Preparing Viable Single Cells from Human Tissue and Tumors for Cytomic Analysis

Leelatian, Nalin; Doxie, Deon B.; Greenplate, Allison R.; Sinnaeve, Justine; Ihrie, Rebecca A.; Irish, Jonathan M.

doi:10.1002/cpmb.37

Cited by 47 publications

(54 citation statements)

References 87 publications

(220 reference statements)

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“…As of February 2019, the median progression free survival (PFS) and overall survival (OS) after diagnosis were 6.3 and 13 months, respectively, similar to those observed in larger populations of patients undergoing standard therapy 27 . Resected tissues were immediately dissociated into single-cell suspensions as previously reported 38 . Cells were stained with a customized antibody panel for mass cytometry designed to capture the expression of known cell surface proteins, intracellular proteins, and phospho-signaling events (Figure 1, 2, Supplementary Table 2, Supplemental Information) that are critical for gliomagenesis and pathogenesis 32,39,40,30,34,35 .…”

Section: Comprehensive Patient-specific Analysis Reveals Glioblastomamentioning

confidence: 99%

“…The second round of data analysis used an equal number of each patient's glioblastoma cells to create a single, common t-SNE map of glioblastoma cell phenotypes across all patients (N = 131,880 cells; 4,710 cells x 28 patients). Prior to creating this common map, mass cytometry standardization beads were used to remove batch effects and to set the variance stabilizing arcsinh scale transformation for each channel following field-standard protocols 11,38,41 . This common t-SNE map was generated using 24 of 34 measured markers (Supplementary Table 2) and was used for automated analysis of risk stratifying cell subsets.…”

Section: Rapid Identifies Prognostic Cell Subsets In Glioblastoma Dismentioning

confidence: 99%

“…Surgical resection specimens of 28 IDH-wildtype glioblastomas collected at Vanderbilt University Medical Center between 2014 and 2016 were processed into single cell suspensions following an established protocol 38 . Only samples that were confirmed to be IDH-wildtype glioblastomas by standard pathological diagnosis were used.…”

Section: Patient Samplesmentioning

confidence: 99%

“…Cells derived from patient samples were prepared as previously described 38 . A multi-step staining protocol was used, which included 1) live surface stain, 2) 0.02% saponin permeabilization intracellular stain, and 3) intracellular stain after permeabilization with ice-cold methanol ( Supplementary Table 2).…”

Section: Mass Cytometry Analysismentioning

confidence: 99%

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High risk glioblastoma cells revealed by machine learning and single cell signaling profiles

Leelatian

Sinnaeve

et al. 2019

Preprint

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Recent developments in machine learning implemented dimensionality reduction and clustering tools to classify the cellular composition of patient-derived tissue in multi-dimensional, single cell studies. Current approaches, however, require prior knowledge of either categorical clinical outcomes or cell type identities. These algorithms are not well suited for application in tumor biology, where clinical outcomes can be continuous and censored and cell identities may be novel and plastic. Risk Assessment Population IDentification (RAPID) is an unsupervised, machine learning algorithm that identifies single cell phenotypes and assesses clinical risk stratification as a continuous variable. Single cell mass cytometry evaluated 34 different phospho-proteins, transcription factors, and cell identity proteins in tumor tissue resected from patients bearing IDH wild-type glioblastomas. RAPID identified and characterized multiple biologically distinct tumor cell subsets that independently and continuously stratified patient outcome. RAPID is broadly applicable for single cell studies where atypical cancer and immune cells may drive disease biology and treatment responses.

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Section: Comprehensive Patient-specific Analysis Reveals Glioblastomamentioning

confidence: 99%

Section: Rapid Identifies Prognostic Cell Subsets In Glioblastoma Dismentioning

confidence: 99%

Section: Patient Samplesmentioning

confidence: 99%

Section: Mass Cytometry Analysismentioning

confidence: 99%

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High risk glioblastoma cells revealed by machine learning and single cell signaling profiles

Leelatian

Sinnaeve

et al. 2019

Preprint

Self Cite

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“…As this panel contains markers expressed in 3 distinct cellular compartments (cell surface, cytoplasm and nucleus), multiple permeabilization protocols were tested to identify one that allowed for optimal detection of all parameters in all compartments. We tested the panel on 3 head and neck solid tumors disaggregated with a standardized protocol for obtaining single cells for mass cytometry analysis of human tissue and tumor biopsies . The protocol as well as information on staining patient samples can be found in the Supporting Information Materials in Section “Panel optimization on tumor biopsies.”…”

Section: Introductionmentioning

confidence: 99%

OMIP‐045: Characterizing human head and neck tumors and cancer cell lines with mass cytometry

2018

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A 42-parameter panel (34 antibody targets, cisplatin for live/dead, iridium for cell identification, and 6 barcodes) was developed for the characterization of cell types and signaling pathways present in tumor tissues or cell lines originating from primary, metastatic and recurrent head and neck squamous cell carcinoma (HNSCC), the most prevalent malignant tumor of the head and neck region and the 6th most common form of non-skin cancer worldwide (1) ( Table 1). Importantly, due to overlap in targets and markers across diverse tumor entities [e.g., HER2 amplification is present in both breast and gastric tumors (2,3)], the described panel may be appropriate for use in preclinical models of additional distinct solid as well as hematological malignancies. This panel has been successfully tested on fresh, formalin-fixed, and frozen cells originating from cell lines derived from primary and metastatic/ recurrent tumors and from patients' tumor tissue.

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Training Novices in Generation and Analysis of High‐Dimensional Human Cell Phospho‐Flow Cytometry Data

et al. 2020

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This article presents a single experiment designed to introduce a trainee to multiple advanced bench and analysis techniques, including high‐dimensional cytometry, profiling cell signaling networks, functional assays with primary human tissue, and single‐cell analysis with machine learning tools. The trainee is expected to have only minimal laboratory experience and is not required to have any prior training in flow cytometry, immunology, or data science. This article aims to introduce the advanced research areas with a design that is robust enough that novice trainees will succeed, flexible enough to allow some project customization, and fundamental enough that the skills and knowledge gained will provide a template for future experiments. For advanced users, the updated phospho‐flow protocol and the established controls, best practices, and expected outcomes presented here also provide a framework for adapting these tools in new areas with unexplored biology. © 2020 by John Wiley & Sons, Inc.Basic Protocol: Phospho‐protein stimulation and mass cytometry data collectionSupport Protocol: Analysis of signaling mass cytometry data

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Preparing Viable Single Cells from Human Tissue and Tumors for Cytomic Analysis

Cited by 47 publications

References 87 publications

High risk glioblastoma cells revealed by machine learning and single cell signaling profiles

High risk glioblastoma cells revealed by machine learning and single cell signaling profiles

OMIP‐045: Characterizing human head and neck tumors and cancer cell lines with mass cytometry

Training Novices in Generation and Analysis of High‐Dimensional Human Cell Phospho‐Flow Cytometry Data

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