Your search keyword '"Chatelain B"' showing total 18 results

1. Analysis of megakaryocytes by flow cytometry.

Author

Baatout, S., Chatelain, B., Staquet, P., Symann, M., and Chatelain, C.

Subjects

*MEGAKARYOCYTES, *BONE marrow cells, *PLOIDY

Abstract

Presents a study that developed a technique that permits the determination of human megakaryocyte ploidy distributions directly from bone marrow samples. Preparation of the bone marrow sample; Applications of the method to the ploidy analysis of megakaryotes of normal individuals and patients with abnormal platlet counts; Advantages of the proposed technique.

Published

1998

2. Influence of apixaban on commonly used coagulation assays: results from the Belgian national External Quality Assessment Scheme.

Author

Van Blerk, M., Bailleul, E., Chatelain, B., Demulder, A., Devreese, K., Douxfils, J., Jacquemin, M., Jochmans, K., Mullier, F., Wijns, W., China, B., Vernelen, K., and Soumali, M. R.

Subjects

*ANTICOAGULANTS, *BIOLOGICAL assay, *FIBRIN, *ORAL drug administration, *QUALITY assurance, *RIVAROXABAN

Abstract

Introduction The Belgian national External Quality Assessment Scheme performed a survey to assess the effect of the direct oral anticoagulant apixaban on the coagulation assays prothrombin time ( PT), activated partial thromboplastin time ( aPTT), fibrinogen and antithrombin as performed with a large number of reagent/instrument combinations. Methods Four lyophilized plasma samples spiked with apixaban (0, 41, 94 and 225 ng/mL) were sent to the 195 Belgian and Luxembourg clinical laboratories performing coagulation testing. Results PT and aPTT were barely influenced at the concentrations tested. At 225 ng/mL apixaban, PT and aPTT clotting times were only 1.15 times longer than at 0 ng/mL. Among PT reagents, RecombiPlasTin 2G® showed a slightly higher sensitivity with 225 ng/mL apixaban prolonging the PT clotting time 1.3-fold. Among aPTT reagents, there was no appreciable difference in sensitivity. Fibrinogen results were unaffected by the presence of apixaban, but antithrombin activity was considerably overestimated when measured with a FXa-based assay. At 225 ng/mL apixaban, the median percentage increase in antithrombin level was 31% when measured with the Liquid Antithrombin® reagent and 44% with the Innovance Antithrombin® reagent. Conclusion Our data provide clinical laboratories with useful information on the impact of apixaban on their routine coagulation assays. [ABSTRACT FROM AUTHOR]

Published

2017

3. Pre-analytical issues in the haemostasis laboratory: guidance for the clinical laboratories.

Author

Magnette, A., Chatelain, M., Chatelain, B., Cate, H. Ten, and Mullier, F.

Abstract

Ensuring quality has become a daily requirement in laboratories. In haemostasis, even more than in other disciplines of biology, quality is determined by a pre-analytical step that encompasses all procedures, starting with the formulation of the medical question, and includes patient preparation, sample collection, handling, transportation, processing, and storage until time of analysis. This step, based on a variety of manual activities, is the most vulnerable part of the total testing process and is a major component of the reliability and validity of results in haemostasis and constitutes the most important source of erroneous or un-interpretable results. Pre-analytical errors may occur throughout the testing process and arise from unsuitable, inappropriate or wrongly handled procedures. Problems may arise during the collection of blood specimens such as misidentification of the sample, use of inadequate devices or needles, incorrect order of draw, prolonged tourniquet placing, unsuccessful attempts to locate the vein, incorrect use of additive tubes, collection of unsuitable samples for quality or quantity, inappropriate mixing of a sample, etc. Some factors can alter the result of a sample constituent after collection during transportation, preparation and storage. Laboratory errors can often have serious adverse consequences. Lack of standardized procedures for sample collection accounts for most of the errors encountered within the total testing process. They can also have clinical consequences as well as a significant impact on patient care, especially those related to specialized tests as these are often considered as "diagnostic". Controlling pre-analytical variables is critical since this has a direct influence on the quality of results and on their clinical reliability. The accurate standardization of the pre-analytical phase is of pivotal importance for achieving reliable results of coagulation tests and should reduce the side effects of the influence factors. This review is a summary of the most important recommendations regarding the importance of pre-analytical factors for coagulation testing and should be a tool to increase awareness about the importance of pre-analytical factors for coagulation testing. [ABSTRACT FROM AUTHOR]

