Altered Mitochondrial Function and Accelerated Aging Phenotype in Neural Stem Cells Derived from Dnm1l Knockout Embryonic Stem Cells

Mitochondria are crucial for cellular energy metabolism and are involved in signaling, aging, and cell death. They undergo dynamic changes through fusion and fission to adapt to different cellular states. In this study, we investigated the effect of knocking out the dynamin 1-like protein (Dnm1l) gene, a key regulator of mitochondrial fission, in neural stem cells (NSCs) differentiated from Dnm1l knockout embryonic stem cells (Dnm1l−/− ESCs). Dnm1l−/− ESC-derived NSCs (Dnm1l−/− NSCs) exhibited similar morphology and NSC marker expression (Sox2, Nestin, and Pax6) to brain-derived NSCs, but lower Nestin and Pax6 expression than both wild-type ESC-derived NSCs (WT-NSCs) and brain-derived NSCs. In addition, compared with WT-NSCs, Dnm1l−/− NSCs exhibited distinct mitochondrial morphology and function, contained more elongated mitochondria, showed reduced mitochondrial respiratory capacity, and showed a metabolic shift toward glycolysis for ATP production. Notably, Dnm1l−/− NSCs exhibited impaired self-renewal ability and accelerated cellular aging during prolonged culture, resulting in decreased proliferation and cell death. Furthermore, Dnm1l−/− NSCs showed elevated levels of inflammation and cell stress markers, suggesting a connection between Dnm1l deficiency and premature aging in NSCs. Therefore, the compromised self-renewal ability and accelerated cellular aging of Dnm1l−/− NSCs may be attributed to mitochondrial fission defects.


Introduction
Mitochondria are essential organelles at the core of cellular energy metabolism and play vital roles in signaling pathways, aging, and cell death [1,2].They are highly plastic and dynamic, allowing them to rapidly adapt to diverse cellular environments and meet the biological demands of different cell types [3][4][5][6][7][8].For example, pluripotent stem cells, such as embryonic stem cells (ESCs), typically contain globular mitochondria, whereas differentiated cells, including somatic stem cells, contain elongated mitochondria [3][4][5][6][7].Furthermore, continuous structural remodeling, known as mitochondrial dynamics, within the mitochondrial network occurs through fusion and fission, which are essential for proper functioning in different cellular states [9].Moreover, maintaining a balanced transition between mitochondrial fusion and fission is vital for ensuring cell adaptability and sufficient energy availability [8].Numerous proteins are involved in mitochondrial fission and fusion.Among these regulatory proteins, dynamin 1-like protein (Dnm1l, known as Drp1 in humans) is directly involved in fission; it is recruited to the outer mitochondrial membrane and forms a ring-like structure that contracts the mitochondrial membrane [10,11].Previous studies using knockout mice have highlighted the importance of Dnm1l for the proper functioning of organs such as the brain and heart [12][13][14].In a recent study, we further demonstrated that Dnm1l knockout resulted in mitochondrial morphology and energy metabolism changes in mouse ESCs without the loss of pluripotency or differentiation potential in the three germ layers [15].The fate of mitochondria is determined by the location of fission.When fission occurs at the periphery of mitochondria, it is degraded via mitophagy [16].Therefore, normal fission of mitochondria by the Dnm1l protein is critical for maintaining mitochondrial function.
In neurogenesis, changes in mitochondrial morphology and function are critical regulatory factors that affect cell fate decisions at the beginning of neural development [17,18].The initiation of neural stem cell (NSC) differentiation entails a shift in the major energy metabolism from glycolysis to oxidative phosphorylation (OXPHOS) [19][20][21].During neuronal differentiation from NSCs, mitochondria undergo dynamic morphological changes.The elongated mitochondria in NSCs become fragmented in the neural progenitor cell (NPC) state and re-elongate once the cells differentiate into neurons [22,23].Considering the role of mitochondria in neural development, it is reasonable to assume that defects in mitochondrial dynamic-related phenotypes could potentially lead to impaired neurogenesis [22,24].Although many studies have shown a correlation between mitochondrial dysfunction and neurological disorders [25,26], the mechanisms that characterize mitochondrial dysfunction in NSCs are poorly understood.
Previously, we demonstrated, through in vitro differentiation and teratoma formation, that Dnm1l −/− ESCs retain their ability to differentiate into the three germ layers [15].However, we did not examine whether Dnm1l −/− ESCs could differentiate into specific cell types and maintain the functional attributes of the resulting cells.In the present study, we assessed the differentiation potential of Dnm1l −/− ESCs into homogenous NSC lines and investigated the characteristics of the Dnm1l −/− ESC-derived NSCs (Dnm1l −/− NSCs).

