

hsPURA I-II with the patient mutation K97E reveals promiscuous domain folding

Discussion

Materials and methods

Acknowledgements

Funding

Author contributions

Disclosure and competing interests statement

Data and materials availability

References

Article and author information

Author information

Marcel Proske†

Robert Janowski†

Sabrina Bacher

Hyun-Seo Kang

Thomas Monecke

Tony Köhler

Saskia Hutten

Jana Tretter

Anna Crois

Lena Molitor

Alejandro Varela-Rial

Roberto Fino

Elisa Donati

Gianni De Fabritiis

Dorothee Dormann

Michael Sattler

Dierk Niessing

Version history

Copyright

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Editors

Marcel Proske

Robert Janowski