Your search keyword '"D. Girelli"' showing total 6 results

1. Interference from immunocomplexes on a high-sensitivity cardiac troponin T immunoassay.

Author

Dalle Carbonare L, Pizzini M, Micheletti V, Lo Cascio C, Bovo C, Girelli D, and Lippi G

Subjects

Acute Coronary Syndrome blood, Acute Coronary Syndrome diagnosis, Adult, Artifacts, Biomarkers blood, Female, Gastritis blood, Gastritis diagnosis, Gastritis drug therapy, Humans, Proton Pump Inhibitors therapeutic use, Sensitivity and Specificity, Antigen-Antibody Complex blood, Immunoassay methods, Troponin T blood

Published

2020

2. Provisional standardization of hepcidin assays: creating a traceability chain with a primary reference material, candidate reference method and a commutable secondary reference material.

Author

Diepeveen LE, Laarakkers CMM, Martos G, Pawlak ME, Uğuz FF, Verberne KESA, van Swelm RPL, Klaver S, de Haan AFJ, Pitts KR, Bansal SS, Abbas IM, Fillet M, Lefebvre T, Geurts-Moespot AJ, Girelli D, Castagna A, Herkert M, Itkonen O, Olbina G, Tomosugi N, Westerman ME, Delatour V, Weykamp CW, and Swinkels DW

Subjects

Calibration, Chromatography, High Pressure Liquid standards, Enzyme-Linked Immunosorbent Assay standards, Hepcidins standards, Humans, Isotope Labeling, Reference Standards, Enzyme-Linked Immunosorbent Assay methods, Hepcidins blood, Tandem Mass Spectrometry standards

Abstract

Background Hepcidin concentrations measured by various methods differ considerably, complicating interpretation. Here, a previously identified plasma-based candidate secondary reference material (csRM) was modified into a serum-based two-leveled sRM. We validated its functionality to increase the equivalence between methods for international standardization. Methods We applied technical procedures developed by the International Consortium for Harmonization of Clinical Laboratory Results. The sRM, consisting of lyophilized serum with cryolyoprotectant, appeared commutable among nine different measurement procedures using 16 native human serum samples in a first round robin (RR1). Harmonization potential of the sRM was simulated in RR1 and evaluated in practice in RR2 among 11 measurement procedures using three native human plasma samples. Comprehensive purity analysis of a candidate primary RM (cpRM) was performed by state of the art procedures. The sRM was value assigned with an isotope dilution mass spectrometry-based candidate reference method calibrated using the certified pRM. Results The inter-assay CV without harmonization was 42.1% and 52.8% in RR1 and RR2, respectively. In RR1, simulation of harmonization with sRM resulted in an inter-assay CV of 11.0%, whereas in RR2 calibration with the material resulted in an inter-assay CV of 19.1%. Both the sRM and pRM passed international homogeneity criteria and showed long-term stability. We assigned values to the low (0.95±0.11 nmol/L) and middle concentration (3.75±0.17 nmol/L) calibrators of the sRM. Conclusions Standardization of hepcidin is possible with our sRM, which value is assigned by a pRM. We propose the implementation of this material as an international calibrator for hepcidin.

Published

2019

3. Sialylated isoforms of apolipoprotein C-III and plasma lipids in subjects with coronary artery disease.

Author

Olivieri O, Chiariello C, Martinelli N, Castagna A, Speziali G, Girelli D, Pizzolo F, Bassi A, Cecconi D, Robotti E, Manfredi M, Conte E, and Marengo E

Subjects

Aged, Apolipoprotein A-I blood, Apolipoprotein A-I isolation & purification, Apolipoprotein C-III isolation & purification, Apolipoproteins E blood, Apolipoproteins E isolation & purification, Chromatography, High Pressure Liquid, Female, Humans, Lipoprotein Lipase metabolism, Lipoproteins, LDL blood, Male, Mass Spectrometry, Middle Aged, Protein Isoforms blood, Protein Isoforms isolation & purification, Solid Phase Extraction, Triglycerides blood, Apolipoprotein C-III blood, Coronary Artery Disease pathology

Abstract

Background: Apolipoprotein C-III (ApoC-III), a key regulator of plasma triglyceride (TG), is present in three isoforms, i.e. non-sialylated (ApoC-III0), monosialylated (ApoC-III1) and disialylated (ApoC-III2). We aimed at quantifying the distribution of the ApoC-III glycoforms in patients with angiographically demonstrated coronary artery disease (CAD) according to levels of total ApoC-III plasma concentration., Methods: ApoC-III glycoforms were quantified by a specifically developed, high-resolution, mass spectrometry method in unrelated CAD patients. Lipoprotein lipase (LPL) activity was estimated by a fluorescence-based method., Results: In 101 statin-treated CAD patients, the absolute concentrations of the three glycoforms similarly increased across ApoC-III quartiles, but the proportion of ApoC-III1 rose whereas that of ApoC-III0 decreased progressively by increasing total ApoC-III concentrations. The proportion of ApoC-III2 was quite constant throughout the whole range of total ApoC-III. A higher proportion of ApoC-III1 reflected an unfavorable lipid profile characterized by high levels of TG, total and low density lipoprotein cholesterol, ApoE and reduced ApoA-I. The correlations between ApoC-III glycoforms and TG were confirmed in 50 statin-free CAD patients. High concentration of total ApoC-III was associated with low LPL activity, while no correlation was found for the relative proportion of glycoforms., Conclusions: Specific patterns of ApoC-III glycoforms are present across different total ApoC-III concentrations in CAD patients. The inhibitory effect of ApoC-III on LPL appears related to total ApoC-III concentration, but not to the relative proportion of ApoC-III glycoforms.

