Fluorescence-activated nuclei sorting (FANS) on human post-mortem cortex tissue enabling the isolation of distinct neural cell populations for multiple omic profiling

Stefania S Policicchio; Barry Chioza; Jonathan P Davies; Joe Burrage; Jonathan Mill; Emma L Dempster

Nov 27, 2024

Version 2

Fluorescence-activated nuclei sorting (FANS) on human post-mortem cortex tissue enabling the isolation of distinct neural cell populations for multiple omic profiling V.2

DOI

dx.doi.org/10.17504/protocols.io.36wgq4965vk5/v2

¹University of Exeter, Exeter, UK

Complex Disease Epigenetics Group

Stefania S Policicchio

University of Exeter Medical School

DOI: dx.doi.org/10.17504/protocols.io.36wgq4965vk5/v2

External link: https://doi.org/10.1038/s41467-022-33394-7

Protocol Citation: Stefania S Policicchio, Barry Chioza, Jonathan P Davies, Joe Burrage, Jonathan Mill, Emma L Dempster 2024. Fluorescence-activated nuclei sorting (FANS) on human post-mortem cortex tissue enabling the isolation of distinct neural cell populations for multiple omic profiling. protocols.io https://dx.doi.org/10.17504/protocols.io.36wgq4965vk5/v2Version created by Barry Chioza

Manuscript citation:

Shireby G,  Dempster EL,  Policicchio S,  Smith RG,  Pishva E,  Chioza B,  Davies JP,  Burrage J,  Lunnon K,  Vellame DS,  Love S,  Thomas A,  Brookes K,  Morgan K,  Francis P,  Hannon E,  Mill J, DNA methylation signatures of Alzheimer’s disease neuropathology in the cortex are primarily driven by variation in non-neuronal cell-types. Nature Communications  doi: 10.1038/s41467-022-33394-7

License: This is an open access protocol distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited

Protocol status: Working

We use this protocol and it's working

Created: October 04, 2023

Last Modified: November 27, 2024

Protocol Integer ID: 88785

Keywords: FANS, post-mortem brain, nuclei, flow cytometry, anti-SOX10, anti-IRF8, anti-NeuN, nuclei sorting

Funders Acknowledgements:

MRC Research Grant

Grant ID: MR/R005176/1

Alzheimer’s Research UK (ARUK)

Grant ID: ARUK-PPG2018A-010

Abstract

Increased understanding of the functional complexity of the genome has led to growing recognition about the role of epigenetic/transcriptional variation in health and disease. Current analyses of the human brain, however, are limited by the use of “bulk” tissue, comprising a heterogeneous mix of different neural cell types. 
As epigenetic processes play a critical role in determining cell type-specific patterns of gene regulation it is important to consider cellular composition in regulatory genomic studies of human post-mortem tissue, and there is a need for methods to purify populations of specific cell-types. Furthermore, the valuable nature of human post-mortem tissue means it is important to use methods that maximize the amount of genomic data generated on each sample. 
This protocol describes a method that uses fluorescence-activated nuclei sorting (FANS) to isolate and profile nuclei from multiple different human brain cell-types from frozen post-mortem tissue. 
This protocol can be used to robustly purify populations of neuronal (NeuN+ve), oligodendrocytes (SOX10+ve), microglia (IRF8+ve) and other glial origin nuclei (NeuN-ve/SOX10-ve/IRF8-ve) from adult post-mortem frozen brain, with each tissue sample yielding purified populations of nuclei amenable to simultaneous analysis of i) DNA modifications (via bisulfite sequencing / array), ii) histone modifications (CUT&Tag), iii) open chromatin analysis (ATAC-seq), and iv) gene expression (snRNA-seq).      

Guidelines

Prior to attempting this protocol please obtain the approval of your Institutional Review Board (IRB) or equivalent ethics committee(s).

