Your search keyword '"Grützner N"' showing total 5 results

1. Analytical validation of an enzyme-linked immunosorbent assay for the quantification of S100A12 in the serum and feces of cats.

Author

Bridges CS, Grützner N, Suchodolski JS, Steiner JM, and Heilmann RM

Subjects

Animals, Biomarkers analysis, Cat Diseases blood, Cat Diseases metabolism, Cats blood, Enzyme-Linked Immunosorbent Assay methods, Feces chemistry, Female, Inflammation blood, Inflammation metabolism, Inflammation veterinary, Male, Reference Values, Reproducibility of Results, S100A12 Protein blood, Cats metabolism, Enzyme-Linked Immunosorbent Assay veterinary, S100A12 Protein analysis

Abstract

Background: Measuring S100A12 concentrations in serum and feces is a sensitive and specific marker of inflammation, such as seen with chronic gastrointestinal inflammation in people and dogs. Biomarkers of inflammation in cats are currently lacking., Objectives: We aimed to analytically cross-validate the canine S100A12-ELISA for the measurement of S100A12 in feline specimens., Methods: The ELISA was analytically validated by assessing dilutional linearity, spiking/recovery, intra- and inter-assay variability. Reference intervals for serum and fecal feline S100A12 concentrations were calculated using samples from healthy cats, and the short-term biological variation of fecal S100A12 was assessed., Results: Observed-to-expected ratios (O/E) for serial dilutions of serum and fecal extracts ranged from 91%-159% (mean, 120%) and 100%-128% (mean, 114%), and for the spiking/recovery method ranged from 106%-263% (mean, 154%) and 52%-171% (mean, 112%). Intra- and inter-assay CV% for serum were ≤5.6% and ≤14.0%, and for fecal extracts were ≤3.8% and ≤19.1%, repsectively. RIs for feline serum and fecal S100A12 concentrations were <43 µg/L and < 20 ng/g, respectively. A mild short-term biologic variation, but large individuality were detected when measuring fecal S100A12 concentrations in healthy cats., Conclusions: The canine S100A12-ELISA is accurate, reproducible, and sufficiently linear and precise for the measurement of S100A12 in feline serum and fecal samples. The use of this assay is a reasonable option for the measurement of S100A12 concentrations in feline specimens and provides a basis for the further evaluation of  S100A12 in cats with gastrointestinal disease. Using a population-based RI for fecal feline S100A12 appears to be of limited value., (© 2019 American Society for Veterinary Clinical Pathology.)

Published

2019

2. Biological variation of serum canine calprotectin concentrations as measured by ELISA in healthy dogs.

Author

Heilmann RM, Ruaux CG, Grützner N, Cranford SM, Bridges CS, and Steiner JM

Subjects

Animals, Biological Variation, Individual, Dogs immunology, Female, Inflammation Mediators blood, Male, Dogs blood, Enzyme-Linked Immunosorbent Assay veterinary, Leukocyte L1 Antigen Complex blood

Abstract

Calprotectin is a useful biomarker of inflammation in dogs. However, the biological variation of serum canine calprotectin is unknown. Indices of biological variation were determined in serial serum samples (n=147) from 11 healthy dogs (males/females: 4/7, median age: 5 years): analytical (3.0%), intra-individual (29.9%), and inter-individual variation (33.2%), reciprocal index of individuality (1.1), and index of heterogeneity (4.9). Serum calprotectin concentrations measured by ELISA and by the previous radioimmunoassay were highly correlated, but a constant and proportional bias exists between both assays. A de novo ELISA-reference interval (RI) for serum calprotectin concentration was established (0.6-11.8mg/L). Moderate changes in serum calprotectin (minimum critical difference: 6.4mg/L) between sequential measurements are needed to be considered relevant, and a population-based RI may or may not be appropriate for serum calprotectin., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

3. Validation of an enzyme-linked immunosorbent assay (ELISA) for the measurement of canine S100A12.

Author

Heilmann RM, Cranford SM, Ambrus A, Grützner N, Schellenberg S, Ruaux CG, Suchodolski JS, and Steiner JM

Subjects

Animals, Dogs, Feces chemistry, Female, Male, Rabbits, Reference Values, Reproducibility of Results, S100A12 Protein blood, Dog Diseases blood, Enzyme-Linked Immunosorbent Assay veterinary, S100A12 Protein analysis

