Literature DB >> 26305912

Endothelial progenitor cells, defined by the simultaneous surface expression of VEGFR2 and CD133, are not detectable in healthy peripheral and cord blood.

Paola Lanuti1,2, Gianluca Rotta3, Camillo Almici4, Giuseppe Avvisati5, Alfredo Budillon6, Paolo Doretto7, Natalia Malara8,9, Mirella Marini4, Arabella Neva4, Pasquale Simeone1,2, Elena Di Gennaro6, Alessandra Leone6, Alessandra Falda7, Renato Tozzoli7, Chiara Gregorj5, Melania Di Cerbo5, Valentina Trunzo8, Vincenzo Mollace8, Marco Marchisio1,2, Sebastiano Miscia1,2.   

Abstract

Circulating endothelial cells (CEC) and their progenitors (EPC) are restricted subpopulations of peripheral blood (PB), cord blood (CB), and bone marrow (BM) cells, involved in the endothelial homeostasis maintenance. Both CEC and EPC are thought to represent potential biomarkers in several clinical conditions involving endothelial turnover/remodeling. Although different flow cytometry methods for CEC and EPC characterization have been published so far, none of them have reached consistent conclusions, therefore consensus guidelines with respect to CEC and EPC identification and quantification need to be established. Here, we have carried out an in depth investigation of CEC and EPC phenotypes in healthy PB, CB and BM samples, by optimizing a reliable polychromatic flow cytometry (PFC) panel. Results showed that the brightness of CD34 expression on healthy PB and CB circulating cells represents a key benchmark for the identification of CEC (CD45neg/CD34bright/CD146pos) respect to the hematopoietic stem cell (HSC) compartment (CD45dim/CD34pos/CD146neg). This approach, combined with a dual-platform counting technique, allowed a sharp CEC enumeration in healthy PB (n = 38), and resulting in consistent CEC counts with previously reported data (median = 11.7 cells/ml). In parallel, by using rigorous PFC conditions, CD34pos/CD45dim/CD133pos/VEGFR2pos EPC were not found in any healthy PB or CB sample, since VEGFR2 expression was never detectable on the surface of CD34pos/CD45dim/CD133pos cells. Notably, the putative EPC phenotype was observed in all analyzed BM samples (n = 12), and the expression of CD146 and VEGFR2, on BM cells, was not restricted to the CD34bright compartment, but also appeared on the HSC surface. Altogether, our findings suggest that the previously reported EPC antigen profile, defined by the simultaneous expression of VEGFR2 and CD133 on the surface of CD45dim/CD34pos cells, should be carefully re-evaluated and further studies should be conducted to redefine EPC features in order to translate CEC and EPC characterization into clinical practice.
© 2015 International Society for Advancement of Cytometry.

Entities:  

Keywords:  CD133; circulating endothelial cells; endothelial progenitor cells; polychromatic flow cytometry; vascular endothelial growth factor receptor 2

Mesh:

Substances:

Year:  2015        PMID: 26305912     DOI: 10.1002/cyto.a.22730

Source DB:  PubMed          Journal:  Cytometry A        ISSN: 1552-4922            Impact factor:   4.355


  22 in total

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7.  Effect of peritoneal dialysis fluid containing osmo-metabolic agents on human endothelial cells.

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Review 8.  Progenitor Cells for Arterial Repair: Incremental Advancements towards Therapeutic Reality.

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9.  Microvesicles Derived from Indoxyl Sulfate Treated Endothelial Cells Induce Endothelial Progenitor Cells Dysfunction.

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10.  Guidelines for the use of flow cytometry and cell sorting in immunological studies (second edition).

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