RÉSUMÉ
BACKGROUND: Manufacture of platelet concentrates (PCs) and plasma may fail to remove all residual red blood cells (rRBCs). Measuring rRBCs for compliance to guidelines has proven challenging, leading to an absence of a consensus methodology. Sysmex hematology analyzers with the Blood Bank mode (BB mode) analysis option offer the potential for automated rRBC counting. We therefore performed a two-site appraisal of the system. STUDY DESIGN AND METHODS: Performance characteristics were determined using platelet and plasma samples spiked with RBCs. Sample stability (n = 47) and the impact of sample type were also assessed. Components (platelets, n = 1474; plasma, n = 77) prepared using different routine manufacturing methods were tested to assess variation in rRBC concentration. RESULTS: Linearity studies up to 19 000 RBCs/µL demonstrated good correlation between expected and observed results (R2 ≥ 0.9731), and flow cytometric results also correlated well with BB mode (R2 = 0.9400). Precision analysis gave a limit of quantitation of 6 to 7 RBCs/µL, and carryover was 0.03%. Ethylenediaminetetraacetic acid and plain tube results were not significantly different (P ≥ 0.10), and samples were stable up to 24 hours. Apheresis PCs produced at two sites had lower rRBC concentrations (medians, 17 and 13 RBCs/µL) than those produced with the buffy coat method either manually (median, 681 RBCs/µL) or with the automated Terumo Automated Centrifuge and Separator Integration process (median, 81 RBCs/µL). All PCs failing visual inspection as having RBCs ≥4000 RBCs/µL were also detected by the BB mode. CONCLUSION: The BB mode had acceptable performance characteristics and has the potential for integration into a fully automated process control system for rRBC enumeration in plasma and PCs.
Sujet(s)
Hémogramme/instrumentation , Transfusion de composants du sang , Numération des érythrocytes/méthodes , Érythrocytes , Anticoagulants , Automatisation , Buffy coat/cytologie , Aphérèse/méthodes , Acide édétique , Cytométrie en flux/instrumentation , Cytométrie en flux/méthodes , HumainsRÉSUMÉ
BACKGROUND: Leukoreduction of blood components was implemented to reduce transfusion-associated risks. The detection level for residual white blood cells (rWBCs) required to demonstrate leukoreduction was originally considered too low for hematology analyzers. Developments enabling cell counts in body fluids have, however, renewed interest in rWBC counting. An assessment of Sysmex XN hematology analyzers with software offering automated rWBC enumeration intended for use on blood components was performed. STUDY DESIGN AND METHODS: Performance characteristics were determined using platelet, red blood cell (RBC), and plasma samples spiked with WBCs. Subsequently, components (platelets, n = 1367; and plasma, n = 80) were tested and results compared with flow cytometry, to monitor leukoreduction efficiency to a level of less than 1 × 106 /unit. Components identified by flow cytometry as having poor leukoreduction, exceeding this limit, were also tested (platelets, n = 3; and RBCs, n = 10). RESULTS: Linearity studies up to 32 WBCs/µL showed good correlation between observed and expected results (R2 > 0.9996). Precision analysis gave an average limit of quantitation of 2 WBCs/µL with coefficients of variation less than 20%. Average carryover was 0.1%. Plain sample tubes were a source of aberrant results with routine components. Using ethylenediaminetetraacetic acid tubes the analyzer gave results greater than 1 × 106 /unit in 2.7% of cases compared with 1.4% by flow cytometry, but overall results were within specification, with more than 90% of components having rWBC values below the limit. All incidences of poor leukoreduction, with flow cytometry results greater than 13 rWBCs/µL were correctly identified, with an excellent correlation between results (R2 = 0.9818). CONCLUSION: The analyzer demonstrated acceptable performance characteristics for enumeration of rWBCs; consequently, additional multisite evaluations are warranted.
