Abstract
The integrated stress response (ISR) is a conserved pathway in eukaryotic cells that is activated in response to multiple sources of cellular stress. Although acute activation of this pathway restores cellular homeostasis, intense or prolonged ISR activation perturbs cell function and may contribute to neurodegeneration. DNL343 is an investigational CNS-penetrant small molecule ISR inhibitor designed to activate the eukaryotic initiation factor 2B (eIF2B) and suppress aberrant ISR activation. DNL343 reduced CNS ISR activity and neurodegeneration in a dose-dependent manner in two established in vivo models – the optic nerve crush injury and an eIF2B loss of function (LOF) mutant – demonstrating neuroprotection in both and preventing motor dysfunction in the LOF mutant mouse. Treatment with DNL343 at a late stage of disease in the LOF model reversed elevation in plasma biomarkers of neuroinflammation and neurodegeneration and prevented premature mortality. Several proteins and metabolites that are dysregulated in the LOF mouse brains were normalized by DNL343 treatment, and this response is detectable in human biofluids. Several of these biomarkers show differential levels in CSF and plasma from patients with vanishing white matter disease (VWMD), a neurodegenerative disease that is driven by eIF2B LOF and chronic ISR activation, supporting their potential translational relevance. This study demonstrates that DNL343 is a brain penetrant ISR inhibitor capable of attenuating neurodegeneration in mouse models and identifies several biomarker candidates that may be used to assess treatment responses in the clinic.
Introduction
Eukaryotic initiation factor 2B (eIF2B) is a heterodecameric protein that plays an indispensable role in regulating translation of mRNA into protein. This process is initiated by the assembly of GTP-bound eIF2 and methionine-carrying initiator tRNA (Met-tRNAi) into a ternary complex (TC) which, along with other initiation factors, delivers Met-tRNAi to the AUG start codon. Upon recognition of the start codon, GTP is hydrolyzed, and the resulting eIF2-GDP dissociates from the complex (Gebauer and Hentze 2004, Sonenberg and Hinnebusch 2009). The continual success of translation initiation is dependent on replenishment of active GTP-bound eIF2 through the exchange of GDP for GTP by eIF2B, a dedicated guanidine exchange factor for eIF2 (Bogorad, Lin et al. 2018, Hanson, Hodgson et al. 2022).
eIF2B activity is dynamically modulated by the integrated stress response (ISR), an evolutionarily conserved signaling pathway that is activated in response to diverse cellular stresses, such as viral infection, amino acid deprivation, protein misfolding, and oxidative stress (Pakos-Zebrucka, Koryga et al. 2016, Costa-Mattioli and Walter 2020). ISR activation centers on the phosphorylation eIF2B binding partner, eIF2, which led to structural changes that alter its interaction with eIF2B, turning it from a substrate into a competitive inhibitor of the guanine nucleotide exchange factor (GEF) activity of eIF2B (Adomavicius, Guaita et al. 2019, Gordiyenko, Llacer et al. 2019, Kenner, Anand et al. 2019, Schoof, Boone et al. 2021). As a result, the availability of eIF2-GTP and the subsequent TC become limited, leading to attenuation of global translation. This also gives rise to the paradoxical increase in translation of some stress response proteins (Harding, Novoa et al. 2000). A common feature of these proteins are upstream open reading frames (uORF) in the 5’ region that act as translational decoys to the main protein coding sequence (MCS). Under non-stress conditions these regulatory elements are translated instead of the MCS. However, during ISR activation, when TC and initiation cofactors are limited, translation of these uORFs are bypassed in place of the MCS due to leaky ribosomal scanning (Wethmar, Smink et al. 2010, Young and Wek 2016, Chen and Tarn 2019, Costa-Mattioli and Walter 2020). One such protein is activating transcription factor 4 (ATF4) (Vattem and Wek 2004), the primary effector of the ISR which regulates the expression of a wide range of adaptive genes aimed at restoring homeostasis or, in the event that the stress signal cannot be mitigated, triggering apoptosis (Walter and Ron 2011).
Dysregulation of the ISR pathway has pathological consequences. In human and rodent models, mutations that lead to persistent activation of the ISR are associated with neurological disturbances (Harding, Zhang et al. 2009, Borck, Shin et al. 2012, Abdulkarim, Nicolino et al. 2015, Kernohan, Tetreault et al. 2015, Skopkova, Hennig et al. 2017) and those that affect the eIF2B subunits cause a rare leukodystrophy called vanishing white matter disease (VWMD) (van der Knaap, Pronk et al. 2006). Additionally, evidence of constitutive pathway activation has been found in neurodegenerative conditions like Amyotrophic Lateral Sclerosis (ALS) (Ilieva, Ayala et al. 2007, Ito, Yamada et al. 2009) and Alzheimer’s disease (Hoozemans, Veerhuis et al. 2005, Unterberger, Hoftberger et al. 2006, Hoozemans, van Haastert et al. 2009, Stutzbach, Xie et al. 2013, Storkebaum, Rosenblum et al. 2023), suggesting that dysregulation of the ISR may contribute to these disorders.
Pharmacological modulation of the ISR is a key area of therapeutic research and has been accomplished through a variety of approaches, including inhibition of upstream ISR kinases, inhibition of eIF2 phosphatases, and activation of eIF2B (Hetz, Axten et al. 2019). Inhibition of upstream kinases such as PERK has been shown to cause on-target toxicity, which limits their therapeutic potential (Halliday, Radford et al. 2015). In contrast, eIF2B activators have proven to be well tolerated in animal models while also improving memory and neurological deficits (Sidrauski, Acosta-Alvear et al. 2013, Chou, Krukowski et al. 2017, Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019, Krukowski, Nolan et al. 2020). The first published eIF2B activator, ISRIB, binds to and stabilizes the eIF2B complex in its decameric form and promotes the GEF activity of eIF2B regardless of the presence of phosphorylated eIF2 (Tsai, Miller-Vedam et al. 2018, Zyryanova, Weis et al. 2018). ISRIB and its analog, 2BAct, were also neuroprotective in an eIF2B mutant mouse model of VWMD that displays ISR-mediated neurodegeneration (Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019). Despite this, further development of ISRIB is hampered by its poor solubility and oral bioavailability (Wang, Tan et al. 2018, Abbink, Wisse et al. 2019), and 2BAct due to its cardiovascular liability in dogs (Wong, LeBon et al. 2019).
DNL343 is an investigational small molecule eIF2B activator that is has completed a Phase 1 clinical trial in healthy participants (NCT04268784) and is now undergoing clinical development for ALS (NCT05006352, NCT05842941). In immortalized cells and iPSC-derived neurons expressing ALS-linked mutations that are exposed to stressors, DNL343 inhibits the ISR and both prevents and reverses stress granule formation (Sun, Tsai et al. 2023). The high potency, selectivity, and pharmacokinetic profile of DNL343 across preclinical species make it an ideal tool for studying ISR inhibition in vivo (Craig, De Vicente et al. 2024).
Here we show that DNL343 reduces ISR activation and neurodegeneration brought on acutely by an optic nerve crush (ONC) injury or chronically by a germline eIF2B LOF mutation in mice. We also show that DNL343 treatment, initiated at a late stage of disease which more accurately replicates a clinical dosing paradigm, reversed these ISR and neurodegeneration biomarkers and prevented premature mortality in the eIF2B LOF mutant. Further, we identified CNS biomarkers of the ISR and neurodegeneration that are measurable in biofluids and showed data that support their translational relevance in samples from patients with VWMD and potentially other indications that are mediated by ISR activation.
Results
DNL343 is a novel brain-penetrant ISR inhibitor
To study the in vivo effects of our investigational small molecule eIF2B activator, DNL343 (Figure 1A), we first demonstrated its suitability for acute and chronic dosing and evaluated brain exposure in wild-type mice (Figure 1B). Following a single dose of DNL343 at 62.5 mg/kg via oral gavage, unbound concentrations in the brain were similar to those in plasma (Figure 1C), supporting high CNS penetrance in mice (Craig, De Vicente et al. 2024). Chronic dosing via a non-invasive self-administration route was then examined by formulating DNL343 in mouse chow. After 5 weeks on medicated chow, dose-dependent increases in plasma and brain exposure of DNL343 were observed in mice (Figure 1D-E). Plasma DNL343 concentrations were similar following 2 or 29 days of dosing, indicating that steady-state conditions were rapidly achieved and sustained throughout the dosing duration (Figure 1D). Further, unbound concentrations of DNL343 in the brain were comparable to those in plasma for all doses at terminal timepoint (Figure 1E). No adverse event/s or effects on body weight (Figure 1F) were observed during the study, indicating that chronic treatment with DNL343 was well tolerated.