Differentiation of Dnm1l −/− ESCs to NSCs In Vitro
In a previous study, we generated Dnm1l −/− ESCs to investigate the effects of Dnm1l deficiency on self-renewal and the dynamics of mitochondrial energy metabolism in ESCs [15].Here, we explored whether somatic stem cells differentiated from Dnm1l −/− ESCs displayed cell type-specific characteristics.For this purpose, we differentiated Dnm1l −/− ESCs into NSCs (Figure 1A) because NSCs can be efficiently derived from ESCs, and the resulting ESC-derived NSCs display homogeneous morphology and marker expression, along with elongated self-renewal ability [27,28].Dnm1l −/− ESCs maintained an undifferentiated state and formed dome-like colonies when cultured in a medium containing fetal bovine serum (FBS) on feeder-layered dishes (Figure 1B).During the onset of differentiation, Dnm1l −/− ESCs underwent a change in colony morphology from dome-shaped to plate-shaped by day 2 of differentiation (Figure 1B).After suspension culture for 5-7 days in the presence of basic fibroblast growth factor (bFGF) and epidermal growth factor (EGF), Dnm1l −/− ESCs formed aggregates (Figure 1D).Aggregates resembling rosette-like structures were selected and transferred to gelatin-coated dishes in NSC expansion medium supplemented with bFGF and EGF.Neural lineage outgrowth spread from the seeded aggregates, exhibiting a branched morphology characteristic of NSCs (Figure 1E).Outgrowths were collected and subsequently passaged every 3-4 days to establish a homogenous NSC population (Figure 1F).Notably, the established Dnm1l −/− NSCs were morphologically similar to brain-derived NSCs (Figure 1F,G).

Characterization of Dnm1l −/− NSCs
We investigated whether the established Dnm1l −/− NSCs possessed characteristic features of brain-derived NSCs.In this study, NSCs from passage 8 were used, and NSC marker expression was assessed using both immunocytochemistry and real-time quantitative reverse transcription PCR (RT-qPCR) and their tripotent differentiation ability.Immunocytochemistry revealed the expression of the NSC markers Nestin and Sox2 in Dnm1l −/− NSCs as well as wild-type ESC-derived NSCs (WT-NSCs) (Figure 2A).However, RT-qPCR showed that the expression levels of NSC markers (Sox2, Nestin, and Pax6) in Dnm1l −/− NSCs were lower than those in WT-NSCs, which exhibited levels similar to brain-derived NSCs (Figure 2B).To evaluate the tripotent differentiation potential, Dnm1l −/− NSCs were differentiated by culturing for 10 days in the absence of bFGF and EGF in culture medium.The presence of astrocytes (GFAP + cells) and oligodendrocytes

