Mutations in the most divergent α-tubulin isotype, α8-tubulin, cause defective platelet biogenesis.

BACKGROUND: In the panel of genes commonly associated with inherited macrothrombocytopenia, an important fraction encodes key cytoskeletal proteins such as tubulin isotypes, the building blocks of microtubules. Macrothrombocytopenia-causing mutations have been identified in the TUBB1 and TUBA4A genes, emphasizing their importance in the formation of platelets and their marginal band, a unique microtubule ring-like structure that supports the platelet typical disc-shaped morphology. This raised the hypothesis that other tubulin isotypes normally expressed in platelets could play a similar role in their formation. OBJECTIVES: To assess whether tubulin isotype genes other than TUBA4A and TUBB1 could be implicated in inherited macrothrombocytopenia. METHODS: We used high throughput sequencing to screen a cohort of 448 French blood donors with mild thrombocytopenia for mutations in a panel of selected genes known or suspected to be involved in platelet biogenesis. RESULTS: We identified six distinct novel mutations in TUBA8, which encodes the most-divergent α-tubulin, as the causative determinant of macrothrombocytopenia and platelet marginal band defects. Functionally, all TUBA8 mutations were found to fully or partially inhibit the incorporation of the mutated α8-tubulin in the microtubule network. CONCLUSION: This study provides strong support for a key role of multiple tubulin genes in platelet biogenesis by discovering variants in a tubulin gene that was previously not known to be important for platelets.

Quality zones automatically identified in water distribution networks by applying data clustering methods to conductivity measurements.

This paper presents a clustering study showing how conductivity measured every five minutes by 215 probes over four years can be used to determine specific quality zones for a large Water Distribution Network (WDN): 8500 km of pipes, 4.6 M customers. Conductivity time-series are compared using Dynamic Time Warping. Then, probes are ordered using a density-based method, and probe clusters are extracted automatically. The clusters are a sound representation of water quality in the WDN, both in terms of water origin and water residence time. More specifically, zones directly impacted by plants or by external water imports, mixing zones and zones influenced by tanks, can be isolated and analyzed. Globally, 82% of the probes were found to be clustered, consistent with expert knowledge on the WDN operation; 13% were unclassified; 3% were erroneously clustered; and 1% seemed to be reasonably clustered, without any physical understanding yet. Besides providing users with an increased understanding of water quality in WDNs, conductivity-based clusters offer an interesting prior tool for contamination warning systems.

Human platelets labeled at two discrete biotin densities are functional in vitro and are detected in vivo in the murine circulation: A promising approach to monitor platelet survival in vivo in clinical research.

BACKGROUND: The production of platelet concentrates (PCs) is evolving, and their survival capacity needs in vivo evaluation. This requires that the transfused platelets (PLTs) be distinguished from those of the recipient. Labeling at various biotin (Bio) densities allows one to concurrently trace multiple PLT populations, as reported for red blood cells. STUDY DESIGN AND METHODS: A method is described to label human PLTs at two densities of Bio for future clinical trials. Injectable-grade PLTs were prepared in a sterile environment, using injectable-grade buffers and good manufacturing practices (GMP)-grade Sulfo-NHS-Biotin. Sulfo-NHS-Biotin concentrations were chosen to maintain PLT integrity and avoid potential alloimmunization while enabling the detection of circulating BioPLTs. The impact of biotinylation on human PLT recirculation was evaluated in vivo in a severe immunodeficient mouse model using ex vivo flow cytometry. RESULTS: BioPLTs labeled with 1.2 or 10 µg/ml Sulfo-NHS-Biotin displayed normal ultrastructure and retained aggregation and secretion capacity and normal expression of the main surface glycoproteins. The procedure avoided detrimental PLT activation or apoptosis signals. Transfused human BioPLT populations could be distinguished from one another and from unlabeled circulating mouse PLTs, and their survival was comparable to that of unlabeled human PLTs in the mouse model. CONCLUSIONS: Provided low Sulfo-NHS-Biotin concentrations (<10 µg/ml) are used, injectable-grade BioPLTs comply with safety regulations, conserve PLT integrity, and permit accurate in vivo detection. This alternative to radioisotopes, which allows one to follow different PLT populations in the same recipient, should be valuable when assessing new PC preparations and monitoring PLT survival in clinical research.