DNL343 reduced ISR activation and neuronal loss in an optic nerve crush injury model in mice
To determine the impact of DNL343 on ISR dependent neurodegeneration, we first utilized an ONC injury model. This model was selected based on the precedence for ISR activation and reproducible degeneration within a relatively short time period following injury (Larhammar, Huntwork-Rodriguez et al. 2017). ONC was performed on the left optic nerve of wild-type mice, following which mice were given either vehicle or increasing doses of DNL343 once daily via oral gavage. (Figure 2A). The mice were euthanized at 2 or 14 days following the ONC procedure. Unbound concentrations of DNL343 measured in plasma or brain were similar, again confirming CNS penetration (Figure 2B). DNL343 exposure increased in a dose-proportionate manner and demonstrated low variability between animals (Figure 2B). We then measured the expression of ISR-dependent transcripts some of which are known to be altered in this model (Larhammar, Huntwork-Rodriguez et al. 2017, Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019) in the retina to confirm DNL343 activity in vivo. We found that many of these transcripts were robustly increased in the ipsilateral retina vs undamaged contralateral control retinas at 2 days and, to a lesser extent, 14 days after the ONC (Figure 2C, Supplemental Tables 1-2). DNL343 modulated the expression level of these ISR-dependent transcripts in a dose-dependent fashion (Figure 2C, Supplemental Tables 1-2) confirming its ability to inhibit ISR in vivo. In addition, the highest dose of DNL343 at 12 mg/kg reduced axonal degeneration (Figure 2D) and the two highest doses, 3 and 12 mg/kg, led to significant reduction in retinal ganglion cell (RGC) loss as measured by immunofluorescence analysis of neuronal markers (Figure 2E-F). Together, these data demonstrate pharmacodynamic and neuroprotective effects of DNL343 in an in vivo model of acute injury.
eIF2B loss of function causes CNS ISR activation in the mouse
We next sought to develop a model that displays chronic ISR activation in the CNS to further test the effect of DNL343 treatment in vivo. To this end, we generated an eIF2B LOF mouse model by knocking in an Eif2b5 R191H point mutation that is homologous to the VWMD-causing human R195H mutation (Fogli, Wong et al. 2002). Homozygous knock-in mice will hereafter be referred to as eIF2B HOM. Previous reports of independently generated Eif2b5 R191H mutant showed ISR overactivation in the CNS and disease phenotypes relevant to human VWMD, such as demyelination and motor function deficit, that ultimately led to premature mortality (Dooves, Bugiani et al. 2016, Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019). In line with this, characterization of select transcript markers in our eIF2B HOM model at 13-19 weeks of age confirmed ISR activation in the brain of mice homozygous for the mutation, but not in heterozygous or wild-type littermates (Supplemental Figure 1A and Supplemental Table 3). The robust elevation of ISR markers were further confirmed in a bulk brain RNA sequencing analysis of a separate cohort of homozygous mutant and wild-type littermates. Known ISR markers rank highly among the 492 protein-coding genes that showed significant differences between eIF2B HOM and wild-type animals (FDR <5%, Supplemental Figure 1B and Supplemental Table 4). Genes reported as upregulated due to eIF2B loss of function (Wong, LeBon et al. 2019) were significantly enriched (gene set enrichment p-value <10-20).
ISR activation appears to be most prominent in the CNS since tissues such as peripheral blood mononuclear cells (PBMC) or spleen have no marked upregulation of the ISR markers in homozygous mice relative to wild-type controls (Supplemental Figure 1C and D and Supplemental Table 5 and 6). This is consistent with the reported CNS and peripheral phenotypes of independently generated models (Dooves, Bugiani et al. 2016, Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019).
Proteomic analysis reveals distinct brain & CSF signatures of ISR activation and neurodegeneration in eIF2B mutant mice
To further characterize the consequences of eIF2B LOF mutation in the mouse brain, we performed bulk brain proteomic characterization on an independent cohort of 11-15-week-old mice. Out of the 7,939 proteins detected, we found 133 proteins that showed significant alteration in the eIF2B HOM genotype relative to wild-type controls (Figure 3A and Supplemental Table 7). Of these, 45 proteins were also dysregulated on a transcriptional level (Supplemental Figure 1B) suggesting some overlap between the transcriptomic and proteomic changes. In keeping with this, proteins that are regulated by ATF4, a transcription factor the levels of which are known to be ISR-dependent (Pakos-Zebrucka, Koryga et al. 2016), are among those that are most significantly elevated, such as solute carrier (SLC) membrane transport proteins (SLC3A2, SLC7A1, SLC7A1), cystathionine γ-lyase (CTH) and phosphoserine aminotransferase 1 (PSAT1) (Figure 3A). Results from the proteomic analysis also show that disturbances in metabolic pathways appear to be the main consequences of the eIF2B LOF mutation on the brain proteome. Indeed, pathways related to amino acid transport and metabolism were found to be significantly (adjusted P <0.05) increased based on gene set enrichment analysis (GSEA) (Figure 3C). Taken together, these results show that eIF2B LOF leads to gross cerebral metabolic derangement that may contribute to the neurodegenerative phenotype associated with this model.
To understand how the ISR-dependent changes in brain proteins correlate to more clinically translatable fluid biomarkers, we also interrogated the CSF proteome of these eIF2B HOM mice. CSF tandem mass tag (TMT) proteomic analysis identified a total of 572 unique proteins, 472 of which were detected in both CSF and the brain. Univariate analysis identified a total of 44 proteins that were changed with unadjusted P <0.05 (Figure 3B and Supplementary Table 7). Notably, the protein with the largest fold decrease in the eIF2B HOM CSF was MUP17 (log2 fold change (FC): -1.3, adjusted P <0.05), a major urinary protein (MUP) and a member of the broader lipocalin protein family, which has been shown to be decreased by ER stress (Weber, Yang et al. 2022). Several proteins associated with microglial activation (PLA2G7, CSF1R, LYSZ, and SIRPA) and intracellular organelle associated proteins (CPE, CTSB, CLSTN1, CTSD, HEXA, GM2A, and ALDH2) were also higher in homozygous mice relative to wild-type controls (Figure 3B and Supplementary Table 7). Analysis of cellular compartment of origin of CSF proteins shows that proteins increased in the CSF were enriched for proteins associated with early endosome, Golgi and membrane bound organelle (Figure 3D). Results also showed decreases in CSF proteins associated with neuron-to-neuron synapse, postsynaptic density and dendritic spine that may be reflecting accelerated neurodegeneration apparent in this model. (Figure 3D and Supplementary Table 7). Alterations in CSF levels of proteins associated with microglial activation and organelle proteins may indicate elevations in inflammatory burden associated with demyelination and neurodegeneration phenotypes seen in humans and other mouse models with mutations in the eIF2B protein (Bugiani, Vuong et al. 2018, Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019). Taken together, our data show very different proteome changes in the brain and CSF from eIF2B HOM mice and collectively, these data point to the CSF proteome representing biomarkers of demyelination and inflammation in the model while the changes in the brain appear to more directly represent cellular ISR dysregulation.
DNL343 reduced brain ISR activation and prevented disease phenotypes in eIF2B HOM mice
Having characterized the eIF2B HOM model, we next tested the ability of DNL343 to inhibit ISR activation in these mice by initiating treatment at 10-17 weeks of age, before disease onset (Figure 4A) (based on clinical signs & plasma biomarker of neurodegeneration (Figure 4F)). Animals received DNL343 medicated chow and intake was steady across all groups, achieving levels equivalent to oral gavage doses of 0, 0.3, 1, 3, or 10 mg/kg (Supplemental Figure 2A-C). DNL343 exposure in the plasma showed a stable and dose-dependent profile from treatment weeks 2-12 (Figure 4B), with similar dose-matched exposure levels between wild-type and eIF2B HOM mice suggesting that DNL343 absorption was not altered in this model (Figure 4B-C). After 13 weeks of dosing, DNL343 exposure in the plasma and brain showed a dose-dependent increase (Figure 4C) that was accompanied by a dose-dependent reduction of ISR transcript markers in the brain of eIF2B HOM mice (Figure 4D and Supplemental Table 8). These data further support the notion that DNL343 is effective at blocking chronic CNS ISR activation in vivo.
Consistent with the characterization of previously published eIF2B mutant models (Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019), eIF2B HOM animals gain less weight over time compared to their wild-type counterparts. The two highest doses of DNL343 (3 and 10 mg/kg) significantly improved body weight increase (Figure 4E and Supplemental Figure 3A), despite a modest reduction in food intake in these groups (Supplemental Figure 2B). This improved disease phenotype was mirrored by a similar dose-dependent prevention of plasma NfL elevation, suggesting that DNL343 is neuroprotective in the model (Figure 4F and Supplemental Figure 3B). Indeed, following 12 weeks of dosing, eIF2B HOM mice also showed a dose-dependent improvement in motor function as assessed by a balance beam test (Figure 4G-I). eIF2B HOM mice treated with DNL343 at doses of 3 and 10 mg/kg were indistinguishable from wild-type controls in the time taken to successfully cross the beam, the numbers of errors measured by foot slips, and falls from the elevated beam (Figures 4G-I).