Sujet(s)
Cytométrie en flux , Leucocytes/cytologie , Contrôle de qualité , Logiciel , Femelle , Cytométrie en flux/instrumentation , Cytométrie en flux/méthodes , Humains , Numération des leucocytes/instrumentation , Numération des leucocytes/méthodes , Mâle , Reproductibilité des résultatsRÉSUMÉ
BACKGROUND: Neonatal haemorrhaging is often co-observed with thrombocytopenia; however, no evidence of a causal relationship with low platelet count has been reported. Regardless, the administration of a platelet transfusion is often based upon this parameter. Accurate measurement of platelet function in small volumes of adult blood samples by flow cytometry is well established and we propose that the use of the same technology could provide complementary information to guide the administration of platelet transfusions in premature neonates. METHODS: In 28 neonates born at 27-41 weeks gestation, platelet function after stimulation agonists was measured using fibrinogen binding and P-selectin expression (a marker of degranulation). RESULTS: Platelets of neonates with gestation of ≤36 weeks (n = 20) showed reduced fibrinogen binding and degranulation with ADP, and reduced degranulation with CRP-XL. Degranulation Scores of 7837 ± 5548, 22,408 ± 5301 and 53,131 ± 12,102 (mean ± SEM) identified significant differences between three groups: <29, 29-36 and >36 weeks gestation). Fibrinogen binding and degranulation responses to ADP were significantly reduced in suspected septic neonates (n = 6) and the Fibrinogen Binding scores clearly separated the septic and healthy group (88.2 ± 10.3 vs 38.6 ± 12.2, P = 0.03). CONCLUSIONS: Flow cytometric measurement of platelet function identified clinically different neonatal groups and may eventually contribute to assessment of neonates requiring platelet transfusion.
Sujet(s)
Cytométrie en flux/méthodes , Prématuré/sang , Tests fonctionnels plaquettaires/méthodes , Transfusion de plaquettes , Dégranulation cellulaire , Femelle , Fibrinogène/métabolisme , Hémorragie/sang , Hémorragie/thérapie , Humains , Nouveau-né , Mâle , Sepsis néonatal/sang , Sélectine P/sang , Activation plaquettaire , Numération des plaquettes , Tests fonctionnels plaquettaires/normes , Thrombocytopénie néonatale allo-immune/sang , Thrombocytopénie néonatale allo-immune/thérapieRÉSUMÉ
Linking non-coding genetic variants associated with the risk of diseases or disease-relevant traits to target genes is a crucial step to realize GWAS potential in the introduction of precision medicine. Here we set out to determine the mechanisms underpinning variant association with platelet quantitative traits using cell type-matched epigenomic data and promoter long-range interactions. We identify potential regulatory functions for 423 of 565 (75%) non-coding variants associated with platelet traits and we demonstrate, through ex vivo and proof of principle genome editing validation, that variants in super enhancers play an important role in controlling archetypical platelet functions.
Sujet(s)
Plaquettes/physiologie , Éléments activateurs (génétique) , Érythroblastes/composition chimique , Variation génétique , Mégacaryocytes/composition chimique , Chromatine , Humains , Régions promotrices (génétique)RÉSUMÉ
The effect of variation in platelet function in platelet donors on patient outcome following platelet transfusion is unknown. This trial assessed the hypothesis that platelets collected from donors with highly responsive platelets to agonists in vitro assessed by flow cytometry (high-responder donors) are cleared more quickly from the circulation than those from low-responder donors, resulting in lower platelet count increments following transfusion. This parallel group, semirandomized double-blinded trial was conducted in a single center in the United Kingdom. Eligible patients were those 16 or older with thrombocytopenia secondary to bone marrow failure, requiring prophylactic platelet transfusion. Patients were randomly assigned to receive a platelet donation from a high- or low-responder donor when both were available, or when only 1 type of platelet was available, patients received that. Participants, investigators, and those assessing outcomes were masked to group assignment. The primary end point was the platelet count increment 10 to 90 minutes following transfusion. Analysis was by intention to treat. Fifty-one patients were assigned to receive platelets from low-responder donors, and 49 from high-responder donors (47 of which were randomized and 53 nonrandomized). There was no significant difference in platelet count increment 10 to 90 minutes following transfusion in patients receiving platelets from high-responder (mean, 21.0 × 109/L; 95% confidence interval [CI], 4.9-37.2) or low-responder (mean, 23.3 × 109/L; 95% CI, 7.8-38.9) donors (mean difference, 2.3; 95% CI, -1.1 to 5.7; P = .18). These results support the current policy of not selecting platelet donors on the basis of platelet function for prophylactic platelet transfusion.