Published

2016

4. Translocation t(14;18) is not associated with inferior outcome in chronic lymphocytic leukemia.

Author

Put, N., Meeus, P., Chatelain, B., Rack, K., Boeckx, N., Nollet, F., Graux, C., Van Den Neste, E., Janssens, A., Madoe, V., Van Hoof, A., Bilhou-Nabera, C., Wlodarska, I., Vandenberghe, P., and Michaux, L.

Subjects

*LETTERS to the editor, *LYMPHOCYTIC leukemia

Abstract

A letter to the editor is presented informing that translocation t(14;18) is not associated with inferior outcome in chronic lymphocytic leukemia.

Published

2009

5. The paradoxical association between inherited factor VII deficiency and venous thrombosis.

Author

Marty, S., Barro, C., Chatelain, B., Fimbel, B., Tribout, B., Reynaud, J., Schved, J.-F., and Giansily-Blaizot, M.

Subjects

*THROMBOSIS, *HEMORRHAGE, *BLOOD coagulation factor VIII, *BLOOD coagulation, *HEMOPHILIA

Abstract

Inherited factor VII (FVII) deficiency is considered to be a haemorrhagic disease. Nonetheless, some patients paradoxically present with venous thrombosis. We assessed whether there was a link between phenotype and genotype in seven patients with inherited FVII deficiency and thrombosis (eleven venous thrombotic events). For each patient (FVII:C < 50%), clinical data were collected, aetiological assessment of risk factors for thrombosis was investigated, and direct sequencing of the nine exons and promoter of the FVII gene ( F7) was performed. We present the second series ever published on FVII patients with thrombosis. In nine of the eleven thrombotic events, there was at least one classical triggering risk factor; clinical ( n = 4), familial antecedent ( n = 2), or biological, defined by phospholipid-binding antibodies or elevated FVIII:C levels ( n = 7). In contrast to a previous series, only two events occurred after surgery, performed both with and without replacement therapy. The thrombotic event remained unexplained in one young patient, highlighting the lack of ‘protection’ against venous thrombosis by low FVII:C levels. Genetic mutations were found to be heterogeneous. Among the seven F7 sequence alterations identified in the present study, only two (p.Ala354Val and p.Arg364Gln) have previously been reported in FVII-deficient patients presenting with venous thrombosis. Our genetic analyses of the F7 mutations in these patients show the complexity of FVII deficiency associated with thrombosis. These data justify a holistic, clinical and biological approach for patients with these specific symptoms. This series also strongly suggest that mild FVII deficiency should not prevent physicians from using antithrombotic prophylaxis in FVII-deficient patients. [ABSTRACT FROM AUTHOR]

Published

2008

6. External quality assessment in the measurement of haemoglobin by blood gas analysers in Belgium.

Author

Van Blerk, M., Coucke, W., Chatelain, B., Goossens, W., Jochmans, K., Meeus, P., Mertens, G., Pradier, O., Rummens, J‐L., Scheiff, J‐M., and Libeer, J‐C.

