Isolation of large numbers of enriched human megakaryocytes from liquid cultures of normal peripheral blood progenitor cells

Mazur, EM; Basilico, David; Newton, JL; Cohen, Joseph L.; Sohl, PA; Narendran, A

doi:10.1182/blood.v76.9.1771.bloodjournal7691771

Cited by 5 publications

(7 citation statements)

References 2 publications

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“…Megakaryocyte culture media consisted of IMDM (GIBCO, Grand Island, NY) supplemented with 1% Glutamine Pen-strep (Irvine Scientific, Santa Ana, CA). Preliminary experiments indicated that 20-30% normal, heparinized, platelet-poor, human AB plasma was required for megakaryocyte development, in agreement with other reports [16][17][18]. By including the following components of a serum-free culture system, the optimal concentration of human plasma could be reduced to 10%: 2-mercaptoethanol ( lo4 M), pyruvic acid (1 10 mg/ml), cholesterol (7.8 mg/ml), adenosine, guanine, cytidine, uridine, thymidine, 2-deoxycytosine, 2-deoxyadenosine, 2-deoxyguanosine (10 mg/ml each, Sigma); human recombinant insulin (10 mg/ml), human transferrin (300 mg/ml), soybean lipids (1%, Boehringer Mannheim, Indianapolis, IN); human recombinant basic fibroblast growth factor ( 2 ng/ml, Genzyme, Cambridge, MA); human recombinant epidermal growth factor (15 ng/ml), platelet-derived growth factor (10 ng/ml, Amgen, Inc., Thousand Oaks, CA).…”

Section: Mediasupporting

confidence: 90%

“…Cells fractionated by CCE were plated at 1.25 and 2.5 x lOs/ml in triplicate. The culture consisted of 15% citrated, platelet-poor, human AB plasma in Iscove's modified Dulbecco's medium (IMDM) with additives as described by Mazur et al [16] and incubated 12 days at 3 7 T , 5% C 0 2 in air. Plates were subsequently fixed with methanol:acetone, stained with antibodies to GPIb and GPIIb/IIIa (Biodesign, Kennebunkport, ME) and a secondary goat anti-mouse fluorescent isothiocyanate ([FITC], Southern Biotechnology Assoc., Inc., Birmingham, AL).…”

Section: Megakaryocyte Progenitor Cell Assaymentioning

confidence: 99%

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Enrichment and characterization of peripheral blood‐derived megakaryocyte progenitors that mature in short‐term liquid culture

et al. 1994

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A population of peripheral blood-derived cells that mature into megakaryocytes within four to eight days of liquid culture is described. This population was enriched from normal leukapheresis units by counterflow centrifugal elutriation and CD34 selection. The cells were incubated in suspension with known megakaryocyte growth or maturation factors. Megakaryocytes were identified within the cultures with antibodies to platelet-glycoproteins (Ib and IIb) and cytologically classified as stage I-IV cells. Plasma from aplastic dogs (APK9) or human recombinant interleukin 3 (IL-3) were the only culture additives which reproducibly resulted in megakaryocyte development. The activity present in APK9 was relatively megakaryocyte-specific while IL-3 was not. The phenotype of the short-term megakaryocyte progenitor cell population was determined by FACS and found to be CD34bright but not CD34dull or CD34-. The population was further characterized as CD34+/CD38+ and CD34+/HLA-DR+. Both CD34+/CD41- and CD34+/CD41+ populations contained megakaryocyte progenitor cells, although megakaryocytes that developed from the latter population were fewer in number. In summary, we have developed an enrichment protocol that, when coupled with a liquid culture assay system, enabled us to characterize short-term megakaryocyte progenitors from peripheral blood. These cells may be important for early platelet recovery in transplantation settings.

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Section: Mediasupporting

confidence: 90%

Section: Megakaryocyte Progenitor Cell Assaymentioning

confidence: 99%

Enrichment and characterization of peripheral blood‐derived megakaryocyte progenitors that mature in short‐term liquid culture

et al. 1994

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“…An average of 4.4 rt 0.3 x lo6 CD34' cells were obtained per unit (n = 25), with an average purity of 90 f 5% (n = 12). Cells were frozen until use [38] then thawed and plated at 5 x 106/ml in megakaryocyte growth medium (meg-GM) [31] with 10% normal human AB plasma (HuAB) [39] and 10 ng/ml purified, mammalian cell-derived, rHuMGDF [ 11. After eight days, cultures were transferred to fresh culture wells and supplemented with 20-50% fresh meg-GM + 10% HuAB. Cultures were monitored for the appearance of proplatelets which occurred one to three days after replating.…”

Section: Cd34+ Cell Isolation and Culture Conditionsmentioning

confidence: 99%

Recombinant human megakaryocyte growth and development factor (rhumgdf), a ligand for c‐mpl, produces functional human platelets in vitro

et al. 1995

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Platelet formation, occurring from bone marrow or lung megakaryocytes, has been difficult to study mechanistically. Recombinant human megakaryocyte growth and development factor (rHuMGDF), a recently described cytokine, has now been used to establish an in vitro system in which this important and little understood process occurs. CD34+ cells cultured with rHuMGDF develop into megakaryocytes which form long cytoplasmic extensions (proplatelets) that fragment into platelet-sized particles (in vitro platelets). Morphologically, in vitro and human plasma-derived platelets (control platelets) are virtually identical with respect to size, dense granule distribution and ultrastructural features. Functionally, in vitro and control platelets have similar aggregation and activation responses, and similarly incorporate mepacrine into dense granules. These findings suggest that rHuMGDF is sufficient to generate platelet-synthesizing megakaryocytes from CD34+ cells and provide an experimental setting in which the study of human platelet formation can be adequately performed.

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“…Cord blood (CB) represents a large and readily available source of HSC. Several investigators [3][4][5][6][7][8][9][10][11][12][13][14][15][16][17][18][19][20][21] have previously made efforts to obtain megakaryocytic progenitors from HSC in bone marrow, peripheral blood, or CB by using a liquid culture system. Furthermore, there have been some clinical trials in which in vitro expanded megakaryocytic progenitors were infused to patients receiving high-dose chemotherapy.…”

Section: Introductionmentioning

confidence: 99%

Ex Vivo Large‐Scale Generation of Human Platelets from Cord Blood CD34 ⁺ Cells

et al. 2006

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Isolation of large numbers of enriched human megakaryocytes from liquid cultures of normal peripheral blood progenitor cells

Cited by 5 publications

References 2 publications

Enrichment and characterization of peripheral blood‐derived megakaryocyte progenitors that mature in short‐term liquid culture

Enrichment and characterization of peripheral blood‐derived megakaryocyte progenitors that mature in short‐term liquid culture

Recombinant human megakaryocyte growth and development factor (rhumgdf), a ligand for c‐mpl, produces functional human platelets in vitro

Ex Vivo Large‐Scale Generation of Human Platelets from Cord Blood CD34 ⁺ Cells

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Isolation of large numbers of enriched human megakaryocytes from liquid cultures of normal peripheral blood progenitor cells

Cited by 5 publications

References 2 publications

Enrichment and characterization of peripheral blood‐derived megakaryocyte progenitors that mature in short‐term liquid culture

Enrichment and characterization of peripheral blood‐derived megakaryocyte progenitors that mature in short‐term liquid culture

Recombinant human megakaryocyte growth and development factor (rhumgdf), a ligand for c‐mpl, produces functional human platelets in vitro

Ex Vivo Large‐Scale Generation of Human Platelets from Cord Blood CD34 + Cells

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Ex Vivo Large‐Scale Generation of Human Platelets from Cord Blood CD34 ⁺ Cells