Characterization of Dnm1l −/− NSCs
We investigated whether the established Dnm1l −/− NSCs possessed characteristic features of brain-derived NSCs.In this study, NSCs from passage 8 were used, and NSC marker expression was assessed using both immunocytochemistry and real-time quantitative reverse transcription PCR (RT-qPCR) and their tripotent differentiation ability.Immunocytochemistry revealed the expression of the NSC markers Nestin and Sox2 in Dnm1l −/− NSCs as well as wild-type ESC-derived NSCs (WT-NSCs) (Figure 2A).However, RT-qPCR showed that the expression levels of NSC markers (Sox2, Nestin, and Pax6) in Dnm1l −/− NSCs were lower than those in WT-NSCs, which exhibited levels similar to brainderived NSCs (Figure 2B).To evaluate the tripotent differentiation potential, Dnm1l −/− NSCs were differentiated by culturing for 10 days in the absence of bFGF and EGF in culture medium.The presence of astrocytes (GFAP + cells) and oligodendrocytes (O1 + cells) was observed in the differentiated cells (Figure 2C).However, early neuronal Tuj1 + cells were not detected even after 10 days of inducement (Figure 2C).(O1 + cells) was observed in the differentiated cells (Figure 2C).However, early neuronal Tuj1 + cells were not detected even after 10 days of inducement (Figure 2C).To verify whether undifferentiated Dnm1l −/− NSCs constituted a homogenous population devoid of differentiated neural subtypes, we stained them for Tuj1, GFAP, and O1 neural subtype markers.Interestingly, Tuj1-expressing cells were detected in the early stages of NSCs at passage 8 (Figure 2D,E), whereas GFAP-and O1-expressing cells were not detected.These results suggest that Dnm1l −/− NSCs retained stemness, but there was ongoing differentiation towards the neuronal lineage under NSC culture conditions.This indicates that the stemness-maintaining ability of NSCs is attenuated by Dnm1l deficiency.