Sujet(s)
Hémorragie/prévention et contrôle , Transfusion de plaquettes , Thrombopénie/thérapie , Donneurs de tissus/classification , Adulte , Sujet âgé , Anémie aplasique/sang , Anémie aplasique/complications , Anémie aplasique/anatomopathologie , Plaquettes/cytologie , Plaquettes/effets des médicaments et des substances chimiques , Plaquettes/physiologie , Maladies de la moelle osseuse/sang , Maladies de la moelle osseuse/complications , Maladies de la moelle osseuse/anatomopathologie , Aplasies médullaires , Méthode en double aveugle , Femelle , Hémoglobinurie paroxystique/sang , Hémoglobinurie paroxystique/complications , Hémoglobinurie paroxystique/anatomopathologie , Hémorragie/sang , Humains , Analyse en intention de traitement , Mâle , Adulte d'âge moyen , Facteur d'activation plaquettaire/pharmacologie , Activation plaquettaire/effets des médicaments et des substances chimiques , Numération des plaquettes , Tests fonctionnels plaquettaires , Thrombopénie/sang , Thrombopénie/étiologie , Thrombopénie/anatomopathologieRÉSUMÉ
Many common variants have been associated with hematological traits, but identification of causal genes and pathways has proven challenging. We performed a genome-wide association analysis in the UK Biobank and INTERVAL studies, testing 29.5 million genetic variants for association with 36 red cell, white cell, and platelet properties in 173,480 European-ancestry participants. This effort yielded hundreds of low frequency (<5%) and rare (<1%) variants with a strong impact on blood cell phenotypes. Our data highlight general properties of the allelic architecture of complex traits, including the proportion of the heritable component of each blood trait explained by the polygenic signal across different genome regulatory domains. Finally, through Mendelian randomization, we provide evidence of shared genetic pathways linking blood cell indices with complex pathologies, including autoimmune diseases, schizophrenia, and coronary heart disease and evidence suggesting previously reported population associations between blood cell indices and cardiovascular disease may be non-causal.
Sujet(s)
Variation génétique , Étude d'association pangénomique , Cellules souches hématopoïétiques/métabolisme , Maladies du système immunitaire/génétique , Allèles , Différenciation cellulaire , Prédisposition génétique à une maladie , Cellules souches hématopoïétiques/anatomopathologie , Humains , Maladies du système immunitaire/anatomopathologie , Polymorphisme de nucléotide simple , Locus de caractère quantitatif , /génétiqueRÉSUMÉ
AIMS: To determine the effects of in vivo S-nitrosoglutathione (GSNO) infusion on cardiovascular function, platelet function, proteinuria and biomarker parameters in early-onset pre-eclampsia. METHODS: We performed an open-label dose-ranging study of GSNO in early-onset pre-eclampsia. Six women underwent GSNO infusion whilst receiving standard therapy. The dose of GSNO was increased incrementally to 100 µg min(-1) whilst maintaining blood pressure of >140/80 mmHg. Aortic augmentation index, aortic pulse wave velocity, blood pressure and maternal-fetal Doppler parameters were measured at each dose. Platelet P-selectin, protein-to-creatinine ratio and soluble anti-angiogenic factors were measured pre- and postinfusion. RESULTS: Augmentation index fell at 30 µg min(-1) S-nitrosoglutathione (-6%, 95% confidence interval 0.6 to 13%), a dose that did not affect blood pressure. Platelet P-selectin expression was reduced [mean (interquartile range), 6.3 (4.9-7.6) vs. 4.1 (3.1-5.7)% positive, P = 0.03]. Soluble endoglin levels showed borderline reduction (P = 0.06). There was a borderline significant change in pre-to-postinfusion protein-to-creatinine ratio [mean (interquartile range), 0.37 (0.09-0.82) vs. 0.23 (0.07-0.49) g mmol(-1) , P = 0.06]. Maternal uterine and fetal Doppler pulsatility indices were unchanged. CONCLUSIONS: In early-onset pre-eclampsia, GSNO reduces augmentation index, a biomarker of small vessel tone and pulse wave reflection, prior to affecting blood pressure. Proteinuria and platelet activation are improved at doses that affect blood pressure minimally. These effects of GSNO may be of therapeutic potential in pre-eclampsia, a condition for which no specific treatment exists. Clinical studies of GSNO in early-onset pre-eclampsia will determine whether these findings translate to improvement in maternal and/or fetal outcome.
