CD34 positive PBPC expanded ex vivo may not provide durable engraftment following myeloablative chemoradiotherapy regimens

Holyoake, Tessa L.; Alcorn, M.; Richmond, Linda; Farrell, Elizabeth; Pearson, C.; Green, R; Dunlop, DJ; Fitzsimons, Edward J.; Pragnell, Ian B.; Franklin, I. M.

doi:10.1038/sj.bmt.1700799

Cited by 107 publications

(78 citation statements)

References 1 publication

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“…Williams et al 26 obtained substantial expansion of myeloid precursors in ex vivo bag cultures of CD34 + leukapheresis cells stimulated with PIXY and subsequent prompt neutrophil recovery in graft recipients. Using other stimulating factors, Holyoake et al 27 reported similar results for the early phase of hematopoietic recovery in four patients. However, further investigations will be necessary to demonstrate the capacity of these expanded cells to induce long-term engraftment in patients who have undergone true myeloablative conditioning.…”

Section: Discussionsupporting

confidence: 61%

Cell culture bags allow a large extent of ex vivo expansion of LTC-IC and functional mature cells which can subsequently be frozen: interest for large-scale clinical applications

Giarratana

Kobari

Nguyen

et al. 1998

Bone Marrow Transplant

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Summary:The aim of this study was to evaluate the ex vivo expansion of normal CD34 + cells in gas-permeable polypropylene bags suitable for clinical use. Cells were cultured for 14 days in serum-free medium supplemented with SCF, IL3, IL6, FLT3-l, G-CSF ؎ MGDF or Epo. The bags supported the expansion of hematopoietic cells in a similar manner to small scale well or flask systems, allowing mean expansions of up to 2193-fold for total nucleated cells, 140-fold for CFU-GM and 66-fold for LTC-IC. Increasing the initial cell concentration from 5 × 10 3 to 1 × 10 5 CD34 + cells/ml induced the production of granulocytic cells with terminal differentiation while simultaneously decreasing the overall extent of expansion of the white blood cells produced. We tested the phagocytic activity and oxidative metabolism of the white blood cells produced. The percentage of phagocytic cells was 39 ؎ 0.5% in expanded cultures derived from fractions initiated at 5 × 10 3 , 10 4 or 10 5 cells/ml and 45 ؎ 6% in cultured cells obtained from starting fractions containing 5 × 10 4 cells/ml, as compared to 58 ؎ 4% in normal controls. A study of the potential for oxygen-dependent microbe killing showed that the expanded cells produced H 2 O 2 , although in lesser quantities than control cells. We subsequently investigated the possibility of freezing expanded cells. Total cell recovery after thawing was 45 ؎ 4%, while recoveries of progenitors and stem cells ranged from 65 to 90%, without any influence of the initial cell concentration. This new approach could be of major interest for clinical practice, as it would allow evaluation of the quality of a graft prior to its infusion and employs experimental conditions which meet the criteria for potential clinical use.

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Section: Discussionsupporting

confidence: 61%

Cell culture bags allow a large extent of ex vivo expansion of LTC-IC and functional mature cells which can subsequently be frozen: interest for large-scale clinical applications

Giarratana

Kobari

Nguyen

et al. 1998

Bone Marrow Transplant

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“…Current methods to ex vivo expand umbilical cord blood cells may introduce defects that lead to engraftment failures as has been reported using expanded 25 or transduced 29 autologous CD34 þ cells. Guenechea et al 30 transplanted fresh and ex vivo-expanded CD34 þ cord blood cells into irradiated non-obese diabetic (NOD)/SCID mice and while they found no differences in engraftment at 4 months, engraftment at 3 weeks was impaired when the expanded cells were used, suggesting that expanded cells might do not facilitate engraftment.…”

Section: Assessment Of Engraftmentmentioning

confidence: 99%

“…Stem cell assays to evaluate UCB expansion With the clinical failure of ex vivo expansion when the expanded product was used as the sole stem cell source 25 and the lack of improvement when the manipulated and unmanipulated products were both infused, 21,24 the current preclinical models and predictive assays for engraftment of all cell lineages deserve further development. Long-term engraftment is dependent upon the number and engraftment ability of the HSC transplanted; therefore, the ideal assay for this purpose must be simple, quantitative and reliably demonstrate engraftment capacity.…”

Section: Current Needs For Successful Hsc Expansionmentioning

confidence: 99%

Ex vivo expansion of umbilical cord blood stem cells for transplantation: growing knowledge from the hematopoietic niche

Hofmeister

Zhang

Knight

et al. 2006

Bone Marrow Transplant

198

172

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Umbilical cord blood transplantation (UCBT) in adults is limited by the small number of primitive hematopoietic stem cells (HSC) in each graft, resulting in delayed engraftment post transplant, and both short-and longterm infectious complications. Initial efforts to expand UCB progenitors ex vivo have resulted in expansion of mature rather than immature HSC, confounded by the inability to accurately and reliably measure long-term reconstituting cells. Ex vivo expansion of UCB HSC has failed to improve engraftment because of resulting defects that promote apoptosis, disrupt marrow homing and initiate cell cycling. Here we discuss the future of ex vivo expansion, which we suggest will include the isolation of immature hematopoietic progenitors on the basis of function rather than surface phenotype and will employ both cytokines and stroma to maintain and expand the stem cell niche. We suggest that ex vivo expansion could be enhanced by manipulating newly discovered signaling pathways (Notch, Wnt, bone morphogenetic protein 4 and Tie2/angiopoietin-1) and intracellular mediators (phosphatase and tensin homolog and glycogen synthase kinase-3) in a manner that promotes HSC expansion with less differentiation. Improved methods for ex vivo expansion will make UCBT available to more patients, decrease engraftment times and allow more rapid immune reconstitution post transplant.