Materials

ABC
       Supplier  Catalogue No.
BD FACSAria™ III Cell Sorter  BD Biosciences    648282-23  
Sorvall WX 80+ Ultracentrifuge  Thermo Scientific™    75000080  
  7mL Dounce Tissue Grinder    DWK Life Sciences    357542  
PA Thin-walled ultracentrifuge tubesThermo Scientific10533934
Table 1: Specifications of the equipment required for FANS protocol
 


ABC
  Supplier    Catalogue No.  
D-Sucrose (Molecular Biology)Fisher Scientific10638403
Calcium chloride (CaCl2) anhydrous, granularSigma-Aldrich  C1016-100G
Magnesium acetate ( Mg(Ace)2), 1M aq. solnAlfa AesarJ60041
UltraPure 0.5M EDTA, pH 8.0Invitrogen15575020
Thermo Scientific 1M Tris-HCI Buffer, pH 8.0Fisher Scientific 15568025
1,4-Dithiothreitol (DTT) - crystalline powderSigma-Aldrich  3483-12-3
Triton X-100Sigma-Aldrich  T9284  
UltraPure DNase/RNase-Free Distilled Water (ddH2O)Fisher Scientific12060346
Bovine Serum Albumin (BSA)Sigma-Aldrich  A9647-500G  
PBS Phosphate-Buffered Saline (10X) pH 7.4Fisher Scientific10722497  
Thermo Scientific™ RiboLock RNase Inhibitor (40 U/µL)Fisher Scientific10389109
TRIzol LS ReagentInvitrogen11588616  
BAMBANKER serum free cell freezing mediumBioCat GmbH BB03-NP 
BD FACSDiva CS&T Research BeadsBD Biosciences  655051  
BD FACS Accudrop BeadsBD Biosciences  345249  
BD FACSFlow Sheath Fluid 20LBD Biosciences  342003  
BD FACS Clean SolutionBD Biosciences  15875858  
BD FACS Rinse SolutionBD Biosciences  340346  
Table 2 : Specification of reagents required for FANS protocol
 


ABC
Lysis Buffer (LB)
StockAmount
0.32M Sucrose              5.47 g     
5mM CaCl21M250 µL   
3mM Mg(Ace)2              1M150 µL    
0.1mM EDTA                   0.5M10 µL  
10mM Tris-HCl, pH 8     1M500 µL    
1mM DTT                        3M17 µL   
0.1% Triton X-100           50 µL
Optional: RiboLock RNase Inhibitor 0.2U/µL40U/ µL5 µL / 1mL
Adjust with ddH2O to  50 mL     
1.8M Sucrose Solution (SS)
1.8M Sucrose                   30.78 g
3mM Mg(Ace)2                  1M150 µL
1mM DTT 3M17 µL
10mM Tris-HCl, pH8         1M500 µL
Adjust with ddH2O to 50 mL
5% BSA Solution (BB)
BSA200 mg
1x PBS4 mL
Staining Buffer (SB)
0.5% BSA5% BSA Solution (BB)400 µL
10X PBS400 µL
Optional: RiboLock RNase Inhibitor 0.2U/µL40U/ µL5 µL / 1mL
Adjust with ddH2O to4 mL  
Table 3 : Recipes for buffers and solutions required
 

 
 
AB
  Supplier    Thermo Scientific™  
  Model    Sorvall™ WX 80+  
  Rotor    TH-641  
  Speed    25,200 RPM / 108670.8 x g  
  Acceleration    9  
  Deceleration    5  
  Temperature    4°C  
Table 4: Ultracentrifuge specification and conditions

  
 
ABCDE
  Antibody    Preconjugated    Supplier    Cat No    Dilution  
Hoechst 33342  --  Abcamab228551    1:500  
Anti-SOX10to NL557R&D systemsNL2864R  1:20
Anti-NeuN  to Alexa Fluor488Millipore  MAB377X    1:1000  
Anti-IRF8  to APCInvitrogen  17-9852-82    1:150  
Table 5: List of antibodies required for FANS protocol
 

 
  
 

Protocol materials

ReagentTRIzol LSFisher ScientificCatalog #11588616 
ReagentBAMBANKERBioCat GmbHCatalog #BB03-NP 

Nuclear prep for FACS separation (using SOX10, IRF8, NeuN and Hoechst)

The protocol below yields at least 1,000,000 NeuN +ve, 1,000,000 SOX10 +ve, 400,000 IRF8 +ve (when the population is present) and 200,000 triple negative (NeuN-ve/SOX10-ve/IRF8-ve) nuclei per Amount500 mg   of frozen human post-mortem cortex tissue. Recovery might vary from sample to sample due to high inter-sample variability (brain collection, cortex sub-areas, fat content of tissue sectioned, and white to grey matter ratio)

Refer to Materials-Table 1  for details about the equipment required and to Materials-Table 2  for specifications of reagents required. 

