Lamin Mutations Accelerate Aging via Defective Export of Mitochondrial mRNAs through Nuclear Envelope Budding

Mirza

Ashley

et al. 2017

Preprint

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SUMMARYDing et al., describe a non-canonical mRNA export pathway in budding yeast similar to that observed in Drosophila. This pathway appears upregulated when the NPC is impaired, nuclear envelope integrity is disrupted, or the export factor Xpo1 (CRM1) is defective.. CC-BY-NC 4.0 International license peer-reviewed) is the author/funder. It is made available under a The copyright holder for this preprint (which was not . http://dx.doi.org/10.1101/224055 doi: bioRxiv preprint first posted online Nov. 22, 2017; ABSTRACTIn eukaryotes, subsets of exported mRNAs are organized into large ribonucleoprotein (megaRNP) granules. How megaRNPs exit the nucleus is unclear, as their diameters are much larger than the nuclear pore complex (NPC) central channel. We previously identified a non-canonical nuclear export mechanism in Drosophila (Speese et al., Cell 2012) and mammals (Ding et al., in preparation), in which megaRNPs exit the nucleus by budding across nuclear envelope (NE) membranes. Here, we present evidence for a similar pathway in the nucleus of the budding yeast S. cerevisiae, which contain morphologically similar granules bearing mRNAs. Wild-type yeast displayed these granules at very low frequency, but this frequency was dramatically increased when the non-essential NPC protein Nup116 was deleted. These granules were not artifacts of defective NPCs; a mutation in the exportin XPO1 (CRM1), in which NPCs are normal, induced similar megaRNP upregulation. We hypothesize that a noncanonical nuclear export pathway, analogous to those observed in Drosophila and in mammalian cells, exists in yeast, and that this pathway is upregulated for use when NPCs or nuclear export are impaired.

Section: Introductionmentioning

confidence: 99%

Nuclear Export Through Nuclear Envelope Remodeling inSaccharomyces cerevisiae

Mirza

Ashley

et al. 2017

Preprint

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“…FISH was performed as described previously (Li et al, 2016) with modifications. Briefly, cultured neurons were washed once with DPBS (Gibco) and fixed with 4% PFA in PBS for 30 min at RT.…”

Section: Fluorescent In Situ Hybridizationmentioning

confidence: 99%

“…The distribution of total poly(A) RNAs in single diMNs was measured by FISH with oligo-dT probes as previously described (Packard et al, 2015;Li et al, 2016). Following hybridization, immunostaining of microtubule-associated protein 2 (MAP2) was used to identify the soma, and the DNA dye HST was used to define the nucleus.…”

Section: Measurement Of Mrna Distribution In Directly Induced Motor Nmentioning

confidence: 99%

Differential Influence of Sample Sex and Neuronal Maturation on mRNA and Protein Transport in Induced Human Neurons

Akter

Zhang

2020

Front. Mol. Neurosci.

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Nucleocytoplasmic transport (NCT) across the nuclear envelope (NE) is tightly regulated in eukaryotic cells and is critical for maintaining cellular homeostasis. Its dysregulation leads to aging and neurodegeneration. Because they maintain aging-associated hallmarks, directly reprogrammed neurons from human fibroblasts are invaluable in understanding NCT. However, it is not clear whether NCT activity is influenced by neuronal maturation and sample sex [a key biological variable emphasized by the National Institutes of Health (NIH) policy]. We examined here NCT activity at the single-cell level by measuring mRNA subcellular distribution and protein transport in directly induced motor neurons (diMNs) from adult human fibroblasts. The results show that mRNA subcellular distribution but not protein transport is affected by neuronal maturation stages, whereas both transport processes are not influenced by the sample sex. This study also provides quantitative methods and optimized conditions for measuring NCTs of mRNAs or protein cargoes, establishing a robust way for future functional examinations of NCT activity in directly induced neurons from diseased human patients.

“…In torsin mutants, disruption of mRNA nuclear export led to slowed growth and impaired development and plasticity of neuromuscular junctions 14 . To examine whether mRNA export was similarly impaired in DYT1 diMNs, we performed fluorescence in situ hybridization (FISH), as previously described 25,33,34 . We used digoxigenin-labeled oligo-dT as probes to detect the subcellular distribution of Poly (A) mRNAs.…”

Section: Dyt1 Dimns Exhibit Dysfunctional Nucleocytoplasmic Transportmentioning

confidence: 99%

Disease modeling with human neurons reveals LMNB1 dysregulation underlying DYT1 dystonia

Tang

et al. 2020

Preprint

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DYT1 dystonia is a hereditary neurological disease caused by a heterozygous mutation in torsin A (TOR1A). While animal models provide insights into disease mechanisms, significant species-dependent differences exist since mice with the identical heterozygous mutation fail to show pathology. Here, we model DYT1 by using human patient-derived motor neurons. These neurons with the heterozygous TOR1A mutation show markedly thickened nuclear lamina, disrupted nuclear morphology, and impaired nucleocytoplasmic transport, whereas they lack the perinuclear blebs that are often observed in animal models. Importantly, we further uncover that the nuclear lamina protein LMNB1 is specifically dysregulated in expression and subcellular localization. LMNB1 downregulation can largely ameliorate all the cellular defects in DYT1 motor neurons. These results reveal the value of disease modeling with human neurons and provide novel molecular mechanisms underlying DYT1 dystonia and potentially other neurological diseases with impaired nucleocytoplasmic transport.