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“…Autologous progeny cells after culture/expansion in cytokine combination including IL-3 have been successfully infused into patients after a nonmyeloablative conditioning regimen [18]. In another study, when patients were given a myeloablative conditioning regimen, cells expanded in IL-3-containing cytokines failed to produce engraftment [19]. More recent data indicated that culture in IL-3 led to a decrease or loss of primitive hematopoietic cells with reconstitution potential [20][21][22][23].…”

Section: Introductionmentioning

confidence: 99%

Correlation Between IL‐3 Receptor Expression and Growth Potential of Human CD34 ⁺ Hematopoietic Cells from Different Tissues

Huang¹,

Chen²,

Yu³

et al. 1999

STEM CELLS

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CD123 (␣-subunit of IL-3 receptor) expression on primitive and committed human hematopoietic cells was studied by multicolor sorting and single-cell culture. The sources of cells included fetal liver (FLV), fetal bone marrow, umbilical cord blood, adult bone marrow and mobilized peripheral blood. Three subsets of CD34 + cells were defined by the levels of surface CD123: CD123 negative , CD123 low , and CD123 bright . Coexpression of lineage markers showed that a majority of CD34 + CD123 bright cells were myeloid and B-lymphoid progenitors, while erythroid progenitors were mainly in the CD34 + CD123 negative subset. The CD34 + CD123 low subset contained a heterogeneous distribution of early and committed progenitor cells. Single CD34 + cells from the CD123 subsets were cultured in a cytokine cocktail of stem cell factor, interleukin 3 (IL-3), IL-6, GM-CSF, erythropoietin, insulin-like growth factor-1, and basic fibroblast growth factor. After 14 days of incubation, a higher cloning efficiency (CE) was observed in the CD34 + CD123 negative and CD34 + CD123 low fractions (37 ± 23% and 44 ± 23%, respectively) than in the CD34 + CD123 bright fraction (15 ± 21%). Using previously published criteria that colonies containing dispersed, translucent cells (dispersed growth pattern, DGP) were derived from primitive cells and that colonies composed solely of clusters were from committed cells, early precursors were distributed evenly in the CD34 + CD123 negative and CD34 + CD123 low subsets. When CD38 and CD90 (Thy-1) were used for further characterization of CD34 + cells from FLV, CE increased from 37 ± 23% in CD123 negative to 70 ± 19% in CD123 negative CD38 -and from 44 ± 23% in CD123 low to 66 ± 19% in CD123 low CD38 -. No significant increase in CE or DGP progenitors was observed when CD34 + cells were sorted by CD90 and CD123. We concluded that: A) high levels of CD123 were expressed on B-lymphoid and myeloid progenitors; B) early erythroid progenitors had little or no surface CD123, and C) primitive hematopoietic cells are characterized by CD123 negative/low expression.

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CD34 positive PBPC expanded ex vivo may not provide durable engraftment following myeloablative chemoradiotherapy regimens

Cited by 107 publications

References 1 publication

Cell culture bags allow a large extent of ex vivo expansion of LTC-IC and functional mature cells which can subsequently be frozen: interest for large-scale clinical applications

Cell culture bags allow a large extent of ex vivo expansion of LTC-IC and functional mature cells which can subsequently be frozen: interest for large-scale clinical applications

Ex vivo expansion of umbilical cord blood stem cells for transplantation: growing knowledge from the hematopoietic niche

Correlation Between IL‐3 Receptor Expression and Growth Potential of Human CD34 ⁺ Hematopoietic Cells from Different Tissues

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CD34 positive PBPC expanded ex vivo may not provide durable engraftment following myeloablative chemoradiotherapy regimens

Cited by 107 publications

References 1 publication

Cell culture bags allow a large extent of ex vivo expansion of LTC-IC and functional mature cells which can subsequently be frozen: interest for large-scale clinical applications

Cell culture bags allow a large extent of ex vivo expansion of LTC-IC and functional mature cells which can subsequently be frozen: interest for large-scale clinical applications

Ex vivo expansion of umbilical cord blood stem cells for transplantation: growing knowledge from the hematopoietic niche

Correlation Between IL‐3 Receptor Expression and Growth Potential of Human CD34 + Hematopoietic Cells from Different Tissues

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Product

Resources

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Correlation Between IL‐3 Receptor Expression and Growth Potential of Human CD34 ⁺ Hematopoietic Cells from Different Tissues