Jun 22, 2023

Public workspaceNuclei isolation from fresh frozen human colon tissue for 10X Genomics Multi-omics (ATAC + GEX) assay

DOI
dx.doi.org/10.17504/protocols.io.5jyl8pn17g2w/v1
  • Antonina Mikorska1,
  • Koen Theunis2,3,
  • Suresh Poovathingal2,3,
  • sam kint1,
  • Sarah Geurs1,
  • Thierry Voet1
  • 1Laboratory of Reproductive Genomics, KU Leuven;
  • 2VIB-KU Leuven Center for Brain & Disease Research;
  • 3Laboratory of Computational Biology, KU Leuven
Antonina Mikorska
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DOI: dx.doi.org/10.17504/protocols.io.5jyl8pn17g2w/v1
Protocol CitationAntonina Mikorska, Koen Theunis, Suresh Poovathingal, sam kint, Sarah Geurs, Thierry Voet 2023. Nuclei isolation from fresh frozen human colon tissue for 10X Genomics Multi-omics (ATAC + GEX) assay. protocols.io https://dx.doi.org/10.17504/protocols.io.5jyl8pn17g2w/v1
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: In development
It works, but we are still developing and optimizing this protocol
Created: June 21, 2023
Last Modified: May 31, 2024
Protocol Integer ID: 83804
Keywords: ASAPCRN
Funders Acknowledgement:
Aligning Science Across Parkinson’s
Disclaimer
This protocol is still being optimized! At the moment, we are testing if we can achieve better results without using the collagenase/dispase as dispase is a proteinase.

The buffers are based on the user guides from 10X Genomics.
Abstract
Nuclei isolation protocol used for sn multi-omics assay on fresh frozen human colon tissue (full thickness and muscularis layer only).
Materials
BUFFERS
Buffers based on 10X Genomics user guides.

Collagenase/Dispase 10269638001 from Sigma

ABCDEF
Collagenase Lysis BufferStock conc Final conc V (µl)
Tris-HCl pH 7.41000mM10mM10,5
NaCl 5000mM10,0mM2,1
MgCl21000mM3mM3,2
DTT1000mM1mM1,1
RNAseIn40U/uL1U/uL26,3
Dispase/collagenase0,1mg/mL0,003mg/mL31,5
NF H2O975,5
Total Volume 1050,0
Wash Buffer 1Stock conc Final conc V (µl)
Tris-HCl (pH 7.4)1000mM10mM28,4
NaCl5000mM10mM5,7
MgCl21000mM3mM8,5
BSA10%1%283,5
Tween-2010%0,1%28,4
DTT1000mM1mM2,8
RNase in plus (promega)40U/ul1U/ul70,9
Water2406,9
Total Volume 2835,0
0.1x LysisStock conc Final conc V (µl)
Tris-HCl (pH 7.4)1000mM10mM5,3
NaCl5000mM10mM1,1
MgCl21000mM3mM1,6
Tween-2010%0,01%0,5
NP-4010%0,01%0,5
Digitonin0,5%0,002%2,1
BSA10%1%52,5
DTT1000mM1mM0,5
Rnase Inhibitor Protector (SIGMA)40U/ul1U/ul13,1
Water447,8
Total Volume 525,0
Wash Buffer 2Stock conc Final conc V (µl)
Tris-HCl (pH 7.4)1000mM10mM10,5
NaCl5000mM10mM2,1
MgCl21000mM3mM3,2
BSA10%1%105,0
Tween-2010%0,1%10,5
DTT1000mM1mM1,1
Rnase Inhibitor Protector (SIGMA)40U/ul1U/ul26,3
Water891,5
Total Volume 1050,0
1X Diluted Nuclei bufferStock conc  Final conc V(µl)
Nuclei buffer20X1X10
DTT100mM1mM2
Rnase Inhibitor Protector (SIGMA)40U/ul1U/ul5
Water183,0
Total Volume 200
Instruments and equipment:
- Kai Medical 2 mm Biopsy punch BP-20F
- WPI Noyes scissors 12 cm S/S 15 mm blades
- VWR®, Disposable Pestles and Cordless Motor for Pellet Mixing
- PluriSelect 40 µm, 20 µm filters
- Flowmi 40 µm Cell strainer for 1000P
- Luna FL Cell Counter
- Swing out rotor centrifuge
Sample preparation
Sample preparation
Place the sample preparation instruments on dry ice: biopsy punch, 1.5 mL EP tube, tweezers, petri dish.
Using 2 mm biopsy punch, aliquot 1.5-2 tissue pieces per patient. Place the pieces in a fresh 1.5 mL EP tube placed on dry ice. Repeat with a fresh biopsy punch for each multiplexed patient.

Experiment preparation
Experiment preparation
Prepare all buffers fresh and on wet ice. Add the the detergents, DTT and RNase inhibitor just before use.
Place all the plastics and filters on wet ice.
Tissue homogenization
Tissue homogenization
Perform all steps on wet ice. Add 500 µL Collagenase Lysis Buffer to the tube with multiplexed patient samples. Let thaw slightly.
Cut the tissue with scissors until there are no more pieces visible. Time = around 4 min (depending on the amount and the characteristics of the tissue).
After cutting, place the scissors in a fresh 1.5 mL EP tube placed on ice.
Further homogenize the tissue using an automatic plastic pellet pestle, for 45 s.
Place the pellet pestle in the EP tube instead of the scissors.
Mince the tissue for 1 min.
Wash the scissors using 250 µL Collagenase Lysis Buffer (while adding it to the tissue).
Homogenize the tissue with the used pellet pestle x15 (by hand).
Wash the pestle with 250µL Collagenase Lysis Buffer and add it to the tissue.
Gently pipet up and down 10X with P1000.
Centrifugate for 5 min at 500g at 4°C, remove the supernatant and resuspend in 1 mL Wash Buffer 1.
With P1000, transfer the sample onto 40 and 20 µm stacked strainers placed on 25 mL EP tube.
Wash the 1.5 mL EP tube with additional 1 mL Wash buffer 1, transfer onto the top filter.
Centrifugate the 25 mL EP tube for 5 min at 500g, 4°C.
Gently remove the supernatant.
Resuspend the pellet in 700 µL of Wash Buffer 1 and filtrate through Flowmi filter into a fresh DNA LoBind 1.5 mL EP tube.
Centrifugate for 5 min at 500g at 4°C
Gently remove the supernatant.
Nuclei permeabilization
Nuclei permeabilization
Resuspend the pellet in 500 µL 0.1x Lysis Buffer, pipette mix X5 with P1000.
Incubate on ice for 1 min (tissue quality dependent).
Add 1000 µL of Wash Buffer 2 and pipette mix 5X with P1000.
Centrifugate for 5 min at 500 g at 5°C.
Very gently remove the supernatant.
Nuclei resuspension and counting
Nuclei resuspension and counting
Resuspend the pellet in 25-50 µL 1X Diluted Nuclei Buffer.
Cell count the nuclei and proceed to the 10X Genomics Chromium Next GEM Single Cell Multiome ATAC + Gene Expression assay.