Comparison of Mitochondrial Morphology and Energy Metabolism between Dnm1l −/− NSCs and Wild-Type ESC-Derived NSCs (WT-NSCs)
Mitochondria are dynamic intracellular organelles that undergo fission and fusion in response to differentiation and cellular states [7,8].Dnm11 plays a crucial role as a key regulator of mitochondrial fission [10,29].Dnm1l −/− NSCs displayed a different mitochondrial morphology than WT-NSCs, indicating impaired mitochondrial fission (Figure 3A).Dnm1l −/− NSCs displayed numerous abnormally swollen mitochondria, and the mitochondrial shape was more elongated in these cells (Figure 3A).To analyze mitochondrial morphology, standard parameters, including the longest axis (c-max) and shortest axis (c-min) of the mitochondria, were determined (n = 76) (Figure 3B).In Dnm1l −/− NSCs, the c-max values were higher, whereas the c-min values were lower than those in WT-NSCs (Figure 3B).When comparing mitochondrial globularity using the c-max/c-min measurement, Dnm1l −/− NSCs showed values approximately two times higher than WT-NSCs, indicating a significantly higher prevalence of elongated mitochondria (Figure 3C).This observation reinforced that the absence of Dnm1l leads to impaired mitochondrial fission, resulting in the elongation and abnormal swelling of mitochondria in Dnm1l −/− NSCs.
Morphological changes in the mitochondria are associated with cellular metabolism [7,8,30,31].We hypothesized that the distinct mitochondrial shapes observed in Dnm1l −/− NSCs would lead to metabolic differences compared with control NSCs.Measurement of the oxygen consumption rate (OCR), which represents mitochondrial respiratory capacity, using a Seahorse analyzer revealed that Dnm1l −/− NSCs showed decreased overall OXPHOS capacity compared with WT-NSCs (Figure 3D).Additionally, Dnm1l −/− NSCs exhibited reduced basal and maximal respiration rates (Figure 3E).Quantitative analysis of OXPHOS (measured using OCR) and glycolysis (measured using extracellular acidification rate [ECAR]) levels represented in 2D graphs showed that Dnm1l −/− NSCs displayed lower OCR and higher ECAR values, indicating an OXPHOS-to-glycolytic shift in energy metabolism caused by Dnm1l knockout (Figure 3F).Furthermore, the contribution of mitochondria to ATP production was lower, whereas that from glycolysis was higher in Dnm1l −/− NSCs than in WT-NSCs (Figure 3G).Collectively, Dnm1l −/− NSCs exhibit structural abnormalities with elongated mitochondria, reduced OXPHOS capacity, and a metabolic shift toward glycolysis for ATP production.These findings suggest that the Dnm1l deficiency affected mitochondrial morphology, leading to altered cellular energy metabolism in the Dnm1l −/− NSCs.Morphological changes in the mitochondria are associated with cellular metabolism [7,8,30,31].We hypothesized that the distinct mitochondrial shapes observed in Dnm1l −/− NSCs would lead to metabolic differences compared with control NSCs.Measurement of the oxygen consumption rate (OCR), which represents mitochondrial respiratory capacity, using a Seahorse analyzer revealed that Dnm1l −/− NSCs showed decreased overall OXPHOS capacity compared with WT-NSCs (Figure 3D).Additionally, Dnm1l −/− NSCs exhibited reduced basal and maximal respiration rates (Figure 3E).Quantitative analysis of OXPHOS (measured using OCR) and glycolysis (measured using extracellular acidification rate [ECAR]) levels represented in 2D graphs showed that Dnm1l −/− NSCs 2.4.Impaired Self-Renewal and Accelerated Cellular Aging in Dnm1l −/− NSCs One of the distinct phenotypes observed in Dnm1l −/− NSCs was their inability to self-renew and survive in long-term culture.Unlike WT-NSCs, Dnm1l −/− NSCs showed reduced capacity to undergo self-renewal and eventually died under prolonged culture conditions (Figure 4A).The proliferation rate of Dnm1l −/− NSCs gradually decreased after passage 16 and almost ceased around passage 22 (Figure 4A), indicating a significant decrease in the proliferation rate compared with WT-NSCs (Figure 4A).Compared with WT-NSCs, which exhibited a high proliferation rate in both knock-out groups, Dnm1l −/− NSCs showed a noticeable reduction in proliferation.This difference became even more pronounced after passage 20, as Dnm1l −/− NSCs struggled to maintain their proliferative capacity (Figure 4A).These results indicate that the Dnm1l deficiency significantly impairs the long-term proliferative potential of Dnm1l −/− NSCs, further highlighting the critical role of Dnm1l in regulating cellular proliferation and self-renewal.
We hypothesized that the loss of the self-renewal ability of Dnm1l deficient NSCs could be attributed to cellular senescence or premature aging.To address this, we analyzed the markers associated with inflammation and endoplasmic reticulum (ER) stress, which are indicators of aging.RT-qPCR analysis revealed that Dnm1l −/− NSCs (passage 18) showed an increased expression of senescence markers, including inflammation (MMP13, IL-1R1, CK68), ER stress (CHOP, IRE1, BiP), and cell cycle (β-galactosidase, P16, P21, and P53) compared with control NSCs (passage 20) (Figure 4B-D).Collectively, our data suggest that mitochondrial dysfunction resulting from Dnm1l knockout may contribute to the reduced proliferation of NSCs.
was higher in Dnm1l −/− NSCs than in WT-NSCs (Figure 3G).Collectively, Dnm1l −/− NSCs exhibit structural abnormalities with elongated mitochondria, reduced OXPHOS capacity, and a metabolic shift toward glycolysis for ATP production.These findings suggest that the Dnm1l deficiency affected mitochondrial morphology, leading to altered cellular energy metabolism in the Dnm1l −/− NSCs.