DNL343 normalized proteins and metabolites in the brain and CSF of eIF2B HOM mice
We next evaluated the effect of chronic DNL343 treatment on the proteomic and metabolomic alterations in eIF2B HOM brains and CSF. The baseline genotype-associated differences observed in the brain and CSF proteomes were largely replicated in this older cohort of animals (5–7 month of age, Supplemental Figure 4 A-B, Figure 3A and B). In addition, targeted metabolomic and lipidomic analyses in the brain revealed profound increases in levels of oxysterols, such as 7-ketocholesterol, and cholesterol esters (CE) in eIF2B HOM mice (Supplemental Figure 4C). These lipids tend to be increased in conditions of rapid demyelination (Nugent, Lin et al. 2020), consistent with the implication of the proteomics data and the phenotypes observed in VWMD patients (Schiffmann, Moller et al. 1994, Bugiani, Vuong et al. 2018).
A 13-week treatment with DNL343 with doses that ranged from 0.3 to 10 mg/kg showed significant (P <0.05) dose-dependent normalization of proteins that were downregulated in brains of eIF2B HOM mice (Figure 5A, top cluster and Supplementary Table 9). These included APOE, SLC7A10, CD63, TST and ETNPPL that are associated with cholesterol, exosome, amino acid transport, detoxification and glycerophospholipid metabolism. Chronic treatment also lowered key ISR proteins that were significantly upregulated in eIF2B HOM brains, including proteins involved in serine/glycine/1-carbon metabolism (PSAT1, ALDH1L2, CTH) and alanine/glutamine/leucine transporters (SLC3A2, SLC7A11, SLC7A3) (Figure 5A, bottom cluster and Supplementary Table 9). Further, we identified proteins of amino acid metabolism pathway to be most significantly enriched in DNL343-vs vehicle-treated eIF2B HOM mice (Figure 5B and Supplementary Table 9). CSF proteomic analysis also showed a clear DNL343 dose-dependent correction of protein biomarkers of microglial activation such as CSF1R, HEXB, CTSS, LYZ2, and CTSB (Figure 5B). As predicted by these results, biological processes that were most impacted by DNL343 were normalization of sulfur amino acid transport and nucleolar large rRNA transcriptions processes (Figure 5D and Supplementary Table 9). As increased abundance of these proteins in the CSF have been associated with higher microglia activation, their correction by DNL343 may reflect downregulation of inflammation observed in the mutant mice. Furthermore, significant increases in 7-ketocholesterol and CE accumulation observed in eIF2B HOM mice were also dose-dependently corrected by chronic DNL343 treatment (Figure 5C and Supplementary Table 9). Together these omics studies revealed that DNL343 can robustly correct biomarkers of ISR activation in the brain and markers of gliosis and demyelination in the CSF of eIF2B HOM mice at doses ≥3 mg/kg.
Potential translational biomarkers are elevated in both eIF2B HOM mice and VWMD patient biofluids
We next sought to interrogate whether the changes observed in markers of ISR and immune activation in eIF2B HOM mice had potential translational relevance to human disease. A select number of proteins were chosen for evaluation in plasma and CSF samples from patients with VWMD (Supplemental Table 10), a neurodegenerative disease that is driven by eIF2B mutations and chronic ISR overactivation (van der Knaap, Bonkowsky et al. 2022), with gene expression and protein levels also being measured in samples from DNL343-treated eIF2B HOM mice. Our selection included growth differentiation factor 15 (GDF-15), an ISR-regulated cytokine and biomarker of clinical inflammation and metabolic distress (Lockhart, Saudek et al. 2020, McGrath, Himali et al. 2020), glial fibrillary acidic protein (GFAP), a marker of reactive astrocytes and an emerging blood biomarker associated with neurodegeneration (Abdelhak, Foschi et al. 2022), tissue inhibitor of metalloprotease 1 (TIMP-1), an astrocyte-released cytokine that has been implicated in neurodegenerative conditions (Lorenzl, Albers et al. 2003), and monocyte chemoattractant protein (MCP-1). These cytokines were largely not detected by TMT proteomics in the brain or CSF of the HOM mice as they are usually present in low abundance and therefore are challenging to detect in broad discovery proteomics method applied in this study. Here we focused on antibody-based immunoassays that are better suited to specifically measure low abundant proteins.
Both mRNA and protein levels of GDF-15 were increased in the eIF2B HOM brains relative to wild-type controls and were dose-dependently reduced by DNL343 treatment (Figure 6A and B). These changes were replicated in a separate cohort of animals (Supplemental Figure 5A and B) and were also detected in the mouse CSF (Supplemental Figure 5C) suggesting that detection of this biomarker in the fluid could be a potential surrogate to assess CNS ISR activation and modulation. GDF-15 protein levels were also elevated in the CSF and plasma of VWMD patients relative to healthy controls (Figure 6C and D) even accounting for the age dependent increase in this biomarker (Lockhart, Saudek et al. 2020) that is particularly apparent in the plasma of patients for which longitudinal samples were available (Supplemental Figure 6A). The astrocyte activation marker GFAP was elevated in eIF2B HOM mice with levels of mRNA in the brain and protein in the plasma both being corrected by DNL343 treatment (Figure 6E and F). In line with these data in the preclinical disease model, GFAP protein concentrations were higher in the CSF and plasma from VWMD patients relative to controls (Figure 6G and H). Although both TIMP-1 and MCP-1 levels were elevated in the eIF2B HOM mice, TIMP-1 levels were not altered in VWMD patients relative to controls in either the CSF or plasma and MCP-1 protein was only elevated in VWMD patient plasma (Figure 6I-P). Additionally, levels of other potential neurodegeneration biomarkers, interleukin 18 (IL-18) and soluble triggering receptor expressed on myeloid cells 2 (sTREM2), did not diverge in VWMD patients relative to controls (Supplemental Figure 6B and C). On the other hand, NfL, a marker of neurodegeneration (Gaetani, Blennow et al. 2019), was significantly elevated in the plasma and CSF of VWMD patients (Figure 6S-R and Supplemental Figure 5D-E) mirroring the changes seen in the eIF2B HOM mice (Figure 4F). In sum, GDF-15, GFAP, and NfL, demonstrated potential translational relevance by having increased gene expression or protein levels in eIF2B HOM mice relative to WT controls, which is reduced by administration of DNL343, as well as showing elevation in VWMD patient biofluids.
DNL343 treatment initiated at advanced stage of disease rescued premature mortality and reversed biomarkers of neurodegeneration in the eIF2B HOM mice
Having shown that DNL343 can robustly prevent ISR activation and disease phenotypes in the eIF2B HOM mouse, we tested the effectiveness of DNL343 to reverse disease in older eIF2B HOM mice after disease onset (based on clinical signs and plasma NfL (Figure 4)). DNL343 was administered in food at a concentration of 100 mg/kg chow for 4 weeks starting when the animals were 19-26 weeks of age, which corresponded to an advanced disease stage (Figure 7A). As expected, and previously established, this led to robust unbound plasma and brain exposure that is equivalent to an oral gavage dose of 10 mg/kg (Figure 7B, Supplemental Figure 2A). Within only 4 weeks of treatment, DNL343 fully restored normal body weight gain (Figure 7C) and reduced the elevated expression of ISR transcripts in the eIF2B HOM brain (Figure 7D and Supplemental Table 11), suggesting that administration of DNL343 can not only prevent ISR activation (Figure 4D), but also reverse it in animals with advanced disease. With this short duration of DNL343 treatment, neither motor function nor plasma NfL were fully rescued (Supplemental Figure 7A and B). Given the robust effects on both ISR markers and weight gain, we evaluated the effects of longer treatment with DNL343 in this treatment paradigm starting when the animals were 24-32 weeks of age (Figure 7A, Supplemental Figure 8A), when independently generated eIF2B mutant mice were approaching their survival limit (Dooves, Bugiani et al. 2016). In line with our hypothesis, 20 weeks of DNL343 treatment normalized the elevated plasma NfL level in eIF2B HOM mice (Figure 7E). This dosing paradigm also reversed the increased level of plasma GFAP in eIF2B HOM mice and normalized it to wild-type control level (Figure 7F). We were unable to evaluate the impact of DNL343 on motor function by the balance beam test as animals of both genotypes were unable to complete the training after 8 weeks of treatment. This impairment appeared to be driven by distinct factors in the two genotypes; age-associated obesity in wild-type animals and severe motor impairment in the eIF2B HOM mice, irrespective of treatment. This and our earlier data (Figure 4G-I) suggest that DNL343 could prevent but not reverse functional deterioration, which is in line with our understanding of DNL343 mechanism of action that does not include neuronal regeneration, a therapeutic effect that is likely required for functional recuperation. Nonetheless, correction in the plasma biomarkers of neurodegeneration was accompanied by a robust extension of survival in the eIF2B HOM mice. As expected, in this 20-week study only 25% (N=3/12) of vehicle-treated eIF2B HOM mice survived to the end of the study. In contrast, 84.6% (N=11/13) of DNL343-treated eIF2B HOM mice survived beyond the study cessation (Figure 7G and Supplemental Figure 8B), confirming that DNL343 can resolve ongoing neurodegeneration and neuroinflammation leading to prolonged lifespan in this model. Together these data demonstrate that DNL343 is a potent, CNS penetrant, ISR inhibitor that can correct or reverse downstream effects of chronic ISR overactivation.
