Use of limiting-dilution type long-term marrow cultures in frequency analysis of marrow-repopulating and spleen colony-forming hematopoietic stem cells in the mouse

Ploemacher, R. E.; Sluijs, JP Van der; Beurden, CA van; Baert, MR; Pl, Chan

doi:10.1182/blood.v78.10.2527.bloodjournal78102527

Cited by 12 publications

(7 citation statements)

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“…Figure 2 shows that, after administration of G-CSF, very few CAFC subsets were detected. In sharp contrast, administration of SD/01 resulted in a massive increase of all CAFC subsets, including large numbers of late-appearing colonies that have been associated with cells with long-term repopulating ability (Ploemacher et al, 1991).…”

Section: Mobilization Potential Of G-csf and Sd/01 On Primitive Cell mentioning

confidence: 90%

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Efficient mobilization of haematopoietic progenitors after a single injection of pegylated recombinant human granulocyte colony‐stimulating factor in mouse strains with distinct marrow‐cell pool sizes

et al. 2000

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We have compared the efficacy of a single injection of SD/01, a newly engineered, pegylated form of recombinant human granulocyte colony stimulating factor (rhG‐CSF), with a single injection of glycosylated rhG‐CSF (Filgrastim). SD/01 was administered to regular and recombinant inbred strains of mice (AKR, C57L/J, DBA/2, C57BL/6, AKXL) known to have widely distinct marrow‐cell pool sizes and proliferation kinetics. A single injection of G‐CSF was unable to mobilize granulocyte–macrophage colony‐forming units (CFU‐GM). In sharp contrast, a single dose of SD/01 resulted in massive mobilization of progenitors and stem cells. Although all mice strains showed qualitatively similar mobilization responses, large interstrain differences remained. C57L and C57BL/6 mice mobilized relatively poorly, whereas AKR and DBA/2 mice showed threefold to tenfold superior responses. In order to explain these different phenotypes, we studied the effects of SD/01 in nine AKXL recombinant inbred strains, derived from well‐responding AKR and poorly responding C57L parental strains. The best predictor for SD/01 responsiveness in these strains was marrow cellularity prior to mobilization. Comparison of the AKXL strain distribution pattern for marrow cellularity with loci previously mapped in these strains showed complete concordance with Aat, a serine protease inhibitor mapping to chromosome 12.

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Section: Mobilization Potential Of G-csf and Sd/01 On Primitive Cell mentioning

confidence: 90%

“…For each of the six cell dilutions used, ten replicate wells were tested. Early appearing CAFCs (d 7) corresponded to relatively committed progenitor cells, whereas late-appearing CAFCs (d 35) reflected more primitive cell subsets (Ploemacher et al, 1991).…”

Section: Methodsmentioning

confidence: 99%

Efficient mobilization of haematopoietic progenitors after a single injection of pegylated recombinant human granulocyte colony‐stimulating factor in mouse strains with distinct marrow‐cell pool sizes

et al. 2000

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“…No significant differences were observed between the genotypes in colony number ( Fig.2b ), morphology or size. Similarly, analysis of the more primitive cell fraction using the long-term culture initiating cell (LTC-IC) assay 10 , demonstrated no significant differences between the WT and KO cells ( Fig.2c ). Taken together, these data demonstrate that deletion of the G s α gene does not alter the differentiation potential of primitive BM MNCs in vitro .…”

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confidence: 88%

Haematopoietic stem cells depend on Gαs-mediated signalling to engraft bone marrow

Adams

Alley²,

Chung

et al. 2009

Nature

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Hematopoietic stem/progenitor cells (HSPC) transition in location during development1 and circulate in mammals throughout life2, moving into and out of the bloodstream to engage bone marrow (BM) niches in sequential steps of homing, engraftment and retention3–5. We show here that HSPC engraftment of BM in fetal development is dependent upon the guanine nucleotide binding protein stimulatory alpha subunit (Gsα). Adult Gsα−/− HSPCs differentiate and undergo chemotaxis, but also do not home to or engraft in the BM in adult mice and demonstrate marked inability to engage the marrow microvasculature. If deleted after engraftment, Gsα did not lead to lack of retention in the marrow, rather cytokine-induced mobilization into the blood was impaired. Testing whether activation of Gsα affects HSPC, pharmacologic activators enhanced homing and engraftment in vivo. Gsα governs specific aspects of HSPC localization under physiologic conditions in vivo and may be pharmacologically targeted to improve transplantation efficiency.

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“…More specifically, during long-term co-culture we observed clusters of phase-dark cells beneath the stromal layer. These clusters are morphologically similar to CAFC that form under stromal cell monolayer when normal HSC are co-cultured with BM stromal cells [25] , [44] , [46] . In this study, immunophenotypic characterization of MCL associated CAFCs reveal that these clusters are composed of cells with a unique and primitive phenotype (CD45+CD19−CD133+) compared to cells that remain in suspension and the bulk population (CD45+CD19+CD133−).…”

Section: Discussionmentioning

confidence: 66%

Cobblestone-Area Forming Cells Derived from Patients with Mantle Cell Lymphoma Are Enriched for CD133+ Tumor-Initiating Cells

et al. 2014

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Mantle cell lymphoma (MCL) is associated with a significant risk of therapeutic failure and disease relapse, but the biological origin of relapse is poorly understood. Here, we prospectively identify subpopulations of primary MCL cells with different biologic and immunophenotypic features. Using a simple culture system, we demonstrate that a subset of primary MCL cells co-cultured with either primary human mesenchymal stromal cells (hMSC) or murine MS-5 cells form in cobblestone-areas consisting of cells with a primitive immunophenotype (CD19−CD133+) containing the chromosomal translocation t (11;14)(q13;q32) characteristic of MCL. Limiting dilution serial transplantation experiments utilizing immunodeficient mice revealed that primary MCL engraftment was only observed when either unsorted or CD19−CD133+ cells were utilized. No engraftment was seen using the CD19+CD133− subpopulation. Our results establish that primary CD19−CD133+ MCL cells are a functionally distinct subpopulation of primary MCL cells enriched for MCL-initiating activity in immunodeficient mice. This rare subpopulation of MCL-initiating cells may play an important role in the pathogenesis of MCL.

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Use of limiting-dilution type long-term marrow cultures in frequency analysis of marrow-repopulating and spleen colony-forming hematopoietic stem cells in the mouse

Cited by 12 publications

References 0 publications

Efficient mobilization of haematopoietic progenitors after a single injection of pegylated recombinant human granulocyte colony‐stimulating factor in mouse strains with distinct marrow‐cell pool sizes

Efficient mobilization of haematopoietic progenitors after a single injection of pegylated recombinant human granulocyte colony‐stimulating factor in mouse strains with distinct marrow‐cell pool sizes

Haematopoietic stem cells depend on Gαs-mediated signalling to engraft bone marrow

Cobblestone-Area Forming Cells Derived from Patients with Mantle Cell Lymphoma Are Enriched for CD133+ Tumor-Initiating Cells

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