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  • 1
    Online Resource
    Online Resource
    Interleukin-2 induces development of dendritic cells from cord blood CD34+ cells
    Oxford University Press (OUP) ; 1998
    In:  Journal of Leukocyte Biology Vol. 63, No. 5 ( 1998-05-01), p. 620-630
    Details
    In: Journal of Leukocyte Biology, Oxford University Press (OUP), Vol. 63, No. 5 ( 1998-05-01), p. 620-630
    Abstract: Dendritic cells (DC) have been shown to develop along a myeloid or lymphoid lineage of differentiation propagated from bone marrow or early thymic precursor cells with hematopoietic cytokines. In our study, we have induced growth and differentiation of DC from cord blood CD34+ cells initiated in interleukin-2 (IL-2) alone or in IL-2 + stem cell factor (SCF) + tumor necrosis factor α (TNF-α)-supplemented medium and cultured with IL-2 or IL-2 + SCF for 28–35 days. Dendritic morphology and antigenic phenotype of DC grown with IL-2 were characteristic for DC cultured in the presence of granulocyte-macrophage colony-stimulating factor (GM-CSF). Growth and differentiation of DC was followed by an increase in expression of MHC II and co-stimulating molecules CD80 and CD86. We have also shown the expression of the IL-2 receptor (IL-2R) γ-chain in CD34+ cells after 2–3 days of culture with IL-2 alone. The co-expression of the IL-2R α, β, and γ subunits in both DC cultured with IL-2- or GM-CSF-containing cocktail of cytokines was also shown. The time curve for induction of IL-2R demonstrated low levels of subunit expression at the beginning of culture. The number of CD1a cells coexpressing CD25, CD122, and CDγ increased to about 24–68 and to 78–95% after 21 and 28–35 days, respectively. Development of natural killer cells was shown along with DC. The proportion of CD56+ cells and cytotoxicity increased in a time-dependent manner.
    Type of Medium: Online Resource
    ISSN: 0741-5400 , 1938-3673
    URL: Article
    DOI: 10.1002/jlb.63.5.620
    RVK:
    XA 10000
    Language: English
    Publisher: Oxford University Press (OUP)
    Publication Date: 1998
    detail.hit.zdb_id: 2026833-6
    SSG: 12
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  • 2
    Online Resource
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    A suitable method for identifying cell aggregates in laser scanning cytometry listmode data for analyzing disaggregated cell suspensions obtained from human cancers
    Wiley ; 2004
    In:  Cytometry Part B: Clinical Cytometry Vol. 59B, No. 1 ( 2004-05), p. 10-23
    Details
    In: Cytometry Part B: Clinical Cytometry, Wiley, Vol. 59B, No. 1 ( 2004-05), p. 10-23
    Abstract: The presence of cell aggregates in cell suspensions obtained from human solid tumors can interfere with the measurement of cell DNA content of cell singlets, and can confound multiparameter analysis of other measurements on the same cells. Flow cytometric corrections for cell aggregates based on signal pulse shape have not proven to be reliable. Mathematical models have been developed to correct for cell aggregates in binned DNA histogram data, but they are not suitable for the correction of correlated non‐DNA measurements obtained on the same cells. Methods A total of 21 samples representing a variety of normal and malignant human cell types, including normal lymphocytes, normal sputum, human breast cancer cell lines, and mechanically disaggregated cell suspensions from primary breast cancers and nonsmall cell lung cancers, were studied by laser scanning cytometry (LSC) using the CompuCyte laser scanning cytometer (Cambridge, MA). Nuclear area, nuclear perimeter, and an LSC‐based cell texture parameter were measured on ≈400 cells in each sample, using an air‐cooled, violet laser emitting at a wavelength of 405 nm for DAPI excitation, and each cell was classified as a singlet or aggregate by its appearance under direct observation. A “saddle function” provided by CompuCyte was used, together with an algorithm based on the measurements of nuclear area, perimeter, and cell texture (the APT algorithm), to identify cell aggregates and exclude them from the listmode data file. Results Proportions of cell aggregates in the uncorrected samples ranging from 6 to 56% (mean, 20%) were reduced to proportions ranging from 0 to 7% (mean, 2.4%) after correction. The discriminant function was “tuned” to maintain both average cell singlet purity and average cell singlet yield at 〉 70% over a broad range of cell DNA contents. Conclusions A combined approach to cell aggregate detection, which utilizes both the saddle function and the APT algorithm, produces list mode data files that exclude 〉 80% of cell aggregates from samples of disaggregated cell suspensions of human tumors and other sources of clinical material. Such data files are suitable for multiparameter analysis. © 2004 Wiley‐Liss, Inc.
    Type of Medium: Online Resource
    ISSN: 1552-4949 , 1552-4957
    URL: Issue
    URL: Article
    DOI: 10.1002/cyto.b.v59b:1
    DOI: 10.1002/cyto.b.20009
    Language: English
    Publisher: Wiley
    Publication Date: 2004
    detail.hit.zdb_id: 2180651-2
    SSG: 12
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