Solution and buffer preps 

Lysis Buffer (LB)
Sucrose Solution (SS)
Staining Buffer (SB)

Solutions should be kept at Temperature4 °C    or TemperatureOn ice  . Refer to Materials-Table  3  for  recipes of solutions and buffers. 
Note
NOTE 1 – LB and SS can be prepared a week in advance, with DTT added on the day of use. Solutions should be stored atTemperature4 °C  once made.


Note

NOTE 2 – SB should be prepared fresh each day.

Note
NOTE 3- Samples are homogenised as bulk tissue using aAmount7 mL   Dounce homogeniser and then equally divided into three ultracentrifuge tubes.

Nuclei isolation
Pre-cool the ultracentrifuge toTemperature4 °C   Duration00:30:00   before starting this stage of the protocol.
All buffers and the Dounce homogenisers should be pre-cooled on ice.
Add DTT (Concentration1 millimolar (mM)   final concentration ) to the SS and LB (i.e. AmountAmount17 µL   3M DTT per Amount50 mL   of SS/LB)
Transfer Amount3 mL   LB to the homogeniser per Amount500 mg   human brain tissue.
Add the dissected tissue sample into the homogeniser.
Wait Duration00:05:00   before douncing the tissue to allow the sample to defrost.

To reduce heat caused by friction, the Dounce homogenisation step should be performed on ice with gentle strokes, and care should be taken to avoid foaming.

Note
NOTE 1 – Using the "TIGHT" pestle helps reduce the number of strokes required to reach full tissue disruption.

Note
NOTE 2 - The number of strokes required to fully homogenise the tissue may vary between samples due to heterogeneity in cellular composition, lipid content, and the amount of connective tissue.


Figure 1  Example of brain tissue sample A) only partially homogenised B) complete homogenisation.
7.  Transfer Amount8 mL   SS to PA thin-walled ultracentrifuge tubes.
8.  Carefully overlay with tissue homogenate (Amount1 mL  per tube) - using a P1000 pipette, releasing slowly down the side of the tube.
9.  Overlay with anotherAmount1 mL   LB – do not worry about disrupting the  homogenate phase
10 .Balance opposite tubes by weight with LB using a fine microbalance.
11. Perform ultracentrifugation for Duration00:45:00  (see Table 4 for centrifuge specification and conditions).

1h 20m

After Ultracentrifugation step 
 Pour off any remaining supernatant, taking care not to dislodge the pellet (90-degree inclination of the tube). If the pellet is hard to see, it is okay to leave  solution in the ultracentrifuge tube.
 Re-suspend pellet in Amount1 mL    SB and gently pipette up and down.
Let samples sit onTemperatureOn ice  for at least  Duration00:15:00  

Blocking step
 Transfer volume into 2 mL Lo-Bind Eppendorf tubes.
 Rinse out ultracentrifuge tubes in order to maximise nuclei collection by adding SB to each      ultracentrifuge tube (Amount1 mL   ) pipetting up and down several times and transferring to the new 2 mL tubes.

Washing step: 
Centifuge tubes atCentrifigation1000 x g for Duration00:05:00  , Temperature4 °C  
 Discard supernatant (pipetting off gently).
 Re-suspend each nuclei pellet in fresh SB ( Amount500 µL    ) 
If the sample was split then pool together pellets from the same sample (Final Volume =Amount1.5 mL  )
  Add DNA dye (Hoechst, 1:1000) and mix thoroughly via inversion.
Pipette out Amount200 µL  of nuclei solution for the Unstained Control (Hoechst dye only) and transfer to a new 2 mL tube
 Bring the volume up to 1 mL for the Unstained tube with fresh SB.
 Replace the volume taken from the Stained" tube with Amount200 µL  of fresh SB  (Final Volume  Amount1.5 mL  ).

20m

Immunostaining

1.  Add the following three antibodies (Ab) to Stained tube (1.5ml): 
       
       SOX10 pre-conjugated antibody (1:20 dilution) – [Amount75 µL   Ab]
       NeuN Alexa488 (1:1000) – [Amount1.5 µL   Ab ]
       IRF8 pre-conjugated antibody (1:150) - [Amount10 µL   Ab]

Refer to Table 5  for specifications of the antibodies used 

2. Incubate tubes for at least Duration01:30:00   on the rotor mixer (speed=11) at Temperature4 °C  , keeping the tubes in the dark
3. Washing step: Centrifigation1000 x g for Duration00:05:00  , Temperature4 °C   (both "Stained" and "Unstained" tubes)
4. Discard supernatant (by aspiration)
5. Re-suspend in fresh SB (Amount0.5 mL   for the Unstained tube, Amount-2 mL   for the Stained tube - depending on pellet size)

Fluorescence-Activated Nuclei Sorting (FANS)

For machine start-up, CST and Accudrop calibrations refer to  BD FACSAria III User’s Guide for guidance and troubleshooting. The following instructions describe FANS using BD FACSAria III. Other FACS platforms can be used but might require modifications to the protocol.