Sujet(s)
Donneur d'oxyde nitrique/usage thérapeutique , Pré-éclampsie/traitement médicamenteux , Protéinurie/traitement médicamenteux , S-Nitroso-glutathion/usage thérapeutique , Adulte , Pression sanguine/effets des médicaments et des substances chimiques , Relation dose-effet des médicaments , Femelle , Hémodynamique/effets des médicaments et des substances chimiques , Humains , Donneur d'oxyde nitrique/administration et posologie , Sélectine P/métabolisme , Activation plaquettaire/effets des médicaments et des substances chimiques , Pré-éclampsie/physiopathologie , Grossesse , Analyse de l'onde de pouls , S-Nitroso-glutathion/administration et posologie , Échographie prénatale/méthodes , Jeune adulteSujet(s)
Plaquettes/anatomopathologie , Pré-éclampsie/sang , Thrombopoïèse , Adulte , Études cas-témoins , Différenciation cellulaire , Femelle , Humains , Progéniteurs mégacaryocytaires/anatomopathologie , Mégacaryocytes/anatomopathologie , Numération des plaquettes , Grossesse , Thrombopénie/sang , Thrombopénie/étiologieRÉSUMÉ
BACKGROUND: Studies show that 1 in 1200 neonates have a low platelet (PLT) count due to alloimmunization against human PLT antigen (HPA)-1a (ß3 -L33). This mainly occurs in HPA-1a-negative mothers who are positive for the human leukocyte antigen (HLA)-DRB3*01:01 allele, but only about one-third of cases will mount an effective alloimmune response. The development of specific treatment modalities requires that the mechanisms driving the maternal alloimmune response against the fetal PLTs be further explored. An antibody reagent that has a different binding affinity to HLA-DRA/DRB3*01:01 with and without the ß3 -L33 peptide would be a valuable reagent to study peptide presentation on maternal antigen-presenting cells. STUDY DESIGN AND METHODS: To identify such antibodies, HLA-DRA/DRB3*01:01 was recombinantly expressed in Drosophilaâ S2 cells. To delineate the epitope of interesting antibodies, seven mutant HLA-DRA/DRB3*01:01 molecules were generated by site-directed mutagenesis introducing naturally occurring amino acid changes encoded by DRB3*02 and DRB3*03 alleles. RESULTS: The murine monoclonal antibody (MoAb) DA2 showed robust binding by enzyme-linked immunosorbent assay to recombinant HLA-DRA/DRB3*01:01, but binding was reduced in the presence of ß3 -L33 peptide. The binding affinity of DA2 to the mutant HLA-DRA/DRB3*0101 in which serine at Position 60 of the ß1-chain was replaced by tyrosine was greatly enhanced. Interestingly the binding of DA2 to the mutant was not reduced by the presence of ß3 -L33 peptide. CONCLUSION: The results of this study generate a molecular model of the interaction of the HLA-DRA/DRB3*01:01 molecule with MoAb DA2. This will inform functional studies with the recombinant Class II molecules.
Sujet(s)
Anticorps monoclonaux/métabolisme , Antigènes HLA/métabolisme , Chaines alpha des antigènes HLA-DR/métabolisme , Chaines HLA-DRB3/métabolisme , Antigènes plaquettaires humains/métabolisme , Sites de fixation , Test ELISA , Chaines alpha des antigènes HLA-DR/composition chimique , Chaines HLA-DRB3/composition chimique , Humains , Intégrine bêta3 , Liaison aux protéines , Structure secondaire des protéinesRÉSUMÉ
Within the healthy population, there is substantial, heritable, and interindividual variability in the platelet response. We explored whether a proportion of this variability could be accounted for by interindividual variation in gene expression. Through a correlative analysis of genome-wide platelet RNA expression data from 37 subjects representing the normal range of platelet responsiveness within a cohort of 500 subjects, we identified 63 genes in which transcript levels correlated with variation in the platelet response to adenosine diphosphate and/or the collagen-mimetic peptide, cross-linked collagen-related peptide. Many of these encode proteins with no reported function in platelets. An association study of 6 of the 63 genes in 4235 cases and 6379 controls showed a putative association with myocardial infarction for COMMD7 (COMM domain-containing protein 7) and a major deviation from the null hypo thesis for LRRFIP1 [leucine-rich repeat (in FLII) interacting protein 1]. Morpholino-based silencing in Danio rerio identified a modest role for commd7 and a significant effect for lrrfip1 as positive regulators of thrombus formation. Proteomic analysis of human platelet LRRFIP1-interacting proteins indicated that LRRFIP1 functions as a component of the platelet cytoskeleton, where it interacts with the actin-remodeling proteins Flightless-1 and Drebrin. Taken together, these data reveal novel proteins regulating the platelet response.
