pubmed-article:9028939 | rdf:type | pubmed:Citation | lld:pubmed |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C0018951 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C0002874 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C0024790 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C1522642 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C0221099 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C0334094 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C0332281 | lld:lifeskim |
pubmed-article:9028939 | lifeskim:mentions | umls-concept:C1457869 | lld:lifeskim |
pubmed-article:9028939 | pubmed:issue | 4 | lld:pubmed |
pubmed-article:9028939 | pubmed:dateCreated | 1997-3-17 | lld:pubmed |
pubmed-article:9028939 | pubmed:abstractText | Paroxysmal nocturnal hemoglobinuria (PNH) results from somatic mutations in the PIG-A gene, leading to poor presentation of glycosylphosphatidylinositol (GPI)-anchored surface proteins. PNH frequently occurs in association with suppressed hematopoiesis, including frank aplastic anemia (AA). The relationship between GPI-anchored protein expression and bone marrow (BM) failure is unknown. To assess the hematopoietic defect in PNH, the numbers of CD34+ cells, committed progenitors (primary colony-forming cells [CFCs]), and long-term culture-initiating cells (LTC-ICs; a stem cell surrogate) were measured in BM and peripheral blood (PB) of patients with PNH/AA syndrome or patients with predominantly hemolytic PNH. LTC-IC numbers were extrapolated from secondary CFC numbers after 5 weeks of culture, and clonogenicity of LTC-ICs was determined by limiting dilution assays. When compared with normal volunteers (n = 13), PNH patients (n = 14) showed a 4.7-fold decrease in CD34+ cells and an 8.2-fold decrease in CFCs. LTC-ICs in BM and in PB were decreased 7.3-fold and 50-fold, respectively. Purified CD34+ cells from PNH patients had markedly lower clonogenicity in both primary colony cultures and in the LTC-IC assays. As expected, GPI-anchored proteins were decreased on PB cells of PNH patients. On average, 23% of monocytes were deficient in CD14, and 47% of granulocytes and 58% of platelets lacked CD16 and CD55, respectively. In PNH BM, 27% of CD34+ cells showed abnormal GPI-anchored protein expression when assessed by CD59 expression. To directly measure the colony-forming ability of GPI-anchored protein-deficient CD34+ cells, we separated CD34+ cells from PNH patients for the GPI+ and GPI-phenotype; CD59 expression was chosen as a marker of the PNH phenotype based on high and homogeneous expression on fluorescent staining. CD34+ CD59+ and CD34+ CD59-cells from PNH/AA patients showed similarly impaired primary and secondary clonogeneic efficiency. The progeny derived from CD34+ CD59- cells were both CD59- and CD55-. A very small population of CD34+ CD59- cells was also detected in some normal volunteers; after sorting, these CD34+ CD59- cells formed normal numbers of colonies, but their progeny showed lower CD59 levels. Our results are consistent with the existence of PIG-A-deficient clones in some normal individuals. In PNH/AA, progenitor and stem cells are decreased in number and function, but the proliferation in vitro is affected similarly in GPI-protein-deficient clones and in phenotypically normal cells. As measured in the in vitro assays, expansion of PIG-A- clones appears not be caused by an intrinsic growth advantage of cells with the PNH phenotype. | lld:pubmed |
pubmed-article:9028939 | pubmed:language | eng | lld:pubmed |
pubmed-article:9028939 | pubmed:journal | http://linkedlifedata.com/r... | lld:pubmed |
pubmed-article:9028939 | pubmed:citationSubset | AIM | lld:pubmed |
pubmed-article:9028939 | pubmed:chemical | http://linkedlifedata.com/r... | lld:pubmed |
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pubmed-article:9028939 | pubmed:chemical | http://linkedlifedata.com/r... | lld:pubmed |
pubmed-article:9028939 | pubmed:status | MEDLINE | lld:pubmed |
pubmed-article:9028939 | pubmed:month | Feb | lld:pubmed |
pubmed-article:9028939 | pubmed:issn | 0006-4971 | lld:pubmed |
pubmed-article:9028939 | pubmed:author | pubmed-author:SatoTT | lld:pubmed |
pubmed-article:9028939 | pubmed:author | pubmed-author:AndersonSS | lld:pubmed |
pubmed-article:9028939 | pubmed:author | pubmed-author:YoungN SNS | lld:pubmed |
pubmed-article:9028939 | pubmed:author | pubmed-author:SloandE MEM | lld:pubmed |
pubmed-article:9028939 | pubmed:author | pubmed-author:MaciejewskiJ... | lld:pubmed |
pubmed-article:9028939 | pubmed:issnType | Print | lld:pubmed |
pubmed-article:9028939 | pubmed:day | 15 | lld:pubmed |
pubmed-article:9028939 | pubmed:volume | 89 | lld:pubmed |
pubmed-article:9028939 | pubmed:owner | NLM | lld:pubmed |
pubmed-article:9028939 | pubmed:authorsComplete | Y | lld:pubmed |
pubmed-article:9028939 | pubmed:pagination | 1173-81 | lld:pubmed |
pubmed-article:9028939 | pubmed:dateRevised | 2004-11-17 | lld:pubmed |
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pubmed-article:9028939 | pubmed:year | 1997 | lld:pubmed |
pubmed-article:9028939 | pubmed:articleTitle | Impaired hematopoiesis in paroxysmal nocturnal hemoglobinuria/aplastic anemia is not associated with a selective proliferative defect in the glycosylphosphatidylinositol-anchored protein-deficient clone. | lld:pubmed |
pubmed-article:9028939 | pubmed:affiliation | Hematology Branch, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, MD, USA. | lld:pubmed |
pubmed-article:9028939 | pubmed:publicationType | Journal Article | lld:pubmed |
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