Purification and Characterization of Glutaminase Free Asparaginase from Enterobacter cloacae: In-Vitro Evaluation of Cytotoxic Potential against Human Myeloid Leukemia HL-60 Cells

Husain, Islam; Sharma, Anjana; Kumar, Suresh; Malik, Fayaz

doi:10.1371/journal.pone.0148877

Cited by 84 publications

(49 citation statements)

References 59 publications

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“…This frequently results in dreadful side effects in patients including a drastic drop in cell counts (WBC and RBC) and severe anemic conditions. Although erythrocytes are not good models for normal cells, to understand whether asparaginase is hemocompatible, hemolysis assay was performed on erythrocytes .The in vitro hemolysis assay results were in concordance with earlier reports of Husain et al and Mahajan et al which showed l ‐asparaginase purified from Enterobacter cloacae and Bacillus licheniformis RAM‐8 was not toxic to human erythrocytes at higher concentrations. This result may suggest that l ‐asparaginase may exert selective cytotoxicity only on leukemic cells, making it an ideal candidate for cancer chemotherapy especially for leukemia.…”

Section: Discussionsupporting

confidence: 85%

“…The DNA fragmentation results were in concordance with earlier reports by Story et al which showed characteristic fragmentation of DNA of mouse lymphoma cell line (LY‐TH) after l ‐asparaginase treatment indicating apoptosis as the mode of cell death. l ‐asparaginase purified from Enterobacter cloacae also showed characteristic laddering pattern of DNA of human myeloid leukemia HL‐60 cell line . The fragmentation of DNA may be due to the activation of caspase 3 which inactivates DFF‐45 (DNA fragmentation factor) and ICDA (Inhibitor of caspase‐activated DNase) which in turn release active DFF‐40 or CAD (caspase‐activated DNase) .…”

Section: Discussionmentioning

confidence: 99%

“…The cytotoxicity of purified l ‐asparaginase was tested against human leukemic cell lines and found decrease in the cell viability of Jurkat cells in a dose‐dependent manner. Several reports earlier suggest the in vitro cytotoxicity of purified l ‐asparaginase against different cell lines such as human myeloid leukemia HL‐60 , human breast cancer MCF‐7 and human myelogenous leukemia K‐562 , human colon cancer CACO‐2 and human cancer prostrate PC‐3 , gastric cancer (AGS) , hepato cellular carcinoma (Hep‐G2) and human gastric cancer cell line (MKN‐28) and human T lymphoblastic leukemia cell line (MOLT‐4) . l ‐asparaginase purified from Penicillium brevicompactum NRC 829 and Aspergillus flavus (KUFS20) was cytotoxic to hepatocellular carcinoma (Hep‐G2) and human breast cancer cells (MCF‐7) with IC 50 value of 43.3 and 120.87 μg/mL, respectively .…”

Section: Discussionmentioning

confidence: 99%

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Growth inhibitory and proapoptotic effects of l‐asparaginase from Fusarium culmorum ASP‐87 on human leukemia cells (Jurkat)

Meghavarnam

Salah

Sreepriya

et al. 2016

Fundamemntal Clinical Pharma

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The objective of this study was to evaluate the anticancer properties of l-asparaginase purified from fungal isolate Fusarium culmorum ASP-87 against human T-cell leukemia cell line (Jurkat). The growth inhibitory and proapoptotic effects of purified l-asparaginase on Jurkat cell lines were investigated by determining its influence on cell viability, colony formation, DNA fragmentation, and cell cycle progression. The results revealed that purified l-asparaginase showed significant decrease in cell survival with IC value of 90 μg/mL (9 IU/mL). The enzyme inhibited colony formation and showed characteristic laddering pattern on agarose gel thereby confirming the induction of apoptosis. Further, cell cycle analysis revealed that the enzyme induced apoptotic cell death by arresting the growth of cells at G -M phase. However, the enzyme did not elicit any toxic effects on human erythrocytes. l-asparaginase purified from F. culmorum ASP-87 showed significant and selective cytotoxic and apoptotic effects on human T-cell leukemic cells in dose-dependent manner. Results of the study give leads for the anticancer effects of fungal l-asparaginase and its potential usefulness in the chemotherapy of leukemia.