General Gating Parameters

For each sample, load stained and unstained tubes individually for data acquisition. A preliminary qualitative analysis of the data acquired is essential to select the appropriate gating strategy to maximize the nuclei capture while excluding unnecessary debris  and to ensure optimal signal/noise ratio.

Gating Parameters (X-axis:Y-axis):

FSC-A:SSC-A (Size, cell granularity or internal complexity)
SSC-W:SSC-A (to gate out doublets)
FSC-A:DAPI-A (to gate the single nuclei population)
DAPI-A:FITC-A (to gate NeuN stained nuclei)
DAPI-A:PE-A (to gate SOX10 stained nuclei)
DAPI-A:APC-A (to gate IRF8 stained nuclei)
FITC-A: PE-A (to visualize the distribution of triple staining)
Note
The SOX10+ve population is gated as a “daughter” population from the NeuN-ve fraction. 
The IRF8+ve population is gated as a “daughter” population of the SOX10-ve fraction.  
Refer to Figure 2 for a visualization of the gating strategy.

Figure 2. FANS gating strategy. 
(a) Particles smaller than nuclei (black dots) were eliminated with an area plot of forward-scatter (FSC-A) versus side-scatter (SSC-A), with gating for nuclei-sized particles inside the gate (box). 
(b) Plots of height versus width in the side scatter channel are used for doublet discrimination with gating to exclude aggregates of two or more nuclei. 
(c) Doublet discrimination gating was used to isolate nuclei determined by subgating on Hoechst 33342.  
Subsequent scatterplots discerning :
(d) NeuN-Alexa Fluor488–conjugated antibody staining (purple) 
(e) SOX10-NL577-stained nuclei (dark pink) 
(f) IRF8-APC stained nuclei (dark blue) 
(g) the distribution of the three main nuclei subpopulations identified through triple staining strategy (NeuN+ve, neurons; SOX10+ve, oligodendrocytes; double–ve, glia). 
The resultant hierarchical colour key ensures that only nuclei that are positive or negative for staining with the NeuN and/or SOX10/IRF8 antibody are passed through each gating condition.

Data recording settings

In line with the experiment design, FSC, SSC, DAPI, FITC, APC and PE are the parameters for which voltage values may need to be slightly adjusted due to experiment/ inter-sample variability. 
It is advisable to set the threshold value between 200 and 500 during data recording. Moreover, in the acquisition dashboard tab, we recommend setting Events to Record ≤3000, Event to display ≤1000 and Flow Rate = 1.0 (1,000 events per second) in order to increase the accuracy of signal detection.
The flow rate can be increased during sample collection to reduce the sort speed (ideally max events per second =1,500 for a 100-micron nozzle). However higher flow rates impact the data resolution and accuracy of events detection, and subsequent sorting of cellular fractions (see BD FACSAria III User’s Guide for details). 
During analysis, recorded data is displayed in plots, while gates are used to define populations of interest for selection. Figure 3 shows a representative example of the two most common outcomes we often observe.


Figure 3. Representative example of inter-individual variability. 
The data shown here are derived from two different control prefrontal cortex specimens of comparable age,  gender, and brain collection  which were processed in parallel following the same procedure. 
A) Optimal sample separation and abundant IRF8+ve fraction vs B) poor sample separation and completely missing a double negative population or an IRF8+ve population.

Sample Collection

DNA LoBind Tubes (Eppendorf, Cat No:30108051) are required to collect nuclei (to maximize sample recovery of nucleic acids by significantly reducing sample–to–surface binding).
Collected fractions can be used directly for downstream applications (e.g. DNA/RNA extraction, ATAC-seq, etc) or stored in  Temperature-80 °C   freezer.          
If you are collecting for DNA or RNA, as soon as the number of events desired is reached, transfer the tubes TemperatureOn ice  , do not hold them at TemperatureRoom temperature   
Note
During collection, it is crucial to regularly pause the sorting to mix the two phases in order to preserve the integrity of resulting RNA preparations.

