Asparaginase: an old drug with new questions

The long-term outcome of acute lymphoblastic leukemia has improved dramatically due to the development of more effective treatment strategies. L-asparaginase (ASNase) is one of the main drugs used and causes death of leukemic cells by systematically depleting the non-essential amino acid asparagine....

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Veröffentlicht in:Hematology, Transfusion and Cell Therapy Transfusion and Cell Therapy, 2020-07, Vol.42 (3), p.275-282
Hauptverfasser: Cecconello, Daiane Keller, Magalhães, Mariana Rodrigues de, Werlang, Isabel Cristina Ribas, Lee, Maria Lucia de Martino, Michalowski, Mariana Bohns, Daudt, Liane Esteves
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Sprache:eng
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Zusammenfassung:The long-term outcome of acute lymphoblastic leukemia has improved dramatically due to the development of more effective treatment strategies. L-asparaginase (ASNase) is one of the main drugs used and causes death of leukemic cells by systematically depleting the non-essential amino acid asparagine. Three main types of ASNase have been used so far: native ASNase derived from Escherichia coli, an enzyme isolated from Erwinia chrysanthemi and a pegylated form of the native E. coli ASNase, the ASNase PEG. Hypersensitivity reactions are the main complication related to this drug. Although clinical allergies may be important, a major concern is that antibodies produced in response to ASNase may cause rapid inactivation of ASNase, leading to a worse prognosis. This reaction is commonly referred to as "silent hypersensitivity" or "silent inactivation". We are able to analyze hypersensitivity and inactivation processes by the measurement of the ASNase activity. The ability to individualize the ASNase therapy in patients, adjusting the dose or switching patients with silent inactivation to an alternate ASNase preparation may help improve outcomes in those patients. This review article aims to describe the pathophysiology of the inactivation process, how to diagnose it and finally how to manage it.
ISSN:2531-1379
2531-1387
2531-1387
DOI:10.1016/j.htct.2019.07.010