4.7 Article

Immobilisation of Neuro-2a cells on electrodes and electrochemical detection of MTT formazan crystals to assess their viability

Journal

BIOELECTROCHEMISTRY
Volume 148, Issue -, Pages -

Publisher

ELSEVIER SCIENCE SA
DOI: 10.1016/j.bioelechem.2022.108274

Keywords

Neuro-2a cell; Electrode; Tetrazolium salt; Ciguatoxin; Tetrodotoxin; Cell -based biosensor

Funding

  1. Ministerio de Ciencia e Innovacion (MICIN)
  2. Agencia Estatal de Investigacion (AEI) [PID2020-112976RB-C21, PID2019-108781RR-C21]
  3. CERCA Programme/Generalitat de Catalunya
  4. MICIN
  5. AEI [PRE2019-088181]

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Marine toxins are potent toxic compounds that need to be detected in seafood to prevent human poisoning. The development of cell-based biosensors for neurotoxins is crucial. This study immobilized Neuro-2a cells on different electrodes and evaluated their presence and viability using MTT detection. The system successfully detected toxicity in standard solutions of CTX1B and TTX, as well as fish extracts containing these toxins.
Marine toxins are potent toxic compounds that may reach humans and poison them. Therefore, their detection in seafood is crucial to prevent intoxication cases. Colorimetric cell-based assays (CBAs) have been developed to analyse marine neurotoxins, such as ciguatoxins (CTXs) and tetrodotoxins (TTXs), and are based on the toxi-cological effect of these toxins on the cells. Cell viability can be quantified by measuring the mitochondrial activity with 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT). With the purpose of moving forward in the development of cell-based biosensors (CBBs) for neurotoxins, Neuro-2a cells were immobilised on electrodes of different materials (carbon, carbon/polyaniline, carbon/poly-L-lysine, carbon/poly(3,4-ethylenedioxythiophene) and gold) and their presence and viability were assessed by the detection of MTT formazan crystals with cyclic voltammetry (CV). Best results in terms of oxidation potential and current intensity were achieved with carbon and carbon/polyaniline electrodes. Light microscopy also proved the presence of immobilised and living cells on electrodes. Cell density, incubation time and MTT concentration were optimised. Appropriate electrochemical responses were obtained incubating 100,000 cells/electrode for 2 h and using 0.86 mg/mL MTT. The system was able to detect toxicity when exposed to CTX1B and TTX standard solutions as well as Seriola dumerili and Lagocephalus sceleratus fish extracts containing these toxins.

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