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

Brumano, Larissa Pereira; Silva, Francisco Vitor Santos da; Costa-Silva, Tales A.; Apolinário, Alexsandra Conceição; Santos, João H. P. M.; Kleingesinds, Eduardo Krebs; Monteiro, Gisele; Rangel-Yagui, Carlota de Oliveira; Benyahia, Brahim; Pessoa, Adalberto

doi:10.3389/fbioe.2018.00212

Cited by 134 publications

(108 citation statements)

References 185 publications

(227 reference statements)

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“…l-Asparaginase from E. coli produces two types of enzyme, l-asparaginase I (ECI), found in the cytoplasm, and l-asparaginase II (ECII) of periplasmic origin. The latter is used for clinical applications and has a higher affinity (K m = 10-15 μM) to l-asparagine than ECI (K m = 3.5 mM) [2,8,120]. l-Asparaginases from E. chrysanthemi (Erc) and E. coli (ECII) have the similar mechanism of action against tumor cells, however their pharmacokinetics, affinity for the substrate (K m ), and immune system sensitization profile varies [120].…”

Section: Sources Of L-asparaginasementioning

confidence: 99%

“…The downstream processing contributes to around 60-80% of the total production costs of a biotherapeutics product. Therefore, it becomes important to explore how traditional methods can be substituted with efficient and cost-effective unconventional methods for recovery and purification of biopharmaceuticals [120]. The efficiency of the protein purification process can be monitored by determining specific activity, yield, and purification fold at each step.…”

Section: Downstream Processingmentioning

confidence: 99%

“…The efficiency of the protein purification process can be monitored by determining specific activity, yield, and purification fold at each step. Specific activity is a measure of enzyme purity and calculated by dividing total enzyme activity by total protein [117,120]. Yield or recovery (percent) is a measure of how well the enzyme activity is retained after each purification step as a percentage of the activity in the crude extract.…”

Section: Downstream Processingmentioning

confidence: 99%

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A comprehensive review on microbial l‐asparaginase: Bioprocessing, characterization, and industrial applications

Chand

Mahajan

Prasad

et al. 2020

Biotech and App Biochem

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l‐Asparaginase (E.C.3.5.1.1.) is a vital enzyme that hydrolyzes l‐asparagine to l‐aspartic acid and ammonia. This property of l‐asparaginase inhibits the protein synthesis in cancer cells, making l‐asparaginase a mainstay of pediatric chemotherapy practices to treat acute lymphoblastic leukemia (ALL) patients. l‐Asparaginase is also recognized as one of the important food processing agent. The removal of asparagine by l‐asparaginase leads to the reduction of acrylamide formation in fried food items. l‐Asparaginase is produced by various organisms including animals, plants, and microorganisms, however, only microorganisms that produce a substantial amount of this enzyme are of commercial significance. The commercial l‐asparaginase for healthcare applications is chiefly derived from Escherichia coli and Erwinia chrysanthemi. A high rate of hypersensitivity and adverse reactions limits the long‐term clinical use of l‐asparaginase. Present review provides thorough information on microbial l‐asparaginase bioprocess optimization including submerged fermentation and solid‐state fermentation for l‐asparaginase production, downstream purification, its characterization, and issues related to the clinical application including toxicity and hypersensitivity. Here, we have highlighted the bioprocess techniques that can produce improved and economically viable yields of l‐asparaginase from promising microbial sources in the current scenario where there is an urgent need for alternate l‐asparaginase with less adverse effects.

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Section: Sources Of L-asparaginasementioning

confidence: 99%

Section: Downstream Processingmentioning

confidence: 99%

Section: Downstream Processingmentioning

confidence: 99%

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A comprehensive review on microbial l‐asparaginase: Bioprocessing, characterization, and industrial applications

Chand

Mahajan

Prasad

et al. 2020

Biotech and App Biochem

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“…Regular supply of asparagine, maintained by asparagines synthetase, is requisite for making proteins in the cell. Leukemic cells however are de cient in asparagines synthetase and depend solely on circulating blood for the supply of L-asparagine (Brumano et al 2019). The immunogenic complications associated with its present microbial sources Escherichia coli, Erwinia caratovora limits its medicinal frontier.…”

Section: Introductionmentioning

confidence: 99%

Fungal endophytes of high altitude ethnomedicinal plants as a bioresource of industrially imperative enzymes

Kapoor

Mushtaque

Gambhir

2020

Preprint

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Endophytic fungi have been in the spotlight as a reservoir of novel agents with diverse bioactivities. Similarity in chemical diversity with the host plant makes them an amenable target for industrial interventions. A wide range of compounds as secondary metabolites and enzymes are manufactured inside the endophytic fungal factory. However, utilization of endophytic fungi as industrially imperative enzyme producers has been a scarce event. The present study was conducted to bio-prospect the fungal endophytes present in the high altitude medicinal plants of Uttarakhand, as industrially imperative enzyme producers. A total of 58 different endophytic isolates were obtained from Pinus sabiniana, Cinnamomum tamala, Cinnamomum verum, Ocimum tenuiflorum and Rhododendron arboreum. Endophytic fungal colonization was highest, 31%, in Pinus sabiniana. The pure isolates were further explored for the production of amylases, cellulases, proteases and L-asparaginase. Out of 58 isolates, 40 isolates exhibited potent enzyme productivity. #7PSSTB isolate was considered as superlative contender on account of its relatively higher production of all the three enzymes viz. amylases, cellulases, proteases. Partial purification of #7PSSTB extract showed compelling enzymatic activity corroborating the existence of exogenous enzyme in the extract. Interestingly, #9 RASTB, #11 RASTB and #17 RASTB exhibited the production of therapeutically imperative L-asparaginase enzyme. The present study puts the spotlight on endophytic diversity in the high altitude medicinal plants as a source of enzymes of industrial interest. Production of L-asparaginase paves the way of pharmaceutical intervention to explore anti-oncogenic effects in the endophytic fungal repository of high altitude regions.

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“…A enzima nativa de E. coli, a nativa de E. coli ligada covalentemente com polietilenoglicol (ASNase peguilada) e por fim a enzima nativa de Dickeya chrysanthemi (erwinase). Também há a formulação da enzima de E. coli produzida de forma recombinante (Spectrila®, Medac) (BRUMANO et al, 2019).…”

Section: A L-asparaginaseunclassified

Expressão da L-asparaginase II de >i<Saccharomyces cerevisiae>/i< recombinante extracelular com glicosilação humanizada em >i<Pichia pastoris>/i<

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

Cited by 134 publications

References 185 publications

A comprehensive review on microbial l‐asparaginase: Bioprocessing, characterization, and industrial applications

A comprehensive review on microbial l‐asparaginase: Bioprocessing, characterization, and industrial applications

Fungal endophytes of high altitude ethnomedicinal plants as a bioresource of industrially imperative enzymes

Expressão da L-asparaginase II de >i<Saccharomyces cerevisiae>/i< recombinante extracelular com glicosilação humanizada em >i<Pichia pastoris>/i<

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