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Immobilization of glucose oxidase on bioinspired polyphenol coatings as a high-throughput glucose assay platform.
Sunoqrot, Suhair; Al-Hadid, Amani; Manasrah, Ahmad; Khnouf, Ruba; Hasan Ibrahim, Lina.
Afiliação
  • Sunoqrot S; Department of Pharmacy, Faculty of Pharmacy, Al-Zaytoonah University of Jordan Amman 11733 Jordan suhair.sunoqrot@zuj.edu.jo +962 64291423 +962 64291511 ext. 197.
  • Al-Hadid A; Department of Pharmacy, Faculty of Pharmacy, Al-Zaytoonah University of Jordan Amman 11733 Jordan suhair.sunoqrot@zuj.edu.jo +962 64291423 +962 64291511 ext. 197.
  • Manasrah A; Department of Mechanical Engineering, Faculty of Engineering and Technology, Al-Zaytoonah University of Jordan Amman 11733 Jordan.
  • Khnouf R; Department of Biomedical Engineering, Faculty of Engineering, Jordan University of Science and Technology Irbid 22110 Jordan.
  • Hasan Ibrahim L; Department of Pharmacy, Faculty of Pharmacy, Al-Zaytoonah University of Jordan Amman 11733 Jordan suhair.sunoqrot@zuj.edu.jo +962 64291423 +962 64291511 ext. 197.
RSC Adv ; 11(62): 39582-39592, 2021 Dec 06.
Article em En | MEDLINE | ID: mdl-35492494
Glucose oxidase (GOx) is an enzyme with important industrial and biochemical applications, particularly in glucose detection. Here we leveraged the oxidative self-polymerization phenomenon of simple polyphenols (pyrogallol or catechol) in the presence of polyethylenimine (PEI) to form adhesive coatings that enabled GOx immobilization on conventional multi-well plates. Immobilization was verified and optimized by directly measuring GOx activity inside the coated wells. Our results showed that incorporating PEI in polyphenol coatings enhanced their enzyme immobilization efficiency, with pyrogallol (PG)-based coatings displaying the greatest enzyme activity. The immobilized enzyme maintained similar affinity to glucose compared to the free enzyme. GOx-immobilized PG/PEI-coated wells exhibited intermediate recycling ability but excellent resistance to urea as a denaturing agent compared to the free enzyme. GOx-immobilized 96-well plates allowed the construction of a linear glucose calibration curve upon adding glucose standards, with a detection limit of 0.4-112.6 mg dL-1, which was comparable to commercially available enzymatic glucose assay kits. The assay platform was also capable of effectively detecting glucose in rat plasma samples. Our findings present a simple enzyme immobilization technique that can be used to construct a glucose assay platform in a convenient multi-well format for high-throughput glucose quantification.

Texto completo: 1 Base de dados: MEDLINE Idioma: En Ano de publicação: 2021 Tipo de documento: Article

Texto completo: 1 Base de dados: MEDLINE Idioma: En Ano de publicação: 2021 Tipo de documento: Article