Discussion
Increasing evidence suggests that the ISR plays a causative role in a broad range of CNS disorders such as ALS and VWMD (Costa-Mattioli and Walter 2020, Storkebaum, Rosenblum et al. 2023). DNL343 is an investigational small molecule eIF2B activator that is developed to address ISR-mediated neurodegeneration. Here, we showed that DNL343 robustly inhibited the ISR in the CNS whether activated acutely by mechanical crush injury to the optic nerve or chronically by an eIF2B LOF mutation. DNL343 also exerted a neuroprotective effect in both models by preventing either degeneration of the RGC or elevation in a plasma biomarker of neurodegeneration, NfL, and motor function deterioration. Initiating DNL343 treatment after disease onset in the eIF2B LOF model led to equally robust inhibition of the ISR and even reversed the elevated levels of plasma markers of neurodegeneration, NfL, and neuroinflammation, GFAP, and prolonged survival in the model. Our study also put forth candidate biomarkers that were identified in the mouse model and cross validated in clinical samples from patients with VWMD to potentially enable clinical assessment of CNS ISR activation and modulation, and their downstream consequences. Together these data demonstrate the therapeutic effects of DNL343 in nonclinical in vivo settings and present clinical biomarker candidates.
DNL343 is a novel small molecule eIF2B activator that was engineered for high CNS penetration. Consistent with this, data across multiple dosing studies in mice showed that DNL343 achieved comparable unbound exposures in the plasma and brain. DNL343 exposure also showed a favorable dose-dependent profile with no notable differences between healthy animals and disease models. In a chronic setting, DNL343 steady-state concentration was rapidly achieved and maintained, and the compound was well tolerated at above neuroprotective exposure levels in the ONC and eIF2B LOF models. In line with its preclinical pharmacokinetic data, DNL343 showed low pharmacokinetic variability and high CSF distribution in healthy volunteers and participants with ALS, supporting its progression as an investigational therapeutic for CNS indications (Sun, Tsai et al. 2023).
Data from our in vivo models showed that DNL343 can inhibit the ISR in multiple mouse models. In an acute ONC model, we showed significant ISR upregulation in the retina 2 days following ONC as previously reported (Larhammar, Huntwork-Rodriguez et al. 2017). This activation persisted but was less pronounced after 14 days suggesting that the ISR is activated most strongly as an early response to acute injury. At both time points, DNL343 dose-dependently normalized the ISR pathway leading to protection against RGC loss with mice treated at doses ≥3 mg/kg showing numbers of surviving RGCs that were comparable to that of uncrushed controls. The neuroprotective potential of ISR inhibition in the model was previously demonstrated using ISRIB (Larhammar, Huntwork-Rodriguez et al. 2017). In contrast to our data however, treatment with ISRIB at a higher and more frequent dose of 10 mg/kg (b.i.d.) led only to a partial correction of Chac1 (an ISR marker that is assessed in both the published data and our study) and RGC survival. This points to improved potency as a potential differentiator between DNL343 and the previous generation ISR inhibitor. Another consideration could be that the greater extent of ISR activation seen in the published data (Larhammar, Huntwork-Rodriguez et al. 2017) exceeded the cellular threshold beyond which ISRIB would have no effect. To date, such a phenomenon had only been demonstrated in vitro in the context of sodium arsenite induced stress (Rabouw, Langereis et al. 2019); whether it also underlies the discrepancy in these in vivo studies remains to be evaluated. Other possible explanations include greater unbound DNL343 exposure in the brain owing to greater CNS penetration and/or lower protein binding, and improved cellular potency (Craig, De Vicente et al. 2024).
The robust ISR inhibition and neuroprotection in the acute nerve injury model led us to study the effect of DNL343 in chronic ISR-dependent neurodegeneration in an eIF2B LOF model. Our independently generated eIF2B LOF mouse exhibits features that are consistent with previously reported models, namely prominent ISR activation in the CNS that was detectable in early adulthood and persisted throughout life, accompanied by stunted body weight growth that does not appear to be driven by hypophagia, and motor function impairment (Dooves, Bugiani et al. 2016, Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019). In addition, we showed a progressive escalation in the level of a plasma neurodegeneration biomarker, NfL, that corresponded to the degree of motor function loss. DNL343 treatment, initiated before overt disease manifestation, dose-dependently normalized these phenotypes with doses ≥3 mg/kg reverting body weight gain, plasma NfL level, and motor function to wild-type-like levels. While preventative modulation of some of the endpoints shown in this study is consistent with published literature utilizing other eIF2B activators (Abbink, Wisse et al. 2019, Wong, LeBon et al. 2019), our data provided further insight to DNL343 effects not previously explored. Our longitudinal data on plasma NfL levels throughout the dosing study allowed us to observe that DNL343, at doses of 3 & 10 mg/kg, not only led to reduction but reversal of plasma NfL elevation that hinted at the potential for this molecule to reverse the consequences of chronic ISR activation. Indeed, when dosed in a therapeutic paradigm starting at ages that corresponded to end of life (Dooves, Bugiani et al. 2016), DNL343 not only suppressed ISR activation in the eIF2B LOF brain but also robustly reversed the elevated levels of plasma NfL and GFAP. Reduction in these markers were apparent after 8 weeks, but not at the earlier timepoint of 4 weeks of treatment and this timeframe appears consistent between the prophylactic and the therapeutic dosing studies, suggesting that resolution of active neurodegeneration & neuroinflammation is predicated on correction of upstream consequences of CNS ISR activation. Further, 4 weeks of therapeutic dosing with DNL343 did not restore motor function. While this could not be further tested, we postulate that prolonging the treatment may not lead to further improvement as motor neurons likely were already degenerated at the time of treatment initiation. On the other hand, longer treatment with DNL343 in the clinically relevant therapeutic dosing paradigm extended the otherwise shortened life span of the eIF2B LOF mouse with most mice surviving past 50 weeks of age when the study was terminated. These key insights that DNL343 can robustly inhibit the ISR, reverse disease biomarkers and extend life span in an in vivo model when treatment was administered after the onset of disease have direct clinical relevance and are a major step forward in understanding the therapeutic potential of eIF2B activators.
We conducted both targeted and unbiased analyses using brain, CSF, and plasma samples from DNL343-treated eIF2B LOF mice to discover biofluid based biomarkers that could be harnessed to monitor CNS ISR activation and modulation, and their downstream consequences in the clinic. We found a disconnect between proteins that were altered in the eIF2B LOF mouse CSF relative to those in the brain. Multi-omics approach undertaken allowed us to cross-validate ATF4-regulated changes in expression of cellular amino acid transport and metabolism at transcriptomic, proteomics level leading to phenotypic alterations in cystathionine and alanine levels. While bulk brain transcriptomic and proteomic analyses show consistent changes in transcripts and proteins that belong to the ISR and amino acid metabolism pathways, as previously published (Wong, LeBon et al. 2019), our CSF proteomic findings identify proteins that represent downstream disease consequences such as demyelination and neuroinflammation. These findings were replicated in 2 cohorts of animals at 3-4 and 5-7 months of age which correspond to stages before and when disease presentation becomes evident in the eIF2B LOF model, respectively, speaking to the robustness of the findings but also highlighting the early onset of neurodegeneration in the model that precedes functional manifestation. Chronic treatment with DNL343 corrected these genotype-associated changes in the respective samples. Targeted analyses of proteins led us to discover additional markers of the ISR and neuroinflammation that could be measured in biofluids. Increased transcript or protein level of GDF-15, GFAP, and TIMP-1 in the eIF2B LOF brain and their dose responsive modulation by DNL343 were reflected by their changes in the CSF (GDF-15 and TIMP-1) and plasma (GFAP). Of these, we showed that GDF-15, a transcriptional target of ATF4, and GFAP, a marker of neuroinflammation and reactive astrocytes, were also elevated in the CSF and plasma of patients with VWMD, a rare neurodegenerative indication that is caused by biallelic recessive mutations in EIF2B1-5 and in which the ISR is a central mechanism. While astrocytes are heavily implicated in the pathophysiology of VWMD (Dietrich, Lacagnina et al. 2005, van der Knaap, Pronk et al. 2006), astrocyte dysfunction is also increasingly being recognized to contribute to the initiation and progression of diverse neurodegenerative disorders (Brandebura, Paumier et al. 2023), so GFAP is of particular interest as a CNS biomarker. NfL, a marker of axonal degeneration that is increased and correlated with disease progression in other neurodegenerative conditions (Huang, Zhu et al. 2020, Uphaus, Steffen et al. 2021, Chelban, Nikram et al. 2022) and in the eIF2B LOF mouse model, was also significantly elevated in both the plasma and CSF from VWMD patients. Inflammatory markers, such as TIMP-1 and MCP-1, that we identified in the mouse model based on changes relative to wild-type control and dose responsiveness to DNL343 were unchanged in samples from patients with VWMD, highlighting contrasts that may be driven by species-specific differences. Nonetheless, the eIF2B LOF mouse serves as an important tool that models the biological consequences of chronic ISR activation in the CNS and from which biomarkers identified have broad applicability in other neurodegenerative indications. To this point, our DNL343 studies in two in vivo models allowed us to observe commonality in ISR transcript markers despite the distinct modes of activation and CNS tissues (acute activation in the retina after ONC and chronic activation in the eIF2B HOM brain). To our knowledge, our study is the first to perform multi-omics characterization of the CNS-adjacent and clinically accessible CSF in an ISR-dependent model of neurodegeneration. The biofluid-based candidate biomarkers we cross-identified in patients with VWMD – GDF-15, GFAP, and NfL – could serve as potential biomarkers to monitor the extent and consequences of ISR activation and therapeutic modulation in the clinic.
