Multicolor flow cytometry in clinical samples for platelet signaling assessment

被引:3
作者
Garcia, Cedric [1 ,2 ]
Dejean, Sebastien [3 ]
Savy, Nicolas [3 ]
Bordet, Jean-Claude [4 ,5 ]
Series, Jennifer [2 ]
Cadot, Sarah [2 ]
Ribes, Agnes [1 ,2 ,6 ]
Voisin, Sophie [1 ]
Rugeri, Lucia [4 ,7 ]
Payrastre, Bernard [1 ,2 ,6 ]
Sie, Pierre [1 ,2 ,8 ,9 ]
机构
[1] CHU Toulouse, Lab Hematol, Toulouse, France
[2] Univ Toulouse, Inst Malad Metab & Cardiovasc INSERM U1048, Toulouse, France
[3] Univ Paul Sabatier Toulouse III, Inst Math, CNRS UMR 5219, Toulouse, France
[4] Hosp Civiles Lyon, Lab Hematol, Lyon, France
[5] Univ Claude Bernard Lyon 1, EA 4609 Hemostase & Canc, Lyon, France
[6] Univ Paul Sabatier Toulouse III, Fac Med, Toulouse, France
[7] Hosp Civils Lyon, Unite Hemostase, Bron, France
[8] Univ Paul Sabatier Toulouse III, Fac Pharm, Toulouse, France
[9] Hop Rangueil, Ctr Reference Pathol Plaquettaires, Lab Hematol, TSA 50032, F-31059 Toulouse, France
关键词
TYROSINE-PHOSPHATASE CD148; VASP PHOSPHORYLATION; ACTIVATION;
D O I
10.1016/j.rpth.2023.100180
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
Background: Availability of multichannel cytometers and specific commercial antibodies makes flow cytometry a new option to simultaneously assess multiple intracellular platelet signaling pathways for clinical purposes, in small volume of blood or low platelet count.Objectives: To describe a multicolor flow cytometry with fluorescent barcoding technique for screening signaling pathways downstream membrane receptors of major platelet agonists (adenosine diphosphate, thrombin, thromboxane, and collagen). Methods: By comparison with immunoblotting, we first selected the target phosphoproteins, AKT, P38MAPK, LIMK, and SPL76; the times of stimulation; and phosphoflow barcoding conditions. We then performed a clinical study on whole blood of patients without evidence of blood platelet disorder on standard biological screening, consulting for trivial or occasionally provoked bleeds without familial antecedent (bleeding of unknown origin, n = 23) or type-1 von Willebrand disease (n = 9). In addition, we included a small group of patients with definite platelet disorders (Glanzmann thrombasthenia, & delta;-storage pool deficiency, and immune glycoprotein VI-related disease withResults: The range, kinetics, and distribution of fluorescence intensity were established for each agonist-target protein combination. Principal component analysis indicates a correlation in response to a target phosphoprotein (AKT and P38MAPK) to different agonists but no correlation in the response of different target phosphoproteins to the same agonist. The heterogeneity of individual responses in the whole population displayed was analyzed using clustering algorithm. Patients with platelet storage pool deficiency were positioned as lowest responders on the heatmap.Conclusion: In complement of functional tests, this study introduces a new approach for rapid platelet signaling profiling in clinical practice.
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页数:12
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