Hcfc1a regulates neural precursor proliferation and asxl1 expression in the developing brain

Castro, Victoria L.; Reyes, Joel F.; Reyes-Nava, Nayeli G; Paz, David; Quintana, Anita M.

doi:10.21203/rs.2.18231/v1

Cited by 4 publications

(29 citation statements)

References 11 publications

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“…We have previously established that nonsense mutation of hcfc1a (co60 allele) causes an increase in asxl1 expression, which promotes increased proliferation of NPCs (Castro et al, 2020). Asxl1 promotes Akt phosphorylation (Youn et al, 2017) and we established that inhibition of PI3K, an upstream regulator of Akt, is sufficient to reduce asxl1 expression and restore the NPC numbers to normal levels in the co60 allele.…”

Section: Resultsmentioning

confidence: 99%

Missense and nonsense mutations of the zebrafishhcfc1agene result in contrasting mTor and radial glial phenotypes

Castro

Paz

Virrueta

et al. 2022

Preprint

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Mutations in theHCFC1transcriptional co-factor are the cause ofcblXsyndrome and X-linked intellectual disability (XLID).cblXis the more severe disorder associated with intractable epilepsy, abnormal cobalamin metabolism, facial dysmorphia, cortical gyral malformations, and intellectual disability.In vitro, Hcfc1regulates neural precursor (NPCs) proliferation and number, which has been validated in zebrafish. However, conditional deletion ofHcfc1in Nkx2.1+ NPCs increased cell death, reducedGfapexpression, and reduced numbers of GABAergic neurons. Thus, the role of HCFC1 in brain development is not completely understood. Recently, knock-in of acblX(HCFC1) andcblX-like (THAP11) were created in mice. Knock-in of thecblX-like allele was associated with increased expression of proteins required for ribosome biogenesis. However, the brain phenotypes were not comprehensively studied due to sub-viability and therefore, a mechanism underlying increased ribosome biogenesis was not described. We used a missense, a nonsense, and two conditional zebrafish alleles to further elucidate this mechanism during brain development. We observed unique subtypes ofcblXsyndrome, each with a unique signature (activation or repression) of Akt/mTor signaling. Differential regulation of mTor was associated with allele dependent radial glial cell phenotypes. Liquid chromatographmass spectrometry and chromatin immunoprecipitation revealed at least two downstream target genes of HCFC1,asxl1andywhab, whose divergent expression correlates with mTor activity in an allele specific manner. These data suggest that differential regulation of mTor across individualcblXmutations may underlie the clinical heterogeneity of patient phenotypes.Summary StatementWe uncovered a novel mechanism whereby HCFC1 regulates brain development through differential regulation of mTor activity and acts as a putative biomarker for subtypes ofcblXsyndrome.

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Section: Resultsmentioning

confidence: 99%

Missense and nonsense mutations of the zebrafishhcfc1agene result in contrasting mTor and radial glial phenotypes

Castro

Paz

Virrueta

et al. 2022

Preprint

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“…In addition, we designed a splice inhibiting morpholino to the 3' splice acceptor of exon 2, but the designed morpholino did not delete exon 3 as predicted, even at the highest concentration injected (2nl of a 0.9mM stock solution). We did, however, utilize a random control morpholino to account for the possibility of morpholino-induced cell death, an endeavor that proved to be rather successful in previous studies (54,55). And, while injection of HS side chains is a potential rescue for the morphant phenotype we observe, there is the possibility that HS/heparin coinjection would fail to rescue because a domain outside of domain I is also essential for regulation of CNCCs.…”

Section: Discussionmentioning

confidence: 98%

“…For all experiments, the morphant experimental group is compared to either a random control group or wildtype non-injected. The randomized control morpholino has been shown through previous literature to have no associated phenotypes, indicating that it does not in uence nal results and therefore is the appropriate control group for comparison (54,55,57). Thus, for statistical analysis, comparisons were performed using a T-test between the random control group and the morpholino.…”

Section: Antisense Oligonucleotide Morpholino Design and Microinjectionmentioning

confidence: 99%

Knockdown of hspg2 is associated with abnormal mandibular joint formation and neural crest cell dysfunction in zebrafish