Subjects

*HEMOGLOBINS, *BLOOD, *POINT-of-care testing, *DIAGNOSIS, *LABORATORIES, *HEMATOLOGY, *RADIOMETERS, *TECHNOLOGY

Abstract

Objective. The Belgian national External Quality Assessment Scheme (EQAS) for haematology organized a survey to assess the reliability of haemoglobin (Hb) measurements with the blood gas analysers (BGAs) currently available in Belgian hospitals. Material and methods. All hospital laboratories received two specimens of fresh EDTA anticoagulated whole blood and were asked to determine the Hb concentration using both the conventional haematology analyser (HA) and all BGAs in the hospital. Ninety-seven hospital laboratories participated in the study and a total of 166 results were reported. The BGAs used (grouped according to technology) were Rapidlab 845, 855, 865 (Bayer 1, n = 41), Rapidlab 1245, 1265, Rapidpoint 405 (Bayer 2, n = 19), GEM Premier 3000 (Instrumentation Laboratory, IL, n = 13), ABL 500 and 600 series (Radiometer 1, n = 13), ABL 700 and 800 series (Radiometer 2, n = 35), Omni C, S5 (Roche 1, n = 7), Omni 3, 6, 9, S2, S4, S6 (Roche 2, n = 21). Results. For the BGAs from Bayer, Radiometer and Roche, interlaboratory variation ranged from 0.6 % to 4.1 %, indicating good precision and close agreement between centres. A significant negative bias observed on the GEM Premier 3000 using the EDTA anticoagulated blood samples did not appear to be present in fresh heparinized whole blood samples. There was no significant difference in imprecision and bias between Hb measurements on BGA situated in and outside the central laboratory. [ABSTRACT FROM AUTHOR]

Published

2007

7. Implementation of a classification strategy of Raman data collected in different clinical conditions: application to the diagnosis of chronic lymphocytic leukemia.

Author

Féré, M., Gobinet, C., Liu, L. H., Beljebbar, A., Untereiner, V., Gheldof, D., Chollat, M., Klossa, J., Chatelain, B., and Piot, O.

Subjects

*CHRONIC lymphocytic leukemia, *RAMAN effect, *RAMAN spectroscopy, *TRANSLATIONAL research, *CELL lines, *DIAGNOSIS

Abstract

The literature is rich in proof of concept studies demonstrating the potential of Raman spectroscopy for disease diagnosis. However, few studies are conducted in a clinical context to demonstrate its applicability in current clinical practice and workflow. Indeed, this translational research remains far from the patient's bedside for several reasons. First, samples are often cultured cell lines. Second, they are prepared on non-standard substrates for clinical routine. Third, a unique supervised classification model is usually constructed using inadequate cross-validation strategy. Finally, the implemented models maximize classification accuracy without taking into account the clinician's needs. In this paper, we address these issues through a diagnosis problem in real clinical conditions, i.e., the diagnosis of chronic lymphocytic leukemia from fresh unstained blood smears spread on glass slides. From Raman data acquired in different experimental conditions, a repeated double cross-validation strategy was combined with different cross-validation approaches, a consensus label strategy and adaptive thresholds able to adapt to the clinician's needs. Combined with validation at the patient level, classification results were improved compared to traditional strategies. [ABSTRACT FROM AUTHOR]

Published

2020

8. Platelet microparticle generation assay: A valuable test for immune heparin-induced thrombocytopenia diagnosis.

Author

Mullier, F., Minet, V., Bailly, N., Devalet, B., Douxfils, J., Chatelain, C., Elalamy, I., Dogné, J.M., and Chatelain, B.

Subjects

*THROMBOCYTOPENIA, *HEPARIN, *BLOOD platelets, *PATHOLOGICAL physiology, *SEROTONIN, *COMPARATIVE studies, *HEALTH outcome assessment, *DIAGNOSIS