Upscaling fixed bed adsorption behaviors towards emerging micropollutants in treated natural waters with aging activated carbon: Model development and validation.

A scale-up procedure was assessed in this study to predict the fixed bed adsorption behaviors with aging granular activated carbon (GAC) for various micropollutants (pesticides, pharmaceuticals). Two assumptions of this upscaling methodology (i.e., involving equal adsorption capacities and surface diffusivities between the batch test and the fixed bed) were studied for the first time to investigate the aging effect on the adsorption capacity and kinetics of carbon at full scale. This study was conducted in natural waters (the Seine River) treated by Veolia Eau d'Ile de France in Choisy-Le-Roi, a division of Syndicat des Eaux d'Ile de France, aiming to monitor real industrial conditions. The isotherms showed that the adsorption capacity for most compounds was significantly affected by aging. For the mass transfer coefficients (i.e., as determined by the homogeneous surface diffusion model (HSDM)), different patterns of adsorbate/adsorbent behaviors were observed, suggesting different competition mechanisms. The model predictions (i.e., HSDM) performed with all parameters obtained during the batch tests tended to overestimate the full-scale pilot adsorption performance. This overestimation could be compensated for by applying a scaling factor. Finally, an empirical pseudo-first order function was used to model the impact of the GAC service time on the characteristic adsorption parameters. Thus, our scale-up procedure may enable the prediction of long-term fixed bed adsorption behaviors and increase the model efficiency for practical implementation.

In Vitro Binding of [³H]PSB-0413 to P2Y12 Receptors.

The P2Y12/ADP receptor plays a central role in platelet activation. Characterization of this receptor is mandatory for studying disorders associated with a P2Y12 receptor defect and for evaluating P2Y12 receptor agonists and antagonists. In the absence of suitable anti-P2Y12 antibodies, radioligand binding assays are the only way to conduct such studies. While various radioligands were employed in the past for this purpose, none were found to be suitable for routine use. Described in this unit are protocols for quantitatively and qualitatively assessing P2Y12 receptors with [³H]PSB-0413, a selective antagonist for this site. The saturation and competition assays described herein make possible the determination of P2Y12 receptor density on cells, as well as the potencies and affinities of test agents at this site.

The P2X1 receptor is required for neutrophil extravasation during lipopolysaccharide-induced lethal endotoxemia in mice.

Extracellular ATP is becoming increasingly recognized as an important regulator of inflammation. However, the known repertoire of P2 receptor subtypes responsible for the proinflammatory effects of ATP is sparse. We looked at whether the P2X1 receptor, an ATP-gated cation channel present on platelets, neutrophils, and macrophages, participates in the acute systemic inflammation provoked by LPS. Compared with wild-type (WT) mice, P2X1(-/-) mice displayed strongly diminished pathological responses, with dampened neutrophil accumulation in the lungs, less tissue damage, reduced activation of coagulation, and resistance to LPS-induced death. P2X1 receptor deficiency also was associated with a marked reduction in plasma levels of the main proinflammatory cytokines and chemokines induced by LPS. Interestingly, macrophages and neutrophils isolated from WT and P2X1(-/-) mice produced similar levels of proinflammatory cytokines when stimulated with LPS in vitro. Intravital microscopy revealed a defect in LPS-induced neutrophil emigration from cremaster venules into the tissues of P2X1(-/-) mice. Using adoptive transfer of immunofluorescently labeled neutrophils from WT and P2X1(-/-) mice into WT mice, we demonstrate that the absence of the P2X1 receptor on neutrophils was responsible for this defect. This study reveals a major role for the P2X1 receptor in LPS-induced lethal endotoxemia through its critical involvement in neutrophil emigration from venules.

