An Amplex Red-based fluorometric and spectrophotometric assay for l-asparaginase using its natural substrate

Karamitros, Christos S.; Lim, Jiseok; Konrad, Manfred

doi:10.1016/j.ab.2013.09.028

Cited by 24 publications

(22 citation statements)

References 21 publications

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“…However, this method has certain limitations such low sensitivity and the fact that it do not measure intracellular ASNase activity (Vaishali and Bhupendra, 2017). After the initial screening, other methods are required for the quantitative evaluation of enzymatic activity such as the aforementioned Nessler's reaction (Peterson and Ciegler, 1969); the L-aspartyl-β-hydroxamic acid (AHA) method, wich evaluates aspartyl β-hydroxamate formation after L-asparagine hydrolysis in the presence of hydroxylamine (Frohweinm et al, 1971); circular dichroism spectroscopy (Kudryashova and Sukhoverkov, 2016); amplex Red method (Karamitros et al, 2014), among others. The screening methods for finding enzymes with reduced glutaminase activity are similar to the plate methods used for ASNase activity detection, i.e., they are based on pH switch, but use GLN instead of ASN as a substrate.…”

Section: L-asparaginase Manufacturing: Production Process and Purificmentioning

confidence: 99%

Development of L-Asparaginase Biobetters: Current Research Status and Review of the Desirable Quality Profiles

Brumano

Silva

Costa-Silva

et al. 2019

Front. Bioeng. Biotechnol.

142

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L-Asparaginase (ASNase) is a vital component of the first line treatment of acute lymphoblastic leukemia (ALL), an aggressive type of blood cancer expected to afflict over 53,000 people worldwide by 2020. More recently, ASNase has also been shown to have potential for preventing metastasis from solid tumors. The ASNase treatment is, however, characterized by a plethora of potential side effects, ranging from immune reactions to severe toxicity. Consequently, in accordance with Quality-by-Design (QbD) principles, ingenious new products tailored to minimize adverse reactions while increasing patient survival have been devised. In the following pages, the reader is invited for a brief discussion on the most recent developments in this field. Firstly, the review presents an outline of the recent improvements on the manufacturing and formulation processes, which can severely influence important aspects of the product quality profile, such as contamination, aggregation and enzymatic activity. Following, the most recent advances in protein engineering applied to the development of biobetter ASNases (i.e., with reduced glutaminase activity, proteolysis resistant and less immunogenic) using techniques such as site-directed mutagenesis, molecular dynamics, PEGylation, PASylation and bioconjugation are discussed. Afterwards, the attention is shifted toward nanomedicine including technologies such as encapsulation and immobilization, which aim at improving ASNase pharmacokinetics. Besides discussing the results of the most innovative and representative academic research, the review provides an overview of the products already available on the market or in the latest stages of development. With this, the review is intended to provide a solid background for the current product development and underpin the discussions on the target quality profile of future ASNase-based pharmaceuticals.

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Section: L-asparaginase Manufacturing: Production Process and Purificmentioning

confidence: 99%

Development of L-Asparaginase Biobetters: Current Research Status and Review of the Desirable Quality Profiles

Brumano

Silva

Costa-Silva

et al. 2019

Front. Bioeng. Biotechnol.

142

View full text Add to dashboard Cite

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“…We measure and compare the kinetics for bead stoichiometries ranging from 1:0 to 1:3. The cascade reaction becomes faster upon increasing the number of aspartate oxidase beads (Figure f), in qualitative agreement with the observation in bulk that the reaction is limited by the amount of aspartate oxidase . We note that the background increase observed in the case of beads containing only the asparaginase‐overexpressing cells is likely to arise from the presence of aspartate oxidase endogenously expressed by our E. coli strains.…”

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confidence: 99%

From Compartmentalization of Bacteria within Inorganic Macrocellular Beads to the Assembly of Microbial Consortia

et al. 2018

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Microorganisms are highly efficient biocatalysts. Yet making use of their capabilities for chemical transformations requiring synergistic interactions between different microbes is challenging as the competition for resources might reduce the diversity and ultimately disrupt the synergies. Here, a new method is proposed for constructing microbial consortia for the integration of multistep transformations. Bacteria are successively grown and trapped within semipermeable inorganic foams produced as millimeter‐sized beads. The beads function as efficient living biocatalysts is demonstrated. These living heterogeneous biocatalysts are manipulated to perform cycles of biochemical reactions and furthermore assembled to perform preprogrammed sequences of reactions. This new family of living advanced biocatalysts should find applications in a wide range of basic research and industrial systems where complex tasks have to be performed by controlled consortia of microorganisms.

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“…ROS concentration was analyzed using the fluorescence microscope (Leica Microsystems). Intracellular H 2 O 2 level was measured by Amplex Red assay as previously reported (17,18).…”

Section: Methodsmentioning

confidence: 99%

Ginkgo biloba extract protects human neuroblastoma SH‑SY5Y cells against oxidative glutamate toxicity by activating redoxosome‑p66Shc

Wang¹,

Jing²,

Zhu³

et al. 2021

Exp Ther Med

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Ginkgo biloba extract (GBE), a traditional Chinese herbal medicine component, is widely used to alleviate symptoms of neurodegenerative diseases. It has been confirmed that GBE exerts its pharmacological effect mainly due to its antioxidant activity; however, the molecular mechanism responsible for this effect remains unclear. The aim of the present study was to investigate the detailed mechanism of GBE, the main component of Gingko biloba dropping medicine, against oxidative glutamate toxicity in human neuroblastoma SH-SY5Y cells. The SH-SY5Y cells were untreated or pretreated with GBE followed by glutamate stimulation. Cell viability was assessed using an MTT assay. In addition, oxidative stress indexes, including intracellular ROS generation and NADPH oxidase and caspase activity, were also measured. The protein expression of key signaling factors involved in the redoxosome-p66Shc pathway was evaluated to elucidate the neuroprotective effect of GBE. The results showed that GBE treatment significantly attenuated the glutamate-induced cytotoxicity in SH-SY5Y cells by suppressing oxidative stress. A mechanical study revealed that redoxosome-p66Shc activation was associated with glutamate-induced cytotoxicity, which caused mitochondrial dysfunction and cell death. Interestingly, GBE treatment attenuated the activation of redoxosome-p66Shc in a dose-dependent manner, which suggested that the protective effect of GBE on SH-SY5Y cells against oxidative glutamate toxicity may be mediated by the modulation of redoxosome-p66Shc signaling. The current findings contribute to a better understanding of the therapeutic effect of GBE and indicate that redoxosome-p66Shc signaling might be a novel therapeutic target in the prevention and/or treatment of neurodegenerative diseases.

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An Amplex Red-based fluorometric and spectrophotometric assay for l-asparaginase using its natural substrate

Cited by 24 publications

References 21 publications

Development of L-Asparaginase Biobetters: Current Research Status and Review of the Desirable Quality Profiles

Development of L-Asparaginase Biobetters: Current Research Status and Review of the Desirable Quality Profiles

From Compartmentalization of Bacteria within Inorganic Macrocellular Beads to the Assembly of Microbial Consortia

Ginkgo biloba extract protects human neuroblastoma SH‑SY5Y cells against oxidative glutamate toxicity by activating redoxosome‑p66Shc

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