Single‐cell mass cytometry adapted to measurements of the cell cycle

Mass cytometry is a recently introduced technology that utilizes transition element isotope‐tagged antibodies for protein detection on a single‐cell basis. By circumventing the limitations of emission spectral overlap associated with fluorochromes utilized in traditional flow cytometry, mass cytomet...

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Published inCytometry. Part A Vol. 81A; no. 7; pp. 552 - 566
Main Authors Behbehani, Gregory K., Bendall, Sean C., Clutter, Matthew R., Fantl, Wendy J., Nolan, Garry P.
Format Journal Article
LanguageEnglish
Published Hoboken Wiley Subscription Services, Inc., A Wiley Company 01.07.2012
Subjects
Animals
Antibodies
Antibodies - chemistry
Bone Marrow Cells - metabolism
Bone Marrow Cells - physiology
cell cycle
Cell Cycle Checkpoints
Cell Differentiation
Cell Line
Cell Proliferation
Cell Separation
Cyclin A - metabolism
Cyclin B1 - metabolism
DNA Replication
Flow Cytometry
Hematopoiesis
Histones - metabolism
Humans
Immunophenotyping
iododeoxyuridine
mass cytometry
Membrane Proteins - metabolism
Mice
retinoblastoma
Retinoblastoma Protein - metabolism
Single-Cell Analysis - methods
Staining and Labeling
T-Lymphocytes - metabolism
T-Lymphocytes - physiology
Transition Elements - chemistry
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Summary:Mass cytometry is a recently introduced technology that utilizes transition element isotope‐tagged antibodies for protein detection on a single‐cell basis. By circumventing the limitations of emission spectral overlap associated with fluorochromes utilized in traditional flow cytometry, mass cytometry currently allows measurement of up to 40 parameters per cell. Recently, a comprehensive mass cytometry analysis was described for the hematopoietic differentiation program in human bone marrow from a healthy donor. The current study describes approaches to delineate cell cycle stages utilizing 5‐iodo‐2‐deoxyuridine (IdU) to mark cells in S phase, simultaneously with antibodies against cyclin B1, cyclin A, and phosphorylated histone H3 (S28) that characterize the other cell cycle phases. Protocols were developed in which an antibody against phosphorylated retinoblastoma protein (Rb) at serines 807 and 811 was used to separate cells in G0 and G1 phases of the cell cycle. This mass cytometry method yielded cell cycle distributions of both normal and cancer cell populations that were equivalent to those obtained by traditional fluorescence cytometry techniques. We applied this to map the cell cycle phases of cells spanning the hematopoietic hierarchy in healthy human bone marrow as a prelude to later studies with cancers and other disorders of this lineage. © 2012 International Society for Advancement of Cytometry
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ISSN:1552-4922
1552-4930
DOI:10.1002/cyto.a.22075