Simultaneous LC–MS determination of glucose regulatory peptides secreted by stem cell–derived islet organoids

Author:

Olsen Christine12ORCID,Wang Chencheng23,Aizenshtadt Aleksandra2,Abadpour Shadab23,Lundanes Elsa1,Skottvoll Frøydis Sved4,Golovin Alexey5,Busek Mathias2,Krauss Stefan25,Scholz Hanne23,Wilson Steven Ray23

Affiliation:

1. Department of Chemistry University of Oslo, Blindern Oslo Norway

2. Hybrid Technology Hub‐Centre of Excellence Institute of Basic Medical Sciences Faculty of Medicine University of Oslo Oslo Norway

3. Department of Transplant Medicine and Institute for Surgical Research Oslo University Hospital Oslo Norway

4. Department of Smart Sensors and Microsystems SINTEF Digital Oslo Norway

5. Department of Immunology and Transfusion Medicine Oslo University Hospital Oslo Norway

Abstract

AbstractFor studying stem cell–derived islet organoids (SC‐islets) in an organ‐on‐chip (OoC) platform, we have developed a reversed‐phase liquid chromatography–tandem mass spectrometry (RPLC–MS/MS) method allowing for simultaneous determination of insulin, somatostatin‐14, and glucagon, with improved matrix robustness compared to earlier methodology. Combining phenyl/hexyl‐C18 separations using 2.1 mm inner diameter LC columns and triple quadrupole mass spectrometry, identification and quantification were secured with negligible variance in retention time and quantifier/qualifier ratios, negligible levels of carryover (<2%), and sufficient precision (±10% RSD) and accuracy (±15% relative error) with and without use of an internal standard. The obtained lower limits of quantification were 0.2 µg/L for human insulin, 0.1 µg/L for somatostatin‐14, and 0.05 µg/L for glucagon. The here‐developed RPLC–MS/MS method showed that the SC‐islets have an insulin response dependent on glucose concentration, and the SC‐islets produce and release somatostatin‐14 and glucagon. The RPLC–MS/MS method for these peptide hormones was compatible with an unfiltered offline sample collection from SC‐islets cultivated on a pumpless, recirculating OoC (rOoC) platform. The SC‐islets background secretion of insulin was not significantly different on the rOoC device compared to a standard cell culture well‐plate. Taken together, RPLC–MS/MS method is well suited for multi‐hormone measurements of SC‐islets on an OoC platform.

Funder

Norges Forskningsråd

Publisher

Wiley

Subject

Clinical Biochemistry,Biochemistry,Analytical Chemistry

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