Sujet(s)
Plaquettes/métabolisme , Analyse de profil d'expression de gènes , Protéines de liaison à l'ARN/métabolisme , Animaux , Extinction de l'expression des gènes , Génotype , Humains , Activation plaquettaire , Protéome/métabolisme , Protéines de liaison à l'ARN/génétique , Protéines de répression/génétique , Protéines de répression/métabolisme , Thrombose , Danio zébré , Protéines de poisson-zèbre/génétique , Protéines de poisson-zèbre/métabolismeRÉSUMÉ
Platelet endothelial cell adhesion molecule-1 (PECAM-1) inhibits platelet response to collagen and may also inhibit two other major platelet agonists ADP and thrombin although this has been less well explored. We hypothesized that the combined effect of inhibiting these three platelet activating pathways may act to significantly inhibit thrombus formation. We demonstrate a negative relationship between PECAM-1 surface expression and platelet response to cross-linked collagen related peptide (CRP-XL) and ADP, and an inhibitory effect of PECAM-1 clustering on platelet response to CRP-XL, ADP and thrombin. This combined inhibition of multiple signaling pathways results in a marked reduction in thrombus formation.
Sujet(s)
Plaquettes/métabolisme , Antigènes CD31/métabolisme , Transduction du signal , ADP/pharmacologie , Plaquettes/effets des médicaments et des substances chimiques , Calcium/métabolisme , Protéines de transport/composition chimique , Protéines de transport/pharmacologie , Cytométrie en flux , Humains , Peptides/composition chimique , Peptides/pharmacologie , Activation plaquettaire/effets des médicaments et des substances chimiques , Antigènes CD31/sang , Glycoprotéines de membrane plaquettaire/métabolisme , Thrombine/pharmacologieRÉSUMÉ
The number and volume of cells in the blood affect a wide range of disorders including cancer and cardiovascular, metabolic, infectious and immune conditions. We consider here the genetic variation in eight clinically relevant hematological parameters, including hemoglobin levels, red and white blood cell counts and platelet counts and volume. We describe common variants within 22 genetic loci reproducibly associated with these hematological parameters in 13,943 samples from six European population-based studies, including 6 associated with red blood cell parameters, 15 associated with platelet parameters and 1 associated with total white blood cell count. We further identified a long-range haplotype at 12q24 associated with coronary artery disease and myocardial infarction in 9,479 cases and 10,527 controls. We show that this haplotype demonstrates extensive disease pleiotropy, as it contains known risk loci for type 1 diabetes, hypertension and celiac disease and has been spread by a selective sweep specific to European and geographically nearby populations.
Sujet(s)
Cellules sanguines , Génome humain , Étude d'association pangénomique , Hémogramme , Cellules sanguines/cytologie , Chromosomes humains de la paire 12 , Maladie des artères coronaires/génétique , Marqueurs génétiques , Humains , Polymorphisme de nucléotide simple , Sélection génétiqueRÉSUMÉ
Human Domain Antibodies (dAbs) that bind to and inhibit the function of platelet glycoprotein VI (GPVI) have been isolated from phage display libraries and their efficacy demonstrated using in vitro models of platelet activation. Here we describe the properties of one such antibody, BLO8-1, which has been shown to specifically inhibit the binding of recombinant human GPVI to cross-linked collagen related peptide (CRP-XL) in vitro. BLO8-1 specifically binds to the platelet cell surface and prevents CRP-XL induced platelet aggregation in platelet-rich plasma, as well as inhibiting thrombus formation in whole blood under arterial shear conditions. Using a series of mutant GPVI molecules, BLO8-1 was shown to recognize an epitope within the collagen binding domain of GPVI, therefore the anti-thrombotic effect of this dAb is predicted to be due to direct blocking of the collagen-GPVI interaction. These data, together with the desirable properties of Domain Antibodies, show that dAbs could potentially be used to generate novel biopharmaceuticals with anti-thrombotic properties.