Abstract

Abstract: Background: Early diagnosis of immune heparin-induced thrombocytopenia (HIT) is essential to improve clinical outcome but remains challenging. The release of platelet microparticles (PMPs) is considered of major pathophysiological significance. Objectives: The aim of this study was to evaluate performances of PMP generation assay (PMPGA) compared to clinical outcome to diagnose HIT. The second objective was to compare PMPGA with performances of 14C-serotonin release assay (SRA) on the same series of patients. Methods: Sera of 53 HIT-suspected patients were retrospectively incubated with citrated-whole blood from healthy donors with 1IU and 500IU/ml of unfractionated heparin (UH). PMPGA was performed using FACSAria® flow cytometer. The clinical diagnosis was established by two blinded independent investigators analysing in a standardized manner the patient’s medical records. Performances of PMPGA and SRA (n=53) were evaluated using ROC curve analysis with clinical outcome as reference. Results: In positive HIT patients, PMPs expressing phosphatidylserine are generated with low UH concentration whereas PMP rate decreases significantly in presence of high UH concentration. Using clinical outcome as reference, sensitivity and specificity of PMPGA reached 88.9% (95% CI: 50.7-99.4) and 100.0% (95% CI: 90.0-100.0). Sensitivity and specificity of 14C-SRA were 88.9% (95% CI: 50.7-99.4) and 95.5% (95% CI: 83.3-99.2). Conclusions: PMPGA is a rapid and reliable assay for HIT diagnosis. PMPGA showed good correlation with 14C-SRA performances and predominately with clinical outcome. [Copyright &y& Elsevier]

Published

2014

9. Rapid exclusion of the diagnosis of immune HIT by AcuStar HIT and heparin-induced multiple electrode aggregometry.

Author

Minet, V., Baudar, J., Bailly, N., Douxfils, J., Laloy, J., Lessire, S., Gourdin, M., Devalet, B., Chatelain, B., Dogné, J.M., and Mullier, F.

Subjects

*HEPARIN, *ELECTRODES, *THROMBOCYTOPENIA, *COMPARATIVE studies, *RETROSPECTIVE studies, *CLINICAL trials

Abstract

Abstract: Background: Accurate diagnosis of heparin-induced thrombocytopenia (HIT) is essential but remains challenging. We have previously demonstrated, in a retrospective study, the usefulness of the combination of the 4Ts score, AcuStar HIT and heparin-induced multiple electrode aggregometry (HIMEA) with optimized thresholds. Objectives: We aimed at exploring prospectively the performances of our optimized diagnostic algorithm on suspected HIT patients. The secondary objective is to evaluate performances of AcuStar HIT-Ab (PF4-H) in comparison with the clinical outcome. Methods: 116 inpatients with clinically suspected immune HIT were included. Our optimized diagnostic algorithm was applied to each patient. Sensitivity, specificity, negative predictive value (NPV), positive predictive value (PPV) of the overall diagnostic strategy as well as AcuStar HIT-Ab (at manufacturer’s thresholds and at our thresholds) were calculated using clinical diagnosis as the reference. Results: Among 116 patients, 2 patients had clinically-diagnosed HIT. These 2 patients were positive on AcuStar HIT-Ab, AcuStar HIT-IgG and HIMEA. Using our optimized algorithm, all patients were correctly diagnosed. AcuStar HIT-Ab at our cut-off (>9.41 U/mL) and at manufacturer’s cut-off (>1.00 U/mL) showed both a sensitivity of 100.0% and a specificity of 99.1% and 90.4%, respectively. Conclusion: The combination of the 4Ts score, the HemosIL® AcuStar HIT and HIMEA with optimized thresholds may be useful for the rapid and accurate exclusion of the diagnosis of immune HIT. [Copyright &y& Elsevier]

Published

2014

10. Assessment of the performances of AcuStar HIT and the combination with heparin-induced multiple electrode aggregometry: A retrospective study.

Author

Minet, V., Bailly, N., Douxfils, J., Osselaer, J.C., Laloy, J., Chatelain, C., Elalamy, I., Chatelain, B., Dogné, J.M., and Mullier, F.

