Pregled bibliografske jedinice broj: 1155729
Assay of haptoglobin, the plasma acute‐phase protein, by hemoglobin binding: Optimization of a novel chromogen
Assay of haptoglobin, the plasma acute‐phase protein, by hemoglobin binding: Optimization of a novel chromogen // 2020 Annual Meeting for ACVP, ASVCP, and ISACP
Chicago (IL), Sjedinjene Američke Države, 2021. str. 104-104 (predavanje, međunarodna recenzija, sažetak, znanstveni)
CROSBI ID: 1155729 Za ispravke kontaktirajte CROSBI podršku putem web obrasca
Naslov
Assay of haptoglobin, the plasma
acute‐phase protein, by hemoglobin binding:
Optimization of a novel chromogen
Autori
Blanka Beer Ljubić ; Vladimir Mrljak ; Romana Turk ; Nicola Brady ; David Eckersall
Vrsta, podvrsta i kategorija rada
Sažeci sa skupova, sažetak, znanstveni
Skup
2020 Annual Meeting for ACVP, ASVCP, and ISACP
Mjesto i datum
Chicago (IL), Sjedinjene Američke Države, 12.10.2020
Vrsta sudjelovanja
Predavanje
Vrsta recenzije
Međunarodna recenzija
Ključne riječi
acute phase protein, haptoglobin, SAT3
Sažetak
Background: Haptoglobin (Hp) can be assayed by a biochemical assay based on its binding to hemoglobin (Hb) and preservation of the Hb peroxidase activity with the peroxidase‐ catalyzed reaction of 4‐aminoantipyrine and 8‐anilino‐1‐ naphthalone sulfonic acid as chromogen. The resulting product has low stability potentially lead‐ ing to poor precision. New peroxidase substrates are available that may improve the Hp assay. Objective: Assess an alternative peroxidase substrate for the assay of Hp. Method: The substrate, N, N’‐bis(2‐hydroxy‐3‐ sulfopropyl)‐ tolidine (SAT‐3, Dojindo, Japan) in buffer was optimized for use on an Architect c4000 Analyzer (Abbot, USA) so that 3 ml of sample was mixed with 157 mL of Hb reagent, 80 mL of SAT‐ 3 solution including H2O2 was added and absorbance at 660 nm determined. Validation was by determination of precision, limit of quantifica‐ tion, interference and detection of clinical changes by monitoring plasma Hp in healthy dairy cows (n = 10) and those with clinical mastitis (n = 10). Results: The SAT‐ 3chromogen product was stable for several min‐ utes post‐reaction with intra‐assay and inter‐ assay CVs below 6.5%. The limit of quantification assay was 0.05 g/L. Lipemia had no effect on Hp results to 0.16 g/L while hemolysis increased the apparent Hp concentration above 0.07 g/L of Hb. Haptoglobin in plasma from healthy cows (n = 10) was <0.05 g/L in all samples, while the median (range) in plasma from cows with clinical mastitis (n = 10) was signifi‐ cantly greater (P = .0011) at 0.15 (<0.05‐0.84) g/L. Conclusion: The use of SAT3 is effective as a peroxidase substrate for the assay of Hp in plasma.
Izvorni jezik
Engleski
Znanstvena područja
Veterinarska medicina
POVEZANOST RADA
Ustanove:
Veterinarski fakultet, Zagreb