Sujet(s)
Anticorps/pharmacologie , Collagène/pharmacologie , Glycoprotéines de membrane plaquettaire/immunologie , Thrombose/prévention et contrôle , Anticorps/usage thérapeutique , Sites de fixation/immunologie , Plaquettes/immunologie , Collagène/métabolisme , Cartographie épitopique , Épitopes , Humains , Banque de peptides , Agrégation plaquettaire/effets des médicaments et des substances chimiques , Agrégation plaquettaire/immunologie , Glycoprotéines de membrane plaquettaire/métabolisme , Thrombose/induit chimiquement , Thrombose/traitement médicamenteuxRÉSUMÉ
Platelet response to activation varies widely between individuals but shows interindividual consistency and strong heritability. The genetic basis of this variation has not been properly explored. We therefore systematically measured the effect on function of sequence variation in 97 candidate genes in the collagen and adenosine-diphosphate (ADP) signaling pathways. Resequencing of the genes in 48 European DNA samples nearly doubled the number of known single nucleotide polymorphisms (SNPs) and informed the selection of 1327 SNPs for genotyping in 500 healthy Northern European subjects with known platelet responses to collagen-related peptide (CRP-XL) and ADP. This identified 17 novel associations with platelet function (P < .005) accounting for approximately 46% of the variation in response. Further investigations with platelets of known genotype explored the mechanisms behind some of the associations. SNPs in PEAR1 associated with increased platelet response to CRP-XL and increased PEAR1 protein expression after platelet degranulation. The minor allele of a 3' untranslated region (UTR) SNP (rs2769668) in VAV3 was associated with higher protein expression (P = .03) and increased P-selectin exposure after ADP activation (P = .004). Furthermore the minor allele of the intronic SNP rs17786144 in ITPR1 modified Ca(2+) levels after activation with ADP (P < .004). These data provide novel insights into key hubs within platelet signaling networks.
Sujet(s)
Plaquettes/physiologie , Dégranulation cellulaire/génétique , Régulation de l'expression des gènes/physiologie , Activation plaquettaire/génétique , Locus de caractère quantitatif/physiologie , Transduction du signal/génétique , Régions 3' non traduites/génétique , Régions 3' non traduites/métabolisme , ADP/génétique , ADP/métabolisme , Allèles , Plaquettes/cytologie , Collagène/génétique , Collagène/métabolisme , Europe , Femelle , Génomique , Génotype , Humains , Récepteurs à l'inositol 1,4,5-triphosphate/biosynthèse , Récepteurs à l'inositol 1,4,5-triphosphate/génétique , Mâle , Sélectine P/génétique , Sélectine P/métabolisme , Polymorphisme de nucléotide simple , Récepteurs de surface cellulaire/biosynthèse , Récepteurs de surface cellulaire/génétique ,RÉSUMÉ
Hematopoiesis is a carefully controlled process that is regulated by complex networks of transcription factors that are, in part, controlled by signals resulting from ligand binding to cell-surface receptors. To further understand hematopoiesis, we have compared gene expression profiles of human erythroblasts, megakaryocytes, B cells, cytotoxic and helper T cells, natural killer cells, granulocytes, and monocytes using whole genome microarrays. A bioinformatics analysis of these data was performed focusing on transcription factors, immunoglobulin superfamily members, and lineage-specific transcripts. We observed that the numbers of lineage-specific genes varies by 2 orders of magnitude, ranging from 5 for cytotoxic T cells to 878 for granulocytes. In addition, we have identified novel coexpression patterns for key transcription factors involved in hematopoiesis (eg, GATA3-GFI1 and GATA2-KLF1). This study represents the most comprehensive analysis of gene expression in hematopoietic cells to date and has identified genes that play key roles in lineage commitment and cell function. The data, which are freely accessible, will be invaluable for future studies on hematopoiesis and the role of specific genes and will also aid the understanding of the recent genome-wide association studies.
