Method Article

Nuclei Isolation and Super-Resolution Structured Illumination Microscopy for Examining Nucleoporin Alterations in Human Neurodegeneration

DOI:

10.3791/62789

September 10th, 2021

In This Article

Summary

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This protocol describes an optimized workflow for nuclei isolation and super-resolution structured illumination microscopy to evaluate individual nucleoporins within the nucleoplasm and NPCs in induced pluripotent stem cell derived neurons and postmortem human tissues.

Abstract

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The nuclear pore complex (NPC) is a complex macromolecular structure comprised of multiple copies of ~30 different nucleoporin proteins (Nups). Collectively, these Nups function to regulate genome organization, gene expression, and nucleocytoplasmic transport (NCT). Recently, defects in NCT and alterations to specific Nups have been identified as early and prominent pathologies in multiple neurodegenerative diseases, including Amyotrophic Lateral Sclerosis (ALS), Alzheimer's Disease (AD)/Frontotemporal Dementia (FTD), and Huntington's Disease (HD). Advances in both light and electron microscopy allow for a thorough examination of sub-cellular structures, including the NPC and its Nup constituents, with increased precision and resolution. Of the commonly used techniques, super-resolution structured illumination microscopy (SIM) affords the unparalleled opportunity to study the localization and expression of individual Nups using conventional antibody-based labeling strategies. Isolation of nuclei prior to SIM enables the visualization of individual Nup proteins within the NPC and nucleoplasm in fully and accurately reconstructed 3D space. This protocol describes a procedure for nuclei isolation and SIM to evaluate Nup expression and distribution in human iPSC-derived CNS cells and postmortem tissues.

Introduction

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The prevalence of age-related neurodegenerative diseases is increasing as the population ages1. While the genetic underpinnings and pathologic hallmarks are well characterized, the precise molecular events leading to neuronal injury remain poorly understood2,3,4,5,6,7,8,9,10,11,12

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Protocol

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All blood samples for iPSC generation and autopsied tissue collections are approved by Johns Hopkins IRB with Johns Hopkins ethics oversight. All patient information is HIPPA compliant. The following protocol adheres to all Johns Hopkins biosafety procedures.

1. Preparation of slides for immunostaining and imaging

  1. Position a positively charged glass microscope slide in an empty cytofunnel and draw a circle with a hydrophobic barrier pen to outline an area to deposit the nuclei.
  2. Add 50 μL of 1 mg/mL collagen solution (diluted in 1x PBS) to the center of the circle drawn in step 1.1 and incubate at room temperature ....

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Results

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To examine the NPC and nucleoplasmic distribution and expression of POM121 in human neuronal nuclei, control, and C9orf72 iPSNs were differentiated as previously described15. Postmortem human motor cortex and day 32 iPSNs were lysed and subjected to nuclei isolation and immunostaining as described above. NeuN positive isolated nuclei were imaged by super-resolution structured illumination microscopy (SIM) using a super-resolution structured illumination microscope (Zeiss) and processed using defau.......

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Discussion

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Given the recent identification of NCT deficits as an early and prominent phenomenon in multiple neurodegenerative diseases16,27,28,30,31, there exists a critical need to thoroughly examine the mechanism by which this pathology occurs. As the NPC and its individual Nup proteins critically control functional NCT39,

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Disclosures

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The authors declare no competing financial interests.

Acknowledgements

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Postmortem human CNS tissues were provided by the Johns Hopkins ALS Autopsy Bank and the Target ALS Postmortem Tissue Core. This work was supported by the ALSA Milton Safenowitz Postdoctoral Fellowship (ANC), as well as funding from NIH-NINDS, Department of Defense, ALS Association, Muscular Dystrophy Association, F Prime, The Robert Packard Center for ALS Research Answer ALS Program, and the Chan Zuckerberg Initiative.

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Materials

List of materials used in this article
NameCompanyCatalog NumberComments
50 mL conical tubesFisher Scientific14-959-49A
Beckman UltracentrifugeBeckman Coulter
Cell ScrapersSarstedt83.183
CollagenAdvanced Biomatrix5005
CoverslipsMatTekPCS-170-1818
CytofunnelThermo Fisher ScientificA78710020
Cytospin 4Fisher ScientificA78300003
Dounce HomogenizersDWK Life Sciences357542
DTTSigma AldrichD0632
Eppendorf tubesFisher Scientific05-408-129
Goat Anti-Chicken Alexa 647Thermo Fisher ScientificA-21449
Goat Anti-Mouse Alexa 488Thermo Fisher ScientificA-11029
Goat Anti-Mouse Alexa 568Thermo Fisher ScientificA-11031
Goat Anti-Mouse Alexa 647Thermo Fisher ScientificA-21236
Goat Anti-Rabbit Alexa 488Thermo Fisher ScientificA-11034
Goat Anti-Rabbit Alexa 568Thermo Fisher ScientificA-11036
Goat Anti-Rabbit Alexa 647Thermo Fisher ScientificA-21245
Goat Anti-Rat Alexa 488Thermo Fisher ScientificA-11006
Goat Anti-Rat Alexa 568Thermo Fisher ScientificA-11077
Goat Anti-Rat Alexa 647Thermo Fisher ScientificA-21247
HemacytometerFisher Scientific267110
Microscope SlidesFisher Scientific12-550-15
Normal Goat SerumVector LabsS-1000
Nuclei PURE Prep Nuclei Isolation KitSigma AldrichNUC201Contains Lysis Buffer, 10% Triton X-100, 2 M Sucrose Gradient, Sucrose Cushion Solution, and Nuclei Storage Buffer; Referenced in protocol as "nuclei isolation kit"
PBSThermo Fisher Scientific10010023
PFAElectron Microscopy Sciences15714-S
Prolong Gold AntifadeInvitrogenP36930Referenced in protocol as "hard mount antifade mounting media"
SW 32 Ti Ultracentrifuge RotorBeckman Coulter369694Referenced in protocol as "ultracentrifuge rotor"
Triton X-100Sigma AldrichT9284
Trypan BlueThermo Fisher Scientific15-250-061
Ultracentrifuge TubesBeckman Coulter344058
Nucleoporin Primary AntibodiesPrimary antibodies suitable for immunofluorescent detection of invidual nucleoporins are available from multiple companies 

References

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  1. Hou, Y., et al. Ageing as a risk factor for neurodegenerative disease. Nature Reviews. Neurology. 15 (10), 565-581 (2019).
  2. Kim, G., Gautier, O., Tassoni-Tsuchida, E., Ma, X. R., Gitler, A. D. ALS genetics: Gains, losses, and implications for future therapies. Neuron

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Tags

Nuclei IsolationStructured Illumination MicroscopyNuclear Pore ComplexNucleoporin AlterationsNucleocytoplasmic TransportSuper Resolution MicroscopyHuman NeurodegenerationiPSC Derived CNS CellsAntibody LabelingPostmortem Tissues
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