Acknowledgements
We thank the VWMD patients and their families for generously donating samples, and we extend our thanks to Dr. Raphael Schiffman and the Baylor Scott & White Research Institute for granting us permission to utilize these valuable patient samples in our research. Finally, the authors dedicate this work to the memory of our beloved colleague and friend, Patrick C. G. Haddick.
Disclosure
Competing Interests: E.Y, J.H.S, M.H.F, R.C, H.S, R.T, A.I.B, I.B, N.B.B, CL.C, T.E, A.A.E, A.G, C.H, K.R.H, R.M, H.N.N, M.O, Y.R, K.R, E.R, T.S, V.T, J.W.L, L.A.K, are current employees and shareholders of Denali Therapeutics. W.E.D, M.L, B.M, P.C.G.H, A.W.L, A.A.N., J.W, K.S.-L, P.E.S are former employees and shareholders of Denali Therapeutics.
Materials and methods
CSF and Plasma from VWMD patients and healthy controls
CSF and plasma from VWMD patients were obtained under a material transfer agreement with Baylor Scott & White Research Institute (Dallas, TX). Samples were collected 15-25 years prior to analysis. Plasma EDTA from healthy controls obtained from BioIVT, Allcells, and Denali Phase 1 clinical trial: NCT04268784. CSF from healthy controls obtained from Biochemed and Denali repository. Healthy control samples were collected 0-2 years prior to analysis.
Quanterix Simoa Assays in human samples
For CSF NfL measurements, CSF was diluted 100x and analyzed using Quanterix Simoa Neurofilament-Light (NfL) kit (Quanterix, # 103400) according to manufacturer’s instructions on the Quanterix SR-X instrument. For plasma measurements of NfL and GFAP, plasma was diluted 4x and analyzed using Quanterix Simoa Neurology 4-Plex A (Quanterix, # 102153) kit according to manufacturer’s instructions on the Quanterix HD-X instrument. Measurements were interpolated against a calibration curve provided with the Quanterix assay kit produced using on-instrument software. All assays run with technical replicates and results averaged.
Electrochemiluminescence-based detection (ECLIA) for the quantitation of (sTREM2) in human samples
MSD GOLD 96-well small spot streptavidin SECTOR plates (MSD, catalog # L45SA) were washed 3 times with 300 μL/well with wash buffer (1X TBST) using a plate washer. To each well, 1 μg/mL Human TREM2 biotinylated antibody, polyclonal goat IgG (R+D, catalog # BAF1828) diluted in PBS was added and the plate was incubated at RT for 1 hour on an orbital shaker at 700 rpm. Plates were washed 3 times with 300 µl wash buffer and blocked with 150 µl per well of MSD Blocker A (MSD, Catalog # R93AA) for 2 hrs at RT on an orbital shaker at 700 rpm. Plates were washed 3 times with wash buffer and sample or standard were added diluted in 25% MSD Blocker A in TBST. hTREM2-His tagged ECD protein standards were prepared at 4X dilutions starting at 50,000 pg/mL. Plates were incubated overnight (16-24 hours) at 4°C on an orbital shaker at 700 rpm. Plates were washed as above and sulfo-tagged Human TREM2 Antibody, polyclonal goat IgG (R+D, catalog # AF1828) detection antibody diluted 1:5000 in 25% MSD Blocker A in TBST was added to each well. Plates were incubated for 1 hr at Rt on an orbital shaker at 700 rpm. Plates were washed again and 150 μL per well of MSD Read Buffer T (MSD, catalog # R92TC-3) diluted 1:1 in water was added to each well. Plates were read on a 1201 MSD SECTOR 600MM plate reader (Meso Scale Discovery, catalog # IC1AA-0) within 30 minutes of adding buffer and data was captured in Methodical Mind (Meso Scale Discovery, version Fall 2020 (1.0.38)). Pg/ml concentrations for each sample were determined by MSD analysis software Discovery Workbench (Meso Scale Discovery, version LSR_4_0_13) using a 4-parameter logistic model. All assays run with technical replicates and results averaged.
MSD assays for additional biomarkers in human samples
CSF and plasma samples were analyzed according to manufacturer’s protocol using the following MSD kits: R-PLEX Human GDF-15 Antibody Set (MSD, catalog # F21YD-3), R-PLEX Human TIMP-1 Antibody Set (MSD, catalog # F21YO-3), V-PLEX Human MCP-1 kit (MSD, catalog # K151NND-2), and U-PLEX Human IL-18 kit (MSD, catalog # K151VJK-2). For CSF only, samples were analyzed according to manufacturer’s protocol using R-PLEX Human GFAP Antibody Set (MSD, catalog # F211M-3). Plates were read on a 1201 MSD SECTOR 600MM plate reader (Meso Scale Discovery, catalog # IC1AA-0) within 30 minutes of adding buffer and data was captured in Methodical Mind (Meso Scale Discovery, version Fall 2020 (1.0.38)). Pg/ml concentrations for each sample were determined by MSD analysis software Discovery Workbench (Meso Scale Discovery, version LSR_4_0_13) using a 4-parameter logistic model. All assays run with technical replicates and results averaged.
Animal care
All procedures in animals were performed with adherence to ethical regulations and protocols approved by Denali Therapeutics Institutional Animal Care and Use Committee. Mice were housed under a 12-h light/dark cycle (lights on at 7 AM, lights off at 7 PM) with ad libitum access to water and a standard chow (Labdiet, #5LG4) unless otherwise indicated. Whenever possible, animals were group housed of up to 5 sex-matched animals/cage.
DNL343 preparation for oral gavage dosing
DNL343 was prepared as a suspension in a 0.5% methylcellulose solution. Briefly, DNL343 was placed in individual glass vials to which purified water (half of the final volume), was added. The mixture was gently mixed using a probe sonicator at 40% amplitude for 10 times, each lasting for 20 seconds on pulse sonication. The result was a suspension with dispersed particles that was uniform throughout the product. Equal volume of a 1% methylcellulose (2X final target concentration, in half of final target volume) solution in purified water was added to the above suspension and vortexed until uniform. Suspension was visually inspected to be uniformly distributed. Dosing solutions were prepared on the first dosing day then weekly thereafter and were maintained at 4°C, on a laboratory rotator, until use. DNL343 suspension was remixed on dosing instances and administered via oral gavage at a volume of 10 ml/kg body weight.
DNL343 preparation for in diet dosing
DNL343 was blended in bacon flavored grain based rodent diet (PicoLab Mouse Diet 20, catalog #5058, gross energy 4.63 kcal/g) and pelleted by Bio-Serv. For every target dose in mg of DNL343/kg body weight per day, DNL343 was formulated based on an estimated daily food consumption of 0.1 kg of chow per kg body weight per day (e.g. 30 mg/kg chow for 3 mg/kg body weight). Bacon flavored base diet was used as placebo control. Coloring was added to differentiate between dosages and to blind experimenters to the treatments.
DNL343 in diet dosing
Animals were group housed whenever possible. Control or medicated food was weighed every week and refreshed every 4 weeks at minimum. Food intake was estimated by taking the difference in hopper weight, normalized for total body weight in each cage and presented per diem. DNL343 intake was estimated by adjusting the food intake for DNL343 concentration in the food. DNL343 exposure in the plasma, collected via submandibular bleed as an in-life procedure or via cardiac puncture at terminal timepoints, and brain was measured using LC/MS/MS.
Tissue collection
For all tissue collection, animals were humanely anesthetized with 2.5% tribromoethanol. Whole blood was collected via cardiac puncture into EDTA coated tubes and spun down at 12,700 rpm for 7 minutes at 4 °C before collecting the top plasma layer for analysis. CSF, if collected, was then extracted via cisterna magna puncture, spun down at 12,700 rpm for 7 minutes at 4 °C, following which the supernatant was collected and stored in a new tube for analysis. Animals were transcardially perfused with ice-cold PBS. Tissues were then collected, weighed, frozen on dry ice and stored at 80 °C for subsequent analysis.
Optic Nerve Crush
Optic nerve crush (ONC) was performed as previously described by (Watkins, Wang et al. 2013) on 12-week-old wild-type male C57Bl/6J mice obtained from the Jackson Laboratory (USA). Animals were deeply anesthetized with inhaled isoflourane. The left eye of each animal was subjected to optic nerve injury via an intraorbital approach. An incision was made on the superior conjunctiva of the left eye, and the optic nerve was exposed. The crush injury was inflicted for 10 seconds using a 45° angled fine tip forceps 1-3 mm from the eyeball. Post-operatively, a drop of 0.5% proparacaine hydrochloride ophthalmic solution was applied to the affected eye as an analgesic measure. A small amount of ophthalmic ointment was applied to the non-procedural eye prior to surgery to prevent drying. Unoperated right eyes (contralateral to the crushed site) were used as controls. Starting from 3 hours after the ONC procedure, mice were administered vehicle or DNL343 at doses of 0.75, 3, or 12 mg/kg once daily via oral gavage. Animals were humanely euthanized on day 2 after ONC (2 hours after the last dose) or on day 14 (20 hours after the last dose).
