Preparation of a Mesoporous Biosensor for Human Lactate Dehydrogenase for Potential Anticancer Inhibitor Screening

Clarissa Cocuzza; Elena Antoniono; Carminna Ottone; Valentina Cauda; Debora Fino; Marco Piumetti

doi:10.1021/acsbiomaterials.3c00582

Preparation of a Mesoporous Biosensor for Human Lactate Dehydrogenase for Potential Anticancer Inhibitor Screening

ACS Biomater Sci Eng. 2023 Nov 13;9(11):6045-6057. doi: 10.1021/acsbiomaterials.3c00582. Epub 2023 Oct 19.

Authors

Clarissa Cocuzza¹, Elena Antoniono¹, Carminna Ottone², Valentina Cauda¹, Debora Fino¹, Marco Piumetti¹

Affiliations

¹ Department of Applied Science and Technology, Politecnico di Torino, Corso Duca degli Abruzzi, 24, 10129 Turin, Italy.
² Escuela de Ingeniería Bioquímica, Pontificia Universidad Católica de Valparaíso, Av. Brasil 2085, Valparaíso 2340000, Chile.

Abstract

Cancer is the second leading cause of death worldwide, with a dramatic impact due to the acquired resistance of cancers to used chemotherapeutic drugs and treatments. The enzyme lactate dehydrogenase (LDH-A) is responsible for cancer cell proliferation. Recently the development of selective LDH-A inhibitors as drugs for cancer treatment has been reported to be an efficient strategy aiming to decrease cancer cell proliferation and increase the sensitivity to traditional chemotherapeutics. This study aims to obtain a stable and active biocatalyst that can be utilized for such drug screening purposes. It is conceived by adopting human LDH-A enzyme (hLDH-A) and investigating different immobilization techniques on porous supports to achieve a stable and reproducible biosensor for anticancer drugs. The hLDH-A enzyme is covalently immobilized on mesoporous silica (MCM-41) functionalized with amino and aldehyde groups following two different methods. The mesoporous support is characterized by complementary techniques to evaluate the surface chemistry and the porous structure. Fluorescence microscopy analysis confirms the presence of the enzyme on the support surface. The tested immobilizations achieve yields of ≥80%, and the best retained activity of the enzyme is as high as 24.2%. The optimal pH and temperature of the best immobilized hLDH-A are pH 5 and 45 °C for the reduction of pyruvate into lactate, while those for the free enzyme are pH 8 and 45 °C. The stability test carried out at 45 °C on the immobilized enzyme shows a residual activity close to 40% for an extended time. The inhibition caused by NHI-2 is similar for free and immobilized hLDH-A, 48% and 47%, respectively. These findings are significant for those interested in immobilizing enzymes through covalent attachment on inorganic porous supports and pave the way to develop stable and active biocatalyst-based sensors for drug screenings that are useful to propose drug-based cancer treatments.

Keywords: MCM-41; NHI-2; covalent attachment; enzyme immobilization; hLDH-A; human lactate dehydrogenase; mesoporous silica.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Biosensing Techniques* / methods
Enzyme Stability
Enzymes, Immobilized / chemistry
Enzymes, Immobilized / metabolism
Humans
L-Lactate Dehydrogenase* / chemistry
L-Lactate Dehydrogenase* / metabolism
Lactate Dehydrogenase 5 / metabolism

Substances

L-Lactate Dehydrogenase
Lactate Dehydrogenase 5
Enzymes, Immobilized