Impaired Self-Renewal and Accelerated Cellular Aging in Dnm1l −/− NSCs
One of the distinct phenotypes observed in Dnm1l −/− NSCs was their inability to selfrenew and survive in long-term culture.Unlike WT-NSCs, Dnm1l −/− NSCs showed reduced capacity to undergo self-renewal and eventually died under prolonged culture conditions (Figure 4A).The proliferation rate of Dnm1l −/− NSCs gradually decreased after passage 16 and almost ceased around passage 22 (Figure 4A), indicating a significant decrease in the proliferation rate compared with WT-NSCs (Figure 4A).Compared with WT-NSCs, which exhibited a high proliferation rate in both knock-out groups, Dnm1l −/− NSCs showed a noticeable reduction in proliferation.This difference became even more pronounced after passage 20, as Dnm1l −/− NSCs struggled to maintain their proliferative capacity (Figure 4A).These results indicate that the Dnm1l deficiency significantly impairs the long-term proliferative potential of Dnm1l −/− NSCs, further highlighting the critical role of Dnm1l in regulating cellular proliferation and self-renewal.
We hypothesized that the loss of the self-renewal ability of Dnm1l deficient NSCs could be attributed to cellular senescence or premature aging.To address this, we analyzed the markers associated with inflammation and endoplasmic reticulum (ER) stress, which are indicators of aging.RT-qPCR analysis revealed that Dnm1l −/− NSCs (passage 18) showed an increased expression of senescence markers, including inflammation (MMP13, IL-1R1, CK68), ER stress (CHOP, IRE1, BiP), and cell cycle (βgalactosidase, P16, P21, and P53) compared with control NSCs (passage 20) (Figure 4B-D).Collectively, our data suggest that mitochondrial dysfunction resulting from Dnm1l knockout may contribute to the reduced proliferation of NSCs.

Discussion
In this study, we conducted a comprehensive analysis of the characteristics of NSCs derived from Dnm1l −/− ESCs.Although Dnm1l −/− NSCs predominantly maintained a homogenous NSC population, differences were observed in the expression levels of NSC markers (Nestin and Pax6), the presence of Tuj1 + cells in the NSC culture conditions, alterations in mitochondrial morphology and energy metabolism, and defective selfrenewal ability.We found that the impaired self-renewal observed in Dnm1l −/− NSCs could be attributed to premature aging or senescence, as evidenced by increased inflammation and cellular stress.These processes are influenced by Dnm1l deficiency and resulting mitochondrial defects.
The expression of NSC markers was lower in Dnm1l −/− NSCs than in control NSCs (WT-NSCs and brain-derived NSCs).Although Dnm1l −/− NSCs predominantly retained a homogenous NSC population, a subset of these cells expressed Tuj1, an early neuronal marker, even during early passages, suggesting the potential effect of mitochondrial abnormalities on NSC stemness and function in sustaining undifferentiated NSCs.Moreover, during long-term culture, Dnm1l −/− NSCs lost their self-renewal ability, ultimately leading to cell death, which may be attributed to premature aging mechanisms.This finding is consistent with previous reports that suggest that mitochondria govern cellular energy metabolism and participate in signaling pathways, aging, and cell death [1,2].Furthermore, the increase in inflammation-and cell stress-associated markers suggests a complex interplay between mitochondrial dynamics and aging-related processes.Further investigations are warranted to explore the underlying molecular