Generation of the eIF2B LOF mouse
The Eif2b5 R191H knock-in mouse model was engineered and maintained on a C57BL/6J background by Ozgene (Australia) using the goGermlineTM technology (Koentgen, Lin et al. 2016). Briefly, a targeting vector was designed against the mouse Eif2b5 gene containing a CGC to CAC codon substitution to replace arginine for histadine at amino acid position 191 in exon 4. An FRT-flanked neomycin selection cassette was targeted between exon 5 and 6 and Flp-mediated recombination was used to excise this cassette. The colony was maintained by heterozygous breeding to obtain littermate wild-type and homozygous knock-in animals. The mouse genotypes were confirmed by PCR.
DNL343 preventative dosing in the eIF2B LOF model
10-17-week-old eIF2B HOM and their wild-type littermates were assigned to receive food containing DNL343 at concentrations of 30-100 mg/kg or base chow. Groups were balanced for differences in body weight, age and sex within each genotype. Food weight and body weight were assessed weekly. Plasma was collected at baseline and every 2 weeks starting at 2 hours after the onset of the light period. Motor function was assessed by a balance beam test after 12 weeks of treatment. Animals were humanely euthanized between 12.9-13.3 weeks of treatment. Mice from all groups are represented on each consecutive necropsy day.
DNL343 therapeutic dosing in the eIF2B LOF model
19-26-week-old eIF2B HOM and their wild-type littermates were assigned to receive food containing DNL343 at a concentration of 100 mg/kg or base chow, accounting for differences in body weight, age, sex and plasma NfL level within each genotype. The body weight was assessed at baseline and after 19 and 28 days of treatment. Motor function was assessed by a balance beam test after 27 days of treatment. Animals were humanely euthanized after 33 days of treatment.
Another cohort of eIF2B HOM and wild-type littermates were treated with DNL343-formulated diet (100 mg/kg chow) or base diet from 24-33 weeks of age for up to 20 weeks. Body weight was assessed at baseline and weekly after. Plasma was collected before and every 4 weeks after study initiation. Animals meeting any one of the following humane endpoints were euthanized: body weight loss of ≥10%, hindlimb paralysis, or inability to right itself within 20 seconds.
Balance Beam Test
To assess balance and motor coordination, animals were trained to walk along a 98.5 cm long x 13 mm diameter wooden beam, elevated at 40 cm above the bench surface lined with a soft foam mattress (104 x 74 x 10 cm). A length of 80 cm was marked on the beam as the distance the animals were required to cross. A spotlight was placed at the starting end to serve as an aversive stimulus. A dark enclosure (black matte acrylic box, 20 x 15 x 20 cm) with bedding material and carton tube was placed at the opposite end to serve as an escape box with a more agreeable condition. A video camera was set in front of the starting end to record foot slips as the animal progressed across the beam.
Animals underwent 3 training runs one day prior to the testing. Each mouse was first placed in the escape box for about 1 minute, then placed at an increasing distance away from the escape box over 3 trials. If an animal paused on the beam, or tried to turn and advance the wrong way, it was gently touched on the hindquarters and encouraged to keep moving toward the escape box. Animals were habituated to the experimental room for at least one hour prior to testing. To begin an experiment, each subject was placed on the starting end of the beam and allowed a cutoff time of 30 seconds (s) to cross. The elapsed time was only recorded while the subject actively moved towards the finish line. If a fall occurred, the subject was restarted at the beginning of the beam. Each subject was given three attempts to complete the balance beam. If a subject failed all three attempts, it was assigned a time of 30 s and a value of 3 falls. The number of foot slips was quantified from the video recording only if the animal completed the task. The balance beam was cleaned with a 70% solution of isopropanol and dried between each subject. The escape box was cleaned with isopropanol and dried, and the bedding and carton tube replaced between animals of different cages. The experiment was video recorded. Time to traverse the beam and number of falls were recorded live by an experimenter who was blinded to the genotypes of the animals. Foot slip scoring was done post-hoc by another experimenter, who was blinded to both genotypes and treatment, using the video recordings.
DNL343 pharmacokinetics
Plasma and brain concentrations of DNL343 were measured using LC-MS/MS by Quintara Discovery. Brain samples were homogenized in 3 volumes of ice-cold water, then further diluted 2-fold with blank mouse plasma. An aliquot of 20 μL of plasma sample or plasma diluted brain homogenate was extracted with 100 μL of acetonitrile containing internal standard (warfarin). The mixture was vortexed on a shaker for 15 minutes and subsequently centrifuged at 4000 rpm for 15 minutes. An aliquot of 70 μL of the supernatant was mixed with 70 μL of 35% acetonitrile in water with 0.1% formic acid for injection to the LC-MS/MS. Calibration standards and quality control samples were prepared by dilutions of the 2 mg/mL DNL343 stock solution with 70% acetonitrile added to blank mouse plasma. These standards and QC samples were extracted alongside unknown samples in each bioanalytical batch. The final extracts were analyzed by reversed-phase liquid chromatography and negative electrospray ionizations (LC-MS/MS) with multiple reaction-monitoring (MRM) of the test article and the internal standard. The standard curve was fitted by linear regression to quantify DNL343 in the matrix using Analyst 1.6.3 software (AB Sciex). Total DNL343 concentrations were adjusted for brain or plasma protein binding (fraction unbound, fu) that were determined in vitro via an ultracentrifugation method and expressed as unbound (free DNL343) exposures.
qPCR Gene Expression Analysis
For analysis of gene expression after ONC, retinas from the left and right eyes were collected into RNAprotect (Qiagen, catalog # 76104) and stored at room temperature until further processing. RNA from the retina was isolated using the RNeasy Plus Micro kit (Qiagen, catalog # 74034). RNA from the brain using the RNeasy Plus Mini Kit (Qiagen, catalog # 74134). RNA was reverse transcribed into cDNA using the Fluidigm Reverse Transcriptase Master Mix (Fluidigm, catalog # 100-6298). Specific target amplification of cDNA was done per manufactures recommendations as the initial step for the real time qPCR on the Biomark HD system (Fluidigm, catalog # BMKHD-BMKHD). Briefly, 20X TaqMan assays were pooled and diluted with DNA Suspension Buffer (Teknova, catalog # T0221) to a final concentration of 0.1X of each assay. PCR reactions were carried out for each cDNA sample with the Taqman assay pooled in 5 μl volumes, each containing 1.2 μL of the pooled assay mix, 1 μL PreAmp Master Mix (Fluidigm, # 100-5580), 1.5 μL of H2O, and 1.25 μL of cDNA. The preamplification PCR was performed at one cycle of 95 °C for 2 minutes, followed by 14 cycles of 95 °C for 15 seconds and 60 °C for 4 minutes, and then 4 °C. Specific target amplification products from the PCR reactions were diluted 5x with DNA Suspension Buffer (Teknova, catalog # T0221). Gene expression analysis was carried out using the 96.96 dynamic arrays IFC (Fluidigm, catalog # BMK-M-96.96) on the Biomark HD system (Fluidigm, catalog # BMKHD-BMKHD). 10x assay mixture and sample pre-mix were prepared, with each assay being prepared in triplicates. Each 10x assay mix contained 2.5 μL of 20x TaqMan gene expression assay (Thermofisher) and 2.5 μL of 2X Assay Loading Reagent (Fluidigm, catalog # 100-7611). All qPCR TaqMan probes (FAM) were ordered from Thermo Fisher Scientific (see Key Resources Table). Sample pre-mix was made by combining 2.5 μL TaqMan Fast Advance PCR Master Mix (Applied Biosystems, catalog # 4444557), 0.25 μL of 20X GE Sample Loading Reagent (Fluidigm, # PN 100-7610) and 2.5 μL pre-amplified cDNA. IFC controller (Fluidigm, catalog # 68000112 I1) were used to prime the 96.96 dynamic arrays IFC Chip (Fluidigm, catalog # BMK-M-96.96) with the 96.96 control line fluid (Fluidigm, catalog # 89000021). 5 μL of each assay and sample mix was then transferred into the appropriate inlets of the primed chip and loaded with the IFC controller. The PCR was performed at 70 °C for 40 minutes, 60 °C for 30 seconds, 98 °C for 1 minute, followed by 35 cycles of 97 °C for 5 seconds, 60 °C for 20 seconds. The data was analyzed with Fluidigm Genetic Analysis software. For relative quantification, the amount of target gene expression was normalized to the geometric means of Actb, Gapdh, and Ubb expression, relative to samples from vehicle-dosed controls and was calculated using the 2−Ct method. The data were analyzed with Real-Time PCR Analysis Software (Fluidigm).