Abstract

Background: Canine S100 calcium-binding protein A12 (cS100A12) shows promise as biomarker of inflammation in dogs. A previously developed cS100A12-radioimmunoassay (RIA) requires radioactive tracers and is not sensitive enough for fecal cS100A12 concentrations in 79% of tested healthy dogs. An ELISA assay may be more sensitive than RIA and does not require radioactive tracers., Objective: The purpose of the study was to establish a sandwich ELISA for serum and fecal cS100A12, and to establish reference intervals (RI) for normal healthy canine serum and feces., Methods: Polyclonal rabbit anti-cS100A12 antibodies were generated and tested by Western blotting and immunohistochemistry. A sandwich ELISA was developed and validated, including accuracy and precision, and agreement with cS100A12-RIA. The RI, stability, and biologic variation in fecal cS100A12, and the effect of corticosteroids on serum cS100A12 were evaluated., Results: Lower detection limits were 5 μg/L (serum) and 1 ng/g (fecal), respectively. Intra- and inter-assay coefficients of variation were ≤ 4.4% and ≤ 10.9%, respectively. Observed-to-expected ratios for linearity and spiking recovery were 98.2 ± 9.8% (mean ± SD) and 93.0 ± 6.1%, respectively. There was a significant bias between the ELISA and the RIA. The RI was 49-320 μg/L for serum and 2-484 ng/g for fecal cS100A12. Fecal cS100A12 was stable for 7 days at 23, 4, -20, and -80°C; biologic variation was negligible but variation within one fecal sample was significant. Corticosteroid treatment had no clinically significant effect on serum cS100A12 concentrations., Conclusions: The cS100A12-ELISA is a precise and accurate assay for serum and fecal cS100A12 in dogs., (© 2016 American Society for Veterinary Clinical Pathology.)

Published

2016

4. Cold Microwave-Enabled Protein Detection and Quantification.

Author

Grützner N, Heilmann RM, Smith AG, Johnson CB, Vitha S, Steiner JM, and Holzenburg AK

Subjects

Animals, Blotting, Western instrumentation, Electrophoresis, Polyacrylamide Gel methods, Enzyme-Linked Immunosorbent Assay instrumentation, Equipment Design, Humans, Immunoblotting instrumentation, Signal-To-Noise Ratio, Blotting, Western methods, Enzyme-Linked Immunosorbent Assay methods, Immunoblotting methods, Microwaves, Proteins analysis

Abstract

Protein screening/detection is an essential tool in many laboratories. Owing to the relatively large time investments that are required by standard protocols, the development of methods with higher throughput while maintaining an at least comparable signal-to-noise ratio is highly beneficial in many research areas. This chapter describes how cold microwave technology can be used to enhance the rate of molecular interactions and provides protocols for dot blots, Western blots, and ELISA procedures permitting a completion of all incubation steps (blocking and antibody steps) within 24-45 min.

Published

2015

5. Cold-microwave enhanced enzyme-linked immunosorbent assays--a path to high-throughput clinical diagnostics.

Author

Grützner N, Heilmann RM, Suchodolski JS, Steiner JM, and Holzenburg A

Subjects

Animals, Dogs, Feces chemistry, Humans, Reproducibility of Results, Sensitivity and Specificity, Cold Temperature, Enzyme-Linked Immunosorbent Assay methods, Leukocyte L1 Antigen Complex blood, Leukocyte L1 Antigen Complex chemistry, Microwaves

Abstract

The enzyme-linked immunosorbent assay (ELISA) constitutes an important clinical diagnostic approach. However, the prolonged incubation times involved lead to turnaround times of typically ⩾1 day, potentially delaying a definitive diagnosis or an adequate treatment plan for individual patients. Here cold-microwave technology (CMT) was employed to significantly reduce the times required for diagnostic ELISAs. The new approach was validated and compared to a conventional ELISA setup measuring canine calprotectin (cCP). Canine serum and fecal specimens were used for the analytical validation of cCP ELISA by conventional and CMT-ELISA. Cross-validation of both ELISA methods consisted of the determination of analytic sensitivity, linearity, accuracy, precision, and reproducibility. The long-term stability of antibody-coated ELISA plates was also evaluated up to 33 days. The ELISA approaches were comparable to each other. The observed-to-expected ratios for linearity and accuracy were 100.2±11.8 and 98.1±10.8% (mean±standard deviation), respectively. Precision and reproducibility were ⩽17.2%. For samples run on precoated ELISA plates over 33 days %CVs were ⩽12.5%. While both ELISA approaches were analytically sensitive, linear, accurate, precise, and reproducible with measurements of cCP concentrations, CMT-ELISA offered a reduction in incubation times by 90-95%, facilitating a very fast turnaround time and suggesting CMT-ELISA for improved human and veterinary clinical diagnostics., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014