Subjects

*HEPARIN, *ELECTRODES, *RETROSPECTIVE studies, *EARLY diagnosis, *IMMUNE system, *THROMBOCYTOPENIA, *DIAGNOSIS

Abstract

Background: Early diagnosis of immune heparin-induced thrombocytopenia (HIT) is challenging. HemosIL® AcuStar HIT and heparin-induced multiple electrode aggregometry (HIMEA) were recently proposed as rapid diagnostic methods. Objectives: We conducted a study to assess performances of AcuStar HIT-IgG (PF4-H) and AcuStar HIT-Ab (PF4-H). The secondary objective was to compare the performances of the combination of Acustar HIT and HIMEA with standardised clinical diagnosis. Methods: Sera of 104 suspected HIT patients were retrospectively tested with AcuStar HIT. HIMEA was performed on available sera (n=81). The clinical diagnosis was established by analysing in a standardized manner the patient’s medical records. These tests were also compared with PF4-Enhanced®, LTA, and SRA in subsets of patients. Thresholds were determined using ROC curve analysis with clinical outcome as reference. Results: Using the recommended thresholds (1.00AU), the negative predictive value (NPV) of HIT-IgG and HIT-Ab were 100.0% (95% CI: 95.9%-100.0% and 95.7%-100.0%). The positive predictive value (PPV) were 64.3% (95% CI: 35.1%-87.2.2%) and 45.0% (95% CI: 23.2%-68.6%), respectively. Using our thresholds (HIT-IgG: 2.89AU, HIT-Ab: 9.41AU), NPV of HIT-IgG and HIT-Ab were 100.0% (95% CI: 96.0%-100.0% and 96.1%-100.0%). PPV were 75.0% (95% CI: 42.7%-94.5%) and 81.8% (95% CI: 48.3%-97.7%), respectively. Of the 79 patients with a medium-high pretest probability score, 67 were negative using HIT-IgG (PF4-H) test at our thresholds. HIMEA was performed on HIT-IgG positive patients. Using this combination, only one patient on 79 was incorrectly diagnosed. Conclusion: Acustar HIT showed good performances to exclude the diagnosis of HIT. Combination with HIMEA improves PPV. [ABSTRACT FROM AUTHOR]

Published

2013

11. Morphology, cytogenetics, and survival in myelodysplasia with del(20q) or ider(20q): a multicenter study.

Author

Mullier F, Daliphard S, Garand R, Dekeyser M, Cornet Y, Luquet I, Talmant P, Richebourg S, Jamar M, Dogné JM, Chatelain C, Michaux L, and Chatelain B

Published

2012

12. Coagulation function in fresh-frozen plasma prepared with two photochemical treatment methods: methylene blue and amotosalen.

Author

Osselaer J, Debry C, Goffaux M, Pineau J, Calomme G, Dubuc E, Chatelain B, Vandendaele M, Hsu J, Rheinschmidt M, and Lin L

Abstract

BACKGROUND: Pathogen inactivation of plasma intended for transfusion is now the standard of care in Belgium. Two methods for treatment of single plasma units are available: amotosalen plus ultraviolet A light and methylene blue plus visible light. This study compared the quality and stability of plasma treated with these two methods. STUDY DESIGN AND METHODS: Plasma units made from a pool of two ABO-matched fresh apheresis units were photochemically treated with either amotosalen (PCT-FFP) or methylene blue (MB-FFP). A total of 12 paired samples were evaluated. Plasma coagulation function was assessed at three time points: immediately after treatment, after 30 days of frozen storage, and an additional 24 hours at 4 degrees C after thawing. Comparison between PCT-FFP and MB-FFP was assessed with the paired t test and a p value of less than 0.05 indicated statistical significance. RESULTS: Based on statistical analysis, mean levels of factor (F)II, FXII, FXIII, von Willebrand antigen, ADAMTS-13, D-dimers, and protein C were equivalent between PCT-FFP and MB-FFP for all three time points. PCT-FFP exhibited shorter mean prothrombin time, activated partial thromboplastin time (two time points), and thrombin time and higher mean levels of fibrinogen, FXI, and protein S than MB-FFP. Retention of FV, FVII, FVIII, FX, or von Willebrand factor:ristocetin cofactor in PCT-FFP was either equivalent to or higher than MB-FFP. MB-FFP contained higher mean levels of plasminogen, antithrombin, and plasmin inhibitor than PCT-FFP. Retention of F IX in MB-FFP was higher than PCT-FFP only after the 4 degrees C storage after thawing. CONCLUSION: There is adequate preservation of therapeutic coagulation factor activities in both PCT-FFP and MB-FFP. The overall coagulation factor levels and stability of PCT-FFP were better preserved than MB-FFP. [ABSTRACT FROM AUTHOR]

Published

2008

13. Biomechanical characterization of earlobe keloid by ring suction test.

Author

Elouneg, A., Lucot, Q., Veyrat-Durebex, E., Lejeune, A., Chambert, J., Lihoreau, T., Chatelain, B., Rolin, G., and Jacquet, E.