Assessment of RGC survival
For immunofluorescence analysis of RGC survival and axonal degeneration, the left (ipsilateral to crush) and right eyes were collected 14 days after the ONC procedure and immediately fixed in 4% paraformaldehyde on ice for 1 hour. Retinas were then dissected from the eyes for wholemount staining. The degree of RGC loss and axonal degeneration at 14 days after ONC was assessed from whole-mount retinas. Floating whole mouse retinas were blocked in 5% normal goat serum in 0.5% Triton X-100 in PBS at 4°C for 2 hours. Primary antibodies were incubated over two nights at 4°C, followed by rinsing and incubation with secondary antibodies in PBS. Immunohistochemistry was performed using the following antibodies: rabbit anti γ-synuclein (1:200, Abcam, ab55424) and mouse anti TuJ1 (1:40, BioLegend, 801203). Retinas were mounted on slides after being cut with four incisions along the radial axes. Retinas were imaged using a spinning disk confocal microscope (Cell Observer CSU-X1, Carl Zeiss MicroSystem). Images were processed for brightness and contrast in Adobe. RGCs, identified as TuJ1 and γ-synuclein double-immunopositive cells, were quantified manually. Retinal axon degeneration was scored based on density of axon bundles immunolabelled with TUJ-1, using a graded scale from 0–5, where 0 corresponds to no degeneration, and five to complete degeneration.
Detection of plasma NfL
Plasma NfL concentrations were measured using Simoa NF-Light® Advantage (SR-X version, Quanterix Catalog # 103400) or the Simoa® Neurology 4-plex A Advantage (HD-X version, Quanterix Catalog # 102153) bead-based digital ELISA kit and read on the Quanterix SR-X or HD-X instrument. All experiments were performed according to kit and instrument instructions as provided by Quanterix. All additional equipment and consumables were procured through Quanterix. Plasma samples were diluted 20x with Sample Diluent (Quanterix Catalog # 103399) before being added to Simoa 96-well microplates (Quanterix Catalog # 101457) alongside kit calibrators and controls. Kit-specific instructions were followed and sample NfL levels were measured using the NF Light analysis protocol on the Quanterix SR-X or Neurology 4-Plex A analysis protocol on the Quanterix HD-X instrument and interpolated against a calibration curve provided with the Quanterix assay kit. Mouse NfL data generated from the two instruments have been established to be comparable (data not shown).
Detection of plasma GFAP
Plasma GFAP was measured using the Simoa Neurology 4-plex A bead-based digital ELISA kit and read on the Quanterix HD-X instrument as described above.
Preparation of brain homogenate for protein analyses
Brains were homogenized in Radio-Immunoprecipitation Assay Buffer (Teknova) made with cOmplete Protease Inhibitor (Roche,Catalog #04693132001) and PhosStop (Roche, Catalog # 04906837001) using the Qiagen TissueLyzer II (Cat No./ID: 85300) for 2 rounds of 3 minutes at 30 Hz. Homogenate was incubated on ice for 20 minutes and spun at 21,100 g for 30 minutes at 4 °C. Subsequent lysate was transferred to a clean 96-well deep plate. Protein concentration of the supernatant was measured with the bicinchoninic acid assay (Pierce™ BCA Protein Assay Kit).
Detection of GDF-15, TIMP-1, and MCP-1
ELISA kits were used to determine the levels of GDF15 (mouse/rat GDF15 Quantikine ELISA Kit, R&D Systems, catalog # MGD150), TIMP-1 (mouse TIMP-1 Quantikine ELISA Kit, R&D Systems, catalog # MTM100) and MCP-1 (Mouse CCL2/JE/MCP-1 Quantikine ELISA Kit, R&D Systems, catalog # MJE00B) in the brain, plasma, or CSF samples.
RNA-Seq library preparation
RNA from bulk mouse brain tissue was extracted using the RNeasy Plus Mini Kit (Qiagen) and resuspended in nuclease-free water. Libraries were generated using the QuantSeq 3’ mRNA-seq Library Prep Kit FWD for Illumina (Lexogen A01173) with the UMI second strand synthesis module to identify and remove PCR duplicates, following the protocol defined by the manufacturer. Briefly, total RNA was used as input for oligo dT priming during reverse transcription, followed by RNA removal. Unique Molecular Identifiers were introduced during second strand synthesis and cDNA was purified using magnetic beads followed by 14 cycles of PCR with dual indexes and PCR purification. Library quantity and quality were assessed with Qubit 1X dsDNA HS Assay Kits (Invitrogen Q33231) and Bioanalyzer High Sense DNA chip (Agilent 5067-4626). Libraries were pooled in equimolar ratios and sequencing reads were generated on an Illumina NovaSeq 6000 instrument (100 bp single end) by SeqMatic (Fremont, CA, USA)
RNA-Seq data preprocessing
Sequencing adapters were trimmed from the raw reads with skewer (version 0.2.2) (Jiang, Lei et al. 2014). Reads were aligned to the mouse genome version GRCm38_p6. A STAR index (version 2.7.1a) (Dobin, Davis et al. 2013) and built with the --sjdbOverhang=50 argument. Splice junctions from Gencode gene models (release M17) were provided via the --sjdbGTFfile argument. STAR alignments were generated with the following parameters: --outFilterType BySJout, --quantMode TranscriptomeSAM, -- outFilterIntronMotifs RemoveNoncanonicalUnannotated, --outSAMstrandField intronMotif, -- outSAMattributes NH HI AS nM MD XS and --outSAMunmapped Within. Alignments were obtained with the following parameters: --readFilesCommand zcat --outFilterType BySJout --outFilterMultimapNmax 20 --alignSJoverhangMin 8 --alignSJDBoverhangMin 1 --outFilterMismatchNmax 999 -- outFilterMismatchNoverLmax 0.6 --alignIntronMin 20 --alignIntronMax 1000000 --alignMatesGapMax 1000000 --quantMode GeneCounts --outSAMunmapped Within --outSAMattributes NH HI AS nM MD XS --outSAMstrandField intronMotif --outSAMtype BAM SortedByCoordinate --outBAMcompression 6. Gene level counts were obtained using featureCounts from the subread package (version 1.6.2) (Liao, Smyth et al. 2014). Gene symbols and biotype information were extracted from the Gencode GTF file.
RNA-Seq differential Expression analysis
Following alignment and expression quantitation, differential expression analysis was performed using the limma/voom framework (Law, Chen et al. 2014). Only samples with at least one million total counts were included in the analysis. To account for remaining differences in library sequence depths, size factors were calculated with the TMM method (Robinson and Oshlack 2010). Genes below the lower limit of quantitation were excluded using the filterByExpr function from the edgeR R package (version 3.42.4) (Robinson, McCarthy et al. 2010). A linear model with the following independent variables was fit for each protein-coding gene with the voomWithQualityWeights function: genotype, sex and age. The comparison of interest was extracted with the eBayes function from the limma R package (version 3.56.2), applying using the robust empirical Bayes procedure of (Phipson, Lee et al. 2016). Genes with FDR <5% were considered significantly differentially expressed.
Gene set enrichment analysis
To compare the expression changes caused by eIF2B loss of function in our study with previous observations, we retrieved the differential expression results published by Wong et al (Wong, LeBon et al. 2019) and performed gene set enrichment analysis (GSEA) with the geneSetTest algorithm from the limma R package. The most significantly upregulated genes reported by Wong et al (e.g. top 100, 200, 300, 400 or 500 genes ordered by Bayes factor) were highly enriched among genes with large t-statistics in our dataset (p-value <10-20). Similar results were obtained with other GSEA algorithms, including camera and fgsea.
Proteomic analysis of the eIF2B LOF brains and CSF
Proteomics analysis was conducted at BGI Americas (San Jose, CA). For mouse CSF, samples were processed via an in-solution digest. Briefly, 4 µl CSF per sample was reduced with DTT and alkylated with iodoacetamide (IAM). 100mM HEPEs pH 8.5 was added and the samples were digested overnight with Tryp/LysC. The digestion was quenched with 10% TFA, desalted using C18 PhyTips (PhyNexus) and dried by SpeedVac and reconstituted in 100mM HEPES, pH 8.5. Samples were assigned respective TMT channels in one of four 8-plexes with the final channel being a pool of all the samples to normalize between TMT plexes. Samples were labelled with respective 8-plex TMT channels at room temperature for 1 hour. Approximately 1% of sample from each channel were mixed, dried down, stage-tipped and injected into the mass spec for label check then the reaction was quenched with 5% hydroxylamine, mixed in equal amounts, dried down and cleaned up using C18 PhyTips (PhyNexus). For mouse CSF, due to the low sample amount no fractionation was performed prior to injection on the MS.
