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001-es BibID:BIBFORM054689
Első szerző:Antal-Szalmás Péter (laboratóriumi szakorvos)
Cím:Measurement of soluble biomarkers by flow cytometry / Péter Antal-Szalmás, Béla Nagy Jr., Ildikó Beke Debreceni, János Kappelmayer
Dátum:2013
Megjegyzések:Microparticle based flow cytometric assays for determination of the level of soluble biomarkers are widely used in several research applications and in some diagnostic setups. The major advantages of these multiplex systems are that they can measure a large number of analytes (up to 500) at the same time reducing assay time, costs and sample volume. Most of these assays are based on antigen-antibody interactions and work as traditional immunoassays, but nucleic acid alterations - by using special hybridization probes -, enzyme- substrate or receptor-ligand interactions can be also studied with them. The applied beads are nowadays provided by the manufacturers, but cheaper biological microbeads can be prepared by any user. One part of the systems can be used on any research or clinical cytometers, but some companies provide dedicated analyzers for their multiplex bead arrays. Due to the high standardization of the bead production and the preparation of the assay components the analytical properties of these assays are quite reliable with a wide range of available applications. Cytokines, intracellular fusion protei ns, activated/phosphorylated components of different signaling pathways, transcription factors and nuclear receptors can be identified and quantitated. The assays may serve the diagnostics of autoimmune disorders, different viral and bacterial infections, as well as genetic alterations such as single nucleotide polymorphisms, small deletions/insertions or even nucleotide triplet expansions can be also identified. The most important principles, technical details and applications of these systems are discussed in this short review.
Tárgyszavak:Orvostudományok Klinikai orvostudományok idegen nyelvű folyóiratközlemény külföldi lapban
Megjelenés:EJIFCC [electronic resource]. - 23 : 4 (2013), p. [1-8]. -
További szerzők:Nagy Béla Jr. (1980-) (labordiagnosztikai szakorvos) Bekéné Debreceni Ildikó (1970-) (biológus) Kappelmayer János (1960-) (laboratóriumi szakorvos)
Internet cím:Intézményi repozitóriumban (DEA) tárolt változat
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2.

001-es BibID:BIBFORM068933
Első szerző:Hudák Renáta
Cím:Laboratory characterization of leukemic cell procoagulants / Renáta Hudák, Ildikó Beke Debreceni, Ivett Deák, Gabriella Gál Szabó, Zsuzsanna Hevessy, Péter Antal-Szalmás, Bjarne Osterud, János Kappelmayer
Dátum:2017
ISSN:1434-6621
Megjegyzések:Background: In acute myeloid leukemias, there is anincreased chance to develop thrombotic disorders. Wehypothesized that in addition to leukemic promyelocytes,monocytic leukemia cells may also have a higher procoagulantactivity.Methods: Fibrin formation was assessed by a one-stageclotting assay using a magnetic coagulometer. The thrombingeneration test (TGT) of magnetically isolated normalhuman monocytes, intact leukemic cells and their isolatedmicroparticles was performed by a fluorimetric assay.Phosphatidylserine (PS) expression of leukemic cells andmicroparticle number determinations were carried out byflow cytometry.Results: All cell lines displayed a significant procoagulantpotential compared to isolated normal human monocytes.In the TGT test, the mean of lagtime and the time to peakparameters were significantly shorter in leukemic cells(3.9?4.7 and 9.9?10.3 min) compared to monocytes (14.9and 26.5 min). The mean of peak thrombin in variousmonocytic leukemia cell lines was 112.1?132.9 nM vs.75.1 nM in monocytes; however, no significant differencewas observed in the ETP parameter. Factor VII-deficientplasma abolished all procoagulant activity, whereas factorXII-deficient plasma did not affect the speed of fibrinformation and thrombin generation but modulated theamount of thrombin. Factor XI-deficient plasma affectedthe time to peak values in one leukemic cell line and alsoattenuated peak thrombin. Leukemia cell-derived microparticlesfrom all three cell lines exerted a procoagulanteffect by significantly shortening the lagtime in TGT; therewas a nonsignificant difference in case of ETP parameter.Conclusions: All investigated monocytic leukemia celllines exhibited significant thrombin generation. This phenomenonwas achieved by the procoagulants on the surfaceof leukemic cells as well as by their microparticles.
Tárgyszavak:Orvostudományok Klinikai orvostudományok idegen nyelvű folyóiratközlemény külföldi lapban
monocytic leukemia
tissue factor
Megjelenés:Clinical Chemistry and Laboratory Medicine 55 : 8 (2017), p. 1215-1223. -
További szerzők:Bekéné Debreceni Ildikó (1970-) (biológus) Deák Ivett Gál Szabó Gabriella Hevessy Zsuzsanna (1966-) (laboratóriumi szakorvos) Antal-Szalmás Péter (1968-) (laboratóriumi szakorvos) Osterud, Bjarne Kappelmayer János (1960-) (laboratóriumi szakorvos)
Pályázati támogatás:TÁMOP-4.2.4.A/2-11-1-2012-0001
TÁMOP
Internet cím:Intézményi repozitóriumban (DEA) tárolt változat
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3.

001-es BibID:BIBFORM054351
Első szerző:Kappelmayer János (laboratóriumi szakorvos)
Cím:Distinct effects of Re- and S-forms of LPS on modulating platelet activation / J. Kappelmayer, I. Beke Debreceni, A. Vida, P. Antal-Szalmás, K. J. Clemetson, B. Nagy Jr.
Dátum:2013
ISSN:1538-7933
Tárgyszavak:Orvostudományok Klinikai orvostudományok idegen nyelvű folyóiratközlemény külföldi lapban
Megjelenés:Journal of Thrombosis and Haemostasis. - 11 : 4 (2013), p. 775-778. -
További szerzők:Bekéné Debreceni Ildikó (1970-) (biológus) Vida András (1979-) (molekuláris biológus, genetikus) Antal-Szalmás Péter (1968-) (laboratóriumi szakorvos) Clemetson, Kenneth J. Nagy Béla Jr. (1980-) (labordiagnosztikai szakorvos)
Internet cím:Intézményi repozitóriumban (DEA) tárolt változat
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