4.7 Article

Functionally modified chitotriosidase catalytic domain for chitin detection based on split-luciferase complementation

Journal

CARBOHYDRATE POLYMERS
Volume 282, Issue -, Pages -

Publisher

ELSEVIER SCI LTD
DOI: 10.1016/j.carbpol.2022.119125

Keywords

Chitin; Chitosan; Chitin binding-module; Chitinase; Chit1; NanoBiT

Funding

  1. Japan Society for the Promotion of Science (JSPS) KAKENHI [JP 20K07487]

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In this study, we developed a reliable method for chitin detection using a luciferase-fragment complementation assay. The use of a CatD mutant allowed for higher sensitivity and structure-specific detection of chitin. Furthermore, a sandwich ELISA using modified CatD showed a low detection limit for soluble chitin.
In this study, we applied a luciferase-fragment complementation assay for chitin detection. When luciferasefragment fused chitin-binding proteins were mixed with chitin, the reconstituted luciferase became active. The recombinant chitin-binding domain (CBD) and a functionally modified catalytic domain (CatD) of human chitotriosidase were employed for this method. We designed the CatD mutant as a chitin-binding protein with diminished chitinolytic activity. The non-wash assay using the CatD mutant had higher sensitivity than CBD for chitin detection and proved to be a structure-specific biosensor for chitin, including crude biomolecules (from fungi, mites, and cockroaches). The CatD mutant recognized a chitin-tetramer as the minimal binding unit and bound chitin at K-D 99 nM. Furthermore, a sandwich ELISA using modified CatD showed a low limit of quantification for soluble chitin (13.6 pg/mL). Altogether, our work shows a reliable method for chitin detection using the potential capabilities of CatD.

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