Tissue samples were lysed in 5% SDS in triethylammonium bicarbonate, pH 7.1 and assayed for concentrations. 6ug of each sample was processed using the STrap MS sample prep device according to the manufacturer’s protocol (Protifi). More specifically: samples were reduced with dithiothreitol (DTT) and alkylated with iodoacetamide (IAM); the IAM reaction was then quenched with DTT; the resulting samples were digested in the STrap device with Trypsin/Lys-C overnight. Digested samples were eluted from the STrap according to the manufacturer’s protocol. An aliquot of 1 µg was taken from each eluted sample; and the aliquots were pooled to form a composite for TMT bridging. 4 aliquots of 5ug were taken out as 4 TMT bridges, with each bridge being used for each TMT batch. All samples were dried by SpeedVac. The samples were reconstituted with 50mM TEAB pH 8.5 and incubated with their assigned TMT channels for 1 hour at room temperature. For each of the four TMT batches: the same amount of each TMT-labelled sample was aliquoted; and the aliquots were pooled and mixed with 1% formic acid. The 4 resulting mixtures were loaded onto the nano LC-MS/MS system for Label Check. After the Label Check was passed, all samples were dried by SpeedVac and reconstituted with 2% formic acid. The reconstituted samples of each batch were combined. The resulting three mixtures were further desalted using EVOLUTE® EXPRESS ABN according to the manufacturer’s protocol (Biotage). The eluted samples were dried by SpeedVac, reconstituted with high-pH reversed-phase buffer A, and loaded onto the offline HPLC for fractionation. Either 8 or 12 fractions were obtained from each sample batch.
All samples were reconstituted with mobile phase A and loaded onto the nano LC-MS/MS system. The same amount of each reconstituted sample was injected for analysis with TMT method on a QE HF-X or Orbitrap Eclipse MS. Peptide search was performed with Sequest HT and TMT quantification was performed with the reporter ions node in Proteome Discoverer 2.5 (PD, Thermo Fisher). Data was searched against reviewed mouse sequences in Uniprot, full trypsin digest, and 20 ppm precursor and 0.5 Da fragment tolerance. N-terminal and Lysine TMT6plex and C carbamidomethyl were set as static modifications, oxidized M and N-terminal acetylation were set as dynamic modifications.
Metabolomic analysis of the eIF2B LOF brains
Sample preparation: 20 mg of snap frozen brain tissues were bead homogenized using 5 mm stainless steel bead (QIAGEN Cat#69989) in 0.4 ml of methanol:water (80:20 v/v; LC-MS grade) solution containing 64 stable internal standards. These samples were homogenized with Tissuelyser for 30 sec at 25 Hz in 4 °C. Crude homogenates were centrifuged at 21,000 x g for 20 min at 4 °C. Resulting supernatants were collected and transferred to 96 glass well plates (Analytical Sales, PN 27350). Two µl of CSF samples were diluted with 8 µl of 18 mW water and centrifuged at 21,000 g for 10 min at 4 °C. To these samples, 100 µl of MS-grade methanol containing 64 stable isotope internal standards was added and vortexed for 5 min at 4 °C. Samples were incubated at -20 °C for 1 hr and subsequently centrifuged at 21,000 x g for 20 min at 4 °C. Resulting supernatants were collected and transferred to 96 glass well plates (Analytical Sales, PN 27350).
Polar metabolomics analysis
Metabolomics analyses were performed using the UHPLC UHPLC ExionLC system coupled to Sciex QTRAP 6500+ electrospray mass spectrometer in positive and negative ionization modes. For positive ionization mode, 5 µL of sample was injected on a BEH amide 1.7 µm, 2.1×150 mm column (Waters Corporation, Milford, Massachusetts, USA) using a flow rate of 0.40 mL/min at 40°C. Mobile phase A consisted of water with 10 mM ammonium formate + 0.1% formic acid. Mobile phase B consisted of acetonitrile with 0.1% formic acid. The gradient was programmed as follows: 0.0–1.0 min at 95% B; 1.0–7.0 min to 50% B; 7.0–7.1 min to 95% B; and 7.1–10.0 min at 95% B. For negative ionization mode, Samples N2 dried and reconstituted in 0.1% formic acid. For each analysis, 5 µL of sample was injected on an Imtakt Intrada Organic Acid 3 µm, 2 x 150 mm (Imtakt USA, Portland, OR USA); using a flow rate of 0.2 mL/min at 60°C. For negative ionization mode, Mobile phase A consisted of acetonitrile/water/formic acid = 10/90/0.1%. Mobile phase B consisted of acetonitrile/ 100mM ammonium formate= 10/90%. The gradient was programmed as follows: 0.0–1.0 min at 0% B; 1.0–7.0 min to 100% B; 7.1 at 0% B; and 7.1-10 min at 0% B. Mass spectrometry setting for the positive mode was as follows; curtain gas at 30 psi; collision gas was set at medium, ion spray voltage at 5500 V; temperature at 600°C; ion source Gas 1 at 50 psi; ion source Gas 2 at 60 psi; entrance potential at 10 V; and collision cell exit potential at 12.5 V. For the negative mode, settings were similar to positive mode with the following modifications: ion spray voltage at -4500 V, entrance potential at -10 V and collision cell exit potential at - 15 V. Peaks were identified and integrated using Multiquant 3.02 (Sciex) based on known retention time and mass transitions and normalized to prespecified stable isotope internal standards. Area ratios were exported as all columns report and used for subsequent data analysis.
Lipidomics analysis
Methanol extracted samples from above were analyzed in electrospray positive and negative ionization modes. For positive ionization mode, Mobile phase A consisted of 60:40 acetonitrile/water (v/v) with 10 mM ammonium formate + 0.1% formic acid; mobile phase B consisted of 90:10 isopropyl alcohol/acetonitrile (v/v) with 10 mM ammonium formate + 0.1% formic acid. For negative ionization mode, Mobile phase composition was same as in positive mode with the exception that 10 mM ammonium acetate and 0.1% acetic acid were used as fortificants. Mass spectrometer settings for positive ionization mode were as follows: curtain gas at 40 psi; collision gas was set at medium; ion spray voltage at 5500 V; temperature at 250°C; ion source Gas 1 at 55 psi; ion source Gas 2 at 60 psi; entrance potential at 10 V; and collision cell exit potential at 12.5 V. Source settings for negative ionization mode were as follows: curtain gas at 30 psi; collision gas was set at medium; ion spray voltage at -4500 V; temperature at 600°C; ion source Gas 1 at 55 psi; ion source Gas 2 at 60 psi; entrance potential at -10 V and collision cell exit potential at -15.0 V. Lipidomics analysis in positive and negative ionization modes were initiated with 5 µl of sample injection using a BEH C18 1.7 μm, 2.1×100 mm column (Waters) as stationary phase with 0.25 mL/min flowrate and column temperature set at 55°C. The gradient was programmed as follows: 0.0-8.0 min from 45% B to 99% B, 8.0-9.0 min at 99% B, 9.0-9.1 min to 45% B, and 9.1-10.0 min at 45% B.
Data pre-processing and analysis for proteomics and metabolomics
Proteomics data pre-processing
TMT data preprocessing was performed using the MSstatsTMT package (2.4.1). Data were median centered and log2 transformed. Features with all missing measurement, shared peptides, or proteins with single feature, features with less than 3 measurements within each run were removed from analysis. All protein features with ≤ 1 feature missing were included in the analysis. Nine proteins with one missing value were imputed using kNN function in VIM package (6.2.2).
Metabolomics and lipidomics data preprocessing
Metabolite/lipid features detected in at least 70% of samples were retained for further analysis. Partially missing values in 44 metabolite/lipid features were imputed using the kNN function in the VIM package. Unwanted variations in data not stemming from relevant biological factors (experimental groups) of interest were detected and removed using the RUV4 function in the ruv (0.9.7.1) package. Top 20th percentile of most abundant Metabolite/lipid features with lowest 10th percentile CV from wild-type control mice were selected as negative control features. RUV adjusted data were used for downstream analysis described below.
Differential expression analysis for proteomics and metabolomics
Unsupervised principal component analysis was performed the FactoMineR (2.8) package. Log2 transformed data were scaled prior to analysis. Univariate analysis of differentially expressed proteins or metabolites were analyzed using limma (3.54.2). Sample specific quality weights were calculated with arrayWeights default method setting. For linear model analysis, a no-intercept model containing the experimental groups of interest (genotype or combination of genotype, treatment, and dose) and covariates (batch) was created. Following linear modeling with lmFit function, contrasts between groups were created using the contrast.fit function to assess group-wise differences. A robust Empirical Bayes moderation was performed with robust argument set to TRUE and minimum logFC set to 1.1. False discovery rate was assessed using the Benjamini-Hochberg procedure. Box plots, volcano plots and heatmaps were generated using the ggplot2 (3.4.2). EnhancedVolcano (1.14), and pheatmap (1.0.12) R packages. Feature overlap and venn diagram analysis were performed using the VennDiagram (1.7.3) package. GSEA was performed using the clusterProfiler (4.10) R package. Protein ranks were created using moderated LogFC with minimum and maximum gene set size set to 3 and 800, respectively. False discovery adjustment when performed used the Benjamini-Yekutieli procedure. All analyses were conducted using R (4.2.1)
Statistical analysis
Data are reported as means ± SEM or as indicated in figures. Statistical analysis of data was performed in GraphPad Prism version 8 or later. Analysis of data from animal studies was performed using t test or one-way analysis of variance (ANOVA) with multiple comparison, or two-way ANOVA followed by multiple comparison test for data obtained from repeated measures of the same subjects. Analysis of data from human samples was assessed on log2 fold change data using Welch’s t test.
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