Subjects

*KELOIDS, *DIGITAL image correlation

Published

2020

14. Biomechanical characterization of earlobe keloid by ring suction test.

Author

Elouneg, A., Lucot, Q., Veyrat-Durebex, E., Lejeune, A., Chambert, J., Lihoreau, T., Chatelain, B., Rolin, G., and Jacquet, E.

Subjects

*KELOIDS, *DIGITAL image correlation

Abstract

Keywords: Ring suction test; keloid scar; earlobe; Clinical investigation EN Ring suction test keloid scar earlobe Clinical investigation S99 S100 2 11/26/20 20200902 NES 200902 1. The device is applied on earlobe after earlobe keloid surgery in order to prevent from keloid recurrency. After validation of the experimental process on the healthy soft tissue, the ring suction test has been applied on a keloid scar situated on a young male African-American earlobe skin. [Extracted from the article]

Published

2020

15. Clearance kinetics of CD34+ cells from peripheral blood: an independent predictor of hematologic recovery after high-dose chemotherapy and hematopoietic stem cell transplantation.

Author

D’Hondt, L, Wuu, J, André, M, van Lerberghe, C, Guillaume, T, Feyens, A-M, Humblet, Y, Dromelet, A, Chatelain, B, Longueville, J, Stewart, F M, D’Hondt, V, and Symann, M

Subjects

*HEMATOPOIETIC stem cell transplantation, *BREAST cancer, *CD antigens, *DRUG therapy

Abstract

We measured the concentration of CD34+ cells in peripheral blood (PB) ½ h prior to and ½, 1, 3, 6, and 12 h following hematopoietic stem cell (HSC) infusion in 34 breast cancer patients treated with high-dose chemotherapy (HDC). The decrease in these concentrations over time enabled us to determine the clearance kinetics of CD34+ cells from PB. The absolute number of CD34+ cells in PB generally peaked at ½ h after infusion, then rapidly declined from 1 to 3 h post infusion and continued to fall until 12 h post transplant, but more slowly. In univariate analysis, CD34+cells/kg infused, CFU-GM/kg infused, the CD34+ count at ½ h, and the 12-h clearance of CD34+ cells from PB were predictors of hematologic recovery, as were each of the two phases of clearance when the slope was divided into rapid and slow phases (from ½ to 3 and from 3 to 12 h post transplant, respectively). We then stratified our population by the number of CD34+ cells/kg infused. In group 1, patients received 7.5 × 106 CD34+ cells/kg; in group 2, >7.5 × 106 CD34+ cells/kg. After adjusting for CD34+ cells injected, age, and purged or unpurged graft in multivariate analysis, the 12 h clearance remained a predictor of hematologic recovery in group 1. In addition, the second phase of clearance (from 3 to 12 h after infusion) was an even better predictor than the 12 h clearance. In group 2, however, no statistically significant correlation was observed, even with the number of HSC injected. Results suggest that rapidity of clearance of CD34+cells from PB is an independent indicator of hematologic recovery in patients receiving lower doses of CD34+ cells. When the cell dose injected is over a threshold, PB clearance correlations with hematologic recovery are masked. [ABSTRACT FROM AUTHOR]

Published

1999

16. Two-site evaluation of high-fluorescent cells for the detection of malignant cells: The importance of clinical information.

Author

Favresse, J., Boland, L., Schellen, M., Chatelain, B., Defour, J., Mullier, F., and Jacqmin, H.