Sujet(s)
Cellules de la moelle osseuse/physiologie , Différenciation cellulaire/génétique , Expression des gènes , Atlas comme sujet , Lignage cellulaire , Cellules cultivées , Cytométrie en flux , Analyse de profil d'expression de gènes , Hématopoïèse , Humains , Séquençage par oligonucléotides en batterie , Facteurs de transcription/métabolismeRÉSUMÉ
Mean platelet volume (MPV) and platelet count (PLT) are highly heritable and tightly regulated traits. We performed a genome-wide association study for MPV and identified one SNP, rs342293, as having highly significant and reproducible association with MPV (per-G allele effect 0.016 +/- 0.001 log fL; P < 1.08 x 10(-24)) and PLT (per-G effect -4.55 +/- 0.80 10(9)/L; P < 7.19 x 10(-8)) in 8586 healthy subjects. Whole-genome expression analysis in the 1-MB region showed a significant association with platelet transcript levels for PIK3CG (n = 35; P = .047). The G allele at rs342293 was also associated with decreased binding of annexin V to platelets activated with collagen-related peptide (n = 84; P = .003). The region 7q22.3 identifies the first QTL influencing platelet volume, counts, and function in healthy subjects. Notably, the association signal maps to a chromosome region implicated in myeloid malignancies, indicating this site as an important regulatory site for hematopoiesis. The identification of loci regulating MPV by this and other studies will increase our insight in the processes of megakaryopoiesis and proplatelet formation, and it may aid the identification of genes that are somatically mutated in essential thrombocytosis.
Sujet(s)
Plaquettes , Chromosomes humains de la paire 7/génétique , Génome humain/génétique , Polymorphisme de nucléotide simple , Locus de caractère quantitatif/génétique , Thrombopoïèse/génétique , Adulte , Sujet âgé , Cartographie chromosomique , Études de cohortes , Femelle , Régulation de l'expression des gènes/génétique , Tumeurs hématologiques/génétique , Humains , Mâle , Adulte d'âge moyen , Numération des plaquettes , Thrombocytémie essentielle/génétiqueRÉSUMÉ
In this study, we demonstrate the suitability of the vertebrate Danio rerio (zebrafish) for functional screening of novel platelet genes in vivo by reverse genetics. Comparative transcript analysis of platelets and their precursor cell, the megakaryocyte, together with nucleated blood cell elements, endothelial cells, and erythroblasts, identified novel platelet membrane proteins with hitherto unknown roles in thrombus formation. We determined the phenotype induced by antisense morpholino oligonucleotide (MO)-based knockdown of 5 of these genes in a laser-induced arterial thrombosis model. To validate the model, the genes for platelet glycoprotein (GP) IIb and the coagulation protein factor VIII were targeted. MO-injected fish showed normal thrombus initiation but severely impaired thrombus growth, consistent with the mouse knockout phenotypes, and concomitant knockdown of both resulted in spontaneous bleeding. Knockdown of 4 of the 5 novel platelet proteins altered arterial thrombosis, as demonstrated by modified kinetics of thrombus initiation and/or development. We identified a putative role for BAMBI and LRRC32 in promotion and DCBLD2 and ESAM in inhibition of thrombus formation. We conclude that phenotypic analysis of MO-injected zebrafish is a fast and powerful method for initial screening of novel platelet proteins for function in thrombosis.
Sujet(s)
Plaquettes/métabolisme , Génomique , Protéines membranaires/métabolisme , Oligonucléotides antisens/pharmacologie , Thrombose/métabolisme , Protéines de poisson-zèbre/métabolisme , Animaux , Technique de Western , Embryon non mammalien/cytologie , Embryon non mammalien/métabolisme , Analyse de profil d'expression de gènes , Humains , Lasers , Protéines membranaires/antagonistes et inhibiteurs , Protéines membranaires/génétique , Séquençage par oligonucléotides en batterie , Phénotype , Agrégation plaquettaire , Thrombose/étiologie , Danio zébré , Protéines de poisson-zèbre/antagonistes et inhibiteurs , Protéines de poisson-zèbre/génétiqueRÉSUMÉ
BACKGROUND: The previously reported platelet (PLT)-specific antigen, Va(a), was defined by an alloantibody detected in the serum sample of a mother who delivered an infant displaying symptoms of severe fetal maternal alloimmune thrombocytopenia (FMAIT). This PLT antigen was localized to the integrin alphaIIbbeta3 (GPIIbIIIa) but its genetic basis was not defined. STUDY DESIGN AND METHODS: Genomic ITGA2B (alphaIIb) and ITGB3 (beta3) DNA from a Va(a)-positive individual were sequenced to identify potential polymorphisms underlying the Va(a) antigen. Recombinant beta3 integrin carrying the putative mutation was then used to assess serologic reactivity with the original maternal Va(a) antiserum. RESULTS: A single-nucleotide polymorphism (SNP; C622>T) in exon 5 of ITGB3 resulting in the replacement of threonine with methionine at residue 195 of the mature beta3 was identified. Calmodulin-tagged soluble recombinant beta3 encoding Met195 was produced in S2 cells and found to react specifically with the Va(a) antiserum. CONCLUSION: With the use of a combination of DNA sequencing and recombinant antigen expression, the molecular basis of the PLT-specific Va(a) antigen (HPA-17bw), a low-frequency antigen implicated in FMAIT, has been resolved. These data further demonstrate the value of using recombinant beta3 peptides for the detection of rare but clinically relevant antibodies.
