Isolation and enumeration of circulating endothelial cells by immunomagnetic isolation: proposal of a definition and a consensus protocol
Background: Circulating endothelial cells (CECs) have been identified as markers of vascular damage in a variety of disorders, such as myocardial infarction, vasculitis, and transplantation. CD146‐driven immunomagnetic isolation has gained widespread use, but the technique is hampered by the lack of...
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| Veröffentlicht in: | Journal of thrombosis and haemostasis 2006-03, Vol.4 (3), p.671-677 |
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| container_title | Journal of thrombosis and haemostasis |
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| creator | WOYWODT, A. BLANN, A. D. KIRSCH, T. ERDBRUEGGER, U. BANZET, N. HAUBITZ, M. DIGNAT‐GEORGE, F. |
| description | Background: Circulating endothelial cells (CECs) have been identified as markers of vascular damage in a variety of disorders, such as myocardial infarction, vasculitis, and transplantation. CD146‐driven immunomagnetic isolation has gained widespread use, but the technique is hampered by the lack of a definition of CECs and the absence of a consensus for their enumeration. Aim: To evaluate several variables influencing immunomagnetic isolation of CECs, formulate a definition for CECs and propose a consensus protocol for their enumeration. Methods: We devised a protocol based on CD146‐driven immunomagnetic isolation and a subsequent confirmatory step with Ulex‐Europaeus‐Lectin‐1 staining. In a multi‐center effort, we evaluated the preanalytical and analytical phases of this protocol. We evaluated the effects of storage, anticoagulation and density centrifugation, and compiled previous experience with this technique. Results: Our protocol permitted unequivocal identification of CECs with acceptable reproducibility. There was an effect of storage time in that median cell numbers declined to only 87.5% of their baseline values during 24 h of storage at 4 °C. Recovery was lower with citrate than with ethylene‐diamine tetra‐acetic acid after 4 h of storage; density centrifugation was also associated with lower recovery. We provide a comprehensive list of technical recommendations and potential pitfalls. Finally, based on our experience with this protocol and a recent consensus workshop, we formulated a working definition for CECs. Conclusion: Our work represents an important step toward consensus regarding the CECs. Our recommendations represent the experience of three major centers and should now be scrutinized by others in the field. |
| doi_str_mv | 10.1111/j.1538-7836.2006.01794.x |
| format | Article |
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In a multi‐center effort, we evaluated the preanalytical and analytical phases of this protocol. We evaluated the effects of storage, anticoagulation and density centrifugation, and compiled previous experience with this technique. Results: Our protocol permitted unequivocal identification of CECs with acceptable reproducibility. There was an effect of storage time in that median cell numbers declined to only 87.5% of their baseline values during 24 h of storage at 4 °C. Recovery was lower with citrate than with ethylene‐diamine tetra‐acetic acid after 4 h of storage; density centrifugation was also associated with lower recovery. We provide a comprehensive list of technical recommendations and potential pitfalls. Finally, based on our experience with this protocol and a recent consensus workshop, we formulated a working definition for CECs. Conclusion: Our work represents an important step toward consensus regarding the CECs. 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Aim: To evaluate several variables influencing immunomagnetic isolation of CECs, formulate a definition for CECs and propose a consensus protocol for their enumeration. Methods: We devised a protocol based on CD146‐driven immunomagnetic isolation and a subsequent confirmatory step with Ulex‐Europaeus‐Lectin‐1 staining. In a multi‐center effort, we evaluated the preanalytical and analytical phases of this protocol. We evaluated the effects of storage, anticoagulation and density centrifugation, and compiled previous experience with this technique. Results: Our protocol permitted unequivocal identification of CECs with acceptable reproducibility. There was an effect of storage time in that median cell numbers declined to only 87.5% of their baseline values during 24 h of storage at 4 °C. Recovery was lower with citrate than with ethylene‐diamine tetra‐acetic acid after 4 h of storage; density centrifugation was also associated with lower recovery. We provide a comprehensive list of technical recommendations and potential pitfalls. Finally, based on our experience with this protocol and a recent consensus workshop, we formulated a working definition for CECs. Conclusion: Our work represents an important step toward consensus regarding the CECs. Our recommendations represent the experience of three major centers and should now be scrutinized by others in the field.</description><subject>CD146 Antigen - analysis</subject><subject>CD146‐driven immunomagnetic separation</subject><subject>Cell Count - methods</subject><subject>Cell Size</subject><subject>circulating endothelial cells</subject><subject>Endothelial Cells - chemistry</subject><subject>Endothelial Cells - immunology</subject><subject>Endothelial Cells - pathology</subject><subject>endothelial damage Ulex Europaeus</subject><subject>Humans</subject><subject>Immunomagnetic Separation - methods</subject><subject>Immunophenotyping</subject><subject>Plant Lectins - analysis</subject><subject>Reproducibility of Results</subject><subject>standardization</subject><subject>Vascular Diseases - pathology</subject><issn>1538-7933</issn><issn>1538-7836</issn><issn>1538-7836</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2006</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNqNUUFOwzAQtBCIlsIXkE_cGuzEsR0kDqgCWlSJSzlbjuMUV4ld4kS0T-DXOKSFK754VzM7o9kFAGIU4fBuNxFOEz5lPKFRjBCNEGYZiXYnYPwLnB7rLElG4ML7DUI4S2N0DkaYEopIisbga-FdJVvjLJS2gNp2tW6G3pVQmUZ1PWzXASpc-64rIyuodFV5mO-hqevOulqurW6NguYodge3jds6H7hBRsJCl8aaXxsJlbNeW9_5ntg65apLcFbKyuurwz8Bb0-Pq9l8unx9XswellNFMCPTXKZxSstcZYQxmsecxpJRotMiCXExo5JJQkoqQ3ZEY44wT2mcUZxnlIehZAJuBt1g_NFp34ra-D6QtNp1XlBGE84zHoh8IKrGed_oUmwbU8tmLzAS_RnERvQbFv22RX8G8XMGsQuj1wePLq918Td42Hsg3A-ET1Pp_b-Fxctq3lfJN4B5mFA</recordid><startdate>200603</startdate><enddate>200603</enddate><creator>WOYWODT, A.</creator><creator>BLANN, A. 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| subjects | CD146 Antigen - analysis CD146‐driven immunomagnetic separation Cell Count - methods Cell Size circulating endothelial cells Endothelial Cells - chemistry Endothelial Cells - immunology Endothelial Cells - pathology endothelial damage Ulex Europaeus Humans Immunomagnetic Separation - methods Immunophenotyping Plant Lectins - analysis Reproducibility of Results standardization Vascular Diseases - pathology |
| title | Isolation and enumeration of circulating endothelial cells by immunomagnetic isolation: proposal of a definition and a consensus protocol |
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