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Section: Discussionsupporting

confidence: 85%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

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Growth inhibitory and proapoptotic effects of l‐asparaginase from Fusarium culmorum ASP‐87 on human leukemia cells (Jurkat)

Meghavarnam

Salah

Sreepriya

et al. 2016

Fundamemntal Clinical Pharma

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“…Removing the presence of glutaminase activity in L-asparaginase preparation will increase the efficacy of ALL treatment. Husain et al (2016), reported the cytotoxicity of purified glutaminasefree asparaginase from Enterobacter cloacae. The purified asparaginase free of glutaminase suppresses the proliferation of cancer cell HL-60 and non-toxic to normal cells in vitro.…”

Section: Isolation and 16s Rrna Analysismentioning

confidence: 99%

Screening of Bacteria Producing Asparaginase Free of Glutaminase and Urease from Hot Springs in West Sulawesi

Setiawan

Larasati

2019

J Bio Bio Edu

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L-asparaginase catalyzes the hydrolysis of asparagine into ammonia and aspartate. It has been used in chemotherapy for patients with acute lymphoblastic leukemia. L-asparaginase presents in animal, plant and microorganism. Long-term application of this enzyme can induce neurotoxicity due to the affinity towards glutamine and urea. The aim of this research was to find new source of glutaminase and urease-free asparaginase from bacteria. Bacteria were isolated from hot springs located in West Sulawesi using R2A media. The identification was employed by amplifying 16S rRNA gene. Screening of asparaginase was conducted using asparagine as single source of Nitrogen. Out of 21 isolates, 76% were Gram-negatives from the genus of Pseudomonas, Acinetobacter, Bosea, Caulobacter, Sphingomonas and Novosphingobium, while the rest of them were Gram-positives from the genus of Mycobacterium, Brachybacterium, Rhodococcus, and Staphylococcus. Twelve isolates which showed asparaginase activity were Caulobacter flavus HS1YWS2 and HS1XWS3, Acinetobacter sp. HS2XWS5, HS2XWS6, HS2XWS8, HS2YWS11, HS2YWS12, HS2YWS13, HS2ZWS14, HS2ZWS15 and HS2ZWS16. Isolates HS1YWS2 and HS1XWS3 were free of glutaminase and urease and showed the highest activity. This study was the first report of asparaginase activity from Caulobacter flavus. This result can further be used to explore the ability of asparaginase free of glutaminase and urease to treat acute lymphoblastic leukemia.

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“…In addition, most L‐asparaginases have low catalytic activity and low stability as well as are only active in a narrow pH range (Jr et al, ; Zuo, Zhang, Jiang, & Mu, ). Many enzymes with L‐asparaginase activity are quite specific for L‐asparagine, but also have a low level of intrinsic L‐glutaminase activity that hydrolyzes the amino acid L‐glutamine, which is an undesirable effect for the food industry (Husain, Sharma, Kumar, & Malik, ; Shrivastava et al, ). Hence, it is necessary to search for novel L‐asparaginases since drawbacks in the food industry are increasingly reported (Zhang et al, ).…”

Section: Introductionmentioning

confidence: 99%

Antitumor activity and ability to prevent acrylamide formation in fried foods of asparaginase from soybean root nodules

2019

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A novel asparaginase (designated srnASNase) has been purified from soybean root nodules and identified by MALDI‐TOF/TOF‐MS. And the enzymatic properties, antitumor activity and the ability to prevent acrylamide formation in fried foods of srnASNase were evaluated. SrnASNase had high specific activity (531.37 U/mg) toward L‐asparagine under optimum conditions (pH 8.0 and 40°C), no activity toward L‐glutamine and D‐glutamine, but trace activity toward D‐asparagine. It was stable in the pH range of 7.0–9.0 and up to 40°C. The Km and Vmax of srnASNase were 0.36 mM and 51.64 mM/min, respectively. Further, in vitro anti‐proliferative activity on human cancer cells assay showed that srnASNase was superior to commercial asparaginase in solution by controlling the tumor cell growth with time. In addition, srnASNase showed more effective acrylamide mitigation than commercial asparaginase in fried foods. These results indicate that srnASNase is a potential candidate for applications in the food processing and pharmaceutical industry. Practical applications L‐asparaginase (L‐asparagine amidohydrolase; EC 3.5.1.1) is an enzyme that catalyzes the hydrolysis of the amide group of the side‐chain of L‐asparagine into aspartic acid and ammonia. It has long been used as a primary component in the treatment of acute lymphoblastic leukemia (All) and other related blood cancers. Apart from its clinical usage, L‐asparaginase has attracted more attention in the food processing industries as a promising acrylamide‐mitigating agent in recent years. This research revealed that soybean root nodules might be good sources of novel asparaginase.

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Purification and Characterization of Glutaminase Free Asparaginase from Enterobacter cloacae: In-Vitro Evaluation of Cytotoxic Potential against Human Myeloid Leukemia HL-60 Cells

Cited by 84 publications

References 59 publications

Growth inhibitory and proapoptotic effects of l‐asparaginase from Fusarium culmorum ASP‐87 on human leukemia cells (Jurkat)

Growth inhibitory and proapoptotic effects of l‐asparaginase from Fusarium culmorum ASP‐87 on human leukemia cells (Jurkat)

Screening of Bacteria Producing Asparaginase Free of Glutaminase and Urease from Hot Springs in West Sulawesi

Antitumor activity and ability to prevent acrylamide formation in fried foods of asparaginase from soybean root nodules

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