Sujet(s)
Antigènes plaquettaires humains/immunologie , Maladies foetales/génétique , Intégrine bêta3/génétique , Polymorphisme de nucléotide simple , Thrombopénie/génétique , Antigènes plaquettaires humains/sang , Exons/génétique , Femelle , Maladies foetales/immunologie , Humains , Intégrine bêta3/composition chimique , Intégrine bêta3/métabolisme , Mâle , Échange foetomaternel , Modèles biologiques , Glycoprotéine-IIb de membrane plaquettaire/métabolisme , Grossesse , Complications de la grossesse , Structure secondaire des protéines , Protéines recombinantes/composition chimique , Protéines recombinantes/métabolisme , Thrombopénie/immunologieRÉSUMÉ
BACKGROUND: Process-induced platelet (PLT) activation occurs with all production methods, including apheresis. Recent studies have highlighted the range and consistence of interindividual variation in the PLT response, but little is known about the contribution of a donors' inherent PLT responsiveness to the activation state of the apheresis PLTs or the effect of frequent apheresis on donors' PLTs. STUDY DESIGN AND METHODS: The relationship between the donors' PLT response on the apheresis PLTs was studied in 47 individuals selected as having PLTs with inherently low, intermediate, or high responsiveness. Whole-blood flow cytometry was used to measure PLT activation (levels of bound fibrinogen) before donation and in the apheresis PLTs. The effects of regular apheresis on the activation status of donors' PLTs were studied by comparing the in vivo activation status of PLTs from apheresis (n = 349) and whole-blood donors (n = 157), before donation. The effect of apheresis per se on PLT activation was measured in 10 apheresis donors before and after donation. RESULTS: The level of PLT activation in the apheresis packs was generally higher than in the donor, and the most activated PLTs were from high-responder donors. There was no significant difference in PLT activation before donation between the apheresis and whole-blood donors (p = 0.697), and there was no consistent evidence of activation in the donors immediately after apheresis. CONCLUSION: The most activated apheresis PLTs were obtained from donors with more responsive PLTs. Regular apheresis, however, does not lead to PLT activation in the donors.
Sujet(s)
Aphérèse , Plaquettes/physiologie , Activation plaquettaire/physiologie , Adulte , Plaquettes/cytologie , Femelle , Cytométrie en flux , Humains , Mâle , Adulte d'âge moyenRÉSUMÉ
We report a 3-generation pedigree with 5 individuals affected with a dominantly inherited macrothrombocytopenia. All 5 carry 2 nonsynonymous mutations resulting in a D723H mutation in the beta3 integrin and a P53L mutation in glycoprotein (GP) Ibalpha. We show that GPIbalpha-L53 is phenotypically silent, being also present in 3 unaffected pedigree members and in 7 of 1639 healthy controls. The beta3-H723 causes constitutive, albeit partial, activation of the alphaIIbbeta3 complex by disruption of the highly conserved cytoplasmic salt bridge with arginine 995 in the alphaIIb integrin as evidenced by increased PAC-1 but not fibrinogen binding to the patients' resting platelets. This was confirmed in CHO alphaIIbbeta3-H723 transfectants, which also exhibited increased PAC-1 binding, increased adhesion to von Willebrand factor (VWF) in static conditions and to fibrinogen under shear stress. Crucially, we show that in the presence of fibrinogen, alphaIIbbeta3-H723, but not wild-type alphaIIbbeta3, generates a signal that leads to the formation of proplatelet-like protrusions in transfected CHO cells. Abnormal proplatelet formation was confirmed in the propositus's CD34+ stem cell-derived megakaryocytes. We conclude that the constitutive activation of the alphaIIbbeta3-H723 receptor causes abnormal proplatelet formation, leading to incorrect sizing of platelets and the thrombocytopenia observed in the pedigree.
