Measurement of key metabolic enzyme activities in mammalian cells using rapid and sensitive microplate‐based assays

Janke, R.; Genzel, Yvonne; Wahl, A.; Reichl, Udo

doi:10.1002/bit.22817

Cited by 30 publications

(46 citation statements)

References 82 publications

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“…Pyruvate Dehydrogenase Activity (PDH) Activity Assay-PDH activity was measured using an NADH cycling assay in the presence of diaphorase to reduce the generated NADH and MTT (3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide) was as an electron acceptor (27). Purified PDH protein from pig heart was incubated with 1 mM MgCl 2 , 5 mM CaCl 2 , 5 mM l-carnitine, 0.2 mM thiamine pyrophosphate, 0.1 mM CoA, 2.5 mM NAD ϩ , 1 mM MTT, and 1 unit/ml diaphorase in 50 mM HEPES/KOH buffer, pH 7.5, at 30°C.…”

Section: Methodsmentioning

confidence: 99%

Inhibition of Mitochondrial Pyruvate Transport by Zaprinast Causes Massive Accumulation of Aspartate at the Expense of Glutamate in the Retina

Cleghorn

Contreras

et al. 2013

Journal of Biological Chemistry

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Background: Pyruvate transport into mitochondria is a key step in energy metabolism. Zaprinast is a well known phosphodiesterase inhibitor.Results: Zaprinast has a strong influence on pyruvate transport into mitochondria. Conclusion: Inhibition of the mitochondrial pyruvate carrier by Zaprinast causes accumulation of aspartate at the expense of glutamate. Significance: Maintenance of normal amino acid levels in the retina relies on pyruvate transport into mitochondria.

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Section: Methodsmentioning

confidence: 99%

Inhibition of Mitochondrial Pyruvate Transport by Zaprinast Causes Massive Accumulation of Aspartate at the Expense of Glutamate in the Retina

Cleghorn

Contreras

et al. 2013

Journal of Biological Chemistry

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“…The assay was conducted according to the protocol of Janke et al 12,13 ATP produced by PK from ADP and phosphoenolpyruvate was fed into the glycerol-3-phosphate cycling assay by glycerol kinase. Optimal conditions for measuring glycerol-3-phosphate levels to indicate maximal PK activity included a cell dilution factor (CDF) of 150, pH 7.0, and 60-minute incubation time.…”

Section: Pk Enzyme Activitymentioning

confidence: 99%

PPARα and fatty acid oxidation mediate glucocorticoid resistance in chronic lymphocytic leukemia

Tung

Shi

Wong

et al. 2013

Blood

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Key Points• Glucocorticoids downregulate PKM2 and metabolism in CLL cells, impairing access to bioenergetic programs needed to repair cell damage.• PPARa and fatty acid oxidation antagonists potentiate the cytotoxic effects of glucocorticoids.High-dose glucocorticoids (GCs) can be a useful treatment for aggressive forms of chronic lymphocytic leukemia (CLL). However, their mechanism of action is not well understood, and resistance to GCs is inevitable. In a minimal, serum-free culture system, the synthetic GC dexamethasone (DEX) was found to decrease the metabolic activity of CLL cells, indicated by down-regulation of pyruvate kinase M2 (PKM2) expression and activity, decreased levels of pyruvate and its metabolites, and loss of mitochondrial membrane potential. This metabolic restriction was associated with decreased size and death of some of the tumor cells in the population. Concomitant plasma membrane damage increased killing of CLL cells by DEX. However, the nuclear receptor peroxisome proliferator activated receptor a (PPARa), which regulates fatty acid oxidation, was also increased by DEX, and adipocyte-derived lipids, lipoproteins, and propionic acid protected CLL cells from DEX. PPARa and fatty acid oxidation enzyme inhibitors increased DEX-mediated killing of CLL cells in vitro and clearance of CLL xenografts in vivo. These findings suggest that GCs prevent tumor cells from generating the energy needed to repair membrane damage, fatty acid oxidation is a mechanism of resistance to GC-mediated cytotoxicity, and PPARa inhibition is a strategy to improve the therapeutic efficacy of GCs. (Blood. 2013;122(6):969-980)

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“…The microplate-based assays offer benefits in terms of fast sample handling, analysis of multiple samples, small volume, continuous monitoring and convenience, which are beneficial to the practical application [21,22]. A few groups reported the assays for thrombin by using microplates as solid support and DNA aptamers as affinity ligands in different formats [23][24][25][26][27][28].…”

Section: Introductionmentioning

confidence: 99%

Microplate based assay for thrombin detection using an RNA aptamer as affinity ligand and cleavage of a chromogenic or a fluorogenic peptide substrate

Líu

Zhao

2016

Microchim Acta

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The authors report on a microplate based thrombin assay by using an RNA aptamer (Toggle-25) as the affinity ligand. The aptamer is nuclease-resistant because it contains nucleobases modified with 2′-deoxyfluoro saccharides. The aptamer is coated on the surface of the wells of microplates where it captures thrombin from a sample. Following a washing step, a chromogenic or a fluorogenic peptide substrate is added which is cleaved by the captured thrombin to form a yellow product (with absorbance at 405 nm) or a blue fluorescent product (with an emission maximum at 444 nm) after incubation at 37°C for 2 h. The assay enables thrombin to be determined with a 10 fM detection limit when using the fluorogenic substrate. The assay is selective in that several other proteins do not interfere. The assay can be applied to the determination of thrombin in diluted human serum and plasma.

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Measurement of key metabolic enzyme activities in mammalian cells using rapid and sensitive microplate‐based assays

Cited by 30 publications

References 82 publications

Inhibition of Mitochondrial Pyruvate Transport by Zaprinast Causes Massive Accumulation of Aspartate at the Expense of Glutamate in the Retina

Inhibition of Mitochondrial Pyruvate Transport by Zaprinast Causes Massive Accumulation of Aspartate at the Expense of Glutamate in the Retina

PPARα and fatty acid oxidation mediate glucocorticoid resistance in chronic lymphocytic leukemia

Microplate based assay for thrombin detection using an RNA aptamer as affinity ligand and cleavage of a chromogenic or a fluorogenic peptide substrate

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