Discussion
In this study, we conducted a comprehensive analysis of the characteristics of NSCs derived from Dnm1l −/− ESCs.Although Dnm1l −/− NSCs predominantly maintained a homogenous NSC population, differences were observed in the expression levels of NSC markers (Nestin and Pax6), the presence of Tuj1 + cells in the NSC culture conditions, alterations in mitochondrial morphology and energy metabolism, and defective self-renewal ability.We found that the impaired self-renewal observed in Dnm1l −/− NSCs could be attributed to premature aging or senescence, as evidenced by increased inflammation and cellular stress.These processes are influenced by Dnm1l deficiency and resulting mitochondrial defects.
The expression of NSC markers was lower in Dnm1l −/− NSCs than in control NSCs (WT-NSCs and brain-derived NSCs).Although Dnm1l −/− NSCs predominantly retained a homogenous NSC population, a subset of these cells expressed Tuj1, an early neuronal marker, even during early passages, suggesting the potential effect of mitochondrial abnormalities on NSC stemness and function in sustaining undifferentiated NSCs.Moreover, during long-term culture, Dnm1l −/− NSCs lost their self-renewal ability, ultimately leading to cell death, which may be attributed to premature aging mechanisms.This finding is consistent with previous reports that suggest that mitochondria govern cellular energy metabolism and participate in signaling pathways, aging, and cell death [1,2].Furthermore, the increase in inflammation-and cell stress-associated markers suggests a complex interplay between mitochondrial dynamics and aging-related processes.Further investigations are warranted to explore the underlying molecular mechanisms in detail and gain a comprehensive understanding of the role of Dnm1l in maintaining stem cell homeostasis.
In our previous study, we compared the three knockout ESC lines: Fis1 −/− , Mff −/− , and Dnm1l −/− ESCs.Notably, Dnm1l −/− ESCs exhibited remarkable changes in mitochondrial morphology, proliferation rates, and reliance on OXPHOS for energy production [15].When comparing differentiation potential, Dnm1l −/− ESCs generated teratomas containing all three germ layer tissues, but the size of the teratomas was significantly smaller than that of the control and other knockout ESC lines (Fis1 −/− and Mff −/− ESCs) [15].This study extends our understanding of Dnm1l deficiency in NSCs, wherein phenotypic alterations similar to those observed in Dnm1l −/− ESCs, including changes in mitochondrial morphology, metabolic patterns, and proliferation rates, were observed.Interestingly, Dnm1l knockout in NSCs resulted in premature aging and eventual cell death during prolonged culture, but Dnm1l knockout in pluripotent ESCs did not induce cell death and led to sustained proliferation, albeit at a reduced rate.This finding holds significance in clinical applications, as the dysregulation of mitochondrial dynamics can cause neurodegeneration, a pathological feature observed in several neurodegenerative disorders.Notably, in neurogenesis, mitochondrial remodeling that occurs after cell division in NSCs determines the fate of daughter cells towards either self-renewal or differentiation [22,23].In addition, abnormal inhibition and activation of mitochondrial dynamics occur in the early stages of many diseases, particularly neurodegenerative disorders [32][33][34].A dominant negative mutation in Dnm1l in humans leads to impaired brain development and neonatal mortality [35].Mutations in Opa1, Opa3, and Opa7, which are crucial genes for regulating mitochondrial dynamics, have been suggested to be associated with autosomal dominant optic atrophy [36].Excessive mitochondrial fragmentation, which disturbs typical mitochondrial dynamics, is observed in Huntington's disease.This disruption ultimately results in diminished motility and compromised respiratory function [32,37].
Although Dnm1l −/− NSCs had elongated mitochondria, they exhibited a lower OCR than WT-NSCs and relied more on glycolysis for energy production.We anticipated that, as demonstrated in ESCs, Dnm1l −/− NSCs, which contain more elongated mitochondria, would be more dependent on OXPHOS than WT-NSCs [15].Wang et al. have demonstrated that a reduction in Dnm1l levels in NSCs leads to mitochondrial elongation and an increase in oxidative phosphorylation (OXPHOS) [38], which may seem contradictory to our result.This is because knock-out of Dnm1l causes mitochondrial elongation, but the mitochondria may not be fully functional, due to the numerous swollen parts of the mitochondria.(Figure 3A).Defects in mitochondrial dynamics lead to depletion of the NSC population in vivo [22].Therefore, it is evident that the knock-out of the Dnm1l gene causes the low expression of NSC markers.Further studies are required to reveal the role of mitochondrial defects in completing ESC differentiation of NSC-like properties.Moreover, in Dnm1l −/− NSCs, premature aging may cause a failure to eliminate dysfunctional mitochondria.This parallels the situation in aged cells, where diminished autophagic capacity hinders the removal of malfunctioning components, consequently contributing to cellular function deterioration [39,40].Mitochondrial fission contributes to the removal of defective components via mitophagy [5,41,42].However, this process is less efficient in aging cells and compromises mitochondrial quality [43,44].The abnormal mitochondrial ultrastructure in Dnm1l −/− NSCs suggests that proper mitophagy is hindered by Dnm1l deficiency, resulting in a decrease in mitochondrial function.
In conclusion, our findings suggested that Dnm1l deficiency leads to morphological and functional alterations in NSC mitochondria.The observed impairment in self-renewal and cellular aging may be linked to mitochondrial dysfunction and altered cellular energy metabolism in Dnm1l −/− NSCs.These results contribute to our understanding of the important role of Dnm1l in regulating NSC properties and highlight its potential implications in cellular aging and neurodevelopmental disorders.
Characterized NSCs were maintained in NSC expansion medium and single-cell dissociation using trypsin was performed every 3-4 days for passaging.In addition, brainderived NSC were obtained from our laboratory as previously reported [46] and maintained in the same condition as ESC-derived NSCs.