Published

2018

4. Hepcidin levels in chronic hemodialysis patients: a critical evaluation.

Author

Valenti L, Messa P, Pelusi S, Campostrini N, and Girelli D

Subjects

Anemia complications, Humans, Iron metabolism, Kidney Failure, Chronic complications, Kidney Failure, Chronic pathology, Renal Dialysis, Hepcidins blood, Kidney Failure, Chronic blood

Abstract

Altered systemic iron metabolism is a key element of uremia, and functional iron deficiency mainly related to subclinical inflammation makes it difficult to maintain proper control of anemia in chronic hemodialysis patients (CHD). In the last decade, the hepatic hormone hepcidin has been progressively recognized as the master regulator of circulating iron levels through the modulation of cellular iron fluxes in response to iron stores, as well as to erythroid and inflammatory stimuli. Hepcidin is cleared by the kidney and progression of renal disease has been associated to increased serum hepcidin levels. This, in turn, reduces iron availability for erythropoiesis, suggesting anti-hepcidin strategies for improving anemia control. Moreover, hepcidin has been recently implicated in the pathogenesis of long-term complications of dialysis, like accelerated atherosclerosis. Initial studies almost invariably reported a sustained increase of serum hepcidin in chronic hemodialysis patients. Noteworthy, such studies included relatively few patients and controls that were poorly matched for major determinants of serum hepcidin at population level, i.e., age and gender. More recent data based on accurately matched larger series challenge the view that hepcidin is intrinsically increased in hemodialysis patients, showing a marked inter- and intra-individual variability of hormone levels. Here we take a critical look to the data published so far on hepcidin levels in CHD, analyze the reasons underlying the discrepancies in available studies and the hepcidin variability in CHD, and point out the need for further studies in large series of well-characterized CHD patients and controls.

Published

2014

5. High resolution melting for the identification of mutations in the iron responsive element of the ferritin light chain gene.

Author

Castiglioni E, Soriani N, Girelli D, Camaschella C, Spiga I, Della Porta MG, Ferrari M, and Cremonesi L

Subjects

Cataract genetics, DNA genetics, Genetic Variation genetics, Humans, Iron Metabolism Disorders genetics, Mutation genetics, Nucleic Acid Denaturation, Sensitivity and Specificity, Syndrome, Apoferritins genetics, DNA Mutational Analysis methods, Iron pharmacology, Response Elements genetics

Abstract

Background: Among the causes of hyperferritinemia, hereditary hyperferritinemia cataract syndrome (HHCS) is an autosomal dominant disease characterized by distinctive cataracts and high serum ferritin. It is caused by mutations in the iron responsive element (IRE) of the ferritin light chain gene (FTL)., Methods: To speed up and simplify mutational scanning in this genomic region, we developed a protocol based on high-resolution melting (HRM) analysis., Results: Validation was carried out using 18 wild-type and 14 DNA samples carrying different mutations, each analyzed in replicates of 20. The method allowed for correct identification and genotyping of all mutant samples, and each variant generated a specific profile distinguishable from the wild type. A 5.5% proportion of false positive results were obtained. In addition, in two patients with HHCS, two new mutations were identified by HRM based on an altered melting profile. These mutations were subsequently characterized by direct sequencing (7C>G+40A>G and 49A>C)., Conclusions: The high reliability of HRM in detecting known and new DNA variations indicate that this could be an effective and sensitive method for molecular scanning of mutations in the IRE of the FTL gene in patients presenting with either HHCS or unexplained hyperferritinemia.

Published

2010

6. Novel serum paraoxonase activity assays are associated with coronary artery disease.

Author

Martinelli N, Girelli D, Olivieri O, Guarini P, Bassi A, Trabetti E, Friso S, Pizzolo F, Bozzini C, Tenuti I, Annarumma L, Schiavon R, Franco Pignatti P, and Corrocher R

Subjects

Coronary Artery Disease diagnosis, Female, Humans, Male, Middle Aged, Risk Factors, Aryldialkylphosphatase metabolism, Coronary Artery Disease blood, Coronary Artery Disease enzymology, Immunoassay methods

Abstract

Background: Serum paraoxonase (PON1) exerts antiatherogenic effects. Novel PON1 enzymatic tests have been recently developed: 5-thiobutyl butyrolactone (TBBL) estimates PON1 lactonase activity, whereas 7-O-diethylphosphoryl-3-cyano-4-methyl-7-hydroxycoumarin (DEPCyMC) is considered a surrogate marker of PON1 concentration. The TBBL to DEPCyMC ratio provides the normalized lactonase activity (NLA), which may reflect the degree of PON1 lactonase catalytic stimulation. The aim of this study was to evaluate for the first time TBBLase and DEPCyMCase activity in patients with coronary artery disease (CAD)., Methods: An angiography-based case-control study was conducted, including 300 sex- and age-matched subjects [100 CAD-free, 100 CAD without myocardial infarction (MI) and 100 CAD with MI]., Results: A low DEPCyMCase activity (lowest vs. highest tertile: OR 2.96, 95% CI 1.18-7.43) and a high NLA (highest vs. lowest tertile: OR 3.25, 95% CI 1.28-8.26) were both associated with CAD, independent of classical atherosclerosis risk factors, lipid-lowering therapy and PON1 genotype. Total TBBLase activity was, however, not different in CAD compared to CAD-free subjects., Conclusions: Novel PON1 activity assays may be associated with CAD. In this study, CAD patients had low DEPCyMCase activity, a possible marker of low PON1 concentration, but showed a high stimulation of PON1 lactonase activity.

Published

2009