Note
For RNA extraction, LoBind Tubes should each contain Amount1 mL  of pre-chilled ReagentTRIzol LSFisher ScientificCatalog #11588616  prior to sorting. 


4. Keep samples TemperatureOn ice   for the entire duration of the sorting.
5. Lightly vortex sample tubes to make the mixture homogeneous (not clumped) before loading the tube into the FACS chamber.
6. Load the UNSTAINED control  tube into the chamber first and proceed with nuclei collection. 
7. Proceed by collecting STAINED tube by simultaneously sorting for NeuN+ve, SOX10+ve , IRF8+ve  or Triple Negative.  
Note
At least  Amount1 µg    genomic DNA at least is expected from Amount500 mg   tissue.  For optimal recovery of high-quality genomic DNA from FANS sorted nuclei we recommend this extraction protocol


Note
The IRF8+ve population may not be detectable in every brain sample processed (high inter-individual variability); when it is, it represents between 5-10% of the total sample, therefore yielding often insufficient material for multiple assays. 
8.  For long term storage of collected nuclei Centrifigation1000 x g , Temperature4 °C    for Duration00:05:00     
9.  Carefully remove supernatant.
10. Add Amount100 µL  ReagentBAMBANKERBioCat GmbHCatalog #BB03-NP per 100,000 nuclei collected to the tube.
11. Gently resuspend.
12. Store in Temperature-80 °C   freezer  

General Recommendations for the user

For every new experiment we recommend performing the following steps:

When loading your tube into the FACS machine, run the unstained / IgG control sample first as this aids in setting the baseline parameters
Check your event rate in the Acquisition Dashboard window. If it is greater than 1500 evt/s turn down the “flow rate” or unload and dilute the sample further. If less than 100  evt/s, turn up the “flow rate” (don’t exceed a flow rate of 5.0 if possible, as the instrument is less focused and more inaccurate at higher flow rates)
In the Acquisition Dashboard window choose the appropriate “stopping gate” and “storage gate” (when working with nuclei, set as “Nuclei” and “All events” respectively)
Choose the range of “events to record” and “events to display” that best suits your purpose (≥ 5000 for both is advised)
Under the “threshold” tab in the Cytometer window, change the threshold (should be set for FSC) so that any small events in the bottom corner of the FSC vs SSC graph (caused by general cell debris and dust) are no longer shown. The threshold should not be set too high so that it causes an arbitrary, artificial cut-off through the left side of your population but not so low that small events caused by debris/dust are visible (ideally between a threshold 200-500).
Under the “parameters” tab in the Cytometer window, adjust the “FSC” and “SSC” values to get your population sitting in the centre of the FSC vs SSC graph (a re-adjustment of the “threshold” may be required at this point). It is essential to select “restart” each time any of the parameters are changed to update the events being displayed to ensure only events are recorded under the new settings.
Adjust or draw a new gate in the FSC vs SSC plot to encompass the population of interest.
Look in the scatter graph of SSC-A vs SSC-W (if you opened a blank experiment you will need to draw one). Right-click on the graph and check it is only displaying the events encompassed by your previous FSC vs SSC gate. Adjust or draw a gate for SSC A vs SSC W to encompass all of the main population to the left of the graph and exclude outliers to the right (these are doublets and other cell debris clumps)
Under the “parameters” tab in the Cytometer window adjust parameters for the fluorochromes selected so the unstained / IgG control sample sits close to 0 for the fluorochrome on a graph of FSC vs fluorochrome.
Load the stained samples and check the stained population has a clear increase in signal for the fluorochrome in comparison to the unstained (signal should not exceed 10x4). Several minor re-adjustments of the fluorochrome’s “parameters" may be necessary for the stained sample at this stage. If so, the unstained / IgG control has to be reset and re-recorded.
Note
WARNING – Do not change parameter settings between samples you wish to compare, if you do you will need to re-record all samples using the changed parameters.

11.  Select the correct option for the collection device in the Sort Layout window ( we recommend “4-Way Purity” for   general collection)
12. Regularly check your “Efficiency” in the Sort Layout window value. Between 80-100% is ideal, 70% is acceptable if less than 70% either the sample is too concentrated or you are sorting a rare population. Although the “flow rate” in the Acquisition Dashboard window can be increased to make the sort quicker, faster flow rates are less efficient.
13. Check the “Electronic abort rate” (N° errors /sec) and “Electronic abort count” (Tot N° of errors) at the bottom of the Acquisition Dashboard window. These parameters measure potential miss-sorts (different from efficiency as efficiency measures undetermined drops which are directed to the “Waste” and therefore lost but do not contaminate).“Electronic abort rate” should be <1% of total events per second.
14. For long sorts, gate positions should be regularly monitored, especially for stained populations as fluorochromes lose intensity over time and the population can shift towards the unstained. Gates can be moved during long sorts to compensate.