OCR Analysis
The OCR was measured using a Seahorse Bioscience XFp analyzer (Seahorse Bioscience, North Billerica, MA, USA).The day before analysis, Dnm1l −/− NSCs and WT-NSCs (7 × 10 4 cells per well) were cultured in XFp cell culture plates coated with 0.1% Matrigel (Corning, 356234, Corning, NY, USA) for overnight incubation.An hour before analysis, the culture medium was changed to an assay medium consisting of XF DMEM base media supplemented with glucose (17.5 mM), sodium pyruvate (0.5 mM), and Lglutamine (2.5 mM).The plates were then incubated in a non-CO 2 incubator.Following the manufacturer's instructions, the cells were supplemented with three chemicals (final concentrations: oligomycin-1.5µM, FCCP-2 µM, and rotenone/antimycin A-0.5 µM) and analyzed according to the Agilent Seahorse XFp Analyzer guidelines.Experiments were performed with biologically duplicated samples.

ATP Production Rate Assay
ATP production was measured using a Seahorse Bioscience XFp analyzer (Seahorse Bioscience, North Billerica, MA, USA).Cell preparation and assay media were the same as those used in the aforementioned OCR analysis.Following the manufacturer's protocol, the cells were supplemented with two chemicals (final concentrations: oligomycin-1.5µM and rotenone/antimycin A-0.5 µM) and analyzed according to the Agilent Seahorse XFp Analyzer guidelines.Experiments were performed with biologically triplicated samples.

RNA Isolation and RT-qPCR
Total RNA was isolated using TRIzol™ Reagent (Invitrogen, 15596026) following the manufacturer's instructions.RNA (1 µg) was reverse transcribed to cDNA using Superi-orScript III RT Master Mix (Enzynomics, RT300S, Daejeon, Republic of Korea) following the manufacturer's protocol.RT-qPCR was conducted using TOPreal™ qPCR 2X PreMIX (Enzynomics, RT500M) on a Roche LightCycler 5480 (Roche, Basel, Switzerland).The primers used for the RT-qPCR are listed in Table 1.Experiments were performed with triplicated samples.) were seeded in gelatin-coated 6-well plates and incubated for 24, 48, and 72 h.Then, cells were harvested and manually counted.All experiments were performed with triplicated samples.

