Dipeptidyl peptidase 4 (DPP4) in fecal samples: validation of the extraction methodology and stability in short-term storage conditions

Author:

Gomes Sandra F.123ORCID,Melo Francisco Jorge13,Silva Rita4,Santiago Mafalda4,Estevinho Maria Manuela135,Dias Sandra4,Dias Cláudia Camila67,Magro Fernando148910

Affiliation:

1. Department of Biomedicine , Unit of Pharmacology and Therapeutics, Faculty of Medicine, University of Porto , Porto , Portugal

2. Department of Public Health and Forensic Sciences and Medical Education , Faculty of Medicine, University of Porto , Porto , Portugal

3. Center for Drug Discovery and Innovative Medicines (MedInUP), University of Porto , Porto , Portugal

4. Portuguese Study Group of Inflammatory Bowel Disease (GEDII) , Porto , Portugal

5. Department of Gastroenterology , Vila Nova de Gaia/Espinho Hospital Center , Vila Nova de Gaia , Portugal

6. Department of Community Medicine , Information and Health Decision Sciences (MEDCIDS), Faculty of Medicine, University of Porto , Porto , Portugal

7. Center for Health Technology and Services Research (CINTESIS) , Porto , Portugal

8. RISE – Health Research Network , Porto , Portugal

9. Department of Gastroenterology , São João University Hospital Center , Porto , Portugal

10. Clinical Pharmacology Unit, São João University Hospital Center , Porto , Portugal

Abstract

Abstract Objectives This study assesses the clinical relevance of dipeptidyl peptidase 4 (DPP4) membrane exopeptidase as a biomarker of inflammatory bowel disease (IBD). A spike-and-recovery approach of DPP4 in fecal samples was used to compare two different methods for protein extraction, followed by a stability assessment. Methods Fecal samples of healthy volunteers spiked with known concentrations of recombinant DPP4 were processed using a standard manual extraction protocol and the CALEX® protocol. The two methods were compared by quantification of fecal DPP4 by ELISA, followed by Bland-Altman analysis. For the stability assays DPP4 was extracted from fecal samples and stored under different conditions of temperature and time after collection. Results In general, the levels of spiked DPP4 in stool samples were lower with the manual protocol than in those obtained with the CALEX® method; this trend was corroborated by Bland-Altman analysis. Nonetheless, variability was within the acceptable limits for both protocols. In the stability assessment, no statistically significant differences were found between the results obtained under the different storage conditions. Conclusions Both manual and CALEX® protocols provided equal extraction ability of DPP4 from stool samples. In addition, DPP4 provided flexibility in terms of sample storage enabling the accurate assessment of samples delivered up to a week before analysis.

Publisher

Walter de Gruyter GmbH

Subject

Biochemistry (medical),Clinical Biochemistry,General Medicine

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