Subjects

*FLUORESCENT probes, *CELLS, *SEROUS fluids

Published

2019

17. Management of the thrombotic risk associated with COVID-19: guidance for the hemostasis laboratory.

Author

Hardy, M., Lecompte, T., Douxfils, J., Lessire, S., Dogné, J. M., Chatelain, B., Testa, S., Gouin-Thibault, I., Gruel, Y., Medcalf, R. L., ten Cate, H., Lippi, G., and Mullier, F.

Subjects

*THROMBOSIS risk factors, *COVID-19 treatment, *ANTICOAGULANTS, *CORONAVIRUS diseases, *FIBRINOGEN, *FIBRINOLYSIS, *HEMOSTASIS, *HEPARIN, *PATHOLOGICAL laboratories, *RISK assessment, *THROMBOEMBOLISM, *THROMBOLYTIC therapy, *VEINS, *FIBRIN fibrinogen degradation products, *COVID-19

Abstract

Coronavirus disease 2019 (COVID-19) is associated with extreme inflammatory response, disordered hemostasis and high thrombotic risk. A high incidence of thromboembolic events has been reported despite thromboprophylaxis, raising the question of a more effective anticoagulation. First-line hemostasis tests such as activated partial thromboplastin time, prothrombin time, fibrinogen and D-dimers are proposed for assessing thrombotic risk and monitoring hemostasis, but are vulnerable to many drawbacks affecting their reliability and clinical relevance. Specialized hemostasis-related tests (soluble fibrin complexes, tests assessing fibrinolytic capacity, viscoelastic tests, thrombin generation) may have an interest to assess the thrombotic risk associated with COVID-19. Another challenge for the hemostasis laboratory is the monitoring of heparin treatment, especially unfractionated heparin in the setting of an extreme inflammatory response. This review aimed at evaluating the role of hemostasis tests in the management of COVID-19 and discussing their main limitations. [ABSTRACT FROM AUTHOR]

Published

2020

18. Focus on pre-processing step to ensure the clinical transferability of Raman data acquired on lymphocytes in different experimental and instrumental conditions.

Author

Féré, M., Piot, O., Liu, L.H, Beljebbar, A., Untereiner, V., Gheldof, D., Chollat, M., Klossa, J., Chatelain, B., and Gobinet, C.

Subjects

*OPERANT conditioning, *CHRONIC lymphocytic leukemia, *PRINCIPAL components analysis, *LYMPHOCYTES, *DISCRIMINANT analysis, *PARTIAL least squares regression, *INSTRUMENTAL variables (Statistics), *B cells

Abstract

• Transferability of models. • Bench-to-bedside. • Pre-processing by EMSC allows multicentric data to be homogenized. The efficiency of Raman spectroscopy for the analysis of biomedical samples has been largely demonstrated at the proof-of-concept stage during one-off measurement campaigns. However, bringing these results to the patient bedside requires to fill the gap for transferability of Raman data acquired in different experimental and instrumental conditions during multicentric measurement campaigns. In this study, we propose to evaluate a solution consisting in the application of Raman data preprocessing specifically developed to remove the spectral variability induced by such different conditions. For this purpose, we compared Raman data of lymphocytes acquired during two independent measurement campaigns from fresh unstained glass blood smears originating from healthy individuals and patients with a B-cell chronic lymphocytic leukemia (CLL) at an advanced stage. The differences between these campaigns were i) the instrumental configuration of the Raman devices, ii) the hospital partner, iii) the smear preparation method. A preprocessing developed previously and efficient for a specific measurement campaign is shown obsolete for these multicentric data. A second preprocessing based on Extended Multiplicative Signal Correction is able to homogenize the data by neutralizing the signal variability between the two measurement campaigns. These conclusions are drawn from the analysis of the data by Principal Component Analysis to study the source of variability between the two campaigns and by Partial Least Squares – Discriminant Analysis to assess the separability between healthy and CLL patients. [ABSTRACT FROM AUTHOR]

Published

2019