Transmission Electron Microscopy (TEM)
For TEM analysis, NSCs were fixed in 4% paraformaldehyde and 2.5% glutaraldehyde in 0.1 M phosphate buffer (PB) for 24 h.After washing with 0.1 M PB, the samples were postfixed in 0.1 M PB supplemented with 1% osmium tetroxide for 1 h.The samples were then serially dehydrated with graded ethanol concentrations (50-100%).For polymerization, samples were embedded in Epon 812 and incubated overnight at 60 • C. Ultrathin sections (60-70 nm-thick) were obtained using an ultramicrotome (Leica UC7 Ultramicrotome, Leica

Figure 1 .
Figure 1.Differentiation of Dnm1l knockout embryonic stem cells (Dnm1l −/− ESCs) into neural stem cells (NSCs).(A) Schematic illustration of the protocol for in vitro differentiation of mouse Dnm1l −/− ESCs into NSCs.(B) Representative image of Dnm1l −/− ESCs cultured on the feeder in the serum/leukemia inhibitory factor (LIF) condition.(C) Morphology of Dnm1l −/− ESCs cultured for 2 days in 15% fetal bovine serum (FBS) medium without feeder and LIF supplementation.(D) Aggregates of differentiating Dnm1l −/− ESCs forming embryonic bodies (EBs) in N2B27 suspension medium supplemented with basic fibroblast growth factor (bFGF) and epidermal growth factor (EGF) for 2 days.(E) Attached EBs forming outgrowths on the gelatin-coated dish.(F) Brightfield images of NSCs at passage 8 cultured in NSC expansion medium.(G) Established NSCs derived from the mouse brain.

Figure 1 .
Figure 1.Differentiation of Dnm1l knockout embryonic stem cells (Dnm1l −/− ESCs) into neural stem cells (NSCs).(A) Schematic illustration of the protocol for in vitro differentiation of mouse Dnm1l −/− ESCs into NSCs.(B) Representative image of Dnm1l −/− ESCs cultured on the feeder in the serum/leukemia inhibitory factor (LIF) condition.(C) Morphology of Dnm1l −/− ESCs cultured for 2 days in 15% fetal bovine serum (FBS) medium without feeder and LIF supplementation.(D) Aggregates of differentiating Dnm1l −/− ESCs forming embryonic bodies (EBs) in N2B27 suspension medium supplemented with basic fibroblast growth factor (bFGF) and epidermal growth factor (EGF) for 2 days.(E) Attached EBs forming outgrowths on the gelatin-coated dish.(F) Brightfield images of NSCs at passage 8 cultured in NSC expansion medium.(G) Established NSCs derived from the mouse brain.
AAA CTT TTG TCC CGG GAA GCG TGT ACT TAT CCT T Pax6 CAG GTA TCC AAC GGT TGT G GCT TAC AAC TTC TGG AGT CG Nestin AGA ACT CTC GCT TGC AGA C GAG AAG GAT GTT GGG CTG A Tuj1 GCT CAC GCA GCA GAT GTT CG GGA TGT CAC ACA CGG CTA CC MMP13 TGA TGA AAC CTG GAC AAG CA GGT CCT TGG AGT GAT CCA GA IL-1R1 GTG CTA CTG GGG CTC ATT TGT GGA GTA AGA GGA CAC TTG CGA AT CD68 GAA ATG TCA CAG TTC ACA CCA G GGA TCT TGG ACT AGT AGC AGT G CHOP CCA CCA CAC CTG AAA GCA GAA AGG TGA AAG GCA GGG ACT CA IRE1 TTG AGA GAG CTT TTA CCA GCA G ACC AGG ACC TGA CGG ATG T BiP TTC AGC CAA TTA TCA GCA AAC TCT TTT TCT GAT GTA TCC TCT TCA CCA GT β-galactosidase GCA CGG CAT CTA TAA TGT CAC C GTA TCG GAA TGG CTG TCC ATC P16 CGC AGG TTC TTG GTC ACT GT TGT TCA CGA AAG CCA GAG CG P21 CCT GGT GAT GTC CGA CCT G CCA TGA GCG CAT CGC AAT C P53 GTC ACA GCA CAT GAC GGA GG TCT TCC AGA TGC TCG GGA TAC β-actin CGC CAT GGA TGA CGA TAT CG CGA AGC CGG CTT TGC ACA TG 4.7.Proliferation Rate Assay WT-NSC and Dnm1l −/− NSC (1 × 10 5