	A	B
	Supplier	Thermo Scientific™
	Model	Sorvall™ WX 80+
	Rotor	TH-641
	Speed	25,200 RPM / 108670.8 x g
	Acceleration	9
	Deceleration	5
	Temperature	4°C

A	B	C
	Supplier	Catalogue No.
BD FACSAria™ III Cell Sorter	BD Biosciences	648282-23
Sorvall WX 80+ Ultracentrifuge	Thermo Scientific™	75000080
7mL Dounce Tissue Grinder	DWK Life Sciences	357542
PA Thin-walled ultracentrifuge tubes	Thermo Scientific	10533934

A	B	C
	Supplier	Catalogue No.
D-Sucrose (Molecular Biology)	Fisher Scientific	10638403
Calcium chloride (CaCl2) anhydrous, granular	Sigma-Aldrich	C1016-100G
Magnesium acetate ( Mg(Ace)2), 1M aq. soln	Alfa Aesar	J60041
UltraPure 0.5M EDTA, pH 8.0	Invitrogen	15575020
Thermo Scientific 1M Tris-HCI Buffer, pH 8.0	Fisher Scientific	15568025
1,4-Dithiothreitol (DTT) - crystalline powder	Sigma-Aldrich	3483-12-3
Triton X-100	Sigma-Aldrich	T9284
UltraPure DNase/RNase-Free Distilled Water (ddH2O)	Fisher Scientific	12060346
Bovine Serum Albumin (BSA)	Sigma-Aldrich	A9647-500G
PBS Phosphate-Buffered Saline (10X) pH 7.4	Fisher Scientific	10722497
Thermo Scientific™ RiboLock RNase Inhibitor (40 U/µL)	Fisher Scientific	10389109
TRIzol LS Reagent	Invitrogen	11588616
BAMBANKER serum free cell freezing medium	BioCat GmbH	BB03-NP
BD FACSDiva CS&T Research Beads	BD Biosciences	655051
BD FACS Accudrop Beads	BD Biosciences	345249
BD FACSFlow Sheath Fluid 20L	BD Biosciences	342003
BD FACS Clean Solution	BD Biosciences	15875858
BD FACS Rinse Solution	BD Biosciences	340346

A	B	C
Lysis Buffer (LB)
	Stock	Amount
0.32M Sucrose		5.47 g
5mM CaCl2	1M	250 µL
3mM Mg(Ace)2	1M	150 µL
0.1mM EDTA	0.5M	10 µL
10mM Tris-HCl, pH 8	1M	500 µL
1mM DTT	3M	17 µL
0.1% Triton X-100		50 µL
Optional: RiboLock RNase Inhibitor 0.2U/µL	40U/ µL	5 µL / 1mL
Adjust with ddH2O to		50 mL


1.8M Sucrose Solution (SS)
1.8M Sucrose		30.78 g
3mM Mg(Ace)2	1M	150 µL
1mM DTT	3M	17 µL
10mM Tris-HCl, pH8	1M	500 µL
Adjust with ddH2O to		50 mL


5% BSA Solution (BB)
BSA		200 mg
1x PBS		4 mL


Staining Buffer (SB)
0.5% BSA	5% BSA Solution (BB)	400 µL
10X PBS		400 µL
Optional: RiboLock RNase Inhibitor 0.2U/µL	40U/ µL	5 µL / 1mL
Adjust with ddH2O to		4 mL

A	B	C	D	E
Antibody	Preconjugated	Supplier	Cat No	Dilution
Hoechst 33342	--	Abcam	ab228551	1:500
Anti-SOX10	to NL557	R&D systems	NL2864R	1:20
Anti-NeuN	to Alexa Fluor488	Millipore	MAB377X	1:1000
Anti-IRF8	to APC	Invitrogen	17-9852-82	1:150

Public workspaceFluorescence-activated nuclei sorting (FANS) on human post-mortem cortex tissue enabling the isolation of distinct neural cell populations for multiple omic profiling V.2

Fluorescence-activated nuclei sorting (FANS) on human post-mortem cortex tissue enabling the isolation of distinct neural cell populations for multiple omic profiling V.2