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Isolation of Murine Myeloid Progenitor Populations by CD34/CD150 Surface Markers.


ABSTRACT: Myeloid progenitors are intermediates between Hematopoietic Stem Cells (HSCs) and Myeloid effector progeny. In mouse bone marrow, they are part of the Lineage- cKit+ Sca1- (LK) compartment. To date, most researchers used CD34 and FcγR surface markers for the dissection of this compartment into various populations. Surprisingly, however, this approach does not provide distinct separation by fluorescence-activated cell sorting (FACS). In this study, we suggest using CD150 instead of FcγR. We re-analyzed published single-cell RNA-Seq data and found that CD34/CD150 provides better sub-populations separation, compared to the "classical" CD34/FcγR-based approach. We confirm our findings by independent FACS analysis. We demonstrate comparable differentiation potential of the newly-obtained LK sub-populations, like previous "classical" ones. Therefore, we suggest the CD34/CD150 gating strategy, utilizing commonly-used surface markers, as a robust and reproducible separation of the LK compartment into distinct sub-populations.

SUBMITTER: Olender L 

PROVIDER: S-EPMC8834359 | biostudies-literature | 2022 Jan

REPOSITORIES: biostudies-literature

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Isolation of Murine Myeloid Progenitor Populations by CD34/CD150 Surface Markers.

Olender Leonid L   Thapa Roshina R   Gazit Roi R  

Cells 20220120 3


Myeloid progenitors are intermediates between Hematopoietic Stem Cells (HSCs) and Myeloid effector progeny. In mouse bone marrow, they are part of the Lineage<sup>-</sup> cKit<sup>+</sup> Sca1<sup>-</sup> (LK) compartment. To date, most researchers used CD34 and FcγR surface markers for the dissection of this compartment into various populations. Surprisingly, however, this approach does not provide distinct separation by fluorescence-activated cell sorting (FACS). In this study, we suggest usin  ...[more]

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