Kinetic development of biofilm on NF membranes at the Méry-sur-Oise plant, France.

The kinetic formation of biofilms developing on nanofiltration (NF) membranes was studied for 2 years in the water production unit of Méry-sur-Oise, France. New membranes were set up in a pilot train integrated to the plant and autopsied after operation for 7, 80, 475 and 717 days. The biofouling layer was studied by confocal laser scanning microscope after 4',6-diamidino-2-phenyindole dihydrochloride and lectin staining, and by attenuated total reflectance-Fourier transform infrared spectroscopy and rheology experiments. Three stages of biofilm growth were discriminated: (1) the presence of sessile microcolonies embedded in an exopolymeric matrix (after filtration for seven days); (2) membrane coverage expansion through microcolony development and biofilm growth in three dimensions (up to 80 days filtration); and (3) biofilm maturation by densification (after filtration for 80-717 days). Biofilm maturation resulted in total coverage of the membrane surface and matrix residue diversification, development of the polysaccharide network, and the strengthening of matrix cohesion through viscosity and elasticity increases. The wettability and permeability of the fouled NF membranes decreased quickly and continuously throughout the biofilm development process. The longitudinal pressure drop (LPD) increased only after the biofilm reached a quantitative threshold. The decline in membrane permeability may be the result of contributions from many fouling mechanisms but the LPD was more substantially influenced by biofilm development.

Analysis and occurrence of odorous disinfection by-products from chlorination of amino acids in three different drinking water treatment plants and corresponding distribution networks.

Previous studies have established that odorous and stable chloraldimines are formed during amino acid chlorination in drinking water treatment. In order to identify at low level (10(-8) M) the presence of these odorous disinfection by-products in drinking water matrixes an analytical method was developed by using head space apparatus (HS) combined with a sorbent trap system linked to a GC with a mass spectrometer detector (HS/Trap/GC/MS). The analyses were carried out in three different drinking water supplies from the Paris area, during the four seasons. Free amino acids were monitored at the inlet of the plant. The odorous disinfection by-products were analyzed at the outlet of each drinking water treatment plant and the different distribution networks were connected to the corresponding plant. The results confirmed that the odorous chloraldimines are produced during chlorination of free amino acids in three different matrixes in different seasons throughout the year (N-chloroisobutaldimine; N-chloromethyl-2-butaldimine; N-chloromethyl-3-butaldimine (6-10 nM). The analytical method (HS/Trap/GC/MS) used to monitor odorous disinfection by-products appeared to be adapted for the detection of these by-products at nM level.

A role of the fast ATP-gated P2X1 cation channel in thrombosis of small arteries in vivo.

The P2X1 receptor is a fast ATP-gated cation channel expressed in blood platelets, where its role has been difficult to assess due to its rapid desensitization and the lack of pharmacological tools. In this paper, we have used P2X1-/- and wild-type mouse platelets, treated with apyrase to prevent desensitization, to demonstrate the function of P2X1 in the response to thrombogenic stimuli. In vitro, the collagen-induced aggregation and secretion of P2X1-deficient platelets was decreased, as was adhesion and thrombus growth on a collagen-coated surface, particularly when the wall shear rate was elevated. In vivo, the functional role of P2X1 could be demonstrated using two models of platelet-dependent thrombotic occlusion of small arteries, in which blood flow is characterized by a high shear rate. The mortality of P2X1-/- mice in a model of systemic thromboembolism was reduced and the size of mural thrombi formed after a laser-induced vessel wall injury was decreased as compared with normal mice, whereas the time for complete thrombus removal was shortened. Overall, the P2X1 receptor appears to contribute to the formation of platelet thrombi, particularly in arteries in which shear forces are high.