Application protocol
Isolation of human tumor cells from tumor tissue samples
In this application protocol, we describe how to isolate untouched human tumor cells in an easy workflow that improves sensitivity and reduces bias in downstream applications, such as next-generation sequencing and tumor cell culture. Solid tumors are dissociated into viable single-cell suspensions and untouched tumor cells are then isolated using MACS® technology.
Protocol
Create a viable single-cell suspension from a solid human tumor using the gentleMACS™ Octo Dissociator with Heaters in combination with the Tumor Dissociation Kit, human. Follow the protocol from the kit data sheet.
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Isolate untouched human tumor cells using the Tumor Cell Isolation Kit, human and LS Columns. Follow the protocol of the kit data sheet.
Download the data sheet
Tumor Cell Isolation Kit, human
We recommend filtering the magnetically labeled cell suspension to guarantee it is single-celled before separating it on the column.
- Place a Pre-Separation Filter (70 µm) on the LS Column.
- Rinse the column 3 times with PBS, ensuring that the filter is pre-wetted.
- Apply the cell suspension and PB buffer to the filter on the column.
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References
Additional resources
The following is a list of additional resources that may be of interest:
Materials
For tumor tissue dissociation
- Tumor Dissociation Kit, human (# 130-095-929)
- gentleMACS™ Octo Dissociator with Heaters (# 130-096-427)
- gentleMACS C Tubes (# 130-093-237)
- RPMI 1640 (# 130-091-440) or DMEM (# 130-091-437) culture media
- MACS® SmartStrainers (70 µm) (# 130-098-462)
- MACSmix™ Tube Rotator (# 130‑090‑753) in combination with an incubator at 37 °C
- (Optional) Red Blood Cell Lysis Solution (10×) (# 130-094-183)
- (Optional) MACS Tissue Storage Solution (# 130-100-008)
- (Optional) ART® 1000 REACH™ pipet tips (Molecular BioProducts, Inc.) for removal of dissociated material from the closed C Tubes
For isolation of tumor cells
- Tumor Cell Isolation Kit, human (# 130-108-339)
- QuadroMACS™ Starting Kit (LS) (# 130-091-051)
- Pre-Separation Filters (70 µm) (# 130-095-823)
- PB Buffer: Prepare a solution containing phosphate-buffered saline (PBS), pH 7.2, and 0.5% bovine serum albumin (BSA) by diluting MACS BSA Stock Solution (# 130‑091-376) 1:20 with PBS. Keep buffer cold (2−8 °C). Degas buffer before use, as air bubbles could block the column. Always use freshly prepared buffer. Do not use autoMACS® Running Buffer or MACSQuant® Running Buffer as they contain a small amount of sodium azide that could affect the results.
- (Optional) Propidium Iodide Solution (# 130-093-233) or 7-AAD for flow cytometry exclusion of dead cells
- (Optional) Fluorochrome-conjugated antibodies for flow cytometry analysis, e.g., CD326 (EpCAM)-VioBlue®. and CD31-PE. Learn more about our antibodies and dyes.
- (Optional) Labeling Check Reagent conjugated to, e.g., APC (# 130-095-237) to evaluate purity of sorted cells
- PBS buffer
Automated protocol
The materials and methods described in this Application are for the manual protocol. Automated cell isolation can be performed with the autoMACS® Pro or the MultiMACS™ Cell24 instruments.
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