Castellanos

Reyes-Nava

Quintana

2020

Preprint

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Background: Heparan sulfate proteoglycan 2 (HSPG2) encodes for perlecan, a large proteoglycan that plays an important role in cartilage formation, cell adhesion, and basement membrane stability. Mutations in HSPG2 have been associated with Schwartz-Jampel Syndrome (SJS) and Dyssegmental Dysplasia Silverman-Handmaker Type (DDSH), two disorders characterized by skeletal abnormalities. These data indicate a function for HSPG2 in cartilage development/maintenance. However, the mechanisms in which HSPG2 regulates cartilage development are not completely understood. Here, we explored the relationship between this gene and craniofacial development through morpholino-mediated knockdown of hspg2 using zebrafish.Results: Knockdown of hspg2 resulted in abnormal development of the mandibular jaw joint at 5 days post fertilization (DPF). We surmised that defects in mandible development were a consequence of neural crest cell (NCC) dysfunction, as these multipotent progenitors produce the cartilage of the head. Early NCC development was normal in morphant animals as measured by distal-less homeobox 2a (dlx2a) and SRY-box transcription factor 10 (sox10) expression at 1 DPF. However, subsequent analysis at later stages of development (4 DPF) revealed a decrease in the number of Sox10 + and Collagen, type II, alpha 1a (Col2a1a)+ cells within the mandibular jaw joint region of morphants relative to random control injected embryos. Concurrently, morphants showed a decreased expression of nkx3.2, a marker of jaw joint formation, at 4 DPF.Conclusions: Collectively, these data suggest a complex role for hspg2 in jaw joint formation and late stage NCC differentiation.

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“…While translation-blocking morpholinos are a simple and effective way in which to knockdown genes of interest, they have been associated with off target effects and non-speci c cell death. We did, however, utilize a random control morpholino to account for the possibility of morpholino-induced cell death, an endeavor that proved to be rather successful in previous studies (58,59). And while injection of heparin side chains is a potential rescue for the morphant phenotype we observed, there is the possibility that heparin sulfate co-injection would fail to rescue because a domain outside of domain I is essential for regulation of CNCCs.…”

Section: Discussionmentioning

confidence: 98%

“…For all experiments, the morphant experimental group is compared to either a random control group or wildtype non-injected. The randomized control morpholino has been shown through previous literature to have no associated phenotypes, indicating that it does not in uence nal results and therefore is the appropriate control group for comparison (58,59,61). Thus, for statistical analysis, comparisons were performed using a T-test between the random control group and the morpholino.…”

Section: Antisense Oligonucleotide Morpholino Design and Microinjectionmentioning

confidence: 99%

Knockdown of hspg2 is associated with mandibular jaw joint fusion and neural crest cell dysfunction in zebrafish

Castellanos

Reyes-Nava

Quintana

2020

Preprint

Self Cite

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Background: Heparan sulfate proteoglycan 2 (HSPG2) encodes for perlecan, a large proteoglycan that plays an important role in cartilage formation, cell adhesion, and basement membrane stability. Mutations in HSPG2 have been associated with Schwartz-Jampel Syndrome (SJS) and Dyssegmental Dysplasia Silverman-Handmaker Type (DDSH), two disorders characterized by skeletal abnormalities. These data indicate a function for HSPG2 in cartilage development/maintenance. However, the mechanisms by which HSPG2 regulates cartilage development are not completely understood. Here, we explored the relationship between this gene and craniofacial development through morpholino-mediated knockdown of hspg2 using zebrafish. Results: Knockdown of hspg2 resulted in abnormal development of the mandibular jaw joint at 5 days post fertilization (DPF). We surmised that defects in mandible development were a consequence of neural crest cell (NCC) dysfunction, as these multipotent progenitors produce the cartilage of the head. Early NCC development was normal in morphant animals as measured by distal-less homeobox 2a (dlx2a) and SRY-box transcription factor 10 (sox10) expression at 1 DPF. However, subsequent analysis at later stages of development (4 DPF) revealed a decrease in the number of Sox10 + and Collagen, type II, alpha 1a (Col2a1a)+ cells within the mandibular jaw joint region of morphants. Concurrently, morphants showed a decreased expression of NK3 homeobox 2 (nkx3.2), a jaw joint molecular marker at 4 DPF. Conclusions: Collectively, these data suggest a complex role for hspg2 in jaw joint formation and late stage NCC differentiation.

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Hcfc1a regulates neural precursor proliferation and asxl1 expression in the developing brain

Cited by 4 publications

References 11 publications

Missense and nonsense mutations of the zebrafishhcfc1agene result in contrasting mTor and radial glial phenotypes

Missense and nonsense mutations of the zebrafishhcfc1agene result in contrasting mTor and radial glial phenotypes

Knockdown of hspg2 is associated with abnormal mandibular joint formation and neural crest cell dysfunction in zebrafish

Knockdown of hspg2 is associated with mandibular jaw joint fusion